9 Endometriosis
9 Endometriosis
9 Endometriosis
Editor
Endometriosis
Pathogenesis
and Treatment
123
Endometriosis
Tasuku Harada
Editor
Endometriosis
Pathogenesis and Treatment
Editor
Tasuku Harada
Department of Obstetrics
and Gynecology
Tottori University
Faculty of Medicine
Yonago, Tottori, Japan
v
Contents
Part I Introduction
vii
viii Contents
Index . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 469
Part I
Introduction
Chapter 1
Endometriosis: A Mysterious Disease
Tasuku Harada
1.1 Introduction
distinguished scientists to contribute a chapter and was happy that all graciously
agreed to do so. Our hope is that this book will provide useful information and fresh
knowledge to all doctors and scientists interested in endometriosis, and that it will
stimulate further research, and lead to more efficacious treatment modalities.
The prevalence of endometriosis in women varies widely: 0.711 % in
populations presenting for health care, 222 % when undergoing surgical steriliza-
tion, 1747 % among infertile women, and 274 % in women with chronic pelvic
pain [2]. An estimated 2.6 million Japanese women have this disease, extrapolating
a prevalence rate of 10 % among reproductive age women. An increase in the
incidence of endometriosis is worrisome because the birth rate in Japanese has
decreased and age of primiparous is reportedly over 30 years old. The number of
newborn babies is decreasing in Japan, while the population over 65 years old is
increasing. In such circumstances, infertility due to endometriosis of women is a
serious socioeconomical problem in Japan.
The assumption that the incidence of endometriosis is increasing is based on the
combination of the implantation theory of retrograde menstruation and the data of
well-known studies on epidemiology. Several well-designed epidemiological stud-
ies reported that shorter menstrual cycles, longer duration of flow, heavier men-
strual flow, and low parity are risk factors for endometriosis [3], indicating an
increased number of menstruation and retrograde reflux may increase risk of the
disease.
The classic theory on the pathogenesis of endometriosis includes implantation
theory, coelomic metaplasia theory, and embryonic Mullerian rests. A recent study
found that extrauterine stem cells originating from bone marrow may differentiate
into endometriotic tissues [4]. Although many researchers argue that modern
technologies of molecular medicine are unveiling the unsolved issues regarding
the pathogenesis of endometriosis, Sampsons implantation theory has never been
discarded.
Redwine raised a question about an intriguing point in Sampsons theory. His
paper entitled Was Sampson wrong? proposed that endometriotic tissues may not
be autotransplanted tissue. After reviewing more than 200 papers on autotransplants
and comparisons of endometriosis and endometrium, Redwine pointed out that a
majority of studies found multiple and significant alterations between ectopic
endometrium (endometriosis) and original endometrium. He suggested that endo-
metriosis is not a simple autotransplant, indicating that endometriosis is not a
displacement (implantation) of normal endometrium. Redwine concluded that
Sampson may be wrong [5].
We investigated the expression of inflammatory cytokines and prostaglandins in
eutopic endometrium and endometriotic tissues [68]. Recently, we obtained inter-
esting data regarding differential expression of inflammatory genes in eutopic
endometrium and endometriosis. We obtained endometriotic tissue from ovarian
chocolate cysts at the time of laparoscopic surgery, collected the two types of
eutopic endometrial tissues, and classified them as follows: (1) the disease-free
(F-Em: patients with benign ovarian tumor) and (2) endometriosis with ovarian
chocolate cysts (C-Em). Gene expression of interleukin-6 (IL-6), IL-8, and
1 Endometriosis: A Mysterious Disease 5
100 b 10.0
80 8.0 b 80
COX-2 mRNA
b
IL-6 mRNA
IL-8 mRNA
60 6.0 60
40 4.0 40
a a
20 2.0 20
a a a a
0 0 0
F-Em C-Em C F-Em C-Em C F-Em C-Em C
Fig. 1.1 Quantitative analysis of IL-6, IL-8, and COX-2 gene expression in human endometrial
and endometriotic tissues. The mRNA levels were evaluated by real-time RT-PCR. The abbrevi-
ations of the three types of tissues are as follows: (1) eutopic endometrial tissues of disease-free,
F-Em (n 15); (2) eutopic endometrium with ovarian chocolate cyst, C-Em (n 15); and (3) the
ovarian chocolate cyst, C (n 15). The mRNA level of F-Em (proliferative phase) set arbitrarily at
1.0. Data are the mean SE of three independent experiments. Bars that do not share a letter are
significantly different (P < 0.05)
References
2.1 Introduction
The term secondary mullerian system was first described by Lauchlan in 1972 [8].
He noted the propensity of the peritoneum which covers the surface of the ovary
and the peritoneal cavity to mullerian differentiation. The surface mesothelial and
the submesothelial stroma of peritoneum exhibit a full spectrum of mullerian
differentiation from benign to malignant. Many lesions of secondary mullerian
system are described, which are benign, such as endosalpingiosis, of the low
grade of malignancy, serous and mucinous and malignant, described as
extraovarian peritoneal serous and mucinous carcinomas, and endometriosis is
considered as the main lesson of the secondary mullerian system [9]. It is proposed
2 Pathological Aspect and Pathogenesis of Endometriosis 11
2.5.1 Transplantation
The theory of transplantation implies that the endometrium is replaced from the
uterus to another location inside the body. Many different ways of dissemination of
endometrial tissue are involved in this concept. Iatrogenic, lymphogenic, and
hematogenic spread account for uncommon, extraperitoneal lesion of endometri-
osis [13, 14]. The most easily understood, scientifically supported, and widely
accepted mechanism for the histogenesis of endometriosis is that, at menstruation,
some effluent flows retrograde through the lumen of fallopian tubes into the
12 R. Honda and H. Katabuchi
Fig. 2.1 Metaplasia of epithelial cells involved in endometriosis. (a) Metaplasia of tubal epithe-
lial cells. (b) Metaplasia of endocervical canal glandular cells. (c) Apocrine metaplasia. (d)
Intestinal metaplasia. Hematoxylineosin stain, (ad) 200 (Reprinted from Okamura and
Katabuchi [12] with permission of Int Rev Cytol.)
peritoneal cavity (Fig. 2.2). Indeed, the high frequency of this phenomenon is
supported by the finding of menstrual blood in the peritoneal fluid of up to 90 %
of women with patent fallopian tubes undergoing laparoscopy during the
perimenstrual period [16]. Although retrograde menstruation explains the physical
displacement of endometrial fragments into the peritoneal cavity, additional steps
are necessary for the development of endometriotic implants. Escape from the
immune clearance system, during the courses of attachment to the ovarian surface
epithelium and peritoneal mesothelium, invasion of the epithelium, establishment
of local neurovascularity, and continued growth and survival are necessary if
endometriosis is to develop from retrograde passage of the endometrium.
The theory of coelomic metaplasia suggests that the mesothelium of the peritoneum
including ovarian surface epithelium (OSE) can be transformed into endometrium
by metaplasia. The mullerian ducts, which constitute the primordial uterus, are
generated through intrusion of the coelomic epithelium in the antenatal stage.
For this reason, it has been proposed secondary mullerian system; the organs derived
2 Pathological Aspect and Pathogenesis of Endometriosis 13
Fig. 2.2 Histogenesis of endometriosis. (a) Exfoliated endometrial tissue (left arrow) floating in
the tubal cavity. (b) Endometrial tissue (left arrow) adhering to the peritoneum. Hematoxylin
eosin stain, (a) 40, (b) 100 (Reprinted from Katabuchi [15] with permission of J Japan Societ
Endo.)
from mullerian duct are generated from the same origin as that of the peritoneal
mesothelium and OSE [8, 17]. The peritoneal mesothelium and OSE may undergo
metaplasia into the endometrial epithelium and stroma, thereby inducing endome-
triosis. We rarely come across the histological evidence for this metaplastic progres-
sion in the ovarian surface as shown in Fig. 2.3 [17]. Moreover, in the observation
of morphological changes in a collagen-embedded culture system of the human
OSE [18], the OSE and the coculture of OSE with endometrial stromal cells
(ES) showed a luminal structure with estradiol (E2) supplementary (Fig. 2.4ac),
and, in the OSE/ES coculture, the nuclear position was deviated toward the basal
side and the appearance of cilia was observed [19]. The OSE/ES coculture was
positive for epithelial membrane antigen (EMA) and cytokeratin, indicating differ-
entiation into glandular cells, while the epithelium of the OSE culture was negative
for EMA. These findings suggest that the OSE can differentiate into glandular cells
and that E2 and endometrial stromal cells are involved in this process. Thus, flow of
endometrial stromal cells in the menstrual blood back through the fallopian tube may
be an important factor in the development of endometriosis [1820].
2.5.3 M
ullerian Ducts Remnants
In the antenatal phase, the coelomic epithelium gives rise to the mullerian ducts,
which constitute the fallopian tubes and the uterus and the upper portion of the
vagina. During the course of differentiation and migration of the mullerian ducts
and fetal organogenesis, some primordial cells might spread in the posterior pelvic
floor. This might explain the findings that endometriosis is frequently found in the
pouch of Douglas, uterosacral ligaments, and rectovaginal septum and even the
presence of endometriosis among young women with MayerRokitanskyKuster
Hauser syndrome.
14 R. Honda and H. Katabuchi
Fig. 2.3 Progression of a cyst enclosed in the ovary to endometriosis. Single layer of the surface
epithelium in the cortex of the ovary, which formed the cyst, moved to the glandular epithelium of
the endometrium (right arrow). Hematoxylin-eosin stain, 150 (Reprinted from Okamura and
Katabuchi [17] with permission of Ital J Anat Embryol.)
Fig. 2.4 Three-dimensional collagen gel-embedded cultures of the ovarian surface epithelium
(OSE). (a) In the OSE culture, a cavity formed after addition of estradiol 17 (10 ng/mL). (b, c) In
a coculture of OSE with the endometrial stoma, an epithelium-stoma structure formed, the surface
epithelium formed a cavity with a threedimensional structure, the position of the nucleus was
biased toward the basal side, and cilia appeared. Hematoxylineosin stain, (a) 200, (b) 400;
Uranyl acetate-lead citrate stain, (c) 17,000 (Reprinted from Ohtake et al. [19] with permission
of Fertil Steril.)
2 Pathological Aspect and Pathogenesis of Endometriosis 15
The upregulation of the antiapoptotic gene BCL-2 in eutopic and ectopic endome-
trium from women with endometriosis is reported, and a genetic alteration of
endometrial cells influencing their tendency to implant may be hereditary [25].
Linkage analysis has elucidated candidate genes with biological plausibility. The
largest of these involved over 1,000 families more than two affected sib pairs and
established significance for a susceptibility locus in the regions of chromosome
10q26 and 7p15 [26, 27].
2.6.3 Inflammation
From the studies of macrophages in the female reproductive organ since the
1980s [28, 29], the conceptualization of endometriosis as a pelvic inflammatory
condition is established. In patients with endometriosis, the peritoneal fluid is
remarkable for an increased number of activated macrophages and important
differences in the cytokine/chemokine profile. Macrophages produce and secrete
16 R. Honda and H. Katabuchi
2.7 Conclusions
The pathogenesis of endometriosis has been studied among major theories; how-
ever, no single theory is sufficient to explain the development of the disease. It has
been suggested that peritoneal endometriosis, chocolate cysts of the ovary, and
adenomyotic nodules of the rectovaginal septum or deeply infiltrating endometri-
osis are three different disease entities, each with a different pathogenesis. This
concept leads that diverse pathological conditions underlie endometriosis and leads
to the proposal of endometriosis as a series of syndromes that develop through
different mechanisms depending on the host tissue or organ. Recently, a combina-
tion of the metastatic and metaplastic theories has been favored to explain that
endometriosis represents a polygenetic disorder, with alterations in multiple bio-
logical pathways leading to a metaplastic process under the irritating effect of
endometrial tissue shed during retrograde menstrual flow. Thus, endometriosis
has a long medical and historical background and is appropriately referred to as
an enigmatic disease. Clinical treatment in line with individual pathology is
required because of the diverse symptoms and findings. Further assessment of the
pathology of endometriosis may open the way for development of new drugs for
this disease.
References
The lesions of early endometriosis are either transparent or translucent because they
still lack formation of vasculatures around them. We named these early lesions as
nonopaque lesions [10] because these lesions contain either of watery, serous, or
mucinous secretion and there is no collection of blood in the stroma by histology.
Once cellular attachment and invasion of endometrial cells are established, the
subsequent growth or maintenance of endometriotic lesions is maintained by
promotion of mitogenesis and angiogenesis with the continuation of menstrual
cycle. The growth-promoting effect of endometriosis is contributed by an orches-
trated action of estrogen and other inflammatory or proinflammatory mediators.
Over proliferation of microvessels in the growing endometriotic lesions causes
oozing of blood in the stroma and appears as blood-filled opaque red lesions by
laparoscope [10]. With the progression of time, there is deoxygenation process from
hemoglobin to methemoglobin or hemosiderin leading to color changes of these
opaque red lesions to black lesion or related lesions. In this stage, collection of
blood in the stroma disappears. Black lesion again changes to white lesion due to
collection of bilirubin or biliverdin and accumulation of fibrous tissue. In this stage,
gland gradually becomes smaller and stroma sometimes disappears due to deposi-
tion of fibrous tissue. Finally old lesions disappear and there is new focus of
endometriosis due to continuation of menstrual reflux. These sequential events
indicate that once exfoliated, the endometrium enters into the pelvic cavity and
becomes attached to the mesothelial layer, and then a process of angiogenesis,
22 K.N. Khan
Fig. 3.1 Shows the diagrammatic representation of the natural course of visible peritoneal
endometriosis in pelvic cavity. After initial attachment of refluxed endometrial cells with perito-
neal cells producing early endometriotic lesions, the consequent events of mitosis, angiogenesis,
metabolic degradation of heme, and appearances of fibrosis result in the generation of different
morphological appearances of peritoneal endometriosis as shown in this figure
heme metabolism, and fibrosis ensue to maintain the natural course of endometri-
osis (Fig. 3.1). A panel of nonopaque lesion, blood-filled opaque lesion, blue berry
spots, and their corresponding histological pictures is shown in Fig. 3.2.
As a cell component of innate immune system, peritoneal fluid (PF) and eutopic/
ectopic endometria derived from women with endometriosis have been shown to
contain higher numbers of activated M than in control women [11, 12]. This
results in the secretion of higher concentrations of growth factors and cytokines in
the PF as produced by the stimulated M in these patients [11]. Red peritoneal
lesions and their adjacent peritoneum had the greatest M infiltration, compared
with black/white lesions or chocolate cyst walls. These results indicate that early
endometriosis with red peritoneal lesions induces a higher inflammatory response
3 Visible and Invisible (Occult) Endometriosis 23
Fig. 3.2 Shows the laparoscopic and corresponding histologic appearance of nonopaque trans-
parent/translucent lesion (A, B), blood-filled opaque red lesion (C, D), and blue berry spots (E, F)
in pelvic cavity of women with peritoneal endometriosis. It can be noted here that nonopaque
endometriotic lesions such as vesicular bleb (A) lack oozing of blood in stroma (B) and opaque red
lesions such as blood bleb with ecchymosis (C) are accompanied by oozing of blood in the stroma
of these lesions (D). In contrast, black lesions such as blue berry spots (E) are manifested by color
change and disappearance of blood from the stroma of these lesions (F)
in the pelvic cavity than advanced endometriosis [12]. The inflammatory reactions
in the eutopic and ectopic endometria suggest that the growth of endometriosis does
not depend on the fibrotic extension of disease; rather, it depends on the tissue
activity of endometriosis. We presume that extension of disease could be related to
pelvic pain, but higher tissue activity of endometriosis associated with abundant
recruitment and infiltration of M could be related to infertility.
We measured endotoxin levels in the menstrual fluid (MF) and PF of women with
and without endometriosis. We found that the concentration of bacterial endotoxin
is two- to fourfold higher in the MF when compared with that in PF. Endotoxin
level in MF/PF was also significantly higher in women with endometriosis than in
control women [16]. We found the highest endotoxin level during the menstrual
phase and persistence of a small amount of endotoxin in the pelvis either in the
proliferative phase or in the secretory phase of the menstrual cycle [16]. This
indicates that MF of women with endometriosis is highly enriched with bacterial
endotoxin followed by the presence of a modest amount in the PF.
There is a possibility that the lower genital tract of women with or without
endometriosis is contaminated with a number of normal bacterial florae including
Escherichia coli (E. coli). Therefore, we speculated that there might be an ascend-
ing migration of E. coli from the vaginal lumen up into the uterine cavity that causes
contamination of menstrual blood and resulting in the subsequent release of endo-
toxin into menstrual blood and back to the peritoneal fluid. After bacteria culture
analysis, we found a significantly higher colony formation (CFU/ml) of E. coli in
the menstrual blood of women with endometriosis than that in control women [16].
3 Visible and Invisible (Occult) Endometriosis 25
The CFU of E. coli was also significantly higher in women containing red perito-
neal lesions than in women having only chocolate cyst.
Based on these findings of our serial experiments, we proposed a new bacterial
contamination hypothesis that may be involved in the growth regulation of visible
peritoneal endometriosis via LPS/TLR4 cascade [16]. This E. coli contamination of
menstrual blood is responsible for higher endotoxin levels in the MF and PF of
women with endometriosis. In search of a mechanistic basis of bacterial contam-
ination of menstrual blood, we found that higher concentrations of PGE2 in MF and
PF of women with endometriosis were involved in E. coli growth by its direct
bacterial proliferation effect or indirect immunosuppressive effect [17].
Fig. 3.3 Microscopically detected three patterns of invisible (occult) endometriosis in visually
normal peritoneum. Pattern I shows presence of typical gland/stroma; pattern II shows reactive
hyperplastic change of endometrioid epithelial cells with surrounding stroma; and pattern III
shows single-layered epithelium-lined cystic lesions with surrounding stromal cells (all in HE
stain, upper column). The identification of glandular epithelial cells, stromal cells, and peritoneal
mesothelial cells was confirmed by the immunoreaction to Ber-EP4, CD10, and calretinin,
respectively, and are shown against each HE-stained slide. Flat mesothelial cells derived from
normal peritoneum and mesothelioma cells as a positive control (inset) immunoreactive to
calretinin are shown at the right panel. The immunoreactions to nonimmune mouse IgG as a
negative control are shown on the extreme right panel. HE stain, hematoxylin and eosin stain.
Magnification of slides (200)
After careful observation and analysis, we collected 227 visually normal peritoneal
samples from 151 women with visible endometriosis and 78 samples from
62 women without any visible peritoneal lesions (control). We detected three
patterns of IME: (I) presence of typical gland/stroma, (II) reactive hyperplastic
change of endometrioid-like epithelium with surrounding stroma, and (III) single-
layered mesothelium- or epithelium-lined cystic lesions with surrounding rim of
stromal cells. All these IME lesions were confirmed by their immunoreactivity to
Ber-EP4 (marker of gland epithelium), CD10 (marker of stroma), and nonreactivity
to calretinin (marker of mesothelial cells) (Fig. 3.3).
We could detect variable patterns of IME in the normal peritoneum derived from
23 women with endometriosis (biopsy samples, n 27) and 4 control women
(biopsy samples, n 4) without visible endometriosis. The detection rate of IME
was as follows: for endometriosis, 15.2 % (23/151) and 11.8 % (27/227) and for
28 K.N. Khan
control women, 6.4 % (4/62) and 5.1 % (4/78) by the number of patients and
number of collected samples, respectively. A higher tendency in the incidence of
IME was found in women with visible endometriosis than in control women
( p 0.06 by patient number and p 0.07 by sample number) [27].
A predominance of IME occurrence was observed in pouch of Douglas and
uterovesical space than in other anatomical sites in pelvis. A dominant presence of
r-ASRM stages III endometriosis and red/black lesions and complaints of dys-
menorrhea were observed in women with visible endometriosis harboring IME in
their peritoneum [27].
The most alarming questions may arise now, how can we decide the origin of IME
lesions? Or is Sampsons theory enough to explain IME lesions? There is no
3 Visible and Invisible (Occult) Endometriosis 29
Fig. 3.4 Some hypothetical proposals that may be linked to the possible origin of invisible
(occult) microscopic endometriosis (IME) lesions. After initial attachment of menstrual debris
to the peritoneum, a sequence of epithelial-mesenchymal transition (EMT) or mesenchymal-
epithelial transition (MET) may be involved in the generation of IME. Hematogenous or
lymphogenous dissemination of shedding endometrial cells during menstruation could be another
mechanism. In addition to possible origin from progenitor cells/stem cells, cellular change of flat
mesothelium to cuboidal or columnar cells (metaplasia theory) or activated cells derived from
residing coelomic epithelium within peritoneum (mulleriosis, induction theory) in response to
pelvic inflammation could be linked to the origin of IME. Cells or tissues derived from mullerian
rests in association with peritoneal pockets can be another explanation for the development of IME
definite answer at this moment. But we argue that we can link each and every
theory supporting the origin of visible endometriosis [28] to the pathogenesis of
IME lesions. If Sampsons theory does not directly support the origin of IME
lesions, it can be indirectly explained by lymphatic or hematogenous spread of
menstrual debris and subsequent localization deep into peritoneum. We cannot
exclude the possibility of genetic factor or metaplastic transformation of peritoneal
mesothelial cells (metaplasia theory) in response to estrogen, inflammation, or
environmental factors. Despite possible origin of IME as a result of epithelial-
mesenchymal transition/mesenchymal-epithelial transition or from stem cells
[29, 30], activation of cells derived from coelomic epithelium (mulleriosis, induc-
tion theory) within peritoneum may be another possible mechanism to explain the
origin of IME [31]. Some hypothetical proposals that might be linked to the
possible origin of IME lesions are shown in Fig. 3.4.
We proposed for the first time a new concept bacterial contamination hypothesis in
endometriosis. Our results suggest that a substantial amount of endotoxin in perito-
neal fluid due to reflux of menstrual blood is involved in pelvic inflammation and
30 K.N. Khan
Acknowledgement I gratefully thank Dr. Michio Kitajima of Nagasaki University Hospital and
Dr. Akira Fujishita of Saiseikai Nagasaki Hospital for their kind assistance in sample collection;
Prof. Masahiro Nakashima of Atomic Bomb Disease Institute, Nagasaki for his experimental
advice; and Prof. Hideaki Masuzaki of Nagasaki University Hospital for reading/advice.
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6. Oosterlynck DJ, Cornillie FJ, Waer M, Vandeputte M, Koninckx PR. Women with endome-
triosis show a defect in natural killer activity resulting in a decreased cytotoxicity to autolo-
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32 K.N. Khan
Tetsuo Maruyama
4.1 Introduction
T. Maruyama (*)
Department of Obstetrics and Gynecology, School of Medicine, Keio University,
35 Shinanomachi, Shinjuku-ku, Tokyo 160-8582, Japan
e-mail: [email protected]
Before discussing the stem cell theory for the pathogenesis of endometriosis, I will
briefly introduce the current paradigm regarding tissue stem cells (adult stem cells),
CSCs, and their roles in cancer formation and metastasis.
Tissue-specific stem cells (also termed somatic stem cells or adult stem cells) are
found in a quiescent, undifferentiated state throughout the body [19]. They self-
renew through symmetric and/or asymmetric cell divisions. Growth is modulated
by physiological signals originating from the microenvironment or stem cell
niche. Asymmetric divisions generate lineage-committed cells that differentiate
and thereby maintain the tissue of origin. The tissue-specific stem cells and the
4 Role of Stem Cells in the Pathogenesis of Endometriosis 35
Stem cell
Undifferentiated
Self-renewal
Quiescent
Multidifferentiation Progenitor cell
Self-tissue reconstitution
Terminally differentiated
cells
Fig. 4.1 Hierarchy of adult stem cell differentiation. Within its microenvironmental niche, adult
stem cells generally remain quiescent. Under the proper conditions, the cells can be stimulated to
undergo asymmetric divisions to renew themselves and produce daughter/progenitor cells. The
latter cell further divides to produce transit-amplifying (TA) cells. The TA cells promptly
proliferate and differentiate into a variety of mature, functional cells
microenvironmental niche work together to keep a balance between the need for
cell replacement and the necessity of retaining a pool of primitive cells. In this
fashion, the structural and functional requirements of organs and tissues can be met
[19]. The hierarchy of tissue stem cells is illustrated in Fig. 4.1.
The classical or stochastic model (clonal evolution model) posits that any normal
(stem) cell, upon acquiring genetic and/or epigenetic modification(s) giving it
selective growth advantage, gives rise to a neoplastic clone of homogenous neo-
plastic cells [14, 15]. Upon the acquisition of additional genetic and/or epigenetic
change(s), it expands as a tumor. In this model, all cells within a tumor have equal
tumorigenic potentials [14, 15].
More recently, a hierarchical or CSC model has been developed. This model is
based upon the hypothesis that tumors consist of a heterogeneous population of
cells, only a small proportion of which are CSCs, also termed tumor-initiating cells
[14, 15, 20]. As depicted in Fig. 4.2, a small, self-renewing population of CSCs is
responsible for tumor initiation and growth maintenance. Thus, CSCs have been
operationally defined by their ability to generate tumors, and tumor-initiating cells
are thought to reflect the operational definition of CSCs [20]. The model states that
CSCs could originate from tissue stem cells or even differentiated cells that
acquired stem cell-like properties (including self-renewal) as a result of genetic
and/or epigenetic modifications [14, 15]. In the CSC model, completely mature
cells can fully dedifferentiate to become CSCs. In addition to genetic/epigenetic
36 T. Maruyama
Differentiation
Angiogenesis
Colonization
Primary tumor
EMT
Migration/Invasion
Intravasation
Systemic dissemination
Secondary tumor Extravasation
formation
Metastasis
De-differentiation
Dormancy
Colonization
Angiogenesis
MET
Normal stem cell Normal non-stem cell Cancer stem cell (CSC)
Fig. 4.2 Cancer stem cell (CSC) model for tumor formation and metastasis. Within tumors, a
small population of self-renewing CSCs is responsible for initiating tumor growth and maintaining
its presence. CSCs might be derived from tissue stem cells or more differentiated cells that gained
stem cell properties (including self-renewal) upon genetic and/or epigenetic modifications. Even
completely differentiated cells can develop into CSCs through dedifferentiation. The tumor
microenvironment (niche) maintains stem cell properties. CSCs that migrate away from the
primary site are capable of invasion, intravasation, systemic dissemination, and extravasation.
This behavior might be due to the EMT. Upon reaching distant tissues, the cells can reverse the
epithelial state by undergoing the MET. This promotes growth and the initiation of angiogenesis.
Alternatively, EMT programs per se might lead to the generation of CSCs
modifications, the tumor microenvironment (the CSC niche) is required for the
maintenance of stem cell properties. It likely includes many components, such as
stromal cells, blood vessels, extracellular matrix (ECM), growth factors, and
cytokines in a hypoxic environment. Exposure of non-CSCs to niche factors
might result in their acquisition of stem cell properties [14, 15].
4 Role of Stem Cells in the Pathogenesis of Endometriosis 37
The metastatic cascade includes tumor cell migration away from the site of the
primary tumor. It is now believed by many researchers that this process requires the
epithelialmesenchymal transition (EMT) [20, 21]. The EMT is a biological process
in which epithelial cells lose their cell polarity and cellcell adhesive properties. In
exchange, the cells gain migratory and invasive properties and undergo multiple
biochemical changes, thereby exhibiting a mesenchymal cell phenotype [22].
The EMT is observed in many processes, including mesoderm and neural tube
formation as well as wound healing, tissue regeneration, and organ fibrosis [22].
Our own data indicated that endometrial epithelial cells undergo EMT during
embryo implantation [23].
CSCs are likely involved in the formation of metastases [20, 21], as they exhibit
invasion, intravasation, systemic dissemination, and extravasation. It is believed that
such processes are enhanced by the EMT conversion [20, 21]. Subsequently, CSCs
that metastasize to distant tissues show colonization and reversion to an epithelial
state through reversal of the EMT, i.e., the mesenchymalepithelial transition
(MET), giving rise to metastatic lesions accompanied by angiogenesis [20].
Alternatively, the activation of EMT programs has been implicated in the generation
of CSCs [20, 21]. Furthermore, in addition to CSCs, non-CSC progeny cancer cells
might become CSCs through dedifferentiation at the metastatic sites and thereby
generate metastatic cancer lesions [20, 21] (Fig. 4.3).
For reference, Fig. 4.2 provides a representative CSC model. However, recent
studies have revealed complexities, such as plasticity of stem cell properties and
clonal diversity of CSCs in certain tumor types requiring revision of the original
CSC model. As a result, more complex models such as the dynamic stemness model
and the combinatory CSC and stochastic models have recently emerged [15].
Based on the principles of the cancer stem cell model illustrated in Fig. 4.2, I here
propose a stem cell model for the pathogenesis of endometriosis as depicted in
Fig. 4.3. This model incorporates the implantation theory, which is the most widely
accepted version among the many theories in this field. Note, however, that the
coelomic metaplasia theory and embryonic rest theory are also compatible with the
second part of this model in which some types of mesothelial cells and/or embry-
onic cell rests of mullerian origin behave as endometriosis-initiating cells
(endometriotic stem cells) and thereby give rise to endometriotic lesions at ectopic
site(s) [18].
38 T. Maruyama
Eutopic endometrium
Menstruation
EMT
Transtubal dissemination
De-differentiation
Hematogenous and lymphatic
dissemination
Intravasation
Extravasation
I. II. III.
Ectopic implantation
Attachment
Migration/Invasion
MET/Differentiation
Colonization
Angiogenesis
Establishment of
endometriotic lesions
Fig. 4.3 Three proposed stem cell models for the pathogenesis of endometriosis extrapolated
from the CSC model. Model I. Endometrial stem cells (EmSCs) are released from eutopic
endometrium most likely upon menstruation. EmSCs are transported to ectopic sites via retrograde
menstruation, lymphatic and vascular dissemination, direct migration, and invasion or some
combination. The EmSCs remain at the ectopic site through attachment, implantation, and/or
extravasation followed by invasion. EmSCs initiate self-renewal and/or asymmetric division to
generate progenitor cells, transit-amplifying cells, and more differentiated endometrial cells.
Because EmSCs and their progeny require a blood supply, angiogenesis is initiated, supporting
the expanding colony/endometriotic lesions. Model II. EmSCs undergo genetic and/or epigenetic
modifications at the eutopic or ectopic sites and thereafter behave as endometriosis-initiating cells
(EmoICs), giving rise to endometriotic lesions as shown in model I. Model III. EmSCs undergo
more extensive genetic and/or epigenetic modifications than in model II. Alternatively, terminally
differentiated endometrial cells undergo multiple and profound genetic and epigenetic changes
and thereby dedifferentiate into EmSC-like cells (not depicted in the schema). In either case, the
EmoICs are capable of generating a variety of endometrial cell components in a fashion similar to
model I
ectopic sites via many routes, including lymphatic and vascular dissemination,
direct migration and invasion, retrograde menstruation, or some combination
thereof. The endometrial stem cells settle ectopically in new sites by attachment,
implantation, extravasation, and, finally, invasion. Upon reaching the ectopic site,
the endometrial stem cells might undergo self-renewal or divide asymmetrically. In
this way, they can self-renew as well as produce progenitor cells, transit-amplifying
cells, and more differentiated endometrial cells (Fig. 4.3, model I). This process is
based on the behavior of general tissue stem cells (Fig. 4.1). Endometrial stem cells
and their proliferating daughter cells require a blood supply to flourish. Therefore,
they induce angiogenesis, permitting them to undergo clonal growth. In this
fashion, endometriotic lesions are formed.
In model II, endometrial stem cells are subject to genetic (or epigenetic) mod-
ifications within the eutopic or ectopic sites. The modifications permit them to act
as endometriosis stem cells, also termed endometriosis-initiating cells, produc-
ing endometriotic lesions. Notably, in this model, they retain the proliferative and
differentiative potential of endometrial stem cell-like cells, allowing them to
generate components of the endometrium, including glandular, stromal, endothe-
lial, and smooth muscle cells. Like CSCs and tumor-initiating cells as mentioned
previously [20], I here operationally define endometriosis stem cells by their stem
cell-like properties and ability to generate endometriosis with high efficiency, and
endometriosis-initiating cells, therefore, reflect the operational definition of
endometriosis stem cells. Thus, endometriosis-initiating cells is used herein
as a synonym of endometriosis stem cells.
In model III, endometrial stem cells undergo additional genetic and/or epige-
netic modifications and thereafter behave as endometriosis-initiating cells, pro-
ducing endometriotic lesions. Alternatively, terminally differentiated endometrial
cells could undergo multiple profound genetic and epigenetic modifications
resulting in dedifferentiation into endometrial stem cell-like cells capable of gen-
erating a variety of endometrial cell populations, including glandular, stromal,
endothelial, and smooth muscle cells. However, it seems likely that such profound
modifications would destroy the cells capability for multipotential differentiation.
Hence, this pathway might result in carcinogenesis. Thus, model III might explain
endometriosis-originated cancers such as clear-cell carcinoma and endometrioid
cancer. In fact, Pten and K-ras double mutations in the mouse give rise to
endometrioid adenocarcinoma of the ovary, whereas single mutation of K-ras
results in pelvic endometriosis [24].
It is important to note that the processes displayed in models IIII are likely
modulated by the microenvironments in which the cells associate themselves.
Microenvironmental influences could include menstrual efflux, peritoneal fluids,
inflammation, and the ECM of the peritoneum, all of which might regulate molec-
ular/cellular events. Thus, invasion, intravasation, extravasation, colonization,
angiogenesis, EMT, and MET could all be affected by the microenvironment. It
should be emphasized that EMT and MET could play critical roles in the passage of
endometrial stem cells from eutopic sites to ectopic sites and the resultant gener-
ation of endometriotic lesions.
40 T. Maruyama
The stem cell theory for the pathogenesis of endometriosis is not merely a hypothesis.
Rather, a number of studies have emerged that support this model [18, 16]. The
supportive evidence is summarized below.
The metastatic cascades initiated by CSCs and non-CSC cancer cells likely involve
the EMT and the MET [20, 21]. In fact, generation of CSCs probably involves the
activation of EMT programs [20, 21]. Thus, it is intriguing that EMT- and
MET-like processes are also involved in the pathogenesis of endometriosis [25].
For example, menstrual effluent can induce the EMT in mesothelial cells [26].
Consider also side population (SP) cells, a population with a high efflux ability of
Hoechst 33342 dye defined by flow cytometric techniques [27]. SP cells constitute
an undifferentiated population that resides in a number of tissues [28]. SP cells have
been isolated from an endometrial cancer cell line, and they represent likely
candidates for endometrial CSCs. These cells possess a high capacity to develop
into mesenchymal cell lineages, a reflection of EMT activity [29]. These data are
consistent with the endometriosis stem cell model. In other words, menstruation
might induce EMT pathways in endometrial stem cells and their progeny. In turn,
this might induce the cells to migrate away from the eutopic endometrium. Once
implanted in an ectopic microenvironment, invasion and establishment of
endometriotic lesions could occur through MET at the ectopic site.
In models II and III, Fig. 4.3, primitive endometriosis-initiating cells are thought to
express several stem cell markers. Thus, clonal expansion generates endometriotic
lesions and the endometriosis-initiating cells retain their original stem cell markers.
Experiments have shown that cells present in or adjacent to endometriotic lesions
express several stem cell markers including OCT4/POU5F1 and ABCG2 [3033].
OCT4/POU5F1 is expressed by embryonic stem cells, germ cells, and some types
of adult stem cells. This protein plays a crucial role in maintaining stem cell
pluripotency [34]. Another stem cell marker is adenosine triphosphate-binding
cassette transporter G2 (ABCG2). ABCG2 is highly expressed in a variety of
stem cells. It is responsible for removing exogenously added fluorescent dye,
Hoechst 33342, and produces the SP phenotype characteristic of stem cells [35].
Thus, the expression of these stem cell markers in endometriotic lesions supports
the presence of stem cells and provides indirect evidence for the stem cell model.
4 Role of Stem Cells in the Pathogenesis of Endometriosis 41
The endometriosis stem cell model predicts that endometriotic lesions should
contain a stem cell-like cell population. Chan et al. reported that ovarian
endometriomas contain a subset of cells displaying a number of somatic stem cell
properties. They include colony-forming activity, self-renewal capacity, and
multipotency [37].
Several theories have been proposed to explain both the origin and pathogenesis of
endometriosis. These hypotheses include retrograde menstruation (implantation),
coelomic metaplasia, and the embryo rest theories [2, 18, 16, 3840]. Retrograde
menstruation (implantation) is the most widely accepted because it is a reasonable
explanation for various types of endometriosis, including peritoneal endometriosis
[38, 40] and even prepubertal endometriosis when neonatal bleeding is taken into
account as a possible cause [41, 42]. In the implantation theory, endometriosis stem
cells originate from stem cells that are present in eutopic endometrium and reach
ectopic sites via many possible routes as discussed above.
Sasson and Taylor [16] and others proposed that the pathogenesis of endome-
triosis could be due to endometriosis stem cells that originate from the bone marrow
of humans [43, 44], data supported by work in mice [45, 46]. These theories are
plausible because a variety of stem/progenitor cells reside in the bone marrow.
In this regard, the presence of mesenchymal stem cells is of particular interest. In
support of this theory, a murine model of endometriosis was used to demonstrate
that bone marrow-derived cells participate in the genesis of epithelial and stromal
cells when endometrium was ectopically transplanted into the peritoneum [45].
42 T. Maruyama
Theories that propose different stem cell origins do not necessarily contradict
one another. It is quite likely that endometrial SP cells include endometrial stem
cells [4751]. Our laboratory showed that endometrial SP cells possess phenotypic
properties that are similar to endothelial progenitor cell (EPC)-like cells [49]. Given
that EPCs originate from bone marrow [52, 53], it is entirely possible that endo-
metrial SP cells have a similar origin. The fact that bone marrow-derived cells are
incorporated into human endometrium at a low level [43, 44] suggests that resident
endometrial stem/progenitor cells such as endometrial SP cells are more likely
responsible for the cyclic renewal and regeneration of endometrium and also
possibly for the establishment of endometriosis than circulating bone marrow-
derived cells [54].
The best current theory for the pathogenesis of endometriosis posits that stem/
progenitor cells in the eutopic endometrium reach ectopic sites through retrograde
menstruation or systemic dissemination. At that point, they give rise to
endometriotic lesions. Integral to this theory is the presence of EmSCs. Below,
the identity and function of EmSCs are discussed.
Endometrial stem/progenitor cells and related cells have been isolated and
characterized by a number of laboratories [18, 17, 55]. Some of the precursors
show plasticity, i.e., the capacity to differentiate into a variety of endometrial
tissue types. For example, endometrial SP cells can differentiate into endothelial,
glandular, smooth muscle, and stromal cells, both in vitro and in vivo [4751].
Endometrial SP cells have been observed in the functional layer of the human
endometrium [49]. Hence, they might contribute to renewal of the endometrium [19].
Intriguingly, when endometrial SP cells are transplanted under the mouse kidney
capsule, they migrate into the kidney parenchyma and initiate the formation of blood
vessels [49]. Endometrial SP cells can be found in the vascular walls of endometrial
small vessels in functional and basal layers, and they have functional properties like
EPCs [49]. Endometrial SP cells might initially trigger neovascularization followed by
propagation and differentiation into various cellular components of the human
endometrium [49].
In addition to endometrial SP cells, endometrial mesenchymal stem cells and
endometrial epithelial progenitor cells have been identified and isolated. This was
achieved through the use of cell surface markers such as CD146, CD140b/
4 Role of Stem Cells in the Pathogenesis of Endometriosis 43
PDGFR-b, EPCAM, and W5C5 [5659]. These cell populations are capable of
self-renewal and multilineage differentiation, at least in in vitro experiments,
except for W5C5-positve cells whose stem cell-like properties are verified in vivo
as well as in vitro [59].
Laboratories isolating endometrial SP cells are not in complete agreement with
regard to the cells properties [4750]. While the endometrial SP cells share some
properties, they appear different in regard to their expression of surface markers,
clonal efficiency, culture requirements, and location within the normal endome-
trium. Thus, it is not clear whether there are multiple types of stem cells in the
human endometrium or whether these differences are the result of subtle variations
in laboratory techniques. In any event, it is an open question whether the endome-
trium contains populations of precursor cells differing in phenotype and function. If
this is indeed the case, it is important to determine their hierarchical relationship.
To better define the nature of endometrial stem cells, our laboratory established a
novel in vivo endometrial stem cell assay [51]. This approach has a number of
advantages, the most important of which is that we could follow multipotential
differentiation through use of cell tracking in combination with in vivo model of
human endometrial regeneration [51, 60]. We found that the efficiency with which
endometrial SP cells reconstituted the endometrium increased when unfractionated
endometrial cells were included as support cells. These data clearly showed the
importance of the microenvironment in supporting primitive undifferentiated cells
[51]. When SP and non-SP cells were labeled with a fluorescent marker by lentiviral
labeling, we found that endometrial SP cells had a greater capacity to differentiate
into vascular, glandular, and stromal structures in vivo compared with non-SP
endometrial cells [51]. These experiments verified that endometrial precursors
possess a range of differentiation potentials. This newly developed in vivo endo-
metrial stem cell assay [51] should prove useful for the identification and analysis
of human endometrial stem/progenitor cells.
cells is similar [64]. The data of the two studies suggest that endometriosis may
originate from the basal layer, which, however, does not exclude a possibility that
endometrial stem cells such as endometrial SP cells present in the functional layer
may also contribute to the cyclic renewal and regeneration of eutopic endometrium
and also the establishment of endometriosis.
Second, attachment, migration, and angiogenesis are essential for the implanta-
tion and survival of endometriosis-initiating cells at ectopic site(s). These cells,
therefore, should have migratory potential and angiogenic capability. Third, to give
rise to endometriotic lesion(s) containing glandular structures, endometriosis-
initiating cells should demonstrate multi-differentiation potentials to produce a
variety of endometrial cell components.
In summary, several groups have shown that endometrial SP cells satisfy most of
the predicted properties of endometriosis-initiating cells. That is, endometrial SP
cells are present in both the functional and basal layers and have migratory,
angiogenic, and stem cell-like properties [49, 50]. These findings strengthen the
stem cell theory of endometriosis and support the retrograde menstruation theory.
The stem cell theory can account for the weakness of the implantation theory. It can
also address the unique characteristics and behavior of endometriosis.
The retrograde menstruation theory has a number of weaknesses. Specifically, it
has been extremely difficult to detect the initial pathological steps, i.e., the attach-
ment of endometrial tissue to the peritoneum and its secondary proliferation and
invasion [6567]. A modified version of the stem cell theory explains this short-
coming. This theory posits that endometriosis arises from EmSCs and/or progenitor
cells in the implanted endometrial fragments. In other words, EmSCs and/or
progenitor cells are both necessary and sufficient for the establishment of endome-
triosis and can be initiated by a single or very few cells. In this scenario, EmSCs
and/or progenitor cells (and not endometrial tissues) implant and give rise to
endometriotic lesions. As such, it would be almost impossible to detect the initial
attachment and proliferation events of these cells. Thus, endometriotic lesions
would only become microscopically detectable after completion of initial events.
Note that non-stem/progenitor cells in the endometrium (the bulk of endometrial
cells) will not give rise to persistent endometriosis even when a large numbers are
present ectopically.
We emphasize that endometrial SP cells, the most likely candidate for endome-
trial stem cells, constitute only ~2 % of the endometrial cell population [49].
Consequently, the chances are low that endometrial stem/progenitor cells will
find an ectopic supportive microenvironment and initiate an endometriotic lesion.
This might explain the apparent discrepancy between the incidence of endometri-
osis and the frequent occurrence of retrograde menstruation.
4 Role of Stem Cells in the Pathogenesis of Endometriosis 45
The stem cell theory of endometriosis is weakened by the fact that the charac-
teristics of endometrial and endometriosis stem cells are not universally accepted.
Without such consensus, the theory necessarily remains an attractive hypothesis.
4.4 Conclusions
The stem cell theory for the pathogenesis of endometriosis seems to account for
many aspects of the pathophysiology of this disease. The theory provides testable
hypotheses and suggests new approaches to the development of novel diagnostic
tests and treatments. The theory, however, largely depends on determining
unequivocally the existence, identity, and function of EmSCs. Such evidence is
growing. However, a consensus has not yet been established. Once EmSC
populations are defined, significant progress in understanding the pathophysiology
of the disease and new clinical approaches can be anticipated.
References
Nagamasa Maeda
Abstract Impaired natural killer (NK) cell activity in women with endometriosis
is thought to promote implantation and the progressive growth of endometrial tissue
in accordance with Sampsons hypothesis. However, the mechanisms responsible
for decreased NK cell activity and the antigens recognized by NK cells in these
women are not clear.
Decreased NK cell activity in the peripheral blood (PB) and peritoneal fluid
(PF) of women with endometriosis was first reported by Oosterlynck et al. and
subsequent investigators have identified the depression of NK cell function in
women with this disorder. Decreased NK cell activity in women with endometriosis
is thought to allow the implantation of endometrial tissue in the manner of a graft,
but the mechanisms underlying the decline of NK cell activity remain uncertain.
We focused on the expression of HLA-G, a ligand of NK cell receptors, and its
changes in eutopic endometrium during the menstrual cycle. HLA-G expression
was only identified in eutopic endometrium during the menstrual phase, but not
during the proliferative or secretory phases. HLA-G-expressing cells were also
detected in peritoneal fluid during the menstrual phase.
Retrograde menstruation may allow HLA-G-expressing endometrial tissue to
enter the peritoneal cavity, where it should be scavenged by the immune surveil-
lance system. Because peritoneal NK cells play an important role in this system,
impairment of their cytotoxicity via HLA-G could allow the survival and implan-
tation of peritoneal endometrial cells.
In this article, we discuss the pathogenesis of endometriosis from the perspective
of intraperitoneal interactions between NK cell receptors and their ligands (anti-
gens) that enter the peritoneal cavity on cells shed from eutopic endometrium via
retrograde menstruation.
NK cells are cytotoxic lymphocytes that constitute a major component of the innate
immune system. Because these cells can attack target cells without requiring
antigen sensitization, they are called natural killer cells [1]. NK cells participate
in host defenses against infection [2], have antitumor activity [3], and are involved
in graft rejection [4]. NK cells can also have an adverse influence on pregnancy [5].
These cells usually express the surface markers CD16 (FcRIII) [6] and CD56
(neural cell adhesion molecule: NCAM) [7] in humans. In addition to killing target
cells, NK cells secrete various cytokines, such as the antiviral cytokine interferon-
(IFN-) [8, 9] and the inflammatory and antitumor cytokine tumor necrosis factor-
(TNF-) [10].
NK cell activity can be assessed by measuring cytotoxicity for NK-sensitive
K562 cells (a chronic myelogenous leukemia cell line) [11, 12]. NK cells do not
require activation in order to kill target cells that lack expression of major histo-
compatibility complex (MHC) class I antigens. Karre et al. [13, 14] have proposed
the missing self hypothesis, which states that NK cells act against target cells that
do not express MHC determinants characteristic of self, while toxicity is
inhibited when cells express these determinants.
This missing self hypothesis has been supported by the identification of killer
cell immunoglobulin-like receptors (KIRs) on NK cells that recognize autologous
MHC class I antigens [15, 16] and inhibit NK cytotoxicity against target cells
bearing these determinants.
Because of their strong cytotoxicity and the potential for autoreactivity, the activity
of NK cells is strictly regulated by several factors. Cytokines play a crucial role in
the regulation of NK cells. Cytokines involved in the activation of these cells
include interleukin (IL)-2 [8], IL-12 [17], IL-15 [18], IL-18 [19], IL-21 [20],
IFN- [8], and granulocyte-macrophage colony-stimulating factor (GM-CSF) [21].
NK cells, as well as macrophages and several other cell types, express the
Fc receptor (FcRIII: CD16/Leu-11 antigen), an activating receptor that binds
the Fc portion of antibodies and allows NK cells to lyse target cells through
antibody-dependent cellular cytotoxicity (ADCC) [22, 23]. Thus, NK cells are
5 Role of NK Cells in Endometriosis 51
In 1991 and 1992, Oosterlynck et al. reported that the NK cell activity against
autologous endometrium in PB and PF was reduced in women with endometriosis
[27, 28]. Impaired NK cell activity in women with this condition is thought to allow
the implantation of endometrial tissue as a graft according to Sampsons
hypothesis [29].
The finding of decreased NK cell activity in women with endometriosis and the
positive correlation of NK cell activity in both the PB and PF with the severity of
this disease has led to consensus about its pathogenesis [3033].
After removal of endometriotic lesions, decreased NK cell activity and the
impaired cytotoxicity of autologous and heterologous lymphocytes against the
endometrium are unchanged, and cytotoxicity is still significantly decreased com-
pared with that in women who do not have endometriosis. These findings suggest a
primary deficiency of NK cell activity in women with endometriosis, which could
explain its frequent relapse after treatment [34].
Survival of endometrial cells in the peritoneal cavity of women with endome-
triosis [35] is mainly due to decreased NK cell activity, but is also related to
resistance of these cells to NK cytotoxicity [3638].
The missing self hypothesis has been supported by the identification of KIRs
on NK cells that recognize self-determinants among MHC class I antigens
andinhibit NK cell cytotoxicity against target cells bearing these determinants. In
women with endometriosis, expression of inhibitory killer immunoglobulin-like
receptors on NK cells from PB and PF is significantly upregulated compared with
the level of expression in women without endometriosis [3941], indicating a
decrease of NK cell activity and cytotoxicity for endometriotic cells.
52 N. Maeda
The KIR genes are polymorphic and highly homologous genes that are located in a
cluster on chromosome 19q13.4 [25]. The KIR proteins are classified by the number
of immunoglobulin (Ig)-like extracellular domain receptors (2 or 3) and by whether
they have a long or short cytoplasmic tail. KIR proteins with a long cytoplasmic tail
transduce inhibitory signals upon ligand binding via an immunoreceptor tyrosine-
based inhibitory motif (ITIM) after binding tyrosine phosphatase SHP1/SHP2,
while KIR proteins with a short cytoplasmic tail that lacks the ITIM associate
with the tyrosine kinase-binding protein ZAP-70/Syk instead transduce activating
signals via an immunoreceptor tyrosine-based activation motif (ITAM) [4244].
Most KIRs are inhibitory, indicating that recognition of MHC antigens by these
receptors suppresses the cytotoxic activity of NK cells, while only a limited number
of KIRs have the ability to activate these cells. The ligands for several KIRs are
subsets of both classical HLA-Ia antigens (HLA-A, HLA-B, HLA-C) and also
nonclassical HLA-Ib antigens (HLA-G) [45, 46].
In women with endometriosis, the decrease of NK cell activity may be related to the
inhibitory KIRs expressed by NK cells.
The percentage of cells expressing KIR2DL1 among NK cells in PF and PB was
reported to be significantly higher in women with endometriosis than in controls,
suggesting that this receptor is probably related to suppression of NK cell activity
in endometriosis [39]. The elevated percentage of KIR2DL1+ NK cells in PB
from women with endometriosis was not reduced by laparoscopic surgery or by
gonadotropin-releasing hormone agonist treatment. Thus, KIR2DL1 overexpression
may be a primary event that represents a risk factor for both the development of
endometriosis and its recurrence after treatment [40].
5.2.2 CD94/NKG2A
Despite its interesting inhibitory function, little has been reported concerning
CD94/NKG2A and endometriosis. Women with stage III and stage IV endometri-
osis were found to have a significantly higher percentage of CD94/NKG2A+
peritoneal NK cells than control women [48], and HLA-E (the CD94/NKG2A
ligand) has been identified in endometriotic tissues [48]. Because target cells
expressing HLA-E show resistance to NK cell-mediated cytotoxicity in a CD94/
NKG2A-dependent manner, the increased expression of CD94/NKG2A by perito-
neal NK cells may mediate the resistance of endometriotic tissues to NK cell
cytotoxicity and thus contribute to the progression of endometriosis [48].
ILT-2 and ILT-4 bind to HLA-G with a three- to fourfold higher affinity than that
for classical MHC class Ia [49], suggesting that ILT/HLA-G recognition may play a
dominant role in regulating the activation of NK cells, T cells, and monocytes.
Although ILT is thus thought to have a role in the pathogenesis of endometriosis,
surprisingly, there has been no report concerning its interaction with this disease.
5.3.2.1 HLA-E
HLA-E is one of a family of molecules known as HLA class Ib and it has a very
specialized role in the recognition of other cells by NK cells. HLA-E is very highly
conserved and presents a small repertoire of peptides of various origins [53]. NK
cells recognize the HLA-E/peptide complex via the heterodimeric inhibitory recep-
tor CD94/NKG2A or the activating receptor CD94/NKG2C. When CD94/NKG2A
is stimulated, it has an inhibitory effect on NK cell cytotoxic activity and prevents
target cell lysis [54].
5 Role of NK Cells in Endometriosis 55
5.3.2.2 HLA-G
HLA-G appears to be mainly recognized by ILT-2 and ILT-4 receptors, which are
expressed by T and B lymphocytes, as well as NK cells and monocytes, and inhibit
the activating signals received by these cells. In addition to ILT, HLA-G can also
react with KIR2DL4 expressed on NK cells and T cells. Although the expression of
ILT2, ILT3, ILT4, and KIR2DL4 is known to be upregulated by HLA-G in antigen-
presenting cells, NK cells, and T cells [55], whether the HLA-G/KIR2DL4 inter-
action leads to activation or inhibition of NK cells remains a complicated and
controversial issue.
Hornung et al. reported that HLA-G was not expressed by eutopic endometrium or
endometriotic tissue [56] and HLA-G protein was not detectable in peritoneal fluid
from endometriosis patients or controls. Moreover, ectopic and normal endometrial
tissues and stromal cells did not express HLA-G during the proliferative phase.
Accordingly, they concluded that immune cell inhibition in endometriosis is medi-
ated by factors other than HLA-G.
In another study, HLA-G expression was identified in the glandular epithelium
of peritoneal endometriotic implants, but not in eutopic endometrium [57]. The
authors concluded that differential expression of HLA-G suggests peritoneal
inflammation or cellular stress may upregulate mechanisms promoting the survival
of ectopic endometrium.
According to our recent findings, KIR2DL4-expressing NK cells can be identi-
fied in both the PB and PF. Interestingly, we found that HLA-G (a ligand of
KIR2DL4) was only expressed by eutopic endometrium during the menstrual
phase and not during the proliferative or secretory phases [47]. In addition, we
detected HLA-G-expressing cells in PF during the menstrual phase [47]. This
suggests that cells bearing HLA-G may enter the peritoneal cavity through retro-
grade menstruation, allowing the antigen to react locally with KIR2DL4.
In 2000, Ibrahim et al. reported that stress, including heat shock and arsenite
treatment, induces an increase in the expression of various HLA-G alternative
56 N. Maeda
5.4 Conclusions
Endometrial cell
HSF-1
Nucleus
Promotor Hsp gene
HSE
HSE HSE
NK cell
Cell lysis
KIR2DL4 (10A/9A)
Fig. 5.1 In the usual menstrual cycle, physiological stresses such as progesterone withdraw,
smooth muscle contraction, spasm of spiral artery, ischemia-reperfusion, oxidative stress, and
transient bacterial infection may occur in the uterus. Increased expression of Hsp70 and HLA-G
in the endometrium during menstruation may result from such stress pathway. Hsp70- and
HLA-G-expressing endometrial cells in the retrograde menstruation may react with immunocom-
petent cells such as NK cells in PF and finally disappear from peritoneal cavity or survive and
develop to endometriosis. HSF heat shock factor, HSE heat shock element, HSP heat shock
protein, KIR killer immunoglobulin-like receptor, ILT immunoglobulin-like transcript
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Chapter 6
Macrophages in Pathophysiology
of Endometriosis
Abbreviations
CD Cluster of differentiation
Cox-2 Cyclooxygenase-2
DCs Dendritic cells
E2 Oestrogen
FGF Fibroblast growth factor
ICAM-l Intercellular adhesion molecule-l
IL Interleukin
IFN- Interferon gamma
ISO-1 ((S,R) 3-(4-hydroxyphenyl)-4,5-dihydro-5-isoxazole acetic methyl
ester
LFA-1 Leukocyte function antigen-l
LPS Lipopolysaccharide
MAPK Mitogen-activated protein kinase
MCP-1 Monocyte chemotactic protein-1
MIF Macrophage migration inhibitory factor
MMPs Matrix metalloproteinases
NF-B Nuclear factor kappa B
NGF Nerve growth factor
NK Natural killer
PGE2 Prostaglandin-E2
PGF2 Prostaglandin-F2
PGs Prostaglandins
PlGF Placental growth factor
RANTES Regulated on activation, normal T cell expressed and secreted
StAR Steroidogenic acute regulatory protein
TGF Tumour growth factor
TIMPs Tissue inhibitors of MMPs
TNF- Tumour necrosis factor-alpha
uNK Uterine natural killer
VEGF Vascular endothelial growth factor
6.1 Introduction
peritoneal fluid [1]. Macrophages are the most abundant nucleated immune cells
found in the peritoneal fluid [2], and their role in endometriosis has been studied for
more than three decades. Haney et al. first reported an increase in the number of
peritoneal macrophages in women with endometriosis [3]. Several studies con-
firmed this observation and further reported an increased activation of these cells in
women with endometriosis [47]. However, activated peritoneal macrophages in
women with endometriosis seem to have a reduced capacity to eliminate misplaced
endometrial cells. Paradoxically, they rather seem to facilitate endometrial cell
survival, invasiveness and growth by secreting growth, angiogenic and tissue
remodelling factors and thereby contribute to the development of endometriosis.
Interestingly, it was reported that even peripheral blood monocytes enhance eutopic
endometrial cell proliferation in women with endometriosis but suppress endome-
trial cell proliferation in healthy women [8]. Puzzling at first, this phenomenon is
being progressively elucidated. It is thus likely that a combination of defects either
in macrophages or in the inherent capability of endometrial cells themselves to
resist immune suppression and apoptosis in the peritoneal environment is involved.
We also believe that activating positive feedback loops and a mutual crosstalk
occur within the pelvic cavity of women with endometriosis (where the disease is
frequently found) between local immune cells, particularly macrophages, and
misplaced or implanted endometriotic cells, which lead to the establishment of a
64 S.F. Ahmad et al.
chronic inflammatory process and a local environment that favours ectopic tissue
growth (Fig. 6.1).
This chapter provides an overview of the current state of knowledge on macro-
phages in endometriosis, the functional impairment of these key immune cells and
their possible role in the pathophysiology of this disease.
Macrophages are mononuclear phagocytic cells derived from blood monocytes [9].
Monocytes originate from haematopoietic stem cells present in bone marrow,
which undergo differentiation. They represent immune effector cells, equipped
with chemokine receptors and pathogen recognition receptors that mediate migra-
tion from blood to tissues during infection. Extravasation of monocytes from blood
to tissue initiates maturation processes leading to mature macrophages or dendritic
cells (DCs) [10]. After migration to peripheral tissue, activated monocytes differ-
entiate to inflammatory DCs and macrophages, which are determined by the
inflammatory milieu, and pathogen-associated pattern recognition receptors present
on the surface of these immune cells. The developmental origin and the function of
tissue macrophage subsets, such as microglia (macrophages in the central nervous
system), dermal macrophages and splenic marginal zone and metallophilic macro-
phages, remain insufficiently understood [11]. Resident macrophages in lymphoid
and non-lymphoid tissues are the phagocytic cells involved in steady-state tissue
homeostasis, and they undergo local activation in response to various inflammatory
and immune stimuli. These macrophages are classified as being elicited, as in the
antigen-non-specific response to a foreign body or a sterile inflammatory agent or as
being classically activated or alternatively activated by an antigen-specific
immune response. It is difficult to distinguish originally resident macrophages
from more recently recruited, elicited or activated macrophages, because cells
adapt to a particular microenvironment [12].
cells that can change from a phenotype to another depending on their microenvi-
ronments [15]. It is a matter of fact that interferon- (IFN-) and lipopolysaccharide
(LPS) generate M1-macrophages, whereas IL-4 and IL-13 activate
M2-macrophages [16]. Furthermore, a pallet of phenotype exists between
the common M1-macrophages and M2-macrophages activation such as decidual
macrophages present in endometrium, which are hybrid M1M2 phenotype
[10, 17, 18]. Scientists finally conclude that the subtle composition of macrophage
environment determines their expression profile and thus their role [10].
Braun et al. have observed a reduction in the number of macrophages in the eutopic
endometrium of women with endometriosis [8]. Their results were surprising
6 Macrophages in Pathophysiology of Endometriosis 67
MMP-9 and CD-36 is suppressed [38, 39]. This significantly inhibits the phagocytic
ability of macrophages and may favour abnormal endometrial tissue growth into the
ectopic host sites.
It is worth mentioning here that an apparent inconsistency seems to emerge
considering the ability of macrophages to phagocytise sperm cells and their inabil-
ity to eliminate ectopic endometrial cells. While it is possible that such a difference
is at least partly due to inherent properties of endometrial cells of women with
endometriosis, the underlying mechanisms remain to be clarified, given their likely
impact on the pathogenesis of the disease and the symptoms it causes.
angiogenesis [55, 56]. MCP-1 has potent direct angiogenic effects on endothelial
cells [57] and may act indirectly via its ability to stimulate macrophage recruitment
and activation and the release of angiogenic factors [52, 58, 59].
RANTES, one of the members of CC chemokine family that mediate monocyte
chemotactic activity, was found to be elevated in peritoneal fluid of women with
endometriosis [60]. RANTES peritoneal fluid levels also correlate with advanced
endometriosis stage, suggesting that it might contribute to the progression of this
disease [60]. Interestingly, our and other studies showed that macrophage-/mono-
cyte-derived pro-inflammatory cytokines such as IL-1 trigger endometriotic cells
to produce this monocyte chemoattractant chemokine [61, 62] and point thereby to
feedforward amplification loops underlying chronic pelvic inflammation in women
with endometriosis.
MIF, originally identified as a protein factor secreted by T cells, inhibits the
migration of macrophages in vitro (hence its name: macrophage migration inhibitory
factor) [63, 64]. MIF is actually expressed by most immune cells such as monocytes,
macrophages or B cells. It has been shown that MIF plays an important role in the
cell-mediated immune response by promoting the Th1 response by the production of
IL-12 by macrophages [65, 66]. MIF is able to inhibit the immunosuppressive effects
of glucocorticoids on the production of pro-inflammatory cytokines such as IL-1 in
activated macrophages [6669]. To illustrate this property, it has been described that
MIF induces the expression of cytoplasmic phospholipase A2 which is an important
component of the pro-inflammatory cascade and usually blocked by the action of
glucocorticoids [70]. Our studies showed that MIF is overproduced by activated
peritoneal macrophages in women with endometriosis [52] and further found abun-
dant levels of this factor in peritoneal fluid [43], peripheral blood [44] and eutopic
endometrial tissue of endometriosis patients [71]. Furthermore, MIF levels varied
according to endometriosis stage and were particularly elevated in women suffering
from endometriosis but also complaining from pelvic pain and/or infertility. This,
together with the increased peritoneal fluid levels of MIF, was corroborated by other
investigators [72, 73]. Our subsequent studies showed that MIF expression is also
elevated in the early stage and highly vascularised endometriotic lesions [43] and
appeared to act at multiple coordinated levels in the PG biosynthesis cascade,
thereby inducing cyclooxygenase-2 (Cox-2) expression in these cells and stimulat-
ing PGE2 [74]. From a cellular mechanism point of view, our work suggests the
involvement of the transcription factor nuclear factor kappa B (NF-B) in MIF gene
activation in ectopic endometrial cells in response to IL-1 [75]. In addition, our
group revealed for the first time the presence of a positive feedback loop by which E2
acts directly on ectopic endometrial cells to up-regulate the expression of MIF,
which, in turn, displays the capability of inducing the expression of aromatase, the
key and rate-limiting enzyme for E2 synthesis [76]. Our studies also revealed that
MIF exerts a potent indirect angiogenic effect by interacting with ectopic endome-
trial cells and inducing the secretion of major angiogenic factors via CD-44 and
CD-74 and mitogen-activated protein kinase (MAPK) signalling pathways [77] and
provide evidence for a possible new mechanism underlying endometriosis develop-
ment and pathophysiology. Angiogenesis or the formation of new blood vessels is
70 S.F. Ahmad et al.
essential for the development and the maintenance of endometriotic lesions. Vascu-
lar endothelial growth factor (VEGF), one of the major angiogenic factors endowed
with the capability of stimulating mitogenesis, migration and differentiation of
endothelial cells, is strongly expressed in endometriotic tissue as well as in perito-
neal macrophages [78, 79]. Peritoneal-activated macrophages are the major source
of VEGF in endometriosis and that this expression is regulated directly by ovarian
steroids [80]. Ovarian steroids regulate the production of this growth factor through
peritoneal macrophages. E2 acts on various macrophage signalling pathways,
influencing in particular those related to sustain the recruitment of inflammatory
cells and the remodelling of inflamed tissues, such as MAPK, phosphatidylinositide-
3-kinase/protein kinase B and NF-B. As a consequence, a deregulated response to
steroids might influence the survival of ectopic endometrial cells and promote the
vascularisation of the lesions [8185]. It is quite established that hypoxia induces the
expression of VEGF [81, 86, 87]. The effects of hypoxia are mainly mediated by
hypoxia-inducible factor-1 (HIF-1) protein complex, which is composed of two
subunits, HIF-l, the inducible unit, and HIF-1, the constitutive unit [88]. In
endometriotic tissue, abnormally high levels of complex HIF-l were found [89],
which makes clear that hypoxia is involved in VEGF production in endometriotic
lesions and presumably by peritoneal macrophages.
It is of note that peritoneal macrophages strongly express Cox-2 [90], one of the
rate-limiting enzyme for PGs secretion. As described in several reports [26, 84, 91,
92], PGE2 and PGF2 themselves induce the over-expression of Cox-2 in macro-
phages and endometriotic stromal cells, leading to an elevated concentration of
their own levels in the peritoneal fluid. On one hand, high levels of PGs act on
macrophages to suppress their phagocytic ability by down-regulating MMP-9 and
CD-36 [37, 39]. On the other hand, PGs stimulate the steroidogenic capacity of
endometriotic stromal cells by up-regulating steroidogenic acute regulatory protein
(StAR) and aromatase [93], which induces aberrant biosynthesis of E2. E2 further
stimulates the production of mitogens such as fibroblast growth factor-9 (FGF-9),
which induces endometriotic cell proliferation [94, 95]. PGE2 can also induce
FGF-9 expression by PGE2 receptor 3-dependent transcriptional up-regulation
[96, 97]. Other main functions of PGs include the induction of the expression of
angiogenic factors such as VEGF and FGF-2 to induce angiogenesis [98, 99]. These
effects may play an important role in the survival and proliferation of endometriotic
cells. Furthermore, elevated PGs concentrations in endometriosis women is
suspected to be involved in pelvic pain and infertility, though more studies will
be required to further elucidate the underlying mechanisms [90, 100, 101].
Obviously, macrophages have a rather heterogeneous array of characteristics
and dramatically modify their environment not only via the production of cytokines
and other pro-inflammatory factors but also via reactive oxygen species (ROS)
[102104]. Production of ROS is known to increase after activation of immune
cells, especially macrophages [105] and their production was reported to be
increased in serum and peritoneal fluid of patients with endometriosis. In addition,
markers of oxidative stress have been found elevated [102104]. ROS role, as a
second messenger of cellular proliferation, has been described. McCubrey
6 Macrophages in Pathophysiology of Endometriosis 71
et al. found that normal cell proliferation correlated with production of endogenous
ROS through the activation of growth-related signalling pathways [106]. Endome-
triosis is considered a benign disease but shares some features with cancer, such as
propensity to invasion, unrestrained growth, neo-angiogenesis, and distant spread-
ing [19, 107]. The known correlation between ROS and proliferation of cancer
cells, along with the increased production of ROS in response to chronic inflam-
mation in endometriosis, thus suggests a possible role for ROS in the regulation of
endometriotic cell proliferation.
The available literature argues in favour of a significant role for macrophages in the
growth and development of endometriotic lesions, the generation of pain through
interaction with nerve fibres and infertility via the impediment of spermatozoids
and/or oocyte functions and endometrial receptivity. It is obvious that little evi-
dence is available as to the existence of a direct cause and effect relationship
between endometriosis-associated macrophage dysfunctions and pain or infertility.
However, chronic pelvic inflammation in women with endometriosis and many
inflammatory and embryotoxic factors involved, abnormally expressed and known
for being secreted by activated endometrial and peritoneal macrophages let, in an
indirect way, believe in such a role.
It is now well known that macrophages are located into decidua (endometrium of
the pregnant uterus) during the implantation window and implicated in the physi-
ological processes of implantation, establishment and maintenance of pregnancy
and labour control. Indeed, decidual macrophages (2025 %) and uNK cells are
predominant decidual leukocytes [115, 116]. While other uterine leukocytes are
diminished during pregnancy, macrophages proportion remains unchanged. During
implantation, macrophages cooperate with developing embryo to insure trophoblast
endovascular invasion and anchorage. At this site, only M2-macrophages are found
infiltrated into endometrial basalis where they will secrete MMP-7 and MMP-9
degrading extracellular matrix to facilitate trophoblast invasion into myometrium
[117]. Moreover, M2-macrophages are able to produce VEGF and placental growth
factor (PlGF) implicated in the profound remodelling of uterine vasculature during
embryonic growth. Furthermore, those phagocytes participate in maternal cell
apoptosis and trophoblast renewal. In fact, maternal decidua cell apoptosis insures
trophoblast invasion to remodelling and development of embryo. It is important to
notice that phagocytosis of apoptotic bodies are vital to avoid secondary necrosis
6 Macrophages in Pathophysiology of Endometriosis 73
and so a harmful inflammatory response generating tissue damage [118, 119]. Even
more, macrophages are fundamental actors of maternal immune tolerance in preg-
nancy. Indeed, these immune cells are not only able to secrete molecules such as
IL-10, known to inhibit T cell activation, but are also to diminish expression of
co-stimulatory molecules (CD-80 and CD-86) and indoleamine 2,3-dioxygenase
[116]. They create a microenvironment capable of containing immune response to
hemi-allogeneic fetal cells even during infection [120]. Interestingly, macrophages
secrete IL-15, an uNK cell chemoattractant, and down-regulate uNK cell cytotoxic
capacity [121]. uNK cells are crucial for implantation knowing that they are
responsible for trophoblast chemoattraction and invasion by secreting IL-8 and
IFN-inducible protein-10 that binds to trophoblasts membrane receptors [122].
Intriguingly, in endometriosis, the number of M2-macrophages is significantly
increased in decidua and peritoneal fluid. As explained in the previous section,
macrophages are differentially activated in endometriosis overproducing a myriad
of pro-inflammatory factors and key processes are crucial for implantation. Decid-
ual macrophages in endometriosis have been shown to secrete elevated concentra-
tions of angiogenic factors (VEGF, MCP-1, IL-8) and to mediate the development
of an anarchic vasculature similar to unstructured tumour vasculature [123,
124]. Such an abnormal angiogenic process might disfavours the functional
crosstalk between maternal decidua and trophoblasts, which is essential for embryo
survival [125]. Acute and controlled inflammation is necessary for pregnancy, but
any chronic inflammation leads to spontaneous abortion [126]. As described pre-
viously, women with endometriosis are characterised by an exaggerated inflamma-
tion that may contribute to infertility in endometriosis [127]. First, disruption of the
phagocytic function in endometriosis may promote accumulation of apoptotic
bodies and secondary necrosis responsible for inflammation. Second, the cocktail
of inflammatory molecules secreted in endometrium generates an acute inflamma-
tion, which is deleterious for trophoblastic implantation. In fact, some relate
miscarriage to TNF- increase and normal pregnancy with high concentrations of
IL-10 [128]. Chronic inflammation may inhibit trophoblast invasion and immune
tolerance [129]. Macrophage phagocytic function is also an issue since sperm
phagocytosis has been described in endometriosis patient. Moreover, an activation
of specific sperm engulfment surely prevents or disturbs oocyte fertilisation [32]. It
seems that endometrial cells express or secrete molecules able to impair phagocy-
tosis in macrophages, but further investigations could provide interesting insights
on this phenomenon. In the meantime, endometriosis is also characterised by an
oxidant environment inauspicious for pregnancy [130]. Both endometriotic cells
and macrophages are responsible for ROS high concentration in peritoneal fluid of
women with endometriosis. More precisely, endometriotic lesions activate induc-
ible nitrogen oxide synthase (iNOS) in macrophages leading to an augmentation of
NO production [131]. Moreover, the antioxidant machinery (secreting ascorbic
acid, GPx, thiol) is down-regulated creating an imbalance in the redox status of
peritoneal environment [132134]. Interestingly, ROS are known to be related to
age-related fertility decline, in vitro fertilisation failure and cigarette smoke
74 S.F. Ahmad et al.
subfertility [135137]. In endometriosis, such redox status may affect sperm via-
bility in peritoneal microenvironment, oocyte and embryo quality [130].
Since macrophages are crucial cells in implantation and pregnancy, it is not
surprising that their dysfunctions may be a significant possible cause of infertility in
endometriosis.
In recent years, a possible link between endometriosis and certain types of cancer,
such as ovarian cancer, has been suggested. It is well established that endometriosis
shares a number of features with cancer such as abnormal cell proliferation and
invasion, the development of new blood vessels [138, 139], the decrease in the
number of cells undergoing apoptosis [140] and its stem cell-like activity
[141]. Macrophages are important inflammatory mediators and have been impli-
cated in endometriosis through their role in chronic inflammation. As discussed
previously in this chapter, macrophages produce a wide range of cytokines which
can also induce the progression of tumorigenesis [78]. IL-1 is a potent mediator of
inflammation produced by macrophages and it promotes tumorigenesis by stimu-
lating the production of other cytokines and growth factors. Among these, VEGF
has been detected in endometriosis-associated ovarian carcinoma [142]. In addi-
tion, it has been proposed that VEGF acts as a growth factor for tumours regardless
of its role in angiogenesis as there was no correlation observed between VEGF
expression and micro-vessel density in ovarian tumours [139].
Taken together, it seems that macrophages might play a role in the development
of cancerous transformation at the site of endometriosis by secreting important
mediators which are responsible for tumour progression and development. How-
ever, further studies are required to ascertain any possible link between endome-
triosis and cancer.
primates. This section of the chapter will summarise the study of macrophages in
the animal models for endometriosis.
6.5.1 Rodents
Mice and rats are the two established experimental animal models among
the rodents. Since rodents do not shed their endometrial tissue and therefore
do not develop endometriosis spontaneously, endometriosis can be induced by
transplanting endometrial tissue to ectopic sites. These models are classified into
two types, homologous and heterologous models. Homologous models have been
employed utilising the surgical transplantation of endometrium of the same or
syngeneic animals in immunocompetent animals, whereas in heterologous models,
human endometrial fragments are transferred either intra-peritoneally or subcuta-
neously to immunodeficient mice.
Nude and Knockout Mice. As mentioned, animal models represent a useful tool
to study in vivo early steps of this disease. The latter approach relies on the transfer
of fragments of endometrial tissue harvested from syngeneic donor mice and
recapitulates important aspects of the disease [143]. The first experimentally
induced endometriosis in mice was reported in 1984 [144], where normal and
ectopic human endometrial tissues were successfully transplanted into the perito-
neal cavity of athymic nude mice [144]. This study demonstrated that endometrial
tissue keeps intact structure and shows the presence of glands and stroma with an
infiltration of macrophages. Since then, several groups have used fluorescent
markers such as green fluorescent protein [16] or bioluminescent markers such as
luciferase expression system to generate endometriosis mouse models [145]. Recent
studies on Tie-2 knockout mice demonstrated that alternatively activated macro-
phages can infiltrate endometriotic lesions and promote angiogenesis
[146, 147]. These data indicate that the recruited macrophages have more than
one effect. Also, it has been shown that knockdown of annexin A2 inhibited the
phagocytic function of macrophages, whereas treatment with annexin A2 recom-
binant protein enhanced phagocytosis [148]. In addition, we have successfully used
the athymic nude mice model to study the role of MIF in the development of
endometriosis [149]. As described previously in this chapter, MIF has been a
regulator of immune system that promotes the pro-inflammatory functions of
immune cells, and its role in angiogenesis, tumorigenesis and autoimmune diseases
is well established [74, 150154]. We have reported previously that expression of
MIF is increased in eutopic endometrial tissue of women with endometriosis, which
is related to the stage of endometriosis [71]. Furthermore, our research in agreement
with others has shown a significant elevation in circulating and local peritoneal
levels of MIF [43, 44]. Taking the advantage of athymic nude mice model of
experimentally induced endometriosis, we have developed a treatment model of
endometriosis. In this study, we have used the in vivo model of experimentally
76 S.F. Ahmad et al.
induced endometriosis and challenge MIF in order to discover a possible target for
the treatment of endometriosis. We used (S,R) 3-(4-hydroxyphenyl)-4,5-dihydro-
5-isoxazole acetic methyl ester (ISO-1), a specific antagonist of MIF [155] where
human endometrial tissue was allowed to implant and grow prior to any treatment.
Thus our group is the first to report that macrophage migration inhibitory factor can
be a suitable target for the treatment of endometriosis as there is no specific targeted
treatment available at present [149].
Rat. Among the rodents, rat is another choice as an experimental model for the
endometriosis for the researchers. Matsubavashi et al. reported the first study where
rats with auto-transplanted endometrium showed the same immunologic changes as
humans with endometriosis [156]. In this study the effect of ectopic endometrial
lesions on the changes of leukocyte subpopulation in the rat model of endometriosis
was reported. This was supported by another independent research where it was
reported that the stromal tissue of uterus-attached peritoneum showed proliferation
and infiltration of macrophages in rat endometriosis models [157]. Furthermore, it
was discovered that an increase in the number of activated macrophages in the
endometriotic lesions has a positive correlation with VEGF [158]. Recently, lipo-
somal bisphosphonate [159] and a selective Cox-2 inhibitor [158] have been used as
therapeutic drugs targeting macrophages in a rat experimental endometriosis
model. These findings have suggested that macrophage depletion effectively
inhibits the initiation and growth of endometriotic implants in a rat endometriosis
model, and further studies are required to confirm these findings in order to use this
approach as a treatment for endometriosis.
In the recent past, researchers have started using rhesus macaque (aka rhesus
monkey) as an animal model for endometriosis since spontaneous development of
the disease requires menstrual shedding. Endometriosis occurs naturally only in
some non-human primate species, making development of lesions more compara-
ble to the establishment of disease in humans. Compared with rodents, the
non-human primate model of endometriosis is advantageous due to a close reca-
pitulation of human disease and physiology [160]. In a recent study, it has been
shown that the activation status of macrophages in endometriosis in the rhesus
monkey is more oriented towards the M2 phenotype, in exactly the same way as
humans [161].
Concisely, non-human primates have been extensively used for the investigation
of endometriosis, but the very high cost of animal handling limits their use. For this
reason, the establishment of rodent models for endometriosis via the intra-
peritoneal transplantation of pieces of endometrial tissue has been greatly exploited
in the recent years.
6 Macrophages in Pathophysiology of Endometriosis 77
Acknowledgement This study is supported by CIHR grants MOP 93716, 120769 and 123259 to
Pr. Ali Akoum, Chercheur National, FRQ-S.
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Chapter 7
Inflammation and Cytokines
in Endometriosis
7.1 Introduction
Endometriosis was first acknowledged more than about 100 years ago, and the usual
definitions of this disease are based on histology and related to glands, stroma,
hemosiderin, and fibromuscular metaplasia [1]. Endometriosis, which occurs in
10 % of reproductive age women, is characterized by the growth of endometrial-
like tissue outside the uterus. Dysmenorrhea and infertility, which are common
symptoms of endometriosis, compromise the quality of life. This disease is thought
to be estrogen dependent. However, the pathogenesis of endometriosis is poorly
T. Iwabe (*)
Department of Obstetrics and Gynecology, Faculty of Medicine,
Sanin Rosai Hospital, Yonago, Japan
e-mail: [email protected]
T. Harada
Department of Obstetrics and Gynecology, Faculty of Medicine,
Tottori University, Yonago, Japan
Fig. 7.1 Laparoscopic findings in pelvic cavity during menstrual period. (a) Retrograde menstru-
ation from fimbria. (b) Cul-de-sac
Peritoneal fluid (PF) containing immune-related cells is often seen in the vesico-
uterine cavity or the pouch of Douglas during gynecologic surgery. PF bathes the
pelvic cavity, uterus, fallopian tubes, and ovaries and may be a major player
controlling the peritoneal microenvironment that influences the development and
progression of endometriosis and endometriosis-associated infertility.
The peritoneal cavity is normally empty except for a thin film of fluid that keeps
surfaces moist. Peritoneal fluid arises primarily from two sources: plasma transu-
date and ovarian exudate. Other sources of peritoneal fluid are tubal fluid, retro-
grade menstruation, and immune cell secretions. Peritoneal fluid depends on
follicular activity, corpus luteum vascularity, and hormonal production. The vol-
ume of PF within the peritoneal cavity varies during the menstrual cycle, reaching a
peak of 20 mL at the time of ovulation [11].
90 T. Iwabe and T. Harada
Changes in fluid volume and the presence of various cells, hormones, and other
compounds during normal menstrual cycles and in pathologic conditions have been
described. Syrop and Halme analyzed PF volume in 426 patients and found that
women with endometriosis had a greater PF volume than fertile controls, patients
with adhesive disease, or those with unexplained infertility [12]. The PF volume in
women with unexplained infertility was also higher than in controls. Therefore,
increased PF volume may be commonly associated not only with endometriosis but
also with long-lasting, unexplained infertility.
PF contains various free-floating cells, including macrophages, mesothelial
cells, lymphocytes, eosinophils, and mast cells. Normally, PF contains leukocytes
in concentrations of 0.52.0 106 mL1, of which approximately 85 % are mac-
rophages. Halme et al. postulated that peritoneal macrophage activation might be a
central contributor to the pathogenesis of endometriosis [13]. Activated macro-
phages in the peritoneal cavity of women with endometriosis are potent producers
of cytokines. Thus, PF contains a rich cocktail of cytokines. The cytokines are
multifunctional proteins whose biological properties suggest a key role in hemato-
poiesis, immunity, infectious disease, tumorigenesis, homeostasis, tissue repair,
and cellular development and growth.
7.3 Cytokines
Cytokines, a large family of more than 100 low molecular weight proteins that
function as growth and differentiation factors and immune cell modulators, also
play a major role in the regulation of immune and inflammatory responses. Immune
cell activation results in a burst and cascade of inflammatory cytokines. These
cytokines have pleiotropic and redundant activities culminating in the recruitment
of numerous cell types to the site of inflammation.
The development of enzyme-linked immunosorbent assay has made it possible
to measure a number of cytokines in the PF of women with endometriosis. These
include interleukin-1 (IL-1) [14], IL-4 [15], IL-5 [16], IL-6 [1721], IL-8 [2224],
IL-10 [20, 25, 26], IL-12 [27, 28], IL-13 [29], IL-17 [30], IL-23 [31], IL-33 [32],
interferon (INF) [19], tumor necrosis factor (TNF) [14, 21], RANTES [33],
monocyte chemotactic protein-1 (MCP-1) [3436], macrophage colony-stimulating
factor (MCSF) [37], transforming growth factor (TGF) [38], and vascular
endothelial growth factor (VEGF) [39, 40]. A number of studies report that the
level of many cytokines is increased in the PF of women with endometriosis.
Cytokines may regulate the actions of leukocytes in the PF or could act directly
on the ectopic endometrium, where they may play various roles in the pathogenesis
and pathophysiology of endometriosis.
7 Inflammation and Cytokines in Endometriosis 91
7.3.2.1 Macrophages
Macrophages are main regulators of the innate response to injured, infected, and
neoplastic tissues. The peritoneal macrophages (PMs) are the major resident cells in
the peritoneal cavity. They kill cells, such as retrograde endometrial tissues, and
their presence is commonly associated with an inflammatory process. Most studies
revealed increased cell numbers and activity of PMs in cases of endometriosis,
although some studies did not [43, 44]. The increased number of PMs in women
with endometriosis may indicate that the presence of endometrial tissue in the
peritoneal cavity represents a foreign entity and needs to be removed. Activated
PMs might synthesize and secrete different cytokines into the PF including various
cytokines and growth factors.
7.3.2.2 T-Lymphocytes
7.3.2.3 Others
Recent studies suggest that endometriotic implants also produce cytokines [45, 46].
We demonstrated that endometriotic cells constitutively express IL-6 mRNA and
produce IL-6 protein and that adding TNF stimulated IL-6 gene and protein
expression in a dose-dependent manner [47]. When we compared IL-6 production
by macrophages and endometriotic stromal cells in patients with endometriosis,
similar levels of IL-6 were found to be produced in stromal cells derived from an
endometrioma and by macrophages under basal- and TNF-stimulated conditions.
Numerous leukocytes are harbored in both stromal and intraepithelial parts of
normal eutopic endometrium. In women with endometriosis, the member of lym-
phocytes is increased both in eutopic and ectopic endometria. We postulated that
immune cells, such as leukocytes or lymphocytes, and endometriotic tissue
interacted via the paracrine mechanism on the source of the cytokines. Therefore,
they may contribute to cytokine production in PF and be involved in cellular growth
and inflammatory reaction. The findings suggest that endometriotic tissue may be
another important source of this cytokine.
compared with patients without endometriosis [46]. This is an important aspect for
recent investigation because it suggests that endometrial cells of women who
develop endometriosis may function differently from those who do not.
In order to implant and grow, endometrial cells must establish cellcell or cell
extracellular matrix (ECM) interactions with the peritoneal lining. In these circum-
stances, cell adhesion molecules are of great importance [51]. A recent report
clearly showed that endometrial stromal cells are the critical cells in endometrial
attachment to the mesothelial surface of the peritoneum and that endometrial
epithelial cells fail to attach to the mesothelium [48]. Most of these interactions
between endometrial cells and ECM are mediated by the integrin family of cell
surface receptors, which are capable of transducing intracellular signals. It has also
been suggested that cellularadhesion itself stimulates chemokine expression [52].
Garcia-Velasco and Arici showed that increasing the dose of IL-8 stimulates
endometrial stromal cells ability to adhere to an ECM protein, fibronectin [53].
They also showed that the adhesion of endometrial stromal cells to different ECM
proteins induces variable levels of IL-8 gene expression and protein secretion and
that this event is integrin-mediated [54]. IL-8 may be relevant for the attachment of
endometrial implants in the pathogenesis of endometriosis.
According to Sampsons theory of retrograde menstruation, deficient cellular
immunity, in particular impaired natural killer (NK) cell function, is one of the
etiological factors that could contribute to the survival and implantation of refluxed
endometrial cells. Several investigators showed a decrease in NK cell activity in the
PF of women with endometriosis compared with women without endometriosis
[8, 55, 56]. This observation suggests that the clearing mechanism of retrograde
menstruated endometrial cells may be impaired in women with endometriosis
because of a defect in the local immune defense system. Oosterlynck et al. found
increased TGF activity in the PF of women with endometriosis [37]. Transforming
growth factor may be a cytokine that inhibits NK activity in the PF of women with
endometriosis.
Intercellular adhesion molecule (ICAM)-1-mediated cellcell adhesion is essen-
tial for various immunological functions, including NK cell-mediated cytotoxicity
against endometrium. Recently, Somigliana et al. reported that soluble intercellular
adhesion molecules (sICAM)-1 were constitutively shed from the surface of endo-
metrial stromal cells obtained from patients with endometriosis into the culture
medium [57]. The enhanced release of sICAM may allow the endometrial stromal
cells of patients with endometriosis to escape immunosurveillance and, therefore, to
implant in ectopic sites. More interestingly, sICAM-1 production from the macro-
phages of patients with endometriosis was upregulated by INF and IL-6 [58].
Interleukin-12 acts on T and NK cells, inducing cytokine production (primarily
INF), enhancing NK cell cytotoxic activity, and favoring the generation of
T-helper 1 response [59, 60]. Concentrations of IL-12 in the PF are low regardless
of the presence or absence of endometriosis, but they are detectable [26]. The
administration of IL-12 was recently shown to significantly prevent ectopic endo-
metrial implantation in a murine model of endometriosis [61]. A direct growth
inhibitory effect on endometrial cells seems unlikely since endometrial cells do not
94 T. Iwabe and T. Harada
express receptors for IL-12. A potential explanation for these results is that IL-12
may enhance the growth and augment the cytolytic activity of both NK and T cells.
These data support the idea that manipulation of cytokine activity in PF is a novel
management approach to controlling the establishment of endometriosis.
7.3.3.2 Angiogenesis
Angiogenesis seldom occurs in adult organs with normal tissues under physiologic
conditions. The endometrium represents an exception: the tightly regulated fluctu-
ation of ovarian steroids, estrogen and progesterone concentrations, cyclically
triggers the remodeling of the organ vasculature, with angiogenesis and
lymphangiogenesis. Angiogenesis, which is the process of generating new capillary
blood vessels, occurs in a variety of normal and pathologic processes. It consists of
the following steps: dissolution of the basement membrane by the protease derived
from vascular endothelial cells, migration and proliferation of the endothelial cells,
and formation of the capillary tube [62]. Each step is regulated by various angio-
genic factors. Neovascularization is likely to be required for the implant to grow
beyond 23 mm during tumor growth [63]. An angiogenic mechanism could be
involved in the pathogenesis of endometriosis. We can postulate that further
outgrowth of these ectopic endometrial implants will depend on new capillary
growth according to several studies that indicate that tumors are angiogenesis
dependent [64].
Vascular endothelial growth factor (VEGF) is a heparin-binding growth factor of
3046 KDa, which is active as a disulfide-linked homodimer and is a potent
mitogen, morphogen, and chemoattractant for endothelial cells. The angiogenic
activity of PF, as well as levels of VEGF in PF, is elevated in women with
endometriosis [38, 65]. McLaren et al. demonstrated that PF macrophages are the
principal source of the angiogenic growth factor, VEGF, and that the anti-VEGF
antibody abolished the enhanced endothelial cell proliferation induced by a condi-
tioned medium from macrophages isolated from the peritoneal cavity of women
with endometriosis [39]. McLarens study suggests that activated macrophages are
a major source of VEGF in endometriosis and that estradiol and progesterone
directly regulate this expression. Since endometriosis is characterized by pro-
nounced vascularization within and surrounding the ectopic tissue, elevated levels
of the potent angiogenic growth factor, VEGF, in the PF and the presence of VEGF-
positive macrophages within the ectopic tissue are clinically important in this
disease. VEGF-induced angiogenesis may therefore be a critical aspect of the
pathophysiology of endometriosis.
IL-8, which is a chemoattractant for neutrophils and an angiogenic agent, induces
the proliferation of human melanoma and glioma cells [66, 67]. Arici et al. reported
that IL-8 is produced in the human endometrium in vivo, mainly in glandular cells,
and that IL-8 induces proliferation of endometrial stromal cell as a potential auto-
crine growth factor [68, 69]. We demonstrated that IL-8 exerts its growth-promoting
actions in endometriotic as well as in normal endometrial cells [24, 70].
7 Inflammation and Cytokines in Endometriosis 95
Surrey and Halme demonstrated a direct stimulatory effect of the cell-free fraction
of PF samples derived from patients with endometriosis on the proliferation of
normal uterine endometrial cells in a short-term culture, indicating that factors in
the PF are involved in the progression of endometriosis [79]. Several cytokines,
such as IL-8 and TNF, have growth-promoting effects on endometrial and
endometriotic cells [24, 69, 70]. These findings suggest that elevated PF levels of
cytokines promote the progression and spread of endometriotic implants in the
peritoneal cavity.
We revealed that PF levels of IL-8 significantly enhanced the proliferation of
stromal cells derived from ovarian endometriomas [24]. Expression of IL-8 recep-
tor type A (CXCR3A) mRNA was detected in endometriotic stromal cells. These
results suggest that IL-8 may promote the progression of endometriosis [70]. We
tested the hypothesis that TNF elevated in PF of patients with endometriosis may
contribute to the progression of endometriosis by inducing the production of IL-8.
Gene and protein expression of IL-8 in the stromal cells of endometriotic tissues are
upregulated by TNF, and TNF also stimulated the proliferation of the
endometriotic stromal cells. This stimulatory effect of TNF was abolished by
adding either anti-TNF antibody or anti-IL-8 antibody. Therefore, the action of
96 T. Iwabe and T. Harada
TNF on stromal cells may occur by mediating the proliferative effects of IL-8. The
expression of type I and type II receptors for TNF was observed in endometriotic
stromal cells. This evidence suggests that TNF action mediated by IL-8 may not
only be an initiating factor that facilitates adhesion of endometrial cells to the
peritoneum, but may also contribute to the development and progression of
endometriosis.
We found that the extent of superficial red endometriotic lesions was related to
increased levels of IL-6, IL-8, and TNF in the PF [21]. Red lesions, such as red
flame-like lesions, gland-like lesions, and red vesicles, were classified as active
lesions of endometriosis because angiogenesis is more pronounced in red lesions
than in black or white lesions and because early red lesions invade the ECM. Thus,
cytokines may play a role in the early stage of endometriosis.
Hepatocyte growth factor (HGF) was originally characterized as a potent mito-
gen for adult hepatocytes. HGF is known as a mesenchymal (stromal)-derived
pleiotropic growth factor that elicits mitogenic and morphogenic activities on
various types of epithelial cells, usually as a paracrine factor [80, 81]. In normal
uterine endometrium, stromal-derived HGF promotes proliferation, migration, and
lumen formation of endometrial epithelial cells [82]. Overexpression of Met, the
receptor for HGF, was observed in several malignant tumors, such as uterine
endometrium and ovary [83]. We also showed that the peritoneum and
endometriotic stromal cells may be major sources of HGF in peritoneal fluid.
Endometrial and endometriotic stromal cells expressed the Met receptor, which
was activated by endogenous and exogenous HGF [84]. HGF enhanced stromal cell
proliferation and invasion. We also demonstrated that the HGF-stimulated stromal
cell invasion was due in part to the induction of urokinase-type plasminogen
activator, a member of the extracellular proteolysis system. HGF increased in PF
and produced by endometrial stromal cells may induce critical changes in mor-
phology of mesothelial cells and then enhance the endometrial cell attachment and
invasion.
7.3.3.4 Infertility
It has also been suggested that IL-6 has important functions in reproductive
physiology, including the regulation of ovarian steroid production, folliculogenesis,
and early events related to implantation [85]. We demonstrated that the addition of
human recombinant IL-6 to culture medium suppressed the rate of blastocyst
formation of mouse embryos, suggesting that increased IL-6 in the PF of endome-
triosis patients may contribute to infertility by adversely affecting embryonic
development [86]. Recently, Banerjee J et al. showed that IL-6 caused the deteri-
oration in morphology of the microtubule and chromosomal alignment in
metaphase-II mouse oocytes [87]. IL-6, generated in the process of oxidative stress,
directly affects the quality of the oocyte and may contribute to infertility.
We used a steroidogenic human granulosa-like tumor cell line, KGN cells, as a
model for granulosa cells collected during the follicular phase [88]. We demon-
strate that IL-6 may reduce aromatase activity and E2 production via the MAPK
signal pathway in human granulosa cells [89]. The results may support the notion
that IL-6 is related to impaired estrogen biosynthesis in patients with endometriosis.
Half of the cause of infertility is the male factor. The key predictors of fertili-
zation capability are sperm count and motility. We showed that IL-6 and sIL-6R
significantly reduced the percentage of motile and rapidly moving sperm [90]. The
inhibition of sperm motility by IL-6 may be involved in the infertility of at least
some patients with endometriosis who have highly elevated levels of IL-6 in PF. PF
diffusing into the tubal and endometrial environment may affect the sperm and their
interaction with the oocyte and embryo development. Many authors have demon-
strated that the PF of patients with endometriosis has detrimental effects on several
steps of the reproductive process.
These findings suggest that endometriotic implants, which can produce various
cytokines, may contribute to reduced fecundity in patients with endometriosis. The
role of PF and cytokines in the pathophysiology of endometriosis-associated infer-
tility is summarized in Fig. 7.2. However, data on cytokines and their role in
infertility are still incomplete, and future investigation that can reveal the critical
roles of cytokines is still needed.
98 T. Iwabe and T. Harada
Many studies have demonstrated that MAPK is involved directly in regulating the
pathogenesis of endometriosis [9193]. MAPK pathways seem to play a pivotal role
as intracellular and extracellular signal transducers in endometriotic cells. In the
MAPK pathway, the activation of p38, c-jun N-terminal kinase (JNK), and ERK1/2
is important for inflammatory cytokine secretion in endometriotic stromal cells. The
most extensively studied mitogen-activated protein kinase (MAPK) pathway is the
extracellular signal-regulated kinase (ERK) pathway in which the MAPKKK is Raf,
the MAPKK is MEK, and the MAPK is ERK. The activation of the MAPK pathway
induced by TNF through Ras, Raf, MEK, and ERK also affected the activation
of AP-1 (Fig. 7.3). We showed that TNF induced the activation of the signal
molecule ERK1/2 of the MAPK cascade in endometriotic cells [94].
Recent studies have shown that p38 mitogen-activated protein kinase (p38
MAPK), an intracellular signal-transducing molecule, plays an important role in
the regulation of a variety of inflammatory responses, including expression of
proinflammatory cytokines, leukocyte adhesion, and chemotaxis. A number of
studies indicated that the p38 MAPK pathway might play an important role in the
development and progression of endometriosis [94]. Increased p38 MAPK activa-
tion in eutopic and ectopic endometrium indicated that p38 MAPK might be one of
the main factors regulating the inflammatory process in endometriosis [9597].
Yoshino et al. revealed that FR 167653, a p38 mitogen-activated protein kinase
inhibitor, inhibits the development of endometriosis, possibly by suppressing peri-
toneal inflammatory status [98]. Zhou et al. also demonstrated that SB203580,
a p38 mitogen-activated protein kinase inhibitor, may suppress the development
7 Inflammation and Cytokines in Endometriosis 99
7.4 Conclusion
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Chapter 8
Epigenetics in Endometriosis
Epigenetics is one of the most promising and expanding fields in the current
biomedical research. The word epigenetics refers to the study of mitotically
and/or meiotically heritable changes in gene expression that occur without changes
in the DNA sequence [1]. The disruption of such changes (epigenetic aberration or
disorder) underlies a wide variety of pathologies including cancer [2, 3]. Epigenetic
regulation includes DNA methylation and histone modifications [4, 5] and is
responsible for a number of gene transcriptions associated with chromatin modifi-
cations that distinguish the various cell types and the states of diseases. Cancer and
many other diseases show aberrant epigenetic regulation [6]. In terms of DNA
methylation, cancer cells show genome-wide (GW) hypomethylation and
site-specific hypermethylation of promoter CpG islands [2]. This may lead to
transcriptional silencing and aberrant transcription from incorrect transcription
start sites [4]. In addition, a recent study comparing colorectal cancer tissue with
its normal counterpart suggests changes at the CpG island shores [7]. In normal
cells, CpG islands and CpG island shores are under the control of physiological
methylation, allowing normal gene transcription.
There is accumulating evidence supporting the concept that endometriosis is an
epigenetic disease [8]. The concept of aberrant DNA methylation in endometriosis
is expanding [9]. Here we describe how the field of epigenetics is reshaping the
current thinking about endometriosis. Firstly, we present our study shedding light
on aberrant aromatase expression in endometriosis from the viewpoint of epigenetic
disorder and then summarize recent advances in endometriosis research using the
epigenetic approach. We subsequently describe the advanced technologies of GW
methylation analysis and GW association study (GWAS) in endometriosis research.
Finally, we refer to environmental factors as a potential background of epigenetic
disorder in endometriosis.
Fig. 8.2 Promoter usage of aromatase mRNA expression. Left: 5-aza-dC-treated endometrial
cells. Right: endometriotic cells
We searched for the unmethylated CpG locus within the aromatase gene in
endometriotic cells [19]. We predicted a CpG island at approximately 20 kb
upstream from the end of exon II (Fig. 8.3). In endometriotic cells, the CpG
sequence was hypomethylated, while in endometrial cells, the upstream half was
hypermethylated and recognized by the methyl-CpG binding proteins, MBD1 and
MeCP2 [19]. The downstream half was hypomethylated in both endometrial and
endometriotic cells. Because the CpG sequence is located at the promoter-distal
region, we speculate that the sequence may act as a cis-acting element under the
control of methylation.
8 Epigenetics in Endometriosis 111
Fig. 8.3 A hypomethylated CpG island at 20 kb upstream from the end of exon II in endometriotic
cells
Estrogen receptor (ER) plays pivotal roles in the pathogenesis and progression of
endometriosis. Earlier studies have focused on the expression of ER as well as
ER in the eutopic endometrium and in endometriotic lesions. Simultaneous
expression of ER and ER indicates that the estrogen action might be transmitted
in a cooperative manner [20, 21]. In contrast to the high ER/ER expression ratio
in the eutopic endometrium, a lower expression of ER and a markedly higher
expression of ER in ovarian endometriomas have been reported [22, 23]. The
higher ER expression in endometriotic tissue may depend on the hypomethylation
of the ER-promoter region [24]. The increased ER expression in endometriotic
tissues may suppress ER expression [25].
tissues, binds to the unmethylated SF-1 promoter and activates its transcription in
endometriotic cells [42]. The SF-1 expression is under epigenetic control that
permits the binding of activator complexes to the SF-1 promoter [41, 42]. SF-1
expression in endometriosis may enhance aromatase expression. Treatment with a
demethylating agent has been shown to increase SF-1 mRNA levels in eutopic
endometrial cells [26].
HOXA10 has been expressed in the endometrium, and its expression is under the
control of estrogen and progesterone [4648]. The roles in endometrial develop-
ment during the menstrual cycle and in establishing uterine receptivity have been
suggested [47, 48]. In women with endometriosis, HOXA10 expression is signif-
icantly decreased in the eutopic endometrium during the secretory phase, indicating
functional defects in uterine receptivity [47, 49]. The promoter region of HOXA10
gene was found to be hypermethylated in the eutopic endometrium from women
with endometriosis [50]. As promoter hypermethylation has been suggested as an
epigenetic marker of gene silencing, the promoter hypermethylation may be related
to the HOXA10 downregulation in the eutopic endometrium of women with
endometriosis [47].
Fig. 8.4 Differentially methylated CpGs in endometriotic cells (a) CpGs, which show more than
10-fold difference, were extracted (b) the classification
The known epigenetic modifications are DNA methylation and histone modifica-
tions, including methylation, acetylation, ubiquitylation, and phosphorylation [62].
The functional and biological significance of the epigenetic alterations accumulate
over a life span. The earliest studies found a pattern of low global DNA methylation
levels in aged mammalian tissues [63]. A recent monozygotic (MZ) twin study
showed a line of evidence that epigenetic variants accumulate during aging inde-
pendently of the genetic sequence [64]. The study tested the epigenetic contribution
to twin discordance and elucidated the effect of environmental characteristics on
gene function. The results revealed that epigenetic difference between siblings is
associated with phenotypic discordance, which might be attributed to an unshared
environment.
The great fidelity with which DNA methylation patterns in mammals are inherited
after each cell division is ensured by the DNA methyltransferases (DNMTs).
116 M. Izawa et al.
However, the aging cell undergoes a DNA methylation drift. Early studies showed
that global DNA methylation decreases during aging in many tissue types [63]. The
loss of global DNA methylation during aging is probably mainly the result of the
passive demethylation of DNA as a consequence of a progressive loss of DNMT
activity [76]. Several specific regions of the genomic DNA become
hypermethylated during aging [77]. Methylation of promoter CpG islands in
nontumorigenic tissues has been reported for several genes, including ER [77].
Interestingly, genes with increased promoter methylation during aging include the
E-cadherin gene [46], which is downregulated and hypermethylated in
endometriotic cells [65]. Aberrant methylation of CpG islands in 50 promoters has
been suggested to be associated with transcriptional silencing or upregulation in
endometriosis [24, 33, 36, 50]. Recent GW methylation studies suggest that tissue-
and cell-type-specific methylation is present only in a small percentage of CpG
islands in 50 promoters, while a far greater proportion of CpG island methylation is
across gene bodies [78, 79]. In addition, functionally different types of DNA
modification, methylation, and hydroxymethylation have been identified [78,
80]. Therefore, methylation of CpG islands in 50 promoters alone may not be a
major player in the aberrant gene expression.
Histone modifications have a defined profile during aging. For example, the
trimethylation of H4-K20, which is enriched in differentiated cells [81], increases
with age [82, 83] and decreases in cancer cells [8387]. A decrease in the histone
trimethylation has been observed in the liver after the long-term treatment with
the hepatocarcinogen tamoxifen [88]. The loss of trimethylated H4-K20 in cancer
can be caused by the loss of expression of the H4-K20-specific methyltransferase
Suv4-20h [74]. Although approximately 100 histone methyltransferases and
demethylases have been identified in human genome, only a subset of histone
methyltransferase inhibitor is in clinical trials for cancer treatment [89].
Acetylation levels of histones are controlled by a balance between histone
acetyltransferases and histone deacetylases (HDACs). Histone acetyltransferases
transfer acetyl groups from acetyl-CoA to lysine residues on the amino-terminal
region of histones and activate gene transcription. Conversely, HDACs restore the
positive charge on lysine residues by removing the acetyl groups and prevent
transcription. HDACs comprise large multiprotein complexes that target promoter
sites through their interaction with sequence-specific transcription sites. HDAC
inhibitors (HDACIs) can inhibit cell proliferation, induce cell differentiation and
cell cycle arrest, and stimulate apoptosis of various cell types [90]. Hyperacetylation
of histones H3 and H4 is often associated with activated transcription, and
hypoacetylation of histones H3 and H4 correlates with transcriptional silencing
or repression [91]. Kawano et al. [92] recently demonstrated that treatment with
HDACIs induced the accumulation of acetylated histones associated with some
8 Epigenetics in Endometriosis 117
8.7 Conclusion
Epigenetics is one of the most promising and expanding fields in the current
biomedical research of diseases including endometriosis. Most important is its
translational application. One of the immediate questions to be clarified in endo-
metriosis is which genome is under epigenetic aberration. Here we focused mostly
on DNA methylation and reviewed current epigenetics studies in endometriosis.
Epigenetics is currently expanding from DNA methylation to histone modifica-
tions (Fig. 8.5) [94]. The development of high-throughput technologies including
Fig. 8.5 Organization and composition of epigenome. (a) A beads-on-a-string chromatin fiber
includes nucleosome cores connected by linker DNA and linker histone H1. Me: methyl group. (b)
The distribution of DNA methylation and a small subset of histone markings, linker histones, and
core histone variants represent a different regulation at active promoters, gene bodies, and
enhancers (top) as compared to silenced and repressed chromatin (bottom)
118 M. Izawa et al.
Acknowledgment This work was supported in part by Grants-in-Aid for Scientific Research
(C) from Japan Society for the Promotion of Science (Nos. 22591824 and 18591800 to M.I.).
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Chapter 9
Roles of Prostaglandin E2 in Endometriosis
9.1 Introduction
Although the etiology of endometriosis remains unclear, there are several hypoth-
eses proposed including retrograde menstruation theory, embryonic rest theory,
coelomic metaplasia theory, and new combined theory [15]. Among these,
Sampsons retrograde menstruation theory is the most accepted one in which it
states that the origin of endometriosis is caused by implanted cast-off endometrial
tissues, the retrograde menstruation [3, 4]. Several clinical observations, which
described that women with cervical or vaginal obstruction have higher risk of
developing endometriosis, are in line with this hypothesis [68]. In addition, an
animal model of baboon showed that the ligation of cervices increases the incidence
of endometriosis [9]. A more convincing evidence is that endometriosis is observed
exclusively in species that menstruate [10]. Nevertheless, retrograde menstruation
theory is insufficient to explain why only 510 % of women with reflux menstru-
ation developed endometriosis when 90 % of women in reproductive age have
retrograde menstruation [11]. Furthermore, before the infiltration of vasculature,
the retrograded tissues have to escape from the surveillance of immune system, gain
the capacity of steroidogenesis (because endometrial cells are highly dependent on
estrogen), and establish a self-support system to maintain proliferation to survive in
the ectopic sites. Therefore, it is clear that other local or even epigenetic factors
must exist to contribute to the pathological processes of this disease. It is obvious
that we cannot discuss all the factors involved in endometriosis pathogenesis;
therefore, in this review chapter, we will primarily focus on the functional roles
of prostaglandin E2 (PGE2) and some other factors that are involved in the regula-
tion of PGE2 biosynthesis.
synthase (mPGES) and PGF synthases, act on PGH2 to produce PGE2 and PGF2,
respectively [1719]. These enzymes coordinate with preferred partners in specific
tissue to produce PGs. For example, in the process of PGE2 synthesis, cytosolic
PGES (cPGES) and COX-1 account for constitutive production of PGE2 [19, 20],
while the coupling of mPGES-1 and COX-2 is responsible for inflammation-
induced PGE2 production [17]. As is the rule for locally acting lipid mediators,
PGE2 is not stored but rapidly metabolized once synthesized. The major enzymes
responsible for the rapid (within minutes) inactivation of PGE2 are the cytosolic
enzymes 15-ketoprostaglandin 13-reductase and 15-hydroxyprostaglandin dehy-
drogenase (15-PGDH).
Early in the mid-1980s, it was discovered that concentrations of PGE2 are elevated
in the peritoneal fluid collected from women with endometriosis compared to that
derived from otherwise healthy women [21]. Later, it became clear that the majority
128 K.-Y. Hsiao et al.
hypoxia-inducible factors (HIFs). There are two kinds of HIF members: the and
subunits, both of which are constitutively transcribed and translated but undergo
differential posttranslational modifications. Under normoxic condition, the
subunit undergoes hydroxylation at two proline residues (Pro402 and Pro564),
which ultimately results in 26S proteasome-mediated degradation of HIF-
protein [32]. In response to hypoxia, the subunit accumulates due to the lack of
oxygen-induced hydroxylation and degradation. In contrast, the subunit does not
respond to oxygen-dependent degradation and is constitutively expressed. Thus, the
level of subunit determines the gene expression profile of a cell. In endometriotic
stromal cells, levels of HIF-1 mRNA and protein were elevated compared to the
eutopic endometrial stromal cells [33]. Elevation of HIF-1 protein or treatment
with hypoxia causes the downregulation of dual-specificity phosphatase-2
(DUSP2), a downstream inactivator of mitogen-activated protein kinase (MAPK)
signaling [3436]. Downregulation of DUSP2 results in a prolonged activation of
ERK and p38 MAPK in ectopic endometriotic stromal cells, which explains the
increased sensitivity of COX-2 promoter to IL-1 stimulation because it is medi-
ated by ERK- and p38 MAPK-dependent signaling pathway [25].
In addition to altered COX-2 regulation, PGE2 transporter/carrier may also play
important roles on the PGE2 production. Up to date, only few transporters/carriers
of PGE2 have been found and are capable of facilitating the uptake or clearance of
PGE2 to regulate pericellular PG levels. The co-expression of prostaglandin trans-
porter, preferentially transporting PGE2, and 15-PGDH, metabolizing PGE2 resides
in cytoplasm, indeed supporting the idea that uptake of PGE2 is essential for its
metabolism [37]. Multidrug resistance-associated protein 4 (MRP4) is one of the
few proteins with high specificity to export PGE1 and PGE2 [38]. Interestingly,
endometriotic tissue expressed lower 15-PGDH but higher MRP4 mRNA compared
to eutopic ones and correlated to higher PGE2 production/release [29, 39].
the survival of endometriotic tissue when the ovarian estrogen is not available? The
answers to this question were revealed by multiple studies showing that
endometriotic stromal cells actually are capable of producing estrogen.
Endometriotic stromal cells not only express proteins/enzymes required for de
novo synthesis of estrogen but even express at higher levels compared to its
endometrial counterpart. The pro-steroidogenic proteins, including steroidogenic
acute regulatory protein (StAR), P450 side chain cleavage enzyme,
3-hydroxysteroid dehydrogenase, 17-hydroxylase 17, 20 lyase, aromatase,
and 17-hydroxysteroid dehydrogenase type I, are either aberrantly expressed or
elevated in ectopic stromal cells [4244], whereas the anti-steroidogenic
protein, 17-hydroxysteroid dehydrogenase type II, is suppressed. Among these
proteins, StAR and aromatase control two of the most important steps for
estrogen production. StAR governs the first step in which hydrophobic cholesterol
is carried through the double-membraned mitochondria where the P450 side chain
cleavage enzyme resides and aromatase converts androstenedione to estrone.
Expression of StAR in endometriotic stromal cells is induced by PGE2 (Fig. 9.2).
This stimulation is unique to endometriotic stromal cells, but not found in eutopic
9 Roles of Prostaglandin E2 in Endometriosis 131
between 24 and 48 h. Taken together, via two different types of receptors, PGE2 is
able to induce the critical survival and proliferating factor, FGF9, to ensure the
progression of endometriosis.
Fig. 9.3 Prostaglandin E2 inhibits phagocytosis. Under low-PGE2 condition, macrophages are
recruited to the peritoneal cavity due to retrogradely transported endometrial tissue-induced
inflammation. Recruited macrophages express high levels of annexin A2 (membrane form and
soluble form), MMP9, and CD36 to facilitate phagocytosis. Therefore, the retrograded tissues will
be engulfed and removed. However, under high concentrations of PGE2 (indicated by red lines),
the expression of annexin A2, MMP9, and CD36 is all suppressed. Thus, macrophages lose their
phagocytic ability and retrogradely transported endometrial tissues are able to implant and grow in
the peritoneum
MMP-9 are reduced, the MMP-9 enzymatic activity is also inhibited [89]. This
markedly impairs macrophages ability to digest the basement membrane of retro-
gradely transported tissues and ultimately contributes to reduced macrophages
phagocytic ability. Since CD36 is one of the first macrophage receptors to be
implicated in the recognition of aged or apoptotic cells [90, 91] and annexin A2
participates in both MMP-9 activation and phagocytosis, reduced expression of
CD36 and annexin A2 severely impairs the phagocytic ability of macrophages.
Indeed, when CD36 or annexin A2 is knocked down from the normal macrophages,
the phagocytic ability is reduced. In contrast, when peritoneal macrophages isolated
from individuals with endometriosis are transfected with exogenous CD36 or
annexin A2, the phagocytic ability is restored [88, 92].
The next question to ask is which factor in the endometriosis peritoneal fluid
exerts such inhibitory effect. Because endometriosis is a chronic inflammatory
disease and many proinflammatory cytokines are elevated in the peritoneal fluid
of endometriosis [24, 9396], it is likely that reduced phagocytic ability of perito-
neal macrophage is mediated by one or some of these proinflammatory cytokines.
Through a series of screens, we identified that PGE2 is the primary factor to inhibit
the expression of MMP-9, annexin A2, and CD36 in peritoneal macrophages [88,
89, 92]. PGE2, via binding to the EP2 and EP4 receptors, activates PKA signaling
pathway to suppress the expression of MMP-9, annexin A2, and CD36. As
expected, treatment of macrophages with PGE2 inhibits phagocytic ability, which
can be reversed by adding EP2 receptor antagonist [92]. The in vitro results of PGE2
action in suppressing phagocytosis are further supported by in vivo autologous
transplanted mouse model. In this model, uterine endometria from donor mice are
peeled off, minced into small pieces, and injected into peritoneal cavity of recipient
mice. Recipient mice are treated with or without PGE2 or selective COX-1/COX-2
inhibitors to blunt the biosynthesis of PGE2 for 4 weeks. Mice treated with PGE2
have more endometriotic tissue-like lesions, lower levels of CD36 and annexin A2
in peritoneal macrophages, and reduced phagocytic ability of peritoneal macro-
phages. In contrast, mice that received selective COX inhibitors develop fewer
lesions, express more CD36 and annexin A2 by the peritoneal macrophages, and
exert greater phagocytic ability of peritoneal macrophages [88, 92]. Taken alto-
gether, these data reveal that PGE2 utilizes the same receptor-mediated signaling
pathway to target three different molecules involved in phagocytosis. Such a
safeguarding system to efficiently inhibit macrophages phagocytic ability by
controlling three target proteins simultaneously is likely due to the evolutional
advantage.
Taking together all currently available data, it is clear that COX-2-derived PGE2
does play a key role in establishing an effective blood supply system either directly
or indirectly during the development of endometriosis. Targeting COX-2-derived
PGE2 signaling pathway to blunt new blood vessel formation may be a plausible
approach to prevent the development of endometriosis.
Fig. 9.4 Positive feed-forward loops of PGE2 actions in endometriosis. Regulation of PGE2
biosynthesis in ectopic endometriotic stromal cells is regulated by predisposition to hypoxic stress,
which inhibits expression of dual-specificity phosphatase-2 (DUSP2) and leads to a prolonged
activation of ERK. Phosphorylated ERK stabilizes HIF-1 and, at the same time, enhances
proinflammatory cytokine-induced COX-2 expression and PGE2 production. These
proinflammatory cytokines also induce COX-2 expression and PGE2 production by peritoneal
macrophages. Elevated concentration of PGE2 stimulates steroidogenesis and angiogenesis to
promote cell proliferation and inhibits phagocytosis to prevent ectopic endometriotic tissues
from destroyed by macrophages. The effects of PGE2 are augmented by three feed-forward
positive regulatory loops: (1) hypoxia-HIF-1-ERK loop, (2) COX-2-PGE2-estrogen loop, and
(3) COX-2-PGE2 proinflammatory cytokine loop. See text for details
Acknowledgment This work was supported by grants from National Science Council of Taiwan
(NSC-101-2320-B-006-030-MY3 to SJT and NSC-101-2314-B-006-043-MY2 to MHW). KYH
wrote the first draft and proof-read the final manuscript. MHW and SJT edited and wrote the final
draft. SJT designed and supervised the project. All authors read and approved the final draft.
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9 Roles of Prostaglandin E2 in Endometriosis 145
Jo Kitawaki
10.1 Introduction
J. Kitawaki (*)
Department of Obstetrics and Gynecology, Kyoto Prefectural University of Medicine,
Graduate School of Medical Science, Kyoto 602-8566, Japan
e-mail: [email protected]
hormone agonist causes regression of the lesions. The recovery of estrogen levels
after discontinuing therapy causes a relapse. Endometriosis may relapse in post-
menopausal women who have been treated with estrogen-replacement therapy,
suggesting that endometriosis progresses and regresses in an estrogen-dependent
fashion.
ER- levels are higher and ER- levels are lower in women with endometriosis than
in those with a normal endometrium. Higher ER- levels are caused by
hypomethylation of a CpG island at the promoter region of this gene. In
endometriotic cells, the excess expression of ER- is responsible for the estrogen-
dependent responses, and this expression inhibits ER- action [12].
The single PR gene is translated into one of two isoforms (PR-A or PR-B) by
activating the corresponding promoters. PR-A is a truncated form of PR-B that
lacks the N-terminal 164 amino acids; PR-A acts as a repressor of PR-B function. In
endometriotic tissue, PR-B is undetectable [13] due to hypermethylation of the PR
gene and PR-A is markedly reduced [14]. Furthermore, excess ER- occupies the
estrogen responsive element at PR promoter region and blocks transcription of PR
that is normally activated by ER- [15].
10 Sex Steroids and Endometriosis 149
10.2.2.1 Aromatase
and diseased endometria, estrogen metabolism is different between the two states.
Furthermore, in endometriotic tissues, progesterone does not stimulate HSD17B2
because there is no PR-B [13], whereas endometrium of women with endometriosis
acquires ability to stimulate HSD17B2 by progesterone.
Both environmental and genetic factors have been implicated in the pathogenesis of
endometriosis. Family and twin studies have indicated that there is a two- to
ninefold increase in the risk of developing endometriosis in first-degree relatives
of women with endometriosis, suggesting it is a genetic disorder with polygenic or
multifactorial inheritance [2830]. Studies have revealed associations between the
polymorphisms of many genes, including the genes involved in steroid metabolism
and endometriosis susceptibility.
10.3.1 ESR1
Polymorphisms in the gene coding for ER- (ESR1) have been investigated in
European and Asian women. Single-nucleotide polymorphisms in intron 1 of
the ESR1 gene have been assessed in PvuII (398 T/C) and XbaI (351A/G)
restriction fragment length polymorphisms. Several studies found statistically sig-
nificant differences between the cases and controls in the distribution of PvuII
alleles [3134], but other studies found no association with PvuII polymorphisms
[3538]. One study found an association with an XbaI polymorphism [34], and
three studies found an association with the TA dinucleotide repeat polymorphism
[31, 36, 39, 40].
10.3.2 ESR2
One study in Japanese women showed association with the gene coding for
ER- (ESR2) AluI polymorphism [35], but other studies found no association
[33, 41]. One study showed that shorter CA dinucleotide repeats in the ESR2
gene were linked to endometriosis in women without infertility [40].
10 Sex Steroids and Endometriosis 151
10.3.3 PR
Several studies in Austria, Italy, and Brazil showed association between the 306-bp
insertion polymorphism in intron G of the PR gene (PROGINS) and the risk of
endometriosis risk [4244].
10.3.4 HSD17B1
Several studies showed that, in an A/G polymorphism of the HSD17B1 gene, the A
allele was found to be associated with a significantly increased risk of endometriosis
[40, 45].
10.3.5 CYP17
10.3.6 CYP19
10.4 Conclusions
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Chapter 11
Aromatase Expression in Endometriosis
and Its Significance
11.1 Introduction
are more potent than those expected from a comparable amount of endocrine
estrogen, possibly because in situ estrogen directly acts on neighboring cells with
neither dilution into the circulating volume nor binding to proteins that interfere
with the hormonal action.
Table 11.1 Association between CYP19A1 gene polymorphisms and the risk of endometriosis
Staging of cases
Nucleotide Range of age Range of age (number of
polymorphisms Location Author Cases (mean SD) Control (mean SD) subjects)a Results
rs 10046 30 untranslated Szczepanska 115 2039 197 1939 I (59), II (56) No associationb
C1558T region of et al.
Exon 10 Lamp et al. 150 1845 199 3050 I (53), II (39), III No association
(32.1 6.1) (39.8 5.3) (36), IV (22)
Vietri et al. 104 2245 86 1848 Undescribed Genotype CC was
(36.8 6.7) (37.8 5.1) overpresented in
cases (48.1 %
vs. 30.2 %)
Hur et al. 224 Undescribed 188 Undescribed III to IV (224) No association
Huber et al. 32 (52.3 5.4) 790 (34.6 7.0) I (0), II (21), III (10), No association
IV (1)
rs700519 Exon7 Wang et al. 300 (34.3 6.9) 337 (52.2 4.2) I (7), II (52), III No association
C > T, (165), IV (76)
Arg264Cys Tsuchiya et al. 79 2045 59 2045 I (21), II (10), III No association
(23), IV (25)
Huber et al. 32 (52.3 5.4) 790 (34.6 7.0) I (0), II (21), III (10), No association
IV (1)
rs2236722 Exon2 Wang et al. 300 (34.3 6.9) 337 (52.2 4.2) I (7), II (52), III No association
T > C, (165), IV (76)
Trp39Arg Hur et al. 224 Undescribed 188 Undescribed III to IV (224) No association
240 A > G, At codon80 Vietri et al. 104 2245 86 1848 Undescribed Genotype AA was
Val80 in exon3 (36.8 6.7) (37.8 5.1) overpresented in
cases (50.0 %
vs. 32.6 %)
Hur et al. 224 Undescribed 188 Undescribed III to IV (224) No association
H. Ishikawa and M. Shozu
11
3 bp insertion/ 50 bp upstream Lamp et al. 150 1845 199 3050 I (53), II (39), III No association
deletion from the (32.1 6.1) (39.8 5.3) (36), IV (22)
(TTTA)n Kado et al. 140 2448 177 (63.8 6.1) I to II (32), III to IV Del/Del was fre-
tract in (36.3 8.1) (108) quently
intron4 observed in
cases
rs1004982 Intron Trabert et al. 256 1849 567 Matched to Undescribed Increased risk of
cases endometriosis
rs18700479 Intron Increased risk of
endometriosis
rs936307 Intron Increased risk of
endometriosis
(TTTA) repeat Intron4 Lamp et al. 150 1845 199 3050 I (53), II (39), III No significant asso-
number (32.1 6.1) (39.8 5.3) (36), IV (22) ciation between
[TTTA] repeat
<7 and [TTTA]
repeat 813
Hur et al. 224 Undescribed 188 Undescribed III to IV (224) No significant asso-
ciation between
[TTTA] repeat
<7 and [TTTA]
Aromatase Expression in Endometriosis and Its Significance
repeat 813
Kado et al. 140 2448 177 (63.8 6.1) I to II (32), III to IV No significant asso-
(36.3 8.1) (108) ciation between
[TTTA] repeat
<7 and [TTTA]
repeat 813
Arvanitis et al. 275 2137 346 2653 Undescribed [TTTA] 10 allele
(27.2 3.2) (34.5 7.4) increased risk by
4.99 times for
endometriosis
a
The staging was assessed by the revised American Society for Reproductive Medicine score
161
b
No statistically significant association was observed among different genotypes
162 H. Ishikawa and M. Shozu
Changes in the methylation status of CpG islands of CYP19A1 have been reported
in endometriosis [26]. A CpG island located approximately 70 kb downstream from
exon 1.1 of CYP19A1 is hypomethylated in endometriosis (stromal cells obtained
from ovarian chocolate cysts) but hypermethylated in the eutopic endometrium
(stromal cells obtained from disease-free women). The methyl-CpG-binding pro-
teins MBD1 and MeCP2, which contain an amino-terminal methyl-CpG-binding
domain and a carboxy-terminal transcriptional repression domain, bind to the
hypermethylated region of the CpG island in eutopic tissues, which in turn may
suppress aromatase expression in the eutopic endometrium [27].
The treatment of endometrial stromal cells with 5-aza-deoxycytidine
(an irreversible inhibitor of DNA methyltransferase1, which is essential for
maintaining the methylation status of genomic DNA) induces aromatase expression
in endometrial stromal cells obtained from disease-free women. The demethylation of
the CpG islands in CYP19A1 may be relevant to the upregulation of aromatase [28],
although other explanations are possible because 5-aza-deoxycytidine alters the
expression level of a broad spectrum of genes that may indirectly or directly affect
aromatase expression.
Histone modifications affect the chromatin structure and the subsequent interaction of
transcription factors with their response elements in the promoters. The acetylation of
histone H3 and histone H4 activates transcription by loosening the chromatin structure
and allowing the recruitment of transcription factors to their response elements.
In contrast, trimethylation of lysine at sites 9 and 27 on histone H3 inactivates
transcription by causing the chromatin to become more condensed. Histone modifi-
cations affect Cyp19a1 mRNA expression in rat granulosa cells [29]. We found
that the acetylation of H3 and H4 at the promoter I.4 region occurs during the
induction of aromatase expression by dexamethasone in breast cancer cell lines.
No histone modification has been reported for aromatase regulation in endometriosis
till date.
miRNAs are short noncoding RNAs that act by targeting partially complementary
sequences within mRNAs. They consist of 1925 nucleotides and commonly exist
in the 30 -untranslated region of the target genes. Traditionally, miRNAs negatively
regulate the transcription of their target genes. A single miRNA may target many
genes, and each of them may in turn be regulated by different miRNAs [30].
11 Aromatase Expression in Endometriosis and Its Significance 163
In addition to the mRNA level, aromatase activity is regulated at the protein level. It
has been reported that phosphorylation and dephosphorylation of amino acids in the
aromatase protein alter the enzymatic activity [34, 35].
Recently we found a novel mechanism underlying posttranslational regulation
by autophagy [36]. Insulin-like growth factor-1 enhances aromatase activity over
50 % as early as 1 h in THP-1 myeloid leukemia cells through the inhibition of
autophagy. A part of the newly synthesized aromatase protein is continuously
transported to the lysosome and is degraded when aromatase protein synthesis is
increased.
Another mechanism underlying posttranslational regulation has been proposed.
A series of transfection experiments revealed that mRNA stability and protein
translation efficiency vary among the 50 -noncoding sequence of exon 1 of aroma-
tase [37]. The 50 -noncoding sequence of exons I.3 and I.4 contains the cis-acting
elements responsible for the modulation of aromatase levels.
No study has reported the posttranslational regulation of aromatase in endome-
triosis where aromatase is highly expressed and translated.
11.4.1 AIs
AIs were originally developed for the treatment of breast cancer. By the 1990s, it
had been revealed that breast cancer tissues synthesize estrogen in situ, which
promotes breast cancer cell growth. After the molecular cloning of aromatase in
the late 1990s, the aberrant expression of aromatase was identified as a cause of the
overproduction of estrogen in situ. AIs were then developed as a new endocrine
treatment of breast cancer. Initial trials showed that AIs reduced the level of
estrogen in situ and suppressed the progression of cancer in postmenopausal
women [59, 60]. Subsequent large-scale studies confirmed the therapeutic advan-
tages over tamoxifen and reported the reduction of cancer development in the
contralateral breast, suggesting a cancer preventive effect [61]. The role of in situ
estrogen in pathology was first exemplified in breast cancer, and this established
aromatase as a molecular target for endocrine therapy.
AIs are now widely used for the treatment of ER-positive breast cancer in
postmenopausal women. The use of AIs shows a survival benefit compared with
that of other endocrine therapies in women with advanced breast cancer [62].
11 Aromatase Expression in Endometriosis and Its Significance 167
11.4.2 Pharmacology
AIs cause undesired health issues related to the presence or absence of estrogen
suppression. Bone loss and fracture are the most important issues, particularly in
postmenopausal women who use AIs for more than 6 months. Concomitant use of
bisphosphonate is recommended for women who have additional risk factors for
fracture [71]. Compared with the use of tamoxifen, long-term use of AIs increases
the odds of cardiovascular disease [72]. Other side effects associated with the use of
AIs are hot flushes, headache, joint stiffness or pain, leg cramps, arthralgia, nausea,
and diarrhea. All of them are generally mild and are therefore tolerable.
It has been reported that AIs + norethindrone acetate or other OCs prescribed for
the treatment of endometriosis cause bone mineral loss, as seen in the case of breast
cancer. The change is significant but not symptomatic. This is partly because of the
shorter duration of therapy compared with that for patients with breast cancer and
partly because of the bone protective action of concomitantly used sex steroids [64].
11.4.4.1 AI Monotherapy
A few reports have provided evidence of the efficacy of AI monotherapy for the
treatment of endometriosis-related pain in premenopausal women. In these studies,
vaginally administered anastrozole (0.25 mg/day) combined with oral elemental
calcium (1.2 g/day) and cholecalciferol (800 IU/day) for 6 months improved
rectovaginal endometriosis-related dysmenorrhea [74].
A prospective randomized clinical trial has been conducted to compare the effect
of short-term letrozole and a GnRH agonist (triptorelin) versus case control on the
pregnancy rate and recurrence of endometriosis after laparoscopic surgery [75]. The
overall pregnancy and recurrence rate of the letrozole group (2.5 mg/day for
2 months) were similar to those of the triptorelin group. The pregnancy and
recurrence rate among the 3 groups were as follows: 23.4 and 6.4 % in the letrozole
group, 27.5 and 5 % in the triptorelin group, and 28.1 and 5.3 % in the control
group, respectively.
Another case report has revealed the efficacy and side effects of AIs in the
treatment of premenopausal patients with endometriosis-related chronic pelvic pain
refractory to conventional treatment. Four premenopausal patients were treated with
either anastrozole (1 mg/day) combined with alendronate (10 mg/day) or letrozole
(2.5 mg/day) combined with calcium (1.5 g/day) and vitamin D (800 U/day) for
6 months, and marked improvement of pelvic pain was observed in all the patients
without significant hormonal change and bone mineral loss [76]. The most common
side effect was irregular bleeding with anastrozole and joint pains with letrozole.
Thus, AI monotherapy for endometriosis-related pain is tolerable for a short
duration, if the prevention of bone mineral loss is adequate.
a rapid, progressive reduction in pain, and the remission lasted over 24 months
after treatment [78].
Another large-scale, prospective, open-label, nonrandomized trial including
82 women with pain caused by rectovaginal endometriosis has been conducted.
Patients received either norethisterone acetate (2.5 mg/day) alone or a combination
of letrozole (2.5 mg/day), norethisterone acetate (2.5 mg/day), elemental calcium
(1,000 mg/day), and vitamin D3 (880 IU/day) for 6 months. Both regimens were
similarly effective for dysmenorrhea; however, the efficacy differed between the
2 regimens with respect to chronic pelvic pain and deep dyspareunia. The reduction
rate of the intensity of the pain scale in the combination therapy was 1.41.5-fold
larger than that in therapy with norethisterone acetate alone [79]. A carryover effect
was not observed in both regimens in terms of pain relief. Side effects, including
joint pain (n 5) and myalgia (n 5), hair loss (n 1), and decreased libido
(n 1), were only reported for the combination therapy (n 41). However, with-
drawal due to side effects was not statistically different between the combination
group (n 4) and the norethisterone acetate group (n 3).
Overall, the use of AIs enhances the therapeutic efficacy of progesterone/progestins
with regard to pelvic pain and deep dyspareunia that are refractory to established
treatments. However, the improvement in the pain relapses soon after the comple-
tion of treatment, and the side effects, albeit minor, are increased. For extended
treatment, great caution is required regarding side effects related to long-term use
of AIs, such as bone loss and arthritis, as reported in case of long-term
AI monotherapy for breast cancer.
The efficacy of AIs for refractory endometriosis has been also examined in
combination with OCPs. A phase 2 prospective open-label trial was conducted on
15 premenopausal women with documented refractory endometriosis and chronic
pelvic pain [80]. The use of anastrozole (1 mg/day) and 1 tablet of ethinyl estradiol
(20 g/day)/levonorgestrel (0.1 mg/day) daily for 6 months significantly relieved the
pain. Side effects were mild, and no adverse effects on major organs were observed.
The efficacy of AIs + OCPs for premenopausal patients with ovarian
endometriomas and chronic pelvic pain, who were previously treated with surgery
and medication with an unsatisfactory result, has been reported. Five women received
letrozole (2.5 mg/day), desogestrel (0.15 mg/day), ethinyl estradiol (0.03 mg/day),
calcium (1,200 mg/day), and vitamin D (800 IU/day) daily for 6 months. Ovarian
endometriomas disappeared and the pain was relieved in all 5 women. Loss of bone
mineral density was not observed [81]. This result is excellent; however, interpretation
is limited because of the small number of patients and the fact that the study was
nonrandomized and did not include controls. In addition, the primary target of the
treatment was ovarian endometrioma and not rectovaginal endometriosis.
Further randomized trials are necessary to elucidate the benefits of a
combination of AIs with OCPs.
11 Aromatase Expression in Endometriosis and Its Significance 171
11.5 Conclusions
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Chapter 12
Apoptosis in Endometriosis
12.1 Introduction
Endometrial cells from women with and without endometriosis have fundamental
differences. Endometrial cells from women with endometriosis has enhanced
proliferation and increased ability to implant and survive in ectopic locations.
Impaired sensitivity of endometrial tissue to apoptosis contributes to abnormal
implantation and growth of endometrium at ectopic sites. The inability of endome-
trial cells to transmit a death signal or their ability to avoid cell death is associated
with increased expression of antiapoptotic factors (e.g., Bcl-2) and decreased
expression of proapoptotic factors (e.g., BAX) [6]. It is unclear whether the
abnormal apoptosis in the eutopic endometrium from patients with endometriosis
is primary in origin or secondary after establishment of pelvic endometriosis
process. This could be attributed to the fact that at the time of clinical presentation
and diagnosis most women have already established disease and therefore, it is very
difficult to investigate the early developmental stages of the endometriosis.
Reflux of endometrial fragments during menstruation into the peritoneal cavity
is a common phenomenon. Under normal conditions, cells that do not adhere to
their extracellular matrix enter apoptosis as they receive different signals from their
12 Apoptosis in Endometriosis 181
adhesion receptors [7]. In endometriosis, these cells have the ability to adhere to
mesothelial cells of peritoneum, to proliferate, and to produce neoangiogenesis
resulting in the development of active endometriosis. The effect of MMPs on
apoptotic factors and their regulation by steroid hormones may provide a link
between endometrial turnover and the invasive process necessary for the develop-
ment of endometriosis. Immunoglobulin-like cell adhesion molecules (nectins and
Necls) involved in apoptosis and cell proliferation have also stronger expression in
eutopic and ectopic endometrium of women with endometriosis [8]. High levels of
VEGF and IL-1 have been found in the PF of patients with endometriosis. VEGF
and IL-1 reduce apoptosis and decrease Bax expression in endometrial epithelial
cells from patients with endometriosis. VEGF and IL-1 may protect endometriotic
cells from undergoing apoptosis favoring the establishment and progression of
endometriotic lesions by promoting the formation of new blood vessels and by
protecting endometriotic cells from undergoing cell death [9].
Intrinsic abnormalities in transplanted eutopic endometrium are contributed to
the pathogenesis of endometriosis. Abnormal signaling pathways in the eutopic
endometrium of women with endometriosis have been recently reported. Two
different groups demonstrated increased activity of the protein kinase A and B
pathways regulating the function of many cellular proteins involved in apoptosis
and proliferation [10, 11]. It was suggested that increased Akt phosphorylation may
be related to the altered apoptosis/proliferation harmony in endometriosis. Another
pathway whose activation confers a resistant to apoptosis phenotype in
endometriotic cell is the NF- [12]. In vivo, NF-B inhibition in early-stage
endometriotic lesions induced in nude mice was found to decrease the proliferation
of endometriotic cells and stimulate their apoptosis [13].
cDNA microarray analysis has provided an interesting insight for altered gene
expression profiles in patients with endometriosis. Arimoto et al. found
97 upregulated and 337 downregulated genes in women with endometriosis [14].
Genes related to apoptosis (GADD34, GADD45A, GADD45B, PIG11) and the
tumor suppressor TP53 gene were downregulated in endometriotic tissues. These
findings are inconsistent with the decreased spontaneous apoptosis observed in
eutopic endometrium from women with endometriosis.
Survivin is a member of the inhibitors of apoptosis family (IAP). IAP proteins
directly inhibit the terminal effector caspases 3 and 7 and thus protect cells from
apoptosis. Endometriotic cells express more survivin genes than normal endome-
trial cells without endometriosis [15]. Survivin plays a critical role in susceptibility
of endometriotic stromal cells to apoptosis and survivin inhibitors may be effective
as treatment for endometriosis [16]. Increased survivin expression was present in
eutopic and ectopic epithelial cells, but only ectopic epithelial cells lost the cyclic
variation of survivin expression during menstrual cycles.
Recently, aberrant miRNA expression has been shown to play an important role
in the pathogenesis of endometriosis as a part of epigenetic mechanisms. A global
miRNA microarray technique used to evaluate the expression of miRNAs in
endometriotic cyst stromal cells [17]. In normal endometrial stromal cells
miR-196b targets c-myc and Bcl-2 expression, inhibits proliferation, and induces
182 A. Kaponis et al.
Apoptosis helps to maintain cellular homeostasis during the menstrual cycle by elim-
inating senescent cells from the functional layer of the uterine endometrium [19].
In normal endometrium, apoptotic cells were identified in the glandular epithelium
of late secretory and menstruating endometrium due to progesterone withdrawal,
while very little apoptosis was detected during the proliferative phase or at the begin-
ning of the secretory phase [20]. The pattern of apoptosis negatively correlates to serum
estradiol concentrations in the proliferative phase [20]. Considering the cyclical nature
of apoptosis in normal endometrium, it seems likely that estrogen and progesterone
can regulate the signals that result in apoptosis in this tissue.
Bcl-2 has been considered to inhibit apoptosis in the endometrium during the
proliferative phase. Bcl-2 cyclically expressed in endometrial glandular and stromal
cells peaks during the late proliferative phase, while it decreases dramatically in the
early and mid-secretory phase to reappear in the late secretory phase. In contrast,
myometrial smooth muscle cells showed consistent Bcl-2 immunoreactivity
throughout the menstrual cycle [21]. Higher expression of Bcl-2 was observed in
the basal layer, whereas death receptor Fas and caspase-3 were higher in the
functional layer of the endometrium [22]. These results fit well with the functional
biology of endometrium. Since the basal layer remains relatively constant through-
out the menstrual cycle, apoptosis is less common in this layer. The functional layer
that undergoes cyclical growth, differentiation, and shedding appears with
increased level of apoptosis.
Susceptibility of any given cells to a potential apoptotic stimulus may be
determined by the ratio of pro- and antiapoptotic Bcl-2 family members presented
in the cell at that time [23]. Bax and Bak are Bcl-2 family members promoting cell
death susceptibility, possibly by countering the effect of Bcl-2 on cellular survival
through heterodimer interaction. BAX and BAK were upregulated in the glandular
12 Apoptosis in Endometriosis 183
epithelial cells during the secretory phase of the normal menstrual cycle [24, 25].
These data imply the existence of a dynamic interplay among many members of the
Bcl-2 family in triggering apoptosis.
The Fas ligand (FasL) belongs to the tumor necrosis factor superfamily. The
Fas/FasL interaction is essential in inducing apoptosis. Fas expression seems to be
unchanged in the different phases of the menstrual cycle [26]. FasL exhibits peak
expression during the secretory and menstrual phases [27]. Taken together, Bcl-2 is
expressed in human endometrial glandular cells during the proliferative phase but
not during the late secretory phase. In contrast, both Fas and FasL are expressed
throughout the cycle in weak or moderate amount, except relatively higher expres-
sion of FasL in the late secretory phase. It is generally accepted that Bcl-2 blocks
apoptosis via the mitochondrial pathway and not the death receptor pathway
induced by the Fas/FasL system. Therefore, in the normal human endometrium,
caspase-8 is initially activated by the Fas/FasL signal, resulting in the caspase
cascade. Activated caspase-8 can switch on both the death receptor pathway and
the mitochondrial pathway via Bid degradation [28]. It is possible that both the
mitochondrial and the death receptor pathways are involved in apoptosis of human
endometrial cells.
endometrium from women with endometriosis when compared with normal endo-
metrium from healthy women [32]. BAX expression was absent in proliferative
endometrium, whereas there was an increase in its expression in secretory endo-
metrium from women with endometriosis and healthy women. The Bcl-xL/Bcl-xS
ratio (antiapoptotic/proapoptotic) was substantially higher in eutopic endometrium
from women with endometriosis compared to endometria from women without
endometriosis [33]. Altered expression of Bcl-2 family members in eutopic endo-
metrium of women with endometriosis resulted to a decreased number of apoptotic
cells and consequently to their abnormal survival in the ectopic locations.
Increased prostaglandin E2 (PGE2) signaling was observed in ectopic
endometriotic tissues compared with eutopic endometrium tissues during the men-
strual cycle [34]. The ability of endometriotic cells to circumvent apoptotic signals
can be the result of increased PGE2 signaling, which is associated with abundant
expression of the antiapoptotic Bcl-2 and Bcl-XL proteins, low expression of
proapoptotic Bax protein, phosphorylation/inactivation of proapoptotic Bad protein,
and activation of multiple cell survival signaling pathways (ERK1/2, Akt, nuclear
factor-, -catenin) [35].
Few studies have been published on the expression of Fas in endometriotic tissues.
Harada et al. found that Fas is expressed randomly in both eutopic and ectopic
glandular endometrial cells [36]. Fas expression was constant in both tissues
throughout the menstrual cycle. Abundant expression of Fas antigen was found in
NKcells of PF of women with early stages of endometriosis [37]. The activated PF
NK-cells can be intensively eliminated via the Fas/FasL apoptosis, thus providing
conditions for the survival of ectopic endometrium cells and the development of the
disease at the initial stages of endometriosis.
In contrast with Fas, many studies indicated that higher expression of FasL by
endometriotic cells contributes to their survival and the development of endome-
triosis. The levels of soluble/active FasL are higher in serum and PF in women with
moderate to severe endometriosis than in women with early-stage disease or in
disease-free women [38]. Higher levels of soluble FasL in the PF of women with
endometriosis may contribute to increased apoptosis of Fas-bearing immune cells
in the peritoneal cavity, leading to their decreased scavenger activity [31]. This may
result in prolonged survival of endometrial cells into the peritoneal cavity.
The sources of the elevated levels of soluble FasL in the peritoneal cavity were
endometriotic lesions and PF leukocytes. Endometrial glandular and stromal cells
presented with increased FasL expression. Peritoneal macrophages in endometri-
osis might stimulate a Fas-mediated apoptosis of immune cells [38]. FasL expres-
sion in the endometriotic cells may protect them from attack by T lymphocytes.
Consequently, ectopic endometrium cells escaping from immune surveillance in
the peritoneal cavity may contribute to the maintenance of the disease. It is,
12 Apoptosis in Endometriosis 185
therefore, possible that many endometriotic cells not only become resistant to
Fas-mediated apoptosis, but additionally they have acquired the ability to utilize
this pathway to their advantage by launching a Fas counterattack against the
hosts immune system.
Upregulation of FasL expression by endometriotic cells could be induced after
the adhesion of these cells to the extracellular matrix proteins laminin, fibronectin,
and collagen IV [39]. MMPs have been implicated in the conversion of FasL to
active/soluble forms, suggesting that these molecules can activate or release factors
involved in the apoptotic process [40]. FasL expression that occurs when endome-
trial stromal cells attach to the extracellular matrix may be one of the critical events
in the development of endometriosis.
Interleukin-8 (IL-8), a chemokine for neutrophils and a potent angiogenic agent,
is elevated in the PF of women with endometriosis [41]. IL-8 promotes proliferation
of stromal cells derived from endometriotic tissues [42], suggesting that it may
facilitate growth of endometriotic implants. Selam et al. demonstrated a
concentration-dependent increase in IL-8-induced FasL expression in endometrial
stromal cells. Elevated IL-8 levels in PF, via stimulation of FasL, induce apoptosis
in activated T lymphocytes and contribute to an immune-privileged environment
around the endometriosis implants supporting their survival [43]. On the other
hand, IL-8 exerts a chemotactic activity primarily on neutrophils and inhibits
their apoptosis even in the presence of Fas engagement. IL-8 is one of the neutro-
phil survival factors in the PF of endometriosis patients. IL-8 exerts the
antiapoptotic effects by activating the PTEN/Akt pathway and mediating the
expression of survivin and Bcl-2 [44]. IL-2 also enhanced survival and invasiveness
of endometrial stromal cells in an autocrine manner by activating Akt and MAPK/
Erk1/2 signal pathway [45]. The impaired clearance of cells responsible for innate
immunity in the PF of patients with endometriosis may be associated with the
development of the disease.
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Chapter 13
Role of Nerve Fibres in Endometriosis
Natsuko Tokushige
Nerve fibres in the body arise from cell bodies in dorsal root ganglia (DRG) and
nerve fibres in the head arise from cell bodies in trigeminal ganglion. Nerve fibres
are categorised into six groups, namely A, A, A, A, B and C fibres. Cell bodies
with the largest diameters give rise to myelinated A, A and A fibres, and cell
bodies with small and medium diameter give rise to thinly myelinated A and B and
N. Tokushige (*)
Department of Obstetrics and Gynaecology, University of Tottori, Tottori, Japan
e-mail: [email protected]
There are two types of nociceptors, namely high threshold mechanoreceptors and
polymodal nociceptors. High threshold mechanoreceptors respond to mechanical
damage such as cutting, crushing or pinching, and polymodal nociceptors respond
to all kinds of damaging stimuli, such as irritating chemicals released from injured
tissue. Information from high threshold mechanoreceptors are rapidly transmitted
to the brain mainly by A fibres, and the location of pain can be recognised.
However, information from polymodal nociceptors is transmitted to the brain
slowly and the location of pain is usually unrecognised.
Nociceptors can be further divided into peptidergic which contains peptides,
such as substance P (SP) and calcitonin gene-related peptide (CGRP), and
non-peptidergic which binds isolectin B4 (IB4) [3]. A and C fibres express
many of the molecules that have been implicated in the pain activation and
sensitisation. These molecules include numerous ion channels and receptors for
chemical mediators in their sensory endings. Most nociceptors express only part of
the receptors, but prolonged inflammation can lead to an up-regulation of receptors
for excitatory compounds. It is likely that the expression of some receptors for
chemical mediators may be increased in endometriosis.
The pain from the periphery enters the spinal cord via DRG and it is passed
to the nociceptive second-order neurons in the dorsal horn of the grey matter.
Second-order neurons are divided into two groups, namely nociceptive-specific
(NS) neurons and wide dynamic range (WDR) neurons [4]. Neurotransmitters such
as glutamic acid and SP are released from the nerve terminals and they can activate
DL--amino-3-hydroxy-5-methylisoxazole-4-propionic acid receptor (AMPA) and
N-methyl-D-aspartic acid (NMDA) receptors on the second-order neurons. The pain
goes to the thalamus and then enters the cerebral cortex or cerebral limbic system.
Not all neurotransmitters activate AMPA or NMDA, and some neurotransmitters
such as gamma-aminobutyric acid (GABA) and serotonin suppress pain sensation.
Neurotransmitters can actually control pain transmission in the brain and spinal cord.
13 Role of Nerve Fibres in Endometriosis 193
The sensitisation and activation of nociceptors after inflammation result from the
release of a variety of chemicals by damaged cells and tissues in the vicinity of the
injury. These substances include bradykinin, histamine, prostaglandins (PGs),
serotonin and nerve growth factor (NGF). They sensitise (lower the threshold) or
activate the terminals of the nociceptor by interacting with cell-surface receptors
expressed by these neurons. Primary sensory neurons have been shown to contain
bioactive peptides that can cause local inflammation. These peptides include SP,
CGRP, neuropeptide Y and vasoactive intestinal polypeptide (VIP). Inflammatory
mediators activate the non-selective cation channel transient receptor potential
vanilloid 1 (TRPV1) which leads to an influx of calcium. Tryptase released from
degranulated mast cells cleaves PAR-2 at the plasma membrane of sensory nerve
endings. Increased calcium causes depolarisation of the nerve and activated PAR-2
stimulates the release of bioactive peptides including SP and CGRP from sensory
nerve endings.
SP and CGRP can contribute to the inflammatory response by causing vasodila-
tion, plasma extravasation (leakage of proteins and fluid from postcapillary venules)
and cellular infiltration by interacting with endothelial cells, arterioles, mast cells,
neutrophils and immune cells [5]. SP acts on mast cells in the vicinity of sensory
nerve endings to evoke degranulation and the release of histamine, which further
induces a release of SP and NGF. SP also acts on platelets to release serotonin,
providing a positive feedback [6]. CGRP inhibits SP degradation by a specific
endopeptidase (SPE) [7] and enhances SP release, amplifying the effects [6].
VIP induces vasodilation and histamine release from mast cells. Histamine and
serotonin levels rise in the extracellular space, secondarily sensitising nearby
nociceptors. This leads to a gradual spread of hyperalgesia and/or tenderness.
Research on nerve fibres in the human uterus began about 1680 [8]. Kilian [9] was
one of the first researchers to investigate nerve fibres in the human endometrium [9].
Frankenhauser [10] reported unmyelinated nerve fibres to the smooth muscle of the
myometrium with branches to the stroma and the lining epithelium of the human
endometrium [10]. Patenko [11], Kostlin [12] and Clivio [13] also demonstrated a
fine plexus of unmyelinated nerve fibres in the submucosa from which fine fibrils
extended to the epithelium of the human endometrium. Von Gawronsky [14]
showed large nerve bundles extending parallel to the endometrial-myometrial junc-
tion, with fine branches into the human endometrial stroma [14]. Labhardt [15] and
Mabuchi [16] were unable to demonstrate nerve fibres in the human endometrium;
however, Dahl [17] described numerous fine nonmodulated nerve fibres in the
human endometrium, ending in small treelike branches in the stroma and as straight
194 N. Tokushige
fibres between the cells of the epithelium. Stohr [18] reported nerve fibres in the
mucosa of the human uterus, even fine fibres to the epithelium. Davis [19] did not
find nerve fibres beneath the mucosa of the body of the human uterus. Brown and
Hirsch [20] reported nerve fibres in the basal layer of the endometrium in the
infantile uterus but were unable to demonstrate the mode of termination in those
tissues. These investigators used the silver reduction methods to stain nerve fibres in
the human uterus. There is a discrepancy between these studies and it is considered
that the silver staining method did not clearly differentiate the nerves and reveal the
nerve fibres in the uterus compared with immunohistochemistry.
State and Hirsch [21] used Goldners modification of Massons trichrome stain
to demonstrate nerve fibres in human uteri with no obvious pathologic changes.
Some nerve fibres were present in the lower third of the basal layer of the
endometrium that have branches terminating in the stroma, in the basolar arterioles
and at the origin of the spiral arterioles. No nerve fibres were detected beyond
the basal layer of the endometrium. They also demonstrated some nerve fibres in the
myometrium and at the endometrial-myometrial junction. In this study, the nerve
fibres in the endometrium were found to be unmyelinated. Koppen [22], Stohr [23],
Krantz [24] and Witt [25] reported that branches of nerve fibres accompanying
arteries had been clearly revealed only in the basal layer of the endometrium and
there were no nerve fibres in the outer two-thirds of the endometrium by Goldners
modification of Massons trichrome stain.
Lerner et al. [26] reported abnormal innervation in the myometrium from
women with chronic pelvic pain and dysmenorrhoea. There was a marked prolif-
eration of unmyelinated nerve bundles in the myometrium, but nerve fibres in the
endometrium were not mentioned in this study. Quinn and Kirk [27] investigated
uterine innervation in normal and some clinical conditions such as adenomyosis
and chronic pelvic pain. They performed immunohistostaining using an antibody
against protein gene product (PGP9.5). They demonstrated nerve bundles at the
endometrial-myometrial interface and throughout the myometrium in nulliparous
and parous subjects with no histologic abnormality. There was nerve fibre prolif-
eration throughout the myometrium with small-diameter nerve fibres eccentric
courses throughout the myometrial stoma in some subjects with chronic pelvic pain.
Some researchers have identified types of nerve fibres in the human uterus. SP- and
CGRP-immunoreactive nerve fibres were present in the human myometrium [28].
Heinrich et al. [29] demonstrated neuropeptide (NPY), SP, neurotensin (NT)
and VIP-immunoreactive nerve fibres in the basal layer of the endometrium and
myometrium in nonpregnant women. Lynch et al. [30] and Helm et al. [31] also
detected VIP-immunoreactive nerve fibres in the endometrium and myometrium in
women with no pathologic abnormality.
Nerve fibres in the endometrium in animals have also been investigated by some
researchers. A number of tyrosine hydroxylase (TH), dopamine -hydroxylase
(DH), NPY and VIP-immunoreactive nerve bundles and fibres were present in
equine endometrium [32], and CGRP-immunoreactive nerve fibres were in equine
13 Role of Nerve Fibres in Endometriosis 195
Quinn and Kirk [27] reported that there was widespread nerve fibre proliferation
(small-diameter nerve fibres) in the uterine isthmus suggesting nerve fibre damage
in the uterine isthmus in women complaining of chronic pelvic pain. Few of these
women had endometriosis, but they did report widespread nerve fibre proliferation
in the uterus and cervix in one woman with advanced endometriosis and with
painful periods and intercourse. These nerve fibres were prominently seen around
196 N. Tokushige
arteries and veins throughout the uterine isthmus. Quinn and Armstrong [50]
reported widespread nerve fibre proliferation with extensive perivascular nerve
fibre proliferation around both arteries and veins in the myometrium in an endo-
metriosis patient with dysmenorrhoea and dyspareunia. In another study, increased
numbers of nerve fibres were seen in the myometrium from women with advanced
endometriosis compared with women without endometriosis [51]. These studies
demonstrated the proliferation of nerve fibres; however, types of nerve fibres in the
endometrium and myometrium from women with endometriosis were not investi-
gated in these studies. It has been demonstrated that no nerve fibres were detected in
the functional layer of the endometrium from women without endometriosis;
however, there were several small nerve fibres present in the functional layer of
the endometrium from women with endometriosis (the mean density of nerve
fibres: 13.4 mm2) [52]. There were more nerve fibres in the basal layer of the
endometrium and myometrium from women with endometriosis than women
without endometriosis. Several thick nerve trunks were seen in the basal layer of
the endometrium or at the endometrial-myometrial interface in women with endo-
metriosis, but these nerve fibres were not seen in women without endometriosis.
Many small nerve fibres were also present throughout the basal layer of the
endometrium, but only a few nerve fibres were seen in women without endometri-
osis. Many more nerve fibres and nerve trunks were seen in the myometrium in
women with endometriosis than in women without endometriosis. In women with
endometriosis, nerve fibres in the functional layer of the endometrium were sensory
C fibres; sensory C, sensory A and adrenergic fibres in the basal layer; and
sensory C, sensory A, adrenergic and cholinergic fibres in the myometrium [53].
These results indicate that abnormal innervation in the uterus may be associated
with pain generation in women with endometriosis who suffer from chronic
pelvic pain.
Progestogens and combined oral contraceptives are often used to treat women
with endometriosis-associated pain. Progestogens and combined oral contracep-
tives significantly reduced the nerve fibre density in the functional and the basal
layers of the endometrium and myometrium from women with hormonally treated
endometriosis compared with that from women with untreated endometriosis [54].
Hormonal treatments may reduce pain symptoms by decreasing nerve fibres in
the endometrium and myometrium in women with endometriosis.
Several groups have studied conscious pain mapping since it has been assumed that
endometriotic lesions are the source of localised pain and tenderness, and conscious
pain mapping may help to identify potential areas causing pelvic pain. Palter and
Olive [55] first described conscious pain mapping to identify a focal source of pain
13 Role of Nerve Fibres in Endometriosis 197
Most women with endometriosis present some kind of pain symptoms such as
dysmenorrhoea or dyspareunia. However, a few endometriosis patients do not show
any pain symptoms. When peritoneal endometriotic lesions from women with
endometriosis who did not have any pain symptoms were stained with PGP 9.5,
some nerve fibres were still detected. Therefore, not only the presence of nerve
fibres but also types of nerve fibres or molecules in endometriotic lesions may be
associated with pain generation in women with endometriosis. There may be some
molecules which can desensitise nerve fibres in those who do not experience pain
symptoms. Further studies will be required as to nerve fibres and substances
secreted from endometriotic lesions from endometriosis patients who do not have
any pain symptoms.
cause pain by directly or indirectly sensitising sensory nerve fibres [88]. NGF in
turn activates mast cells and neutrophils which can release additional inflammatory
mediators such as histamine, serotonin and bradykinin to cause hypersensitivity
[89]. NGF has also been reported to promote angiogenesis [90]. NGF induces
proliferation of endothelial cells [91] and of vascular smooth muscle cells [92]
and stimulates the production of vascular endothelial growth factor (VEGF)
[93]. NGF is expressed in vascular endothelial cells [94] and a variety of cell
types such as T and B lymphocytes [95], mast cells [96], eosinophils [97], mono-
cytes/macrophages [98], neutrophils and basophils [99]. Increased angiogenesis in
eutopic endometrium in women with endometriosis demonstrated by several stud-
ies [100, 101] and increased numbers of immune cells may lead to further produc-
tion of NGF, promoting further nerve fibre outgrowth and pain sensation.
It is well established that oestrogen has multiple effects on the female reproductive
system and peripheral nervous system including pain sensitivity and neural regu-
lation of vascular function. Endometriosis is oestrogen dependent for continued
growth and proliferation, and it usually becomes less active with menopause as the
oestrogen level decreases. However, oestrogen replacement therapy can reactivate
the disease. Oophorectomy significantly decreased NGF and BDNF levels while
oestrogen treatment increased these levels [102, 103], and oestrogen also
up-regulated NGF and BDNF expressions in the endometrium [104106]. Several
studies have shown that neuroprotective effects of oestrogen were blocked by ER
antagonists [107109]. Ovariectomy caused a significant decrease in NGF protein
content in the uterus, and short-term treatment of ovariectomised mice with
oestrogen and/or progesterone increased uterine NGF mRNA and restored NGF
protein to concentrations similar to intact control mice [110].
In animals, stronger immunostaining of NGF and TrkA was observed in luminal
epithelial cells and glandular cells in the estrous period and early pregnancy as
compared to the non-breeding period in the uterus of the wild ground squirrels [111].
p75 was immunolocalised only in luminal epithelial and glandular cells during the
estrous period, early pregnancy and non-breeding period. The mean mRNA levels of
NGF and TrkA and p75 were significantly higher in the estrous period and early
pregnancy as compared to the non-breeding period.
Strong immunostaining of NGF and its receptors NTRK1 and TNFRSF1B was
observed in uteri of golden hamsters on the day of proestrus as compared to the
other stages of the estrous cycle [112]. There was a positive correlation between
uterine NGF expression and plasma concentrations of estradiol-17beta, and
estradiol-17beta stimulated expression of NGF and its two receptors in the uterus.
Neutral endopeptidase (NEP) is the enzyme responsible for degradation of SP and
oestrogen treatment of ovariectomised rats resulted in a four-fold decrease in uterine
NEP relative to control ovariectomised rats, resulting in increased SP levels [113].
13 Role of Nerve Fibres in Endometriosis 201
factors, such as IL-8 [152], hepatocyte growth factor (HGF) [153], erythropoietin
[154], angiogenin [155], macrophage migration inhibitory factor [156], neutrophil-
activating factor [157] and TNF- [158], and these proangiogenic factors may also
have neurotrophic effects and be involved in nerve fibre growth in endometriosis.
13.13 Conclusions
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208 N. Tokushige
14.1 Introduction
Mice are the most common animal models capable of investigating the pathophys-
iology of endometriosis; however, they do not spontaneously develop endometri-
osis. To induce endometriosis in mice, endometrial tissue must be transplanted into
the peritoneal cavity using several methods [1821], which can be classified into
two basic types, homologous and heterologous. Both models produce comparable
phenotypes, which are then morphometrically evaluated.
In homologous or autologous models, normal endometrial tissue is transplanted
into the peritoneal cavity of immunocompetent recipients and starts to grow in an
estrogen-dependent manner. In almost all models, uterine endometrial fragments
from a donor mouse are directly introduced via injection into the peritoneal cavity
of an immunocompetent syngeneic recipient without suturing the implants. In
heterologous models, human endometriotic lesions are transplanted into the peri-
toneal cavity of immunodeficient mice [22, 23]. Human endometriotic implants
were sutured to the peritoneum of immunocompromised mice [24, 25]. This xeno-
transplantation model using the nude mouse is also used, but is limited by the lack
of a normal immune system. Despite the advantage of being based on human
endometrial tissues, the number of endometriotic lesions in the heterologous
model that will develop varies from one animal to another. In both models, with
or without suturing the endometrial implant, the drugs influence on growth of
endometrial or endometriotic transplants is evaluated.
These established endometriosis models in mice are under discussion. Indeed,
mice do lack a menstrual cycle and do not develop spontaneous endometriosis. It
should be established whether transplanting normal endometrium into the perito-
neal cavity of a non-menstruating species reflects all pathophysiological aspects of
human endometriosis. Although the murine endometriosis model is not exactly the
same as human endometriosis, their endometriotic lesions develop in some ways
the same as human endometriotic lesions.
The murine model of endometriosis is a versatile one used to study how the
immune system, hormones, and environmental factors affect endometriosis and
how endometriosis affects fertility and pain. A novel study design also enables the
evaluation of molecular mechanisms that are critical for disease initiation [26, 27].
In Table 14.1, the recent representatives of mouse endometriosis models are shown.
Additional and ideal models of endometriosis are needed. In the next section, we
demonstrate the results in a murine endometriosis model that expands the capability
of conducting both mechanistic and translational research.
216 F. Taniguchi and T. Harada
Fig. 14.1 Cystic lesion in the murine endometriosis model. (a) An endometriosis-like lesion
developed in the murine abdominal cavity. (b) Representative of a large excised lesion. (c) and (d)
HE staining of lesion
14.5 Discussion
we and the other investigators provided crucial evidence of both the development of
endometriosis-like lesion growth and donor tissue responsiveness. Recently, Pelch
et al. described a detailed method of a mouse surgically induced endometriosis
model by autotransplantation of uterine tissue [45].
The rodent endometriosis models using mice or rats are widely used in research,
but may have limitations and may not mimic all aspects of human pathophysiology.
For example, in homologous rodent models, healthy uterus is cut into fragments
and transplanted into the peritoneum, whereas it has been suggested that the eutopic
endometrium of women suffering from endometriosis may already be abnormal [2].
Nude mice lacking an intact immune system are employed in the heterologous
model, which cannot mimic the inflammatory response normally seen in human
endometriotic lesions [23]. Although heterologous rodent endometriosis models are
responsive to drugs and manipulations that induce a hypoestrogenic state, such as
ovariectomy, GnRH agonists, aromatase inhibitors, danazol, and selective estrogen
receptor modulators, it may be difficult to analyze novel target families in which,
for example, the murine ligand does not bind to the receptor of the human
transplant.
Whereas cell-based in vitro experiments provide a framework for testing molec-
ular mechanisms, eventually confirming their role in disease causality in vivo can
only be accomplished by a suitable animal model. For a disease as diverse as
endometriosis, a single animal model would unlikely be sufficient to represent the
entire diversity in etiology, pathogenesis, and pathology. Each model has design-
related strengths and limitations. For example, a recently described disease model
consists of introducing endometrial tissue via direct injection into the peritoneal
cavity of immunocompetent mice without suturing [21, 27, 28]. In mice, the
injected tissue forms cyst-like endometriosis lesions; however, the injection method
does not seem to work in rats because the tissue fails to attach to and invade the
peritoneal cavity [9]. Since all endometriosis lesions in each model are attached to
the peritoneum and/or mesenterium with or without suturing, evaluating attachment
or invasion of lesions would be difficult. Furthermore, to quantify the injected
endometrial fragments, this model may be insufficient to evaluate precisely the
endometriotic lesions.
The rodent model is used extensively to study the etiology, pathology, and risk
factors of endometriosis [21, 22, 27, 30, 33, 35, 46, 47] as well as to explore novel
therapeutics [28, 29, 31, 32, 34, 3640, 4851]. In conclusion, this murine model of
endometriosis provides an important tool to evaluate a therapeutic approach to the
disease. This model will help to better understand disease evolution in the living
animal and permit faster and more accurate characterization of a drugs effect on
experimental endometriosis.
220 F. Taniguchi and T. Harada
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Chapter 15
Malignant Transformation of Endometriosis:
Underlying Mechanisms
Abstract Although it is well known that ovarian cancer, especially clear cell and
endometrioid carcinoma, sometimes develops from endometriotic cyst, the precise
mechanism of carcinogenesis is not clarified yet. Recently, several molecules,
including HNF-1, AKT/PI3K/Met, and ARID1A, have been shown to be involved
in this carcinogenic process. Some of them are included in the OCCC signature
genes which we identified as a gene group specifically expressed in clear cell
carcinoma among ovarian cancers. OCCC signature genes contain many stress-
related genes and were induced by treatment with the fluid of endometriotic cysts.
The fluid of endometriotic cysts contained significantly high concentration of free
iron and oxidative stress-related products. These findings suggest that microenvi-
ronment within the endometriotic cyst may play an important role in the malignant
transformation of endometriosis and development of clear cell carcinoma, a rare
histotype among ovarian cancers.
M. Mandai (*)
Department of Obstetrics and Gynecology, Faculty of Medicine, Kinki University,
377-2 Ono-Higashi, Osaka-Sayama, Osaka 589-5811, Japan
e-mail: [email protected]
K. Yamaguchi N. Matsumura I. Konishi
Department of Gynecology and Obstetrics, Graduate School of Medicine,
Kyoto University, Kyoto, Japan
15.1 Introduction
SO/omentectomy
with post-operative
pathology of clear
cell carcinoma
Given the fact that endometriosis is a neoplastic disorder, it may have precancerous
potential. Most endometrioses show a benign character, but malignant transformation
may accompany some morphologic and genetic alterations. In pathology, we some-
times encounter the so-called atypical endometriosis, a putative intermediate between
benign endometriosis and endometriosis-associated ovarian cancer (EAOC).
Sampson first described ovarian cancer in endometriosis and defined a criterion
for EAOC [10]. In a review of 194 cases of ovarian endometriosis, Czernobilsky
and Morris found severe cytological atypia in 3.6 % of the cases [11]. Moreover,
in their study, 2.0 % of the cases showed adenomatous, hyperplasia-like lesions.
LaGrenade and Silverberg presented four cases of ovarian carcinomas contiguous
with atypical glandular epithelial changes in endometriosis [12]. Subsequently,
Fukunaga et al. reported that as many as 61 % of the cases of endometriosis coexisting
with ovarian cancer had atypical endometriosis foci, while only 1.7 % of the cases
of endometriosis without ovarian cancer exhibited atypical lesions [13]. Ogawa
et al. reported that atypical endometriosis was found in 78 % of the cases with
EAOC [14]. In their investigations, the transition from typical to atypical endometri-
osis was detected in 22 of 37 cases, and the transition from atypical endometriosis to
226 M. Mandai et al.
carcinoma was found in 23 cases. These pathological observations suggest that benign
endometriosis develops into ovarian cancer in some cases via atypical endometriosis,
a premalignant stage.
There are several ways of analyzing LOH. LOH is usually used to estimate the
locus of a tumor suppressor gene associated with a corresponding event, the
development and malignant transformation of endometriosis in this case. Using
DNA from 40 cases of endometriosis, Jiang et al. analyzed candidate ovarian tumor
suppressor loci on chromosome arms 6q, 9p, 11q, 17p, l7q, and 22q [17]. LOH was
detected on chromosomes 9p (18 %), 1lq (18 %), and 22q (15 %), and, in total, 11 of
40 (28 %) cases demonstrated LOH at one or more of these loci. The same
investigators subsequently examined 14 cases of endometriosis synchronous with
ovarian cancer for LOH on 12 chromosome arms and for X chromosome inactiva-
tion. In all four of the cases in which the carcinoma had arisen within the endome-
triosis and in five of the seven cases in which the carcinoma was adjacent to the
endometriosis, common genetic lesions were detected to be consistent with a
common lineage [17]. Prowse et al. analyzed LOH in 10 EAOCs with coexisting
endometriosis using 82 microsatellite markers and found that, of 63 LOH events
detected in the carcinoma samples, 22 were also detected in the corresponding
15 Malignant Transformation of Endometriosis: Underlying Mechanisms 227
endometriosis samples [18]. Goumenou et al. reported that LOH in p16, GALT,
and p53, as well as APOA2, a region frequently lost in ovarian cancer, occurred in
endometriosis, even in stage II of the disease [19]. Sato et al. examined 20 ovarian
endometrioid carcinomas, 24 clear cell carcinomas, and 34 solitary endometrial
cysts of the ovary for LOH at 10q23.3 [20]. In five endometrioid carcinomas
synchronous with endometriosis, three cases displayed LOH events common to
both the carcinoma and the endometriosis. In seven clear cell carcinomas that are
synchronous with endometriosis, three displayed LOH events common to both
the carcinoma and the endometriosis. No LOH events were found in solitary
endometriosis. These findings indicate that attenuation of tumor suppressor genes
is associated with the malignant transformation of endometriosis.
Mutations and altered expression of several genes have been implicated in the
malignant transformation of endometriosis.
According to Yamamoto et al., exons 9 and 20 of the PIK3CA gene were analyzed
in 23 clear cell carcinomas with synchronous putative precursor lesions [23].
Somatic mutations of the PIK3CA gene were detected in 10/23 (43 %) carcinomas
and in the coexisting endometriotic epithelium adjacent to the carcinoma in 9/10
(90 %) cases. Moreover, in six of the nine lesions, the mutation was identified even in
the endometrioses lacking cytological atypia. The authors suggested that mutations
of the PIK3CA gene are early events in tumorigenesis, most likely initiating the
malignant transformation of endometriosis.
In our bodies, live cells are continuously exposed to oxidative stresses, which
are produced internally or externally. Internal stress consists of mitochondrial
respiratory stress, cytochrome P450 metabolism, and inflammatory responses.
External stresses are generated by various agents, including chemicals, xenobiotics,
irradiation, and metal ions, including Fe ions. One of the well-known mechanisms
15 Malignant Transformation of Endometriosis: Underlying Mechanisms 229
120 80
100
60
80
60 40
40
20
20
0 0
endometriotic other epithelial endometriotic other epithelial
cyst cyst cyst cyst
Fig. 15.2 Differences in Fe concentration/oxidative stress between endometriotic cysts and other
benign epithelial cysts
by which metal ions produce intracellular ROS is called the Fenton reaction [29].
During this reaction, highly toxic dOH and anoxidized metal ions are generated
from H2O2. Metal-induced ROS causes DNA damage, including single- or double-
strand breaks, base modifications, deoxyribose modifications, and DNA cross-
linking, which ultimately contributes to carcinogenesis.
In normal conditions, ROS overproduction is avoided by endogenous antioxi-
dants, including superoxide dismutase (SOD), catalase (CAT), and glutathione
peroxidase (GPx). If the balance between the cellular antioxidant defense and
ROS generation is impaired, excessive ROS can cause oxidative stress. Prolonged
and excessive oxidative stress mediates a variety of chronic and degenerative
diseases, including cancers, inflammation, aging, and neuronal disorders [29].
The content of endometriotic cysts consists of old blood containing a high concen-
tration of iron derived from hemoglobin. We compared the concentrations of free
iron in endometriotic cysts with those in other ovarian cysts, including serous and
mucinous cystadenoma, and found that the concentrations were significantly higher
in endometriotic cysts [30] (Fig. 15.2). Likewise, lactose dehydrogenase (LDH)
(a marker of tissue damage), potential antioxidant (PAI) (an antioxidant marker),
lipid peroxidase (LPO) (Fig. 15.2) (a marker of oxidative stress), and 8-hydroxy-2-
deoxyguanosine (a marker of DNA damage) were all significantly elevated in
endometriotic cysts compared with other ovarian cysts. These data strongly suggest
that the epithelial cells of the endometriotic cyst are constantly exposed to exces-
sive oxidative stress and are subjected to cellular and DNA damage (Fig. 15.3).
To elucidate the mutagenic property of the fluid in chocolate cysts, we
conducted an experiment in vitro, which demonstrated that the fluid in chocolate
230 M. Mandai et al.
DNA injury/mutation
Oxidative stress
Old blood
containing Fe
cysts is more mutagenic than that in other cysts [30]. There are several reports
suggesting a link between a stressful microenvironment and cancer development.
(1) Chromosomal aberrations are more frequent in ovarian endometriotic cysts than
in extra-gonadal endometriosis [31]. (2) Malignant transformation of endometriotic
cysts increases with the duration of endometriosis [32].
genetic alteration
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chromatin remodeling, is a tumor suppressor in gynecologic cancers. Cancer Res. 2011;71
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27. Katagiri A, Nakayama K, Rahman MT, Rahman M, Katagiri H, Nakayama N, Ishikawa M,
Ishibashi T, Iida K, Kobayashi H, Otsuki Y, Nakayama S, Miyazaki K. Loss of ARID1A
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28. Yamamoto S, Tsuda H, Takano M, Tamai S, Matsubara O. PIK3CA mutations and loss of
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29. Lee JC, Son YO, Pratheeshkumar P, Shi X. Oxidative stress and metal carcinogenesis.
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30. Yamaguchi K, Mandai M, Toyokuni S, Hamanishi J, Higuchi T, Takakura K, Fujii S. Contents
of endometriotic cysts, especially the high concentration of free iron, are a possible cause of
carcinogenesis in the cysts through the iron-induced persistent oxidative stress. Clin Cancer
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molecular biology, pathology, and clinical management. Int J Clin Oncol. 2009;14(5):38391.
36. Mandai M, Matsumura N, Baba T, Yamaguchi K, Hamanishi J, Konishi I. Ovarian clear cell
carcinoma as a stress-responsive cancer: influence of the microenvironment on the carcino-
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Hamanishi J, Kang HS, Matsui S, Mori S, Murphy SK, Konishi I. Sorafenib efficacy in ovarian
clear cell carcinoma revealed by transcriptome profiling. Cancer Sci. 2010;101(12):265863.
Chapter 16
Potential New Drugs for Endometriosis:
Experimental Evidence
16.1 Introduction
Apoptosis plays a critical role in maintaining tissue homeostasis, and its function is
to eliminate excess cells and dysfunctional cells. Apoptosis can be initiated by
extracellular or intracellular death signals, and it results from a series of related
morphologic and biochemical processes. Morphologically, apoptotic cells present
with condensed chromatin, multiple membrane-bound organelles (apoptotic bod-
ies), and shrunken appearance. Biochemically, apoptosis is characterized by mono-
meric or multimeric 180-base pair nucleosomal fragments resulting from the
cleavage of double-stranded nuclear DNA [5]. Apoptosis is controlled by the
expression of a number of regulatory genes, including c-myc, p53, Fas, NF-B,
and members of the B-cell lymphoma/leukemia (Bcl)-2 family [611].
16 Potential New Drugs for Endometriosis: Experimental Evidence 237
Estradiol
TNF- Lipopolysaccharide
Receptors
NF-
MAPKK NIK Akt NF-B
inhibitors
IKK
Phosphorylated
NF-B
inhibitors
NF-
Autologous activation ECM
stimulation remodeling
Cytokine Proliferation
production
Apoptosis
Progression of endometriosis
led Anaf et al. [50] to suggest that endometriotic stromal cells can differentiate to
-SMA-positive myofibroblasts.
To establish a model of fibrosis formation in endometriosis, we used a 3D
collagen culture system with human endometriotic stromal cells [51, 52]. We
cultured the cells in floating collagen lattices to reorganize the collagen fibers and
make them compact, resulting in contraction of the collagen gels. This culture
system provided a model for mechanically relaxed tissue with low tensile strength,
comparable to the early stages of an endometriotic lesion. We found that
endometriotic stromal cells cultured in floating 3D gels have an enhanced contrac-
tile profile compared to normal endometrial stromal cells [51]. This suggested that
endometriotic stromal cells may acquire fibrogenetic ability or fail to avoid
fibrogenesis during the pathogenesis of endometriosis.
Members of the Rho family of small guanosine triphosphatase (GTPase) are
known to regulate cell shape, motility, cell-substratum adhesion, and cell contrac-
tion through the reorganization of actin cytoskeletons [5365]. The active form of
Rho is GTP-bound [54, 62], and many polypeptides have been reported as targets of
activated Rho, including ROCK-I/p160ROCK and Rho-kinase/ROCK-II [66].
ROCKs phosphorylate the myosin light chain (MLC) [67] and the myosin-binding
subunit of myosin phosphatase [68], and they inhibit myosin II regulatory light
chain phosphatase activity [68] in cultured fibroblasts. Rho and ROCKs have been
implicated in myosin II-dependent force generation [69]. Thus, the activation of
ROCKs by Rho can promote the assembly of focal adhesions, actin stress fiber
formation, and contraction of non-muscle cells [62, 68], in which RhoA regulates
-SMA expression [70].
Based on these observations in fibroblasts, we have investigated the signaling
pathway underlying endometriotic stromal cell-mediated contractility by using 3D
cultures. Our data indicated that human endometriotic stromal cells undergo
myofibroblastic differentiation and show increased expression of RhoA, ROCK-I,
and ROCK-II proteins, resulting in enhanced contractility [51]. Thus, we evaluated
several inhibitors of mevalonate-Rho/ROCK pathways as candidate drugs for the
treatment and prevention of endometriosis-associated fibrosis [51, 52, 7173].
16.2.3 Statins
Statins are potent inhibitors of cholesterol biosynthesis that are widely used to
reduce serum cholesterol levels in hyperlipidemic patients [74, 75]. Statins are
divided into three categories: natural statins (i.e., lovastatin and pravastatin),
semisynthetic statins (i.e., simvastatin), and synthetic statins (i.e., atorvastatin,
fluvastatin, and cerivastatin) [75, 76]. These three subtypes of statin exhibit mark-
edly different hydrophobicities, with simvastatin as the most hydrophobic and
pravastatin as the most hydrophilic.
Statins competitively inhibit 3-hydroxy-3-methylglutarylcoenzyme A
(HMG-CoA) reductase to block the conversion of HMG-CoA to L-mevalonate, a
240 K. Nasu et al.
rate-limiting step in cholesterol synthesis [77]. By inhibiting the initial step of the
cholesterol synthesis pathway, statins reduce the synthesis of several important
lipid intermediate compounds including isoprenoids such as farnesyl pyrophos-
phate (FPP), a precursor of cholesterol, and geranylgeranyl pyrophosphate (GGPP),
which is synthesized from FPP [78]. Both FPP and GGPP are important isoprenoid
intermediates and serve as lipid attachments for a variety of intercellular proteins to
the plasma membrane, including Rho proteins, resulting in their activation [59, 79].
By inhibiting the activation of Rho proteins, statins also regulate both the
Rho/ROCK pathways and the mevalonate pathway [80, 81].
Simvastatin has been demonstrated to inhibit the proliferation of endometriotic
stromal cells as well as the collagen gel contraction mediated by these cells [71].
Attenuation of the endometriotic stromal cell attachment to collagen fibers is
involved in this mechanism. Lovastatin also inhibited cell proliferation and angio-
genesis in endometriosis [82], whereas simvastatin and mevastatin inhibited the
MCP-1 production by endometriotic cells [83]. Atorvastatin also exhibited
antiproliferative and anti-inflammatory effects in endometriotic cells [84]. Oktem
et al. [85] demonstrated that atorvastatin induced the regression of endometriotic
implants in a rat model. Similarly, Bruner-Tran et al. [86] demonstrated that
simvastatin induced the regression of endometriotic implants in a nude mouse
model.
16.2.5 Heparin
16.2.6 HDACIs
VPA was used in a pilot study of three patients with endometriosis and
adenomyosis who had moderate to severe dysmenorrhea [125]. A VPA dose of
1,000 mg/day was used for 3 months. Complete relief of pain in all cases and an
average reduction of one-third in uterine size were reported. The disappearance or
reduction of palpable tender nodules in the cul-de-sac was also reported.
16.3 Conclusions
Acknowledgments This work was supported in part by a Grant-in-Aid for Scientific Research
from the Japan Society for the Promotion of Science (no. 13237327 to K. Nasu, no. 25861500 to
Y. Kawano, and no. 23592407 to H. Narahara).
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Chapter 17
Altered Biological Characteristics of Eutopic
and Ectopic Endometrium
C.G.T. Silveira
Department of Gynecology and Obstetrics, University of Lubeck, Lubeck, Germany
A. Agic
Department of Gynecology and Obstetrics, Diakonissenkrankenhaus Karlsruhe Ruppurr,
Diakonissenstr. 28, 76199 Karlsruhe, Germany
G.O. Canny
Geneva Foundation for Medical Education and Research, Versoix, Switzerland
D. Hornung (*)
Department of Gynecology and Obstetrics, University of Lubeck, Lubeck, Germany
Department of Gynecology and Obstetrics, Diakonissenkrankenhaus Karlsruhe Ruppurr,
Diakonissenstr. 28, 76199 Karlsruhe, Germany
e-mail: [email protected]
17.1 Introduction
transforming growth factor (TGF), epidermal growth factor (EGF) and EGF
receptors, as well as insulin-like growth factor-1 (IGF-1) in response to estrogen
were shown and associated with endometrial cell proliferation and decidualization.
Interestingly, these growth factors are also believed to modulate the effects of
estrogen or progesterone or each other by altering growth factor receptor or binding
protein expression [1214].
Indeed, the architecture and function of the endometrium are maintained by the
dynamic relationship between epithelial and stromal cells and the complex micro-
environment that includes the extracellular matrix (ECM), diffusible growth fac-
tors, cytokines, and other paracrine messengers, as well as a variety of other cell
types such as endothelial cells, lymphocytes, and macrophages [15, 16]. Thus, it has
become evident that the abnormal interactions between these cellular components
and their microenvironments may disrupt tissue homeostasis and precede the
development of several endometrial pathologies, including endometriosis. So far,
numerous studies have pointed out that the onset and progression of endometriosis
are potentially supported by the interruption of this well-balanced cellular
equilibrium [15, 1721] potentially resulting from genetic [22] and epigenetic
changes [23].
Similar to intrauterine endometrium, ectopic endometrial tissue consists of
endometrial-like epithelial and stromal cells although cases of only stromal endo-
metriosis have also been reported [24]. In ectopic loci, such as the peritoneum and
ovary, both endometriotic epithelial and stromal cells are functional and respond
actively to steroid hormones during the menstrual cycle. On the other hand,
endometriotic tissue displays a distinct production of cytokines and prostaglandins,
diverse estrogen biosynthesis and metabolic pathways, as well as an altered
response to progesterone, e.g., progesterone resistance [25], that seem to favor
ectopic endometrial growth and maintenance.
In addition to altered steroid content and metabolism, ectopic endometrium also
retains other peculiar characteristics that contribute to disease development.
Although peritoneal, ovarian, and rectovaginal endometriotic lesions are consid-
ered distinct entities with a different pathogenesis [2628], a general consensus
exists regarding the critical role of the cross talk between endometriotic cells, host
peritoneum and infiltrating leukocytes, endothelial cells, and fibroblasts. This all
appears to support the development of the disease [16].
implants originate from uterine endometrium and those proposing that implants
arise from tissues or cells other than the uterus. Intrinsic to these theories are
inciting factors (i.e., immune, endocrine, and environmental factors) and genetic
susceptibilities whose roles are beginning to be delineated, although they are still
insufficient to fully explain the cause and development of disease. For instance,
acquired genomic alterations and several physiological changes were shown to
represent a potential source for a conferred proliferation and survival advantage to
endometriotic implants [29].
In this context, the potential involvement of eutopic endometrium seems to be
particularly critical in the pathogenesis of endometriosis, evinced by Sampsons
retrograde menstruation theory in 1921 [30], the most widely accepted hypothesis,
which nonetheless does not fully explain the etiology. In accordance with this
theory, it is presumed that the establishment of endometrial cells from refluxed
menses in ectopic sites is supported by the following characteristics: (a) the endo-
metrial debris, including both epithelial and stromal cells, must exist in the reflux
menses; (b) these two cellular components must be viable and able to evade
immune attack within the pelvic cavity; (c) both epithelial and stromal cells must
have the potential ability to attach and implant into the pelvic mesothelium; and
(d) ultimately, once implanted at an ectopic location, endometriotic cells must be
able to survive and develop a neovascular system [31]. Indeed, the link between
altered eutopic endometrium and the risk for developing endometriosis may possi-
bly justify the morbidity of the disease in only 1015 % of the women with
menstrual reflux [32, 33] and at least partially explain the high rate of recurrence
after medical and/or surgical treatment [34].
In fact, important functional and biochemical differences between eutopic endo-
metrium of women with and without endometriosis have been reported in the
literature [35, 36]. In particular, a large number of differentially expressed gene
transcripts, miRNAs, and proteins have been detected and they appear to mostly
encode molecular signals mediating cross talk between epithelial and stromal cells,
cell proliferation, differentiation and survival, as well as endometrial receptivity
[3743]. For instance, aberrant production of cytokines, growth and angiogenic
factors, different steroid receptor expression and signaling, and abnormal expres-
sion of specific cancer-related genes presented in eutopic endometrial cells are
thought to predispose to growth and survival of endometrial foci outside the uterus
and to produce disease-related symptoms such as reduced fertility and implantation
failures.
The role of the eutopic endometrium as a major and active contributor for the
development of endometriotic lesions has also been supported by the accumulat-
ing evidence implying the involvement of stem cells. Stem cells are rare undiffer-
entiated cells characterized by high proliferative, self-renewal, and differentiation
potential that are present in virtually all adult tissues and organs [44]. The
presence of aberrant stem cells has been associated with the pathogenesis of
several tumors and proliferative disorders in female reproductive organs [45].
As thoroughly addressed in Chap. 4, endometrium-derived stem/progenitor cells
residing in the basalis and/or functionalis have been suggested to reach the
17 Altered Biological Characteristics of Eutopic and Ectopic Endometrium 255
of the menstrual cycle that were not fully considered in most studies despite their
well-known influences on gene expression in eutopic and ectopic tissues [7375].
In spite of these limitations, significant and interesting findings have been
provided by microarray-based analyses of eutopic and ectopic endometrium
which have been confirmed by subsequent investigations using other conventional
and sophisticated methodologies. Collectively, these published data highlight dif-
ferences in the expression of gene-encoding proteins involved in multiple biolog-
ical process and hypothesized to be responsible for the establishment of ectopic
endometrial implants, including cell adhesion, extracellular matrix remodeling,
migration, proliferation, apoptosis, immune system regulation, inflammatory
pathways, sex hormone-related signaling and neuroangiogenesis [16, 6468, 75]
that will be thoroughly addressed in the following sections.
Also noteworthy are the observations on the differential expression pattern of
microRNAs (miRNAs) in ectopic versus eutopic endometrium [76, 77]. miRNAs
are small noncoding RNA molecules that have a critical role in posttranscriptional
regulation of gene expression by repression of target mRNA translation. A rela-
tively recent microarray-based investigation in paired eutopic and ectopic endome-
tria has identified more than 80 differentially expressed miRNAs. Interestingly,
most of them are predicted to regulate a large fraction of protein-coding genes
associated with genetic (i.e., cancer) and immunological disorders and involved in
cellular growth and proliferation, apoptosis, cellular movement, cell-mediated
immune response, cell-to-cell signaling and interaction, as well as gene expression
regulation [78].
Evidence for molecular abnormalities in eutopic and ectopic endometria has also
been revealed through proteomic approaches. In particular, large-scale proteomic
studies including mass spectrometry and protein microarray-based technologies
have enabled the simultaneous evaluation of several hundred proteins in eutopic
and ectopic endometrium as well as biological fluids and provided valuable infor-
mation regarding their expression pattern, functions, localization, posttranslational
modifications, and interactions [79]. Investigations focusing on the comparative
proteomic analysis of paired eutopic and ectopic endometrial tissues are still limited
although they are currently gaining more attention. For instance, a recent study
combining two-dimensional electrophoresis and mass spectrometry demonstrated a
remarkable difference in the protein repertoire of endometriotic lesions compared
with its uterine counterpart [80]. Interestingly, significant differences comprised
proteins primarily involved in cellular spreading and attachment, cell homeostasis
and survival, mRNA processing and transport, immune response, and protein
trafficking [80].
In addition to differences between eutopic and ectopic endometrium, increasing
evidence in the literature has also suggested that the biological characteristics of
endometriotic cells might differ between different forms of endometriosis [28, 81].
These findings may possibly account for the high heterogeneity observed in endo-
metriosis pathogenesis and disease-related symptoms and imply that a single
universal treatment is perhaps not effective for all forms of endometriosis.
258 C.G.T. Silveira et al.
Accumulating evidence suggests that endometrial cells from women with and
without endometriosis exhibit fundamental differences in their apoptotic capacity.
Endometrial cells from women with endometriosis have enhanced proliferation and
an increased ability to implant and survive in ectopic locations. Impaired sensitivity
of endometrial tissue to spontaneous apoptosis contributes to the abnormal implan-
tation and growth of endometrium at ectopic sites.
The inability of endometrial cells to transmit a death signal or their ability to
avoid cell death is associated with increased expression of anti-apoptotic factors
(Bcl-2) and decreased expression of pre-apoptotic factors (BAX) [89]. However, it
remains unclear whether abnormal apoptosis in the eutopic endometrium from
patients with endometriosis is a primary or a secondary process after establishment
of the pelvic endometriosis process. This could be attributed to the fact that at the
time of clinical presentation and diagnosis, most women already have established
disease and, therefore, it is difficult to investigate the early developmental stages of
endometriosis.
Reflux of endometrial fragments during menstruation into the peritoneal cavity
is a common phenomenon. Under normal conditions, cells which do not adhere to
17 Altered Biological Characteristics of Eutopic and Ectopic Endometrium 259
their extracellular matrix enter apoptosis as they receive different signals from their
adhesion receptors [90]. However, in women with endometriosis, these cells have
the ability to adhere to mesothelial cells of the peritoneum, proliferate, and induce
neoangiogenesis resulting in the development of active endometriotic implants. The
effect of MMPs on apoptotic factors and their regulation by steroid hormones may
provide a link between endometrial turnover and the invasive process necessary for
the development of disease.
Recent studies from Gonzalez-Ramos et al. [91, 92] showed constitutive NF-B
activation in peritoneal endometriosis. They reported that the NF-B pathway is
implicated in the development of endometriotic lesions in vivo and that NF-B
inhibition reduces intracellular adhesion molecule-1 expression and cell prolifera-
tion, but increases apoptosis of endometriotic lesions, diminishing the initial devel-
opment of endometriosis in an animal model. This and other observations support
the notion that endometriosis is characterized by persistent inflammation and
proliferation.
Murk et al. [93] described extracellular signal-regulated kinase (ERK1/2) activ-
ity in human endometrium. ERK1/2 plays key intracellular roles in activating
cellular survival and differentiation processes. The authors found that ERK1/2-
mediated steroid inhibition in endometrial stromal cells reduced proliferation and
increased apoptosis. They suggested that abnormally high levels of ERK1/2 activity
may be involved in endometriosis, possibly by stimulating endometrial cell
survival.
Some studies have suggested that genetic factors are likely to influence
individual susceptibility to endometriosis. Genetic alterations in somatic chromo-
somes [94] and DNA deletions that inactivate some tumor suppressor genes
(e.g. PTEN) are likely to be involved in the initiation, persistence, and progression
of endometriosis [95, 96].
cDNA microarray analysis provided an interesting insight into altered gene
expression profiles in endometriosis patients. Using this method, Arimoto
et al. [37] found 97 upregulated and 337 downregulated genes in women with
endometriosis. Genes related to apoptosis (GADD34, GADD45A, GADD45B,
PIG11) and the tumor suppressor TP53 gene were downregulated in endometriotic
tissues. On the other hand, Eyster et al. [66] found that only a few genes in apoptosis
resistance pathways were differentially expressed in endometriosis cells compared
to normal endometrial cells. They suggested that the presence of ligands to activate
the apoptotic pathway or the apoptosis resistance pathways may be more important
than whether specific members of the pathway are over- or underexpressed.
Braun et al. [97] demonstrated that the transcript abundance ratio of anti-
apoptotic to pro-apoptotic isoforms of the Bcl-X gene favors survival in eutopic
and ectopic endometrial cells from women with endometriosis, but not control
endometrial cells. This was found throughout the menstrual cycle for ectopic
endometrial cells. Eutopic but not ectopic endometrial cells also expressed
increased transcript abundance of the anti-apoptotic DAD-1 gene in endometriosis.
Eutopic and ectopic endometrial cells from women with endometriosis expressed
decreased transcript abundance of p53 and caspase-1 compared to endometrial cells
260 C.G.T. Silveira et al.
Both circumstantial and laboratory evidence strongly supports the notion that
estrogen is an extremely strong mitogen for endometriotic tissue. The biologically
active estrogen 17 beta estradiol (E2), which is secreted by the ovary or locally
produced by in endometriotic tissue, acts as a classical steroid hormone to regulate
growth of endometrial or endometriotic tissue. E2 enters cells and binds to the ER
in estrogen-responsive cells. ER subtypes and are proteins with high affinity for
E2 and are encoded by separate genes. The classical human ER was cloned in
1986, and a second estrogen receptor, ER, was cloned from rat prostate and human
testis in 1996 [130132]. Although both ER and ER are present in the endome-
trium, ER seems to be the primary mediator of estrogenic action in this tissue
[133]. Studies using ER-deficient mice have revealed the central role of this
receptor in reproductive function, at all levels of the hypothalamicpituitary
gonadal axis [134]. Despite its sensitivity to estrogen, endometriosis appears to
have an altered steroid hormone receptor profile compared with that of its normal
tissue counterpart, the eutopic endometrium. For example, several investigators
reported markedly higher levels of ER and lower levels of ER in human
17 Altered Biological Characteristics of Eutopic and Ectopic Endometrium 263
endometriotic tissues and primary stromal cells compared with eutopic endometrial
tissues and cells [56, 135, 136]. Moreover, the levels of both isoforms of PR,
particularly PR-B, are significantly lower in endometriosis compared with eutopic
endometrium [137, 138].
The E2-receptor complex acts as a transcription factor that becomes associated
with the promoters of E2-responsive genes via direct DNA binding or binding to
other docking transcription factors at basal promoter regions [139]. This interaction
brings about ER-specific initiation of gene transcription, which promotes the
synthesis of specific mRNAs and proteins [139]. PR is one of many
E2-responsive genes, and E2 acts in eutopic endometrial tissues and stromal cells
to promote endometrial responsiveness to progesterone [140]. In contrast, PR
mRNA and protein levels are not elevated in biopsied endometriotic tissues
exposed to high E2 levels during late proliferative phase or in endometriotic cells
treated with E2, indicating that E2 induction of PR expression in endometriosis is
markedly blunted [138].
The immune status has been suggested to play an important role in both initiation and
progression of endometriosis. T and B lymphocytes and natural killer cells seem to
play essential roles in determining if endometrial and endometriotic cells accept or
reject survival, implantation, and proliferation [156, 157]. Several studies have shown
a reduced activity of cytotoxic T cells and NK cells, cytokine secretion by helper T
cells, and autoantibody production by B lymphocytes in women with endometriosis
[156158]. As alluded to in a previous section, NF-B transcriptional activity modu-
lates inflammatory key cell processes contributing to the initiation and progression of
endometriosis [159]. It has further been shown that immuneendocrine interactions are
likely to be involved in the pathogenesis of endometriosis.
Endometriosis is associated with an increased inflammatory activity, as seen
by elevated serum levels of inflammatory markers such as CA-125 [160] and
C-reactive protein [161]. Changes in peritoneal fluid inflammatory markers of
peritoneal fluid have also been observed in women with endometriosis [162]. The
generalized inflammatory activity may lead to more generalized clinical effects
where some women with endometriosis suffer from fever and a general feeling of
sickness, especially AT times when they experience more pain.
17 Altered Biological Characteristics of Eutopic and Ectopic Endometrium 265
Recent evidence indicates that ectopic endometriotic implants recruit their own
unique neural and vascular supplies through neuroangiogenesis. It is believed that
these nascent nerve fibers in endometriotic implants influence dorsal root neurons
within the central nervous system, increasing pain perception in patients [163].
Several studies have suggested that endometrial biopsies with the detection of
nerve fibers provide a reliability of diagnosing endometriosis [164, 165]. Newer
studies however were not able to demonstrate any differences in the amount of
nerve fibers or neuronal markers in endometrium of women with endometriosis
compared to women without endometriosis. The neuronal markers, PGP9.5,
NGFp75, and VR1, are expressed in the endometrium at levels that do not differ
between women with and without endometriosis [166].
Endometrial functional layer nerve fibers were identified in 22 % of biopsies
overall including 19 % of cases with histologically confirmed peritoneal endome-
triosis and 29 % of cases without endometriosis. There was no correlation between
the presence of functional layer nerve fibers and the presenting symptoms, endo-
metrial histology, or current hormonal therapy. Endometrial functional layer nerve
fibers assessment performed using standard immunohistochemical techniques on
routine biopsy specimens proved neither sensitive nor specific for the diagnosis of
endometriosis [167]. In conclusion, much rigorous research to better understanding
this complex pathology and to find specific and sensitive biomarkers remains
to be done.
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Although science has not yet addressed directly, there are extensive scientific and
clinical resources applicable to the prevention of endometriosis, especially when
regarded as the systemic inflammatory, autoimmune and endocrine disease. Fur-
ther, dioxin and endocrine-disrupting environmental toxicants that modify the
inflammatory process have been strongly associated with endometriosis [1].
Endometriosis shares pathophysiological characteristics such as immune
response alterations, increased inflammation, elevated levels of tissue-remodeling
components, altered apoptosis, increased local and/or systemic levels of cytokines.
Growth factors including fibroblast growth factor (FGF), vascular endothelial
growth factor (VEGF), platelet-derived growth factor (PDGF), epidermal growth
factor (EGF), transforming growth factor-h (IGF-h) and granulocyte/macrophage-
colony-stimulating factor (GM-CSF) and inflammatory mediators like IL-1, TNF-a,
IL-2, IL-6, IL-8, IL-10, IL-11, MCP-1, and interferon-g (IFN-g) produced by
peritoneal leukocytes are all elevated in the peritoneal fluid of women with
endometriosis.
There is an association between the presence of endometriosis and common
autoimmune and atopic diseases, such as systemic lupus erythematosus, Sjogrens
syndrome, rheumatoid arthritis, Crohns disease, psoriasis. chronic fatigue immune
dysfunction syndrome, multiple sclerosis, hypothyroidism and fibromyalgia.
Research has suggested that endometriosis may increase the risk of ovarian and
breast cancer, non Hodgkins lymphoma, melanoma, thyroid, kidney and brain
tumors. There are also concerns about the risk for birth defects in the children of
women with endometriosis. Therefore, prevention of the disease processes involv-
ing endometriosis may also reduce the risk for these other health problems and their
sequelae [13].
To be able to prevent or delay the development of endometriosis and hopefully
other associated comorbidities, known risk factors for endometriosis should be
defined at the first place. The plethora of risk factors for endometriosis may reflect
varying methodologies such as study populations, definitions utilized for risk
factors, and diagnostic accuracy. Infertility by itself is a significant risk factor for
endometriosis. An infertility history increases the odds of an endometriosis diag-
nosis in both the operative (OR, 2.43; 95 % CI, 1.573.76) and population (OR,
7.91; 95 % CI, 1.6937.2) cohorts [4]. Increasing age, alcohol use, early menarche,
family history of endometriosis, infertility, intercourse during menses, low body
weight, prolonged menstrual flow, and short cycle interval are known risk factors
[58]. Endometriosis has been negatively associated with exercise and smoking
[9]. Recently, red hair [10], blue or green eyes, and freckles have been reported to
increase the odds of diagnosis [11]. It is possible that there may not be a classic set
of risk factors generic to all women with endometriosis. Rather, risk factors may
need tailoring to the subgroups of women by their behavioral and clinical
characteristics.
18 Prevention of Endometriosis 279
First degree relatives of a woman with endometriosis carry 410 times higher
risk of also having endometriosis when compared to the general population.
Candidate genes such as ESR1, COMT, IL6, IL10, CYP17A1, CYP19A1,
CYP1A1, MMP1, and MMP9 studied in genomic DNA showed no association
with endometriosis [12].
In more than 1,000 families with two or more members with surgically documented
endometriosis from Australia and the UK, significant linkage to 10q26 and 20p13
was demonstrated. However, no causative gene was identified [13]. It is likely that
endometriosis is a common polygenic/multifactorial disease caused by an interaction
between genes as well as the environment [14, 15].
Early age at menarche (11 years old) might increase a womans exposure to
menstruation during her reproductive lifetime and consequently increase the risk of
endometriosis. The data, however, do not present strong evidence for the clinical
utility of a history of early menarche in the evaluation of endometriosis [16]. The
lowest risk was seen in those whose age at menarche was 15 years [17].
Increased exposure to menstruation in terms of short cycle length, long duration
of flow, and low parity have frequently been identified as possible risk factors. The
use of tampons does not seem to confer a risk for endometriosis.
Dysmenorrhea is likely to be a precursor to disease development, and shorter
cycles may possibly suggest increased risk [18, 19].
In contrast to past studies, data of a recent study found no relationship between
endometriosis and menstrual cycle history, including age at menarche, average
cycle length, and number of menstrual cycles in the past 12 months. However,
>80 % of the women in all groups in this study had a history of oral contraceptive
use. This contraceptive use may have altered both recent menstrual cycle patterns or
possibly the presence or absence of endometriosis [4].
Therefore, the potential role of menstrual cycle characteristics in the actual
development of endometriosis remains an open question. At best they may be
used to guide diagnostic and therapeutic strategies if other symptoms point to
endometriosis as a possible diagnosis.
Several studies have found that a lower body mass index (BMI) during adolescence
and early adulthood is a risk factor for endometriosis. Taller women tend to have
higher follicular-phase estradiol levels and thus may have an increased risk
280 E.H. Biberoglu and K.O. Biberoglu
with migraine. The subgroup of migraineurs with endometriosis is more likely to have
other comorbid conditions affecting mood and pain [56]. Angiogenic cytokines are
hypothesized to play a critical role in the pathogenesis of endometriosis and migraine,
possibly by stimulating matrix metalloproteinases (MMPs) [62]. There may also be a
neuro-immuno-endocrine link between endometriosis and migraine, fibromyalgia,
irritable bowel syndrome, chronic fatigue syndrome, interstitial cystitis (painful
bladder), and mood disorder through increased mast cell activation [63]. Mast cell
activation without allergic degranulation has been documented to occur in response to
stress and lead to painful sterile inflammatory states [64]. An increased prevalence of
hypothyroidism, fibromyalgia and chronic fatigue syndrome, and autoimmune inflam-
matory diseases in women with endometriosis compared with the general female
population was previously reported. The coexistence of all these conditions suggests
an underlying role for the immune system in fibromyalgia and chronic fatigue
syndrome [50].
18.1.10 Contraception
18.2.1 Vaccines
18.2.6 Simvastatin
Statins reduce the rate of endometrial stromal growth and angiogenesis, interfere
with the development and attachment of endometriotic implants, and also protect
the subject from the development of endometriosis by virtue of their anti-
inflammatory and antioxidant properties [145]. Considering its safety and minimal
side effects, use of statins in treatment of endometriosis holds promise [146].
18.2.7 Pentoxifylline
limited the increased migration of ectopic MSC. Targeting the stem cell population
may be relevant in achieving the complete eradication of endometriotic
implants [151].
Puerarin, the main isoflavone glycoside derived from the Chinese medicinal herb
Radix puerariae, exhibits antiestrogenic activity by suppressing P450arom and
interferes with the invasion of endometrial stromal cells (ESC) and angiogenesis
of ectopic tissues, in a model of endometriosis. This might be a good option for
avoiding the relapse of endometriosis after the initial surgical and/or medical
therapy, since it can be used for long periods without severe side effects, unlike
the classical antiestrogenic medical treatment modalities [167].
According to several clinical studies in the medical literature, treatment with
Chinese herbal medicine (CHM) involving formulae of between 10 and 20 separate
herbal ingredients selected from a materia medica of several hundred commonly
herbs that are administered as pills, enemas, and intramuscular injections prevents
the recurrence of endometriosis after a conservative operation with fewer adverse
18 Prevention of Endometriosis 293
18.3.2 Diet
Over the past decade, many studies have provided evidence that higher intakes of
fruit and vegetables, rich in antioxidants, among other micronutrients, improve the
function of the immune system and fight free radical damage [173]. Manipulation
of dietary polyunsaturated fatty acid (PUFA) composition demonstrably affects the
proinflammatory activities of many cell types involved in the immune response,
inflammatory reactions, and cytokine network and on the synthesis and biological
activity of prostaglandins and cytokines such as IL-1, IL-2, IL-6, TNF, and inter-
feron [174, 175]. In the presence of high n-6:n-3 PUFA ratios of dietary intake,
biosynthesis of their metabolites steadies a prominent production of 2-series
prostaglandins (PGE2, PGF2a), thromboxane A2, and 4-series leukotrienes, in
294 E.H. Biberoglu and K.O. Biberoglu
associations between physical activity and the risk of endometriosis, with relative
risks ranging from 0.2 to 0.6 [9, 34, 182]. 70 % decreased risk of developing an
endometrioma with recent, frequent, and regular high intensity physical activity, as
characterized by 3 times/week, 30 min/episode, 10 month/year for 2 years.
Another study found a 40 % lower risk for women who reported regular exercise
for 37 h/week and an 80 % risk reduction for those who exercised more than 7 h/
week when compared with nonexercisers [183]. On the contrary to the others, in the
Nurses Health Study II, activity reported 6 years prior to diagnosis and inactivity
have not been found to be associated with endometriosis [184].
Although adult physical activity has been mostly associated with lower endo-
metriosis risk [9, 34, 182, 183, 185], little is known about the influence of childhood
or adolescent physical activity on endometriosis.
One of the studies reported a 27 % increased risk of endometrioma for any
physical activity at 1221 years of age [182], and the other one, the Nurses Health
Study II, also found a positive linear relationship between strenuous physical
activity at 1213 years of age and endometriosis risk [186], suggesting that the
early adolescent period is a critical window of exposure for the implantation of
endometriosis lesions, which physical activity might promote at that age.
adult exposure [33]. Based on these evidences, one can hypothesize that during
embryogenesis, EDC exposure has an organizational effect that increases suscep-
tibility for endometriosis, but subsequent adult hormone, immune, and/or EDC
irregularities are required for disease onset.
Although estrogen is necessary for the progression of endometriosis, other
factors also influence this progression. The most toxic dioxin, TCDD, induces
endometriosis, not in ovariectomized mice but with an intact ovary [34]. Also, in
women with peritoneal endometriosis, immune dysfunction by TCDD has been
blamed since the immune system fails to prevent implantation of endometrial
debris, despite high levels of activated macrophages and inflammatory cytokines
in the peritoneal environment [189], suggesting that the progression of endometri-
osis is dependent on both hormonal and immune environments.
Increasing experimental evidence suggests an influence of environmental organ-
ochlorines, a class of xenobiotic chemicals on endometriosis development, includ-
ing dioxin or dioxin-like compounds [190, 191] which are known to disrupt
endocrine and immune functions [192].
Human endometrium is a known site for estrogen, and many environmental
chemicals have been detected there [193] or may induce inflammation and the
chronic stimulation of proinflammatory cytokines. At the same time, they have
been associated with immunologic changes, downregulating natural killer cells or
interleukin-1 and interleukin-12 [194].
Recently, organochlorine pesticides have also been shown to increase endome-
triosis risk in a laparoscopic cohort of US women [195] and other studies have
reported increased risks with higher concentration of phthalates [196, 197],
polychlorinated dibenzodioxins and polychlorinated dibenzofurans, and
polychlorinated biphenyls [198, 199].
Experiments on rodents suggest that both adult and in utero exposure to dioxin
can promote endometriosis during adulthood. Increased endometriotic lesion size
was observed in mice exposed to TCDD during both perinatal and adult life
stages [33].
Since in utero and lactational exposure to TCDD reduces circulating estradiol
in vivo [200] and decreases ovarian estradiol production in cultures [201], and also
causes degradation of ER- [202], it is possible that fetal exposure to TCDD
promotes adult endometriosis through altered P action, because PR expression is
reduced in the uterus of adult mice that were exposed to TCDD in utero [35] and P
insensitivity is characteristic of women with endometriosis [189, 203]. TCDD
which is an immunosuppressant [36] might promote endometriosis by altering the
immune function, thereby enabling establishment and growth of peritoneal endo-
metriosis under the influence of E2, proangiogenic, proliferative, and antiapoptotic
factors. Alternatively, TCDD could activate the expression of K-ras in the ovarian
surface resulting in peritoneal endometriosis [37]. Endometriotic lesions have
increased expression of aromatase and 17-HSD type 1 and decreased expression
of 17-HSD types 2 and 4, resulting in an increase in production of estradiol [39].
If this expression pattern is established during fetal development via
epigenetic mechanisms, then endometriosis could manifest during adulthood after
18 Prevention of Endometriosis 297
postpartum period, whether there will be any remobilization or not of adipose tissue
resulting in increased circulating levels of previously stored EDCs, thereby increas-
ing the levels in breast milk, is unknown [219].
Parents should be advised to avoid plastic bottles and not to store foods including
breast milk or formula for baby in plastics to avoid bisphenol A. There are also
toxins including dioxin, xylene, ethylbenzene, and styrene in disposable diapers
made of bleached paper and plastic [220]. Infants whose skin are exposed to lotion,
powder, and shampoo reveal increased urinary concentrations of phthalates [221].
Since food is the primary exposure to EDCs, eating organic instead of geneti-
cally modified foods is very critical [222]. Another way to reduce exposure is to eat
more vegetables, grains, fruits, and less animal products [223]. One might skip meat
completely and go vegetarian. On the other hand, soy, corn, potatoes, squash,
canola oil, cottonseed oil, papaya, and tomatoes are among the most commonly
genetically engineered foods. Consuming lignin-containing vegetables like cab-
bage, cauliflower, broccoli, and Brussels sprouts, which helps in the removal of
excess estrogen, is another way to reduce exposure [224]. In brief, contaminated
fish, meats, dairy, eggs, processed oils and fast foods, fried foods, and refined
processed foods should better be reduced or even avoided.
Avoiding pesticides and herbicides from other, non-food, sources is also important.
Pesticides have been linked to some immune abnormalities seen in endometriosis,
infections, asthma, and allergies. PVC, a source of phthalates, is prevalent worldwide
in building materials, plumbing, shoes, rain gear, shower curtains, flooring, and toys.
Dental sealants, used to protect teeth from decay-causing bacteria, typically contain
bisphenol A [225]. Children who have been exposed to pesticides are 37 times
more likely to develop non-Hodgkins lymphoma than children who have not been
exposed to pesticides and this risk was similar for pesticide exposure to the
mother during pregnancy and direct exposure after birth [226]. Since women with
endometriosis have 40 % higher risk for developing hematopoietic malignancies,
mainly non-Hodgkin lymphoma, this may be a problem which requires extra
caution [227].
Menarche is correlated to percent body fat with about 17 % body fat required for
menarche and 22 % body fat reported to be required to maintain or restore
menstruation [228]. Since fat cells produce estrogen, heavier girls usually begin
sexual development and periods earlier [229]. Fat cells also make cytokines,
therefore keeping down fat should also avoid inflammation [230]. The fat con-
sumed as a child may be even more an important risk than the fat consumed as an
adult. Exercise is another way to keep body fat low and achieve the goal of delaying
puberty and menarche [231].
The Nurses Health Study II (NHS II), in a well-characterized cohort, has
reported that low birth weight, multiple gestation, and DES are associated with a
diagnosis of endometriosis [23]. Another study demonstrated lower odds of the
diagnosis with in utero exposure to cigarette smoking [232]. Women eventually
diagnosed with endometriosis were leaner from childhood through diagnosis
relative to women without endometriosis [21]. This finding was subsequently
18 Prevention of Endometriosis 299
corroborated in the large Nurses Health III Cohort Study [233]. Despite some
indirect evidence suggestive of an early origin for endometriosis, some recent
studies failed to demonstrate an association between in utero exposures and
increased odds of an endometriosis diagnosis [234, 235].
18.5 Conclusion
In conclusion, medical literature have not yet addressed the prevention of endome-
triosis. However, there is extensive scientific and clinical data applicable to pre-
vention of endometriosis when it is regarded as a systemic inflammatory,
endocrine, and immunological disease. We hope this review will stimulate further
basic and clinical research on this very critical health problem of women.
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Chapter 19
MR Imaging of Endometriosis
Shinya Fujii
S. Fujii (*)
Division of Radiology, Department of Pathophysiological and Therapeutic Science,
Faculty of Medicine, Tottori University, Yonago, Japan
e-mail: [email protected]
Fig. 19.1 A 39-year-old woman with bilateral ovarian endometriotic cysts. Axial T1-weighted
MR image (a) shows bilateral hyperintense ovarian masses (arrows). T2-weighted image shows
shading with hyperintensity in both lesions (arrows) (b). On fat-suppressed T1-weighted image,
these masses remain hyperintense (c)
Fig. 19.2 A 32-year-old woman with left ovarian endometriotic cyst. Axial T2-weighted images
demonstrate left ovarian hypointense cystic mass (arrow). The shading sign is more prominent at
3 T (a) than at 1.5 T (b)
Adhesion is diagnosed when there is obliteration of fat planes with a lack of a clear
interface between adjacent organs, spiculated hypointensity stranding between the
organs, and angulation and distortion of adjacent bowel loops [14]. These findings
are usually subtle, and we should detect the findings carefully.
The following findings are related to posterior cul-de-sac obliteration:
retroflexed uterus, elevated posterior vaginal fornix, intestinal tethering and/or a
tethered appearance of the rectum in the direction of the uterus, faint strands
between the uterus and intestine, and fibrotic plaque and/or nodule covering the
serosal surface of the uterus [14] (Fig. 19.3). Particularly, the following findings are
proposed as the major criteria for diagnosing cul-de-sac obliteration because of
their good specificity: intestinal tethering and/or a tethered appearance of the
rectum in the direction of the uterus, strands between the uterus and intestine, and
a fibrotic plaque covering the serosal surface of the uterus. Additionally, the most
accurate combination of two findings is intestinal tethering in the direction of the
uterus and fibrotic plaque in the uterine serosal surface, and the next highest
combination is retroflexed uterus and intestinal tethering in the direction of the
uterus [14].
Fig. 19.3 A 34-year-old woman with bilateral ovarian endometriotic cysts and posterior
cul-de-sac obliteration. The uterus is retroflexed on sagittal T2-weighted image (a). An irregular
hypointense area at posterior serosal surface of uterus is found (curved arrows). The posterior
vaginal fornix (arrow) is elevated toward this area. Axial T2-weighted image (b) shows faint
strands between uterus and rectum (arrowhead), tethered appearance of the rectum in the direction
of the uterus (bold arrow)
pain, dysuria, and lower gastrointestinal symptoms. The lesion can involve the
posterior cul-de-sac, uterosacral ligaments, rectovaginal septum, ureters, bowel,
and bladder. Endometriotic implants usually elicit an intense desmoplastic response
in the surrounding tissues, leading to the formation of adhesions, fibrotic bands, and
plaques. The histologic finding of deep pelvic endometriosis is mainly characterized
by fibromuscular hyperplasia surrounding foci of endometriosis. Previous report has
demonstrated the high accuracy in the prediction of deep pelvic endometriosis
with a sensitivity of 90.3 %, specificity of 91 %, and accuracy of 90.8 % [15].
Additionally, 3.0 T MR imaging has high accuracy in the diagnosis and staging of
deep endometriosis [16].
Deep endometriosis shows typically hypointensity with punctate hyperintensity
on T1-weighted imaging, hypointensity on T2-weighted imaging, and contrast
enhancement, which findings correspond to fibrous tissue. Punctate foci of
hyperintensity reflect hemorrhage surrounded by solid fibrous tissue. Additionally,
tiny hyperintensities within the lesion, which represent endometrial glands, can be
shown on T2-weighted imaging.
Irregular fibrotic thickening and nodularity with regular or stellate margins along
the course of the uterosacral ligament suggests deep pelvic endometriosis
(Fig. 19.4) [15]. MR imaging for the diagnosis of uterosacral ligament endometri-
osis has a sensitivity of 69.290 % and a specificity of 7694.3 % [17]. Thin-section
oblique axial T2-weighted imaging can improve the depiction of uterosacral liga-
ment endometriosis [18]. However, 3D T2-weighted imaging in combination with a
multi-planar reconstruction technique has no significant different accuracy from
that of conventional 2D axial T2-weighted imaging [17].
19 MR Imaging of Endometriosis 315
Fig. 19.4 A 29-year-old woman with deep pelvic endometriosis of bilateral uterosacral ligaments.
Axial T2-weighted image (a) demonstrates hypointense fibrotic plaque (arrow) with punctate
hyperintense foci on fat-suppressed T1-weighted image (arrow) (b) and irregular thickening of the
right uterosacral ligament (arrowheads)
Fig. 19.5 A 30-year-old woman with deep pelvic endometriosis infiltrating the rectosigmoid.
Rectosigmoid involvement shows hypointense fan-shaped configuration on sagittal T2-weighted
image (a) and contrast enhancement on enhanced T1-weighted image (arrow). An irregular
hypointensity area at posterior serosal surface of uterus is also found (arrowhead)
Fig. 19.6 A 34-year-old woman with bilateral ovarian endometriotic cysts. Bilateral
endometriotic cysts (arrows) show hyperintensity with subtle shading on axial T2-weighted
images obtained before hormone therapy (a). The size and signal intensity of the cysts (arrows)
decreased after hormone therapy (b)
Decidual changes of the ectopic endometrial stroma during pregnancy are well
known. Decidual changes of endometrial tissue in endometriomas during preg-
nancy may manifest as mural nodules and mimic malignant transformation. The
mural nodules indicating decidualization are demonstrated as linear, small nodular,
broad-based nodular, or polypoid structures, which show isointensity with the
nomotopic decidualized endometrium on T1- and T2-weighted images, balanced
fast field echo images, and diffusion-weighted images [2729]. Additionally, the
apparent diffusion coefficient of decidualized mural nodules is significantly higher
than that of ovarian cancers [29]. These MR imaging characteristics can help to
differentiate decidualized endometriotic cyst from malignant transformation.
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23. Del Frate C, Girometti R, Pittino M, et al. Deep retroperitoneal pelvic endometriosis: MR
imaging appearance with laparoscopic correlation. Radiographics. 2006;26:170518.
24. Busard MP, Mijatovic V, Luchinger AB, et al. MR imaging of bladder endometriosis and its
relationship with the anterior uterine wall: experience in a tertiary referral centre. Eur J Radiol.
2012;81:210611.
25. Bazot M, Jarboui L, Ballester M, et al. The value of MRI in assessing parametrial involvement
in endometriosis. Hum Reprod. 2012;27:23528.
26. Sugimura K, Okizuka H, Kaji Y, et al. MRI in predicting the response of ovarian
endometriomas to hormone therapy. J Comput Assist Tomogr. 1996;20:14550.
27. Miyakoshi K, Tanaka M, Gabionza D, et al. Decidualized ovarian endometriosis mimicking
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33. Tanaka YO, Okada S, Yagi T, et al. MRI of endometriotic cysts in association with ovarian
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Chapter 20
Biomarkers of Endometriosis
A semi-invasive test could be developed for peritoneal fluid and eutopic endometrium.
The development of such a test from initial biomarker discovery to be a clinically
approved biomarker assay is a long, difficult, and uncertain process and includes four
different phases. A review of the existing literature is provided in this chapter. Overall,
most endometriosis biomarker studies remain at the level of phase I, with only a few
currently in phase II of biomarker development. There is a need for a well-designed
multinational study including academic and industrial partners for phase II and
phase III trials.
20.1 Introduction
The last few years, tremendous work has been published regarding biomarkers.
In 2009 and 2013, researchers proposed that the development of reliable noninva-
sive test of endometriosis is one of the top research priorities in endometriosis
[16, 24]. A clinically reliable test for endometriosis can be expected to have a
profound impact on the reduction of health care and individual costs by:
1. Reducing time to diagnosis and the time wasted to see numerous health-care
professionals
2. Subsequently reducing the time before individualized specialist care is invoked
3. Subsequently reducing expensive hit-and-miss treatments
4. Subsequently reducing expensive fertility treatments if the disease is under
control before fertility is impaired [25]
Highly relevant markers known to be involved in the pathogenesis of endometriosis
have been studied such as glycoproteins, inflammatory and noninflammatory
cytokines, adhesions, and angiogenic and growth factors [20]. At present, neither a
single biomarker nor a panel of biomarkers measurable in peripheral blood has been
validated as a noninvasive test for endometriosis [19]. The measurement of serum
CA-125 levels has no value as a diagnostic tool compared to laparoscopy [15].
Although previous studies have shown that various tumor markers, cytokines, and
angiogenic and growth factors show altered levels in peripheral blood (plasma or
serum) of women with endometriosis when compared to controls [19, 26], so far none
of them, alone or in combination, have been validated as a noninvasive test for
endometriosis [19]. Furthermore, at present there is no consensus on the value of
inflammatory factors as biomarkers for endometriosis [20]. Comparable serum IL-6
[27, 28], IL-8 [27, 29], TNF-alpha, and IL-1 [27, 28, 30] levels were previously
reported in women with and without endometriosis. However, other investigators
reported elevated peripheral levels of IL-6 [30, 31], IL-8 [32, 33], TNF-alpha [31, 34],
and IFN-gamma [30] in endometriosis patients compared with controls [20].
20 Biomarkers of Endometriosis 325
So far, studies evaluating panels of biomarkers [3538] have been limited with
respect to the number of biomarkers analyzed, the statistics used, and the lack of
validation in an independent test set of patients [20]. One study proposed two panels
of four biomarkers (annexin V, VEGF, CA-125, and glycodelin or sICAM-1)
measured in plasma samples obtained during menstruation allowed the detection
of ultrasound-negative endometriosis with high sensitivity (82 %) and acceptable
specificity (6375 %) in an independent test data set [39]. In the same study, three
biomarkers (VEGF, annexin V, and CA-125) present in plasma obtained during
menstruation allowed the diagnosis of endometriosis (minimalsevere endometri-
osis, both with and without ultrasound evidence) with 8594 % sensitivity and 62
75 % specificity in an independent test data set [39]. These results are promising but
need to be validated in a prospective study. Surprisingly, inflammatory molecules
did not emerge as biomarkers in this study [39].
Recently, a diagnostic model including patient-reported clinical data derived
from a validated questionnaire predicted any-stage endometriosis poorly, but stages
III and IV accurately, with menstrual dyschezia and a history of benign ovarian
cysts as the strongest predictive factors [40]. More research is needed to add clinical
factors to diagnostic models based on plasma or endometrial analysis.
The development of a noninvasive diagnostic test, from initial biomarker dis-
covery to a clinically approved biomarker assay, is a long, difficult, and uncertain
process [41] and occurs in four different phases as described below:
Phase IPreclinical discovery phase. This phase consists of exploratory preclinical
studies aiming to identify potential biomarkers. In endometriosis research, the
state of the art in this field has recently been reviewed by May et al. [19].
Phase IIPreclinical assay development and validation of a clinically useful
noninvasive diagnostic test in the preclinical setting, as has been done in the
context of endometriosis in our most recent paper [39].
Phase IIIProspective clinical validation and determination of clinical utility. This
phase establishes the diagnostic accuracy and predictive value in the target
population, but this phase has not yet been reached in endometriosis biomarker
research so far.
Phase IVCommercialization: product development by industry, which has not
yet been done successfully for noninvasive endometriosis biomarkers.
Overall, most endometriosis biomarker studies remain at the level of phase I [19]
and only a few have made it to phase II studies. There is a need for well-designed
phase II and phase III trials to make progress in this field.
The abovementioned data were not confirmed by Newman and coworkers, com-
paring 20 patients with endometriosis (minimalmild n 20, moderate n 4, and
severe n 4) to 25 controls [52]. No significant difference was observed between
the disease and control group in PGP 9.5-positive nerve fibers, visualized by
immunohistochemistry [52]. Using western blotting as a quantitative method to
detect the neural markers, all three markers were expressed in endometrium from
both endometriosis cases and controls (PGP 9.5: P 0.0991, VR I: P 0.0621,
NGFp75: P 0.2586) [52].
In another study, no statistical difference was observed in endometrial nerve
fiber density, determined by PGP 9.5 staining, between women with (n 47) and
without endometriosis (n 21) [53]. This study, however, was marked by several
methodological drawbacks. Firstly, threshold for endometrial biopsy quality was
low (one low-power field of well-oriented endometrial mucosa sample perceived to
be sufficient to being classified as satisfactory). Secondly, the exact endometrial
nerve fiber density was not mentioned, since data were classified as positive or
negative depending on the presence or absence of nerve fibers [53]. This study
highlighted that methodological factors such as the method of endometrial biopsy
sampling and image analysis might influence the consistency of results for this
semi-invasive diagnostic test [53]. Taking into account the uneven distribution of
the nerve fibers in a biopsy, reliable results may require inspection of more than one
section per biopsy [45]. Furthermore, the whole surface of an endometrial section
should ideally be examined [49] as opposed to counting endometrial nerve fibers in
randomly chosen fields [45]. Additionally, it is crucial that background staining
during immunohistochemistry is reduced as much as possible, which can be
challenging. In a research context, results should be analyzed by an experienced
pathologist. While it is essential to refine methodology, it is equally important to
select and phenotype the study population. All cases in the endometriosis group
should have laparoscopically confirmed endometriosis, preferably with histological
confirmation of the presence of endometrial glands and stroma in the lesions [49].
In some of the studies, this criterion was not met, as only in a part of the cases
histological confirmation of endometriosis was available [45, 47]. Further,
according to the modified QUADAS (Quality Assessment of Diagnostic Accuracy
Studies) criteria [19], detailed information should be available regarding the demo-
graphics such as disease stage and cycle phase [49]. Study patients ideally have not
received hormonal medication 3 months prior to surgery, because systemic expo-
sure to hormonal medication might reduce the presence of nerve fibers in eutopic
endometrium [43]. However, this medication-free period was as short as 1 month in
one study [50] and could have been even shorter in another study stating that
patients were not on medication only at the time of laparoscopy [45]. Additionally,
one study included three patient groups (one on current hormonal therapy (n 11),
one without hormonal therapy (n 44), and a group with unknown status (n 13))
and found an overall poor sensitivity for the test that was independent of the
treatment status [53]. This lack of significance might have been due to the
low sample size in each group. The control group should be equally well charac-
terized and should have absence of endometriosis confirmed by laparoscopy
20 Biomarkers of Endometriosis 329
20.2.2.1 Endometrium
Recently, several studies of miRNA in peripheral blood have been performed in the
context of endometriosis [7678]. One study, investigating circulating miRNAs in
plasma, showed a significant downregulation of miR-17-5p ( p 0.011), miR-20a
( p 0.0020), and miR-22 ( p 0.0002) in women with endometriosis (n 23)
compared with women without endometriosis (n 23) [78]. Receiver operating
characteristic (ROC) curve analysis permitted the calculation of the area under the
curve (AUC) (0.74, 0.79, and 0.85 for miR-17-5p, miR-20a, and miR-22, respec-
tively) after which a cutoff value could be set to determine sensitivity (70.0, 60.0,
90.0 % for miR-17-5p, miR-20a, and miR-22, respectively) and specificity (70.0,
90.0, 80.0 % for miR-17-5p, miR-20a, and miR-22, respectively) to differentiate
between women with and without endometriosis [78]. Combined assessment of the
three miRNAs resulted in an AUC of 0.90 [78]. Additionally, another study showed
that discrimination was possible between plasma of healthy controls (n 20) and
endometriosis patients (n 33) with 88 % sensitivity and 60 % specificity
(AUC 0.90), based on the assessment of miR-16, miR-191, and miR-195 which
were all highly expressed in endometriosis [77]. Endometriosis and endometriosis-
associated ovarian cancer (EAOC) (n 14) could be distinguished from each other
through a combination of miR-21, miR-362-5p, and miR-1274a with 57 % sensi-
tivity and 91 % specificity and an AUC of 0.92. Distinction of endometriosis and
serous ovarian cancer (SOC) (n 21) was possible with 90 % sensitivity and 73 %
specificity (AUC 0.88), based on the assessment of miR-362-5p, miR-628-3p, and
miR-1915 [77]. A trend of elevated plasma miRNA expression compared with
healthy controls was found in endometriosis cases and even more so in EAOC
cases. This suggests that endometriosis might be a precursor stage of EAOC and the
possibility for miRNA signatures to act as disease progression markers [77].
In serum of patients with endometriosis (n 60) and controls (n 25) the
combination of miR-199a, miR-122, miR-145*, and miR-542-3p could predict
endometriosis with 93.22 % sensitivity and 96.00 % specificity (AUC 0.994) [76].
Currently, there is no agreement on which circulating miRNA can be used for
data normalization. One group selected U6 as a normalization control because of its
use as internal control in other studies [76]. However, other investigators preferred
miR-16 as endogenous control because it is more stable and less variable in
circulation than other miRNAs [78]. Yet another research group used miR-132
for data normalization, as they found this miRNA to be homogeneously expressed
across all samples [77].
It is also important to distinguish the presence of miRNAs in either plasma
or serum. Although higher miRNA concentrations were observed in plasma than
332 A. Fassbender et al.
in serum in one study [79], this was not confirmed in another study [80].
This discrepancy might have been due to pre-analytical variability concerning
blood tube type or differences in sample-processing protocols [79]. Conversely,
other studies have shown an increased concentration of miRNAs in serum samples
when compared to plasma samples of the same patient, although they conclude that
plasma might be the sample of choice because miRNAs that are released during
the coagulation process in serum samples may interfere with the true miRNA
profile [81].
Interestingly, miRNAs are exceptionally stable in plasma, serum, and tissue
samples, making them excellent candidates for biomarker research [80]. Possibly
miRNA is protected from RNases in blood by being packaged in vesicles or bound
to RNA-binding proteins [82].
Despite the potential advantages of a miRNA-based blood test for endometri-
osis, some possible pitfalls should be taken into consideration. It should be noted
that apart from their best known function as transcriptional repressor, miRNAs can
act as translational activators [83]. Therefore the relationship between miRNA
and target mRNA is not necessarily an inverse one [72]. Additionally, in most
miRNA studies, specific mRNA targets are often not experimentally verified, but
only predicted by various computational algorithms [65, 72]. Beside the influence
of the choice of mathematical algorithm, one mRNA can be the target of multiple
miRNAs that might not all be altered, rendering validation in an in vitro
setup essential to determine the effect of the dysregulation of the miRNA of interest
[65, 72].
Since miRNA patterns change under the influence of reproductive hormones and
are thus altered in different phases of the menstrual cycle [84], an adequate control
group should be chosen, preferably without any other illness as this could also
influence the miRNA profile [78].
The discrepancies observed in different miRNA results can be explained by
differences in patient selection, microarray protocol, and choice of housekeep-
ing genes for data normalization. Therefore a standardized methodological
approach needs to be determined and controls and patients need to be selected
according to the QUADAS criteria. The rationale for implementing next-
generation sequencing is that a larger amount of miRNAs can be examined,
without being dependent on the availability of probes [66]. Exceptionally
important is the role of advanced statistical methodology in studies where
many variables are compared. Therefore, all data should be controlled for
multiple testing [85].
In conclusion, miRNAs are interesting subjects in the further development of
biomarker research, although more extensive research in a larger population and
validation in independent test sets should be conducted with full awareness of
methodological issues and the complexity of miRNA mechanisms.
20 Biomarkers of Endometriosis 333
20.3 Conclusions
Despite its gradual progress, the biomarker research field still faces the challenge of
successfully developing a clinically approved biomarker assay for endometriosis [20].
Up to now, no semi- or noninvasive diagnostic test exists for endometriosis [19].
Most studies so far have included limited numbers of patients, limited assessment
of different cycle phases and endometriosis stages, limited number of biomarkers
analyzed, limited statistical analysis (mostly univariate statistical analysis only),
and the lack of validation in an independent test set of patients [20].
In the past, collaborations between research centers have been limited and
standard operating procedures (SOPs) are different among centers [20]. Most
biomarker studies remain at the level of phase I, the preclinical discovery phase,
as reviewed by May et al. [19, 42]. Only a few biomarkers make it to phase II, the
preclinical assay development and validation [39, 47, 86].
To develop a diagnostic test for endometriosis, semi-invasive techniques utiliz-
ing endometrial biopsies have been explored [87]. An increased amount of small
unmyelinated nerve fibers in the functional layer of eutopic endometrium of
endometriosis patients has been reported [45, 49, 88]. However, prospective vali-
dation of this method in a blinded fashion is needed in a larger patient population,
using a standardized biopsy sampling technique and standard immunohistochemi-
cal and statistical methods. Validation should be carried out in a patient population
experiencing pain/infertility with a 30 % prevalence of endometriosis.
At present, neither a single biomarker nor a panel of biomarkers measurable in
peripheral blood has been validated as a noninvasive test for endometriosis [19],
although panels with reasonable specificity and sensitivity have recently been
published [39]. Panels of biomarkers that have been proposed as diagnostic tests
in phase I and II trials should be validated in prospective phase III studies [20].
In this phase, diagnostic accuracy of the proposed panel needs to be confirmed in
an independent test population with infertility/pain scheduled for surgery [20].
The predicted outcome should be compared with the actual presence of endome-
triosis. Future studies should also focus on the large and clinically relevant
population of endometriosis patients using hormonal medication, which is under-
represented in published biomarker discovery studies.
In order to improve the specificity and sensitivity of previously proposed
diagnostic models, several choices are possible: using advanced protein technology
to discover new and unknown biomarkers, combining a blood test with a semi-
invasive test, or adding clinical factors to a model.
Advanced protein technologies such as antibody-based large-scale protein
arrays, allowing concurrent detection of up to 1,000 proteins, might be required
to improve the diagnostic power of a noninvasive blood test for endometriosis.
Antibody-based microarrays have already been applied in biomarker screening for
334 A. Fassbender et al.
sample collection, processing, and storage along with reporting uniform clinical
information are crucial to compare results between studies and to enable a multi-
center biobanking approach [16, 95]. Collaborations are essential to obtain the large
sample sizes that are required for the statistical power of validation studies [16].
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20 Biomarkers of Endometriosis 339
21.1 Introduction
Since the first descriptions of endometriosis by Lockyer et al. in 1918 [1] and
Sampson et al. in 1921 [2] it became necessary to classify the disease with the aim
to include histological differentiation as well as differentiation according to loca-
tion and severity of the disease. Ideally, a classification has a common language that
specifies the diagnosis, thereby allowing a standardisation of disease assessment.
Furthermore, it enables research, as well as the clinical community to compare
findings.
The early classification systems were based on the anatomical localisation of the
disease and its similarity to malignancy. The classification systems before 1973
described mainly the anatomical distribution of endometriosis and did not correlate
with the clinical outcome; thus they have not received widespread clinical accep-
tance. The Acosta classification [3] was the first one where a direct relationship
could be established with different stages of the disease and clinical pregnancy
rates. As a further development, the staging system of Kistner [4] tried to reflect
the natural progression of the disease with moving from early peritoneal implants
to ovarian and fallopian tube-ovarian involvement and dissemination within the
pelvis. One of the most precise and detailed classification systems was the Buttram
classification [5], which, however, has not received widespread acceptance.
Table 21.1 gives an overview of the most common classification systems, which
have been made since 1918.
An ideal classification would require that a consensus be reached over empiri-
cally as well as scientifically based data that are comprehensive for all cases. Terms
would need to be defined unambiguously, and anatomic lesions, extent of disease,
severity of pain, impact on fertility and organ function within the pelvis as well as
social impact would need a simple translation into a verbal description. Founding
variables would need to be recognised and the risk of complications should be
indicated. Finally the ideal classification would also guide the treatment and
estimate risk for recurrence.
To date, we are far from having an ideal endometriosis classification.
In this chapter we are introducing and analysing the currently used classification
systems.
21 Classification of Endometriosis 343
None of the classifications before 1978 have been widely accepted in the clinical
practice, which motivated the American Fertility Society (AFS) to form a panel and
introduce a new classification that has been published in 1979 [12]. The first
revision was published in 1985 [13] and appeared in its final version in 1996
when the society had changed its name into American Society of Reproductive
Medicine [14].
Even though it is called a classification, it rather is a scoresheet, where the
peritoneum, the ovaries, the tubes and the cul-de-sac are listed (Fig. 21.1).
The size and depth of lesion corresponds to points, which by analogy are also
assigned for adhesions on the ovaries and fallopian tubes as well as points for partial
or complete obliteration of the cul-de-sac. A schematic drawing is provided where
the localisation of lesions and adhesions can be drafted. The summing up of all
points yields in a score, which then allows classifying the endometriosis into four
grades of severity: stage I (minimal endometriosis: 15 points), stage II (mild
endometriosis: 615 points), stage III (moderate endometriosis: 1640 points) and
21 Classification of Endometriosis 347
Fig. 21.1 The revised American Society for Reproductive Medicine classification of endometri-
osis. With permission from Elsevier (Fertility and Sterility, Licence number: 3184950406638)
348 H.-R. Tinneberg et al.
The most widely used rASRM and Enzian scores (see below) describe properly the
anatomical distribution of the respective superficial and deep infiltrating
endometriotic lesions and concomitant adhesions, but are not eligible to provide
information about the clinical outcome, the pain reduction and the reproductive
performance after surgery.
In 2010 Adamson and Pasta analysing the clinical characteristics and reproduc-
tive results after surgical intervention of 569 infertile endometriosis patients in the
USA in a prospective study, proposed a new staging system, the endometriosis
fertility index (EFI) [18]. EFI predicts pregnancy rates in patients with surgically
scored endometriosis who attempt non-ART conception. EFI could be regarded as a
specifically further developed form of the rASRM classification, focusing on the
reproductive outcome, and is not intended to assess the pain symptoms or predict
the pain-reducing effect of the surgery.
The EFI score is based on three surgical factors and on one history factor
that are presented in Fig. 21.2.
In the first step the least function (LF) score at conclusion of surgery is defined.
LF reflects the predicted function of the fallopian tubes, the fimbriae and the
ovaries, each scored from 0 to 4, depending on absent or nonfunctional state, severe
dysfunction, moderate dysfunction, mild dysfunction and normal state. Table 21.2
represents the description of least function terms.
The better the function the higher the score. Scores are added and give the least
function score. The LF score is completed with the categorised and valued rASRM
lesion score as well as the rASRM total score.
The historical factors contribute to age, duration of infertility and history of prior
pregnancies. The lower the age, the lower the duration of infertility, and the higher
the number of previous pregnancies, the higher the historical score (Fig. 21.2).
350 H.-R. Tinneberg et al.
Fig. 21.2 Endometriosis fertility index (EFI). With permission from Elsevier (Fertility and
Sterility, licence number: 3184941294427)
The total historical as well as the total surgical scores sum up to a score ranging
between 0 and 10, with 0 representing the poorest and 10 the best prognosis. A
coloured graph shows the respective estimated percentage of pregnancy likelihood
depending on time after surgery and EFI score.
21 Classification of Endometriosis 351
Table 21.2 Least function terms after Adamson and Pasta [18]
Structure Dysfunction Description
Tube Mild Slight injury to serosa of the fallopian tube
Moderate Moderate injury to serosa or muscularis of the fallopian tube; moderate
limitation in mobility
Severe Fallopian tube fibrosis or mild/moderate salpingitis isthmica nodosa;
severe limitation in mobility
Nonfunctional Complete tubal obstruction, extensive fibrosis or salpingitis isthmica
nodosa
Fimbria Mild Slight injury to fimbria with minimal scarring
Moderate Moderate injury to fimbria, with moderate scarring, moderate loss of
fimbrial architecture and minimal intrafimbrial fibrosis
Severe Severe injury to fimbria, with severe scarring, severe loss of fimbrial
architecture and moderate intrafimbrial fibrosis
Nonfunctional Severe injury to fimbria, with extensive scarring, complete loss of
fimbrial architecture, complete tubal occlusion or hydrosalpinx
Ovary Mild Normal or almost normal ovarian size; minimal or mild injury to
ovarian serosa
Moderate Ovarian size reduced by one-third or more; moderate injury to ovarian
surface
Severe Ovarian size reduced by two-thirds or more; severe injury to ovarian
surface
Nonfunctional Ovary absent or completely encased in adhesions
Besides introducing the new EFI score, Adamson has prospectively validated
and proven the effectiveness of the new scoring system analysing the predicted and
actual reproductive results of 222 North American surgically treated endometriosis
patients [18]. Three further external studies, performed in China, France and
Belgium, have validated as well the clinical usefulness of the EFI score. In the
study of Wei et al., 350 infertile patients were studied retrospectively. Within
3 years after surgery the cumulative pregnancy rates with EFI scores 8, 9 and
10 were 62.5, 69.8 and 81.1 % and with EFI scores 5, 6 and 7, 49.8, 43.9 and 41.6 %
respectively, in accordance with the estimated pregnancy rates [19]. A French study
of Yacoub et al. investigated in a retrospective study 132 infertile endometriosis
patients and found that EFI showed a significant association between the severity of
endometriosis, infertility and postoperative cumulative birth rates. However, the
rASRM score fall short to predict pregnancies. The authors suggested that the EFI
should be the main component in the choice of the postoperative ART
management [20].
A further study performed in a Belgian population with 233 infertile endome-
triosis patients has also validated the effectiveness of the EFI and found the LF
score the most important contributor to the total EFI score among all the other
variables [21]. The authors concluded that the EFI classification system is a useful
tool in counselling infertile endometriosis patients about their reproductive chances
after surgery.
352 H.-R. Tinneberg et al.
Several approaches have been published in the literature to classify deep infiltrat-
ing endometriosis (http://www.endometriose-sef.de) [2224]. The intention of
Chapron et al. was to propose a classification based on where the DIE lesions are
located. The deep infiltrating lesions have been divided into two major compart-
ments, anterior (DIE of the bladder) and posterior compartment (DIE of the
sacrouterine ligaments, the vagina and intestines) and a subsequent operative proce-
dure has been defined [22]. Another descriptive classification system of Koninckx
tried to reflect all the possible manifestation and severity of endometriosis, classifying
the so-called subtle, typical, cystic, deep and adenomyotic lesions [23]. In the
meantime the group of German-speaking gynaecologist has developed a classifica-
tion system, called Enzian, with the intention to describe deep infiltrating lesions in
those compartments where the appropriate surgical removal can be performed.
In 2005 Tuttlies et al. [24] published the Enzian classification, which has been revised
in 2010 and 2011. The latest version was published in 2012 at the homepage of the
SEF (Stiftung fur Endometriose-Forschung) (http://www.endometriose-sef.de).
The Enzian classification is exclusively devoted to describe deep infiltrating
endometriosis and is supposed to be used additionally with the rASRM classifica-
tion. Enzian is not an acronym or abbreviation for endometriosis issues but refers to
a beautiful blue-coloured flower and also to the name of a hotel in the Alpes, where
a group of Austrian and German experts since 2002 annually meet under the
patronage of the SEF in order to discuss endometriosis-related problems.
The development of this classification followed in the early versions the master
model of the TNM classification for cervical cancer inspired by the fact that deep
infiltrating endometriosis shows significant characteristics of a malignant tumour,
like crossing organ boundaries and likely infiltrating adjacent structures like blad-
der, ureter or intestines.
When comparing the rASRM classification, which has been established over
decades, with the Enzian classification, the list of common sites demonstrates only
little overlapping. The Enzian classification was designed to describe exclusively
deep infiltrating endometriosis, which means that it is limited to a special, but
challenging, clinically relevant situation. The Enzian classification is based on
different topographic areas following a surgical way of separation of involved
anatomic structures.
There are two main subclasses introduced to describe the clinical presentation of
deep infiltrating endometriosis. On the one hand there is a group of three topo-
graphic relevant compartments in the posterior pelvis and on the other hand there
21 Classification of Endometriosis 353
Fig. 21.3 Example for surgical route for successful separation of compartments A and
C. Segmental rectum resection of two transmural infiltrative endometriotic lesions of 4 and
2 cm, respectively, Enzian C3 FI Sigma
The three posterior pelvic compartments were entitled A, B and C (Fig. 21.4)
and embrace the pelvic manifestation of deep infiltrating endometriosis including
the rectovaginal space, the vagina, the rectum and also the sacrouterine ligament
with the pelvic sidewall.
The second group with the capital letter F (far) was designed to add important
information about the location of infiltrative endometriosis, which is not directly
involved to the pelvic site or distant from the cardinal posterior compartments of the
pelvis as described above. Only important and typical presentations of DIE are
listed, such as infiltration of the bladder, intrinsic ureter endometriosis,
adenomyosis as infiltration of the uterus and distant bowel infiltration.
Compartment A (signed with red colour) includes the rectovaginal space from
the pouch of Douglas along a longitudinal direction downwards to the vagina.
Compartment B (signed with green colour) follows a horizontal line divided in a
left and a right part starting from the sacrouterine ligament; further lateral obstruc-
tions like the external ureter compression as well as the involvement of the cardinal
ligament up to the pelvic sidewall are included. Involvement of the splanchnic
nerves may also be an important issue in extended pelvic sidewall infiltration.
Compartment C (signed with blue colour) describes the dimension of rectal
21 Classification of Endometriosis 355
Of uppermost importance for the imaging of patients suffering from deep infiltrat-
ing endometriosis is the detection and description of all manifestations of endome-
triosis in order to provide a reliable roadmap for surgical and conservative therapy.
MRI has been established for diagnostic and pretherapeutic imaging of patients
suspected to suffer from endometriosis [25]. Inherent to the method in contrast to
ultrasound, clinical examination or laparoscopy, which offers only a limited field of
view, spaces of the pelvis are equally accessible. For complete diagnostic evalua-
tion of all pelvic spaces including the rectum, retrocervical space and vaginal
fornices, careful preparation of the patient is indispensable [26]. For most scanning
protocols 50 mL aqueous gel (ultrasound gel) is administered intravaginally (for
distension of the vaginal cavity, assessment of the retrocervical area and vaginal
fornices) and 150200 mL water is administered into the rectum to obtain disten-
sion and increase contrast between bowel wall and lumen. Scopolamine-N-butyl
bromide is intravenously injected immediately prior to MRI in order to reduce
bowel movements and contractions of the uterus [27]. The bladder should be filled
21 Classification of Endometriosis 357
lesions is measured. Points are added separately for f (fertility) and s (structures)
according to Table 21.3 (Fig. 21.6 represents an example of MRI classification of
a 28-year-old patient with deep infiltrating endometriosis). In cases of bilateral
involvement (i.e. ovaries or fallopian tubes), first the more severely affected side is
rated followed by the side with the smaller lesion. According to Table 21.3 MARIE
classification for f and e values is assigned following the scheme MARIE f s.
21 Classification of Endometriosis 359
21.5 Discussion
Even though many classifications as well as scoring systems have been proposed
since the first mentioning of endometriosis as a disease entity, no widespread
agreement on a classification for endometriosis is obtained. This review describes
four examples in more detail. The rASRM classification differentiates endometri-
osis in minimal, mild, moderate and severe stages and provides a score that includes
superficial endometriotic implants as well as adhesions. The assignment of points
according to the clinical situation was not developed on the basis of empirical data,
but based on theoretical background and estimations. In case of a superficial
non-infiltrating endometriosis, which is only manifested on the peritoneal surface,
this scoring system including a graph makes a lot of sense; however, any sub- and
retroperitoneal deep infiltrating manifestation is not considered with the rASRM
classification. The most commonly used classification system to describe deep
360 H.-R. Tinneberg et al.
infiltrating endometriosis is the Enzian string code, which is used additionally to the
rASRM. In addition to the rASRM and Enzian classification Hackethal et al. [29]
showed that even in stage 1 endometriosis (rASRM classification) 25 % of those
patients were suffering from deep infiltrating endometriosis. Even though this is in
accordance with the initial aim of the rASRM classification omitting DIE can lead to
a marked misjudgement of the impact of the disease and necessary treatment [30].
Since the EFI is a specific further development of the rASRM classification, DIE
with no peritoneal, ovarian or tubal infiltration would not have been reflected in the
EFI score; however it could be responsible for infertility. This would apply to DIE of
the rectovaginal space as well as adenomyosis. However, only limited data are
available on the impact of such manifestations of DIE on fertility. Therefore, the
EFI will likely not be suitable to fully reflect the impact of different locations and
manifestations of endometriosis on fertility. It is probably because of this reason that
EFI gives major importance on historical factors as it is very well known that the
duration of infertility, age of a patient and prior history of pregnancies are extremely
strong predictors.
Haas et al. [31] compared the rASRM classification with the Enzian classifica-
tion. They clearly concluded that the Enzian classification is a clear supplement to
the rASRM classification with regard to the description of the manifestations of
DIE. They found an overlapping of description, especially in peritoneal disease of
the pouch of Douglas or cul-de-sac, which could be repetitive in the Enzian
classification as well as in rASRM classification.
The development of a radiological classification system is extremely useful in
the preparation of the surgical procedure and counselling patients preoperatively
about the required surgical steps. It has to be kept in mind that endometriosis
surgery is almost never easy and straightforward. A presurgical adequate classifi-
cation of disease can potentially improve patients outcome by the organisation of
multidisciplinary surgical teams or referral of patients to specialised surgical
endometriosis centres.
Unfortunately there is no ideal classification of endometriosis at the moment that
would be able to reflect all the aspects of endometriosis, the pathogenesis, anatom-
ical distribution, clinical manifestation, progression and recurrence. The way to
define the perfect classification system is long and lots of basic research as well as
well-conducted clinical trials in a large multicentre set-up are needed to better
understand the clinical nature of the disease and develop a classification system,
which encompass all these aspects.
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362 H.-R. Tinneberg et al.
Sun-Wei Guo
22.1 Introduction
In this chapter, I shall critically review the evidence in support of the link, point
out the challenges in proving the causal link, and, in the end, sketch some ways to
solve this problem. Due to space limitation, I shall restrict my attention to epide-
miological and clinical data. While there is a growing body of literature
documenting shared molecular aberrations between endometriosis and ovarian
cancer, suffice to say that, due to the nature of these studies, many such aberrations
are indicative of association, only suggestive for a causal link, simply because the
temporality of the link is difficult to prove.
22.2 Methods
A systematic and comprehensive search of PubMed was performed for all studies
published up to June 18, 2013, using the following combination of search terms of
endometriosis, ovarian cancer, epidemiology, and association. The studies
had to report epigenetic aberrations in endometriosis. The search was limited to
publications written in English.
For each retrieved case-control studies, the OR and its 95 % confidence interval
(CI) and the standard error (SE) of the log OR were extracted. The choice of log OR
was simply due to the fact that, in contrast to the OR, its SE is unaffected by the
magnitude of the log OR. For cohort studies, the standardized incidence ratio (SIR),
rate ratio (RR), or hazard ratio (HR) and their SEs were extracted.
Funnel plots were used to examine asymmetry, in which the risk estimates such
as OR were plotted on a logarithmic scale against the inverse of their corresponding
standard errors, a measure of precision [8]. If bias is absent, small studies will have
ORs that are widely scattered but symmetric about the OR estimates provided by
larger, more precise studies. In this case, the plot would resemble an inverted funnel
with the tip pointing roughly towards the true log OR. If publication bias is present,
the plot will be asymmetric because some negative studies are not published
All computations were made with R statistics software system version 3.0.9 [9].
The statistical routine rmeta was used.
The sponsor of the study had no role in study design, data collection, data analysis,
data interpretation, or writing of this report.
366 S.-W. Guo
As early as 1925, Sampson proposed histopathological criteria for inferring that the
malignancy arose from endometriosis, or the causal relationship between endometri-
osis and malignancy: (1) clear evidence of endometriosis close to the tumor (prox-
imity); (2) the carcinoma must be seen to arise in endometriosis and not to be
invading it from other sources (arising from endometriosis); and (3) presence of
tissue resembling endometrial stroma surrounding characteristic glands (endometrial
stroma plus glands) [10]. Scott later added one more criterion: the demonstration of a
histology-proven transition from benign endometriosis to cancer (transition) [11].
Clearly, these criteria are all based on histological evidence, which, in turn, are
based on tissue samples taken from patients. While the proximity and endome-
trial stroma plus glands criteria may be relatively easy to establish, the inference of
arising from endometriosis and transition has, by necessity, to be based on a
single snapshot, in contrast to serial observations, of the histological images or
morphologic features during a presumably long period of tumorigenesis and, as
such, can be challenging to establish. It is no wonder that these criteria, considered
to be stringent, are rarely fulfilled [1, 12].
The morphologic data can tell us something, but only to a certain extent. For
example, ovarian cancer was once regarded as a single disease since by morphology
the tumor seemingly originated from ovary but now a dualistic model of carcino-
genesis of ovarian cancer based on distinctive clinicopathologic and molecular
genetic features seems to have replaced the older view [7, 13]. Also, just by
morphology or histological data, it would be very difficult to find that there are
4 main subtypes of breast cancer caused by different subsets of genetic and
epigenetic abnormalities [14]. In addition, since the choice of tissue sections entails
certain degree of selection, it may be susceptible to attribution error, especially
when the pathologists are inexperienced.
That is, when ovarian cancer is rare (indeed it is), the OR obtained from case-
control studies is merely an approximation to RR.
By Bayes theorem and after some simple algebra, it is easy to see that RR
P(E|O)[1P(E)]/(P(E)/[1P(E|O)]). That is, the true RR depends only on the
prevalence of endometriosis (which we have a fairly good idea) and the prevalence
of endometriosis among women with ovarian cancer (which can be estimated from
data, at least in theory). Note that this RR does not depend on the prevalence of O.
Hence we can calculate RR even for some specific histotypes of ovarian cancer, such
as clear cell or endometrioid ovarian cancers. It is noted that RR can be expressed in
a more revealing form, as RR rO/r, where rO P(E|O)/[1P(E|O)], the odds
of having endometriosis given that the woman has O, and r P(E)/[1P(E)],
the odds of having endometriosis in the general population.
The prevalence data extracted from 13 studies reporting the prevalence of endo-
metriosis in women with ovarian cancers, along with the estimated RR using either
the 10 % prevalence for endometriosis or the 5 % for ovarian endometriomas, are
listed in Table 22.1. It can be seen that there are enormous variations in the reported
prevalence, and, consequently, the RR estimates also vary greatly from study to
study. It should be noted that the reported prevalence of endometriosis in women
with ovarian cancer is likely to be an underestimate of P(E|O), since some
endometriotic lesions may not have been found by the surgeon who performed
the operation, or pathologists who performed histologic examination may not have
found any lesion which might still exist. On the other hand, P(E|O) is prone to be
overestimated if one is single-mindedly trying to find all cases of ovarian cancer-
associated endometriosis while dismissing or discarding cases with ovarian cancer
but no endometriosis, consciously or otherwise. Anyhow, it can be seen from
Table 22.1 that some RR estimates based on the reported prevalence still
deviate greatly from the OR estimates reported from case-control studies, espe-
cially for clear cell and endometrioid histotypes. In fact, all, except one, OR
368
Table 22.1 Prevalence of endometriosis in women with ovarian cancers and the estimated relative risk of developing ovarian cancer in women with
endometriosis vs. women without
Overall Clear cell and endometrioid
Year of RR RR RR RR
ID Author publication Prevalence (%) (P 10 %) (P 5 %) Prevalence (%) (P 10 %) (P 5 %) Remark
A71 Aure et al. [15] 1971 4.2 (35/831) 0.39 0.83 12.5 (34/271) 1.29 2.71
K72 Kurman et al. [16] 1972 NR 10.2 (5/49) 1.02 2.16
R79 Russell [17] 1979 11.3 (46/407) 1.15 2.42 34.3 (36/105) 4.70 9.92
B89 Brescia et al. [18] 1989 NR 18.4 (14/76) 2.03 4.28
V93 Vercellini et al. [19] 1993 11.1 (52/466) 1.12 2.37 25.0 (38/152) 3.00 6.33
C96 De La Cuesta et al. 1996 NR 40.0 (16/40) 6.00 12.67
J97 Jimbo et al. [20] 1997 14.5 (25/172) 1.53 3.22 35.6 (16/45) 4.96 10.50
F97 Fukunaga et al. [21] 1997 24.1 (54/224) 2.86 6.03 49.4 (40/81) 8.79 18.55
O00 Ogawa et al. [22] 2000 29.1 (37/127) 3.69 7.80 66.0 (33/50) 17.47 36.88
V00 Vercellini et al. [23] 2000 43.5 (91/209) 6.93 14.63 60.7 (54/89) 13.90 29.35 Only unilateral
cancer and
left-sided lesions
were considered
O03 Oral et al. [24] 2003 7.7 (14/182) 0.75 1.59 26.3 (5/19) 3.21 6.79
D11 Dzatic-Smiljkovic 2011 11.0 (23/210) 1.11 2.35 33.3 (19/57) 4.49 9.49
et al. [25]
K12 Kondi-Pafiti et al. [26] 2012 5.9 (1/17) 0.56 1.19 0.0 (0/16) 0.00 0.00
S.-W. Guo
22 The Association of Endometriosis with Ovarian Cancer: A Critical Review. . . 369
0.25
K12
O03
0.20
1/sqrt(sample size)
C96
0.15
J97
K72 O00
D11
B89
F97
0.10
V00
R79
V93
A71
-4 -2 0 2 4
log RR
Fig. 22.1 Funnel plot for the 13 log-transformed prevalence-based RRs, using data extracted from
Table 22.1 and assuming a 5 % prevalence of endometriosis in the general population. The dashed
line represents RR 1. The alphabet-numeric combinations are the IDs shown in Table 22.1, and
each ID represents one study. Note that for study K12, a Bayes estimate for binomial distribution
assuming a non-informative prior (uniform distribution) was used, since otherwise the data would
yield a RR of 0
estimates are pretty large. It is unclear as to whether some seemingly high preva-
lence estimates are genuine or a result of ascertainment bias, population idiosyn-
crasy, or chance events.
Based on all published prevalence estimates listed in Table 22.1, one can get a
pooled estimate of prevalence for all histotypes of ovarian cancer weighted by the
sample size, which is 12.9 %, yielding an RR estimate of 1.33 if a prevalence of
10 % is assumed, or 2.81 if a prevalence of 5 % is assumed. For clear cell and
endometrioid ovarian cancers, the pooled estimate of prevalence is 28.0 % and
the corresponding RR estimates are 3.51 and 7.40, respectively, depending on the
endometriosis prevalence.
Note that, since RR rO/r, where rO P(E|O)/[1P(E|O)] and r P(E)/[1
P(E)], r is a constant when P(E) is assumed to be a fixed number (say, 5 %); hence
we can calculate the standard error of log RR, which is equivalent to the standard
error of log rO, or log[P(E|O)]log[1P(E|O)]. By delta method, it is easy to
see that the standard error of log RR is inversely proportional to the squared root of
the sample size n. Hence, we can plot the log RR listed in Table 22.1 against the
squared root of the sample size n reported in the study (Fig. 22.1).
It is interesting to see from Fig. 22.1 that when the estimated log RRs were
plotted against the squared root of the sample size of the study, the seemingly large
RRs seen in Table 22.1, when all placed in the funnel plot in Fig. 22.1, seem to
gravitate to a point close to 1, but perhaps slightly greater than 1.
370 S.-W. Guo
In a typical cohort study, two cohorts or two groups of people, one with and one
without a particular attribute (in our case, women with or without endometriosis),
are identified and followed up longitudinally. The incidence of a particular event
quite often, disease (ovarian cancer, in our case)in the two groups is evaluated
and compared. In this way, whether having the particular attribute (exposure)
would increase or decrease the incidence can be investigated.
Due to constraint in time and resources, cohort studies are seldom conducted
concurrently or truly prospectively. Instead, many cohort studies are conducted
retrospectively. In the latter case, the cohorts are identified and assembled in the
past based on archived records. In this case, the occurrence of the event of interest is
often retrieved from the records as well. While retrospective cohort studies require
much less resources and time, their major disadvantage is their exclusive reliance
on available information, sometimes the subjects own memory. Consequently, the
quality of exposure or disease data can be compromised (e.g., recall bias).
In epidemiology, the outcome is frequently a disease. One common outcome
measure in cohort studies is incidence, or the risk of developing certain disease
within a specified period of time given no occurrence prior to that time period. It
can be expressed either in cumulative incidence (incidence proportion) or incidence
rate with a denominator (called incidence density rate or person-time incidence
rate). In analytical epidemiology, one measure that is used very frequently is the
standardized incidence ratio (SIR), which is a ratio or percentage quantifying the
increase or decrease in incidence of a study cohort with reference to the general
population.
While the SIR provides a succinct measure of the change from the incidence
from the reference population or cohort, it becomes a bit cumbersome when there
are some confounding factors that need to be controlled for, especially in retro-
spective cohort studies. In these circumstances, the rate ratio (RR, also called ratio
of incidence densities) or hazard rate (HR) would be more convenient, and their use
would render the use of some sophisticated statistical models such as the Cox
regression model possible, facilitating elaborate statistical analysis. The RR gives
the ratio of the event rate in the cohort of interest (say, women with endometriosis)
vs. that in the reference group after adjustment for other known confounders. Both
SIR and RR provide a measure of causality (or, rather, association, especially for
retrospective cohort studies) between exposures and outcomes.
So far, seven cohort studies, with varying qualities, on endometriosis-ovarian
cancer link can be identified (Table 22.2). Some of them were population-based and
prospective studies, and others were hospital-based or retrospective cohort studies.
These studies yielded either SIR or RR estimates, along with 95 % confidence
intervals (CIs) (Table 22.2).
22 The Association of Endometriosis with Ovarian Cancer: A Critical Review. . . 371
Table 22.2 Published cohort studies reporting ovarian cancer risk in women with endometriosis
Length
Year of #
of Cohort follow- of
ID Author publication size up cases SIR or RR S.E. 95 % CI
B97 Brinton 1997 20,686 11.4 29 1.92 0.38 1.32.8
et al. [27]
O02 Olson 2002 1,392 13 13 0.78* 0.74 0.25
et al. [28] 2.44
B04 Brinton 2004 1,919 18.8 13 1.26* 0.29 0.62.6
et al. [29]
B05 Brinton 2005 2,491 NA 50 1.69* 0.09 1.27
et al. [30] 2.25
M06 Melin 2006 66,187 12.7 122 1.43 0.133 1.19
et al. [31] 1.71
M07 Melin 2007 63,630 13.4 134 1.37 0.12 1.14
et al. [32] 1.62
K07 Kobayashi 2007 6,398 12.8 46 8.95 2.85 4.12
et al. [33] 15.3
A10 Aris [34] 2010 2,854 10 333 1.6* 0.10 1.12
2.09
S12N Stewart 2012 3.11* (for 0.52 1.13
et al. [35] nulli- 8.57
parous
women)
S12P 1.52* (for 0.76 0.43
parous 6.75
women)
SIR standard incidence ratio, RR rate ratio, SE standard error, CI confidence interval
*SIR or RR column are RR estimates
From these SIRs and their CIs, their standard errors (SEs) can be easily calcu-
lated. Since all the RRs were calculated based on logistic or Poisson regression
models after adjusting for possible confounding factors, the SE of the
log-transformed RR can be calculated based on RRs and their CIs.
In evaluating risk estimatesbe it SIR, RR, or OR if from case-control studies
from various studies, funnel plots are often employed [36]. In funnel plots, risk
estimates, such as RRs or log RRs, are placed on the horizontal axis against some
measure of study size or precision, such as their standard errors, on the vertical axis.
The funnel plot is so named because of its shape: in the absence of selection biases
(such as publication bias and bias in inclusion criteria), true heterogeneity (i.e., size
of effect differs according to study size), and data irregularities (such as poor
methodological design of small studies, inadequate analysis, and fraud), studies
of large or small sample sizes should be more or less symmetrically scattered
around the true log RR. Hence the plot should have the shape of a funnel with
wide opening on the top (due to sampling variability), with the tip of the funnel
pointing to the bottom and centering on the true log RR [36]. The choice of log OR
instead of OR is due to the fact that the standard error of RR is related with the odds
372 S.-W. Guo
Fig. 22.2 Funnel plot for Funnel plot for log SIRs/RRs
the 9 log-transformed SIRs/
K07
RRs, using data extracted
from Table 22.2. The
2.5
dashed line represents
SIR 1 or RR 1.
The alphabet-numeric
2.0
combinations are the IDs
Standard error
shown in Table 22.2,
and each ID represents
1.5
one study
1.0
O02
0.5
S12P
B97
B04
M06
M07A10 S12N
B05
0.0
-2 -1 0 1 2
log SIR/RR estimate
ratio, while the standard error of log OR is purely a function of sample sizes in
different exposure-disease status combinations. The use of log OR also renders ORs
that are greater than 1 or less than 1 symmetric about 1 (0 on the log scale).
When plotting the 9 log-transformed SIRs/RRs against their SEs in a funnel plot
(Fig. 22.2), two features can be noted. First, the plot looks like an asymmetric
funnel, with its tip gravitating towards somewhere near log SIR or log RR 0, i.e.,
SIR 1 or RR 1. Since there is no indication of bias in inclusion criteria or
heterogeneity, this suggests that there may be a publication bias towards favoring
positive studies and higher estimates of odds ratios may well be a chance variation.
In addition, the plot seems to suggest that the true SIR or RR is near 1.
Second, the SIR estimate, K07 in the plot, provided by Kobayashi et al. [33] is
situated at the rim of the funnel, suggesting that while it gave a larger SIR estimate,
it is not a precise estimate.
The paper by Aris [34] gave P(E) 0.107 and P(E|O) 0.14, yielding
RR 1.36 as discussed above. This is very close to the RR estimate of 1.6 reported
by the paper.
the observed association may result from bias, confounding, and/or chance, and the
extent to which they may be described as causal [37]. A case-control study
compares cases (in our case, women with ovarian cancer) and controls (women
without ovarian cancer, say) with respect to their exposure (or lack thereof) or
levels of exposure to a suspecting risk factor (in our case, having endometriosis).
When the risk factor at hand is a dichotomous variable, such as having endometri-
osis or not, the outcome measure is typically the odds of exposure in cases as
compared with that in controls, or OR. When the occurrence of disease is rare, such
as ovarian cancer, the OR estimated from case-control studies becomes an accept-
able approximation to the relative risk. Case-control studies can be a powerful tool
in the investigation of exposure-disease relationship when both the disease and the
exposure are rare. A prime example is the uncovering of the relationship between in
utero exposure to diethylstilbestrol (DES) and vaginal adenocarcinomas in the
daughters [38]. That study was based on just eight cases, each with four matched
controls. Seven out of eight cases had been exposed to DES in utero, but in contrast
none of the 32 controls had.
As with SIR or RR used in cohort studies, the OR or relative risk (RR) used in
case-control studies is the measure of association between disease and exposure.
However, the association could be causal but also could be merely a correlation. For
women with endometriosis (E), or with ovarian cancer (O), the association between
E and O could be due to a variety of scenarios. Figure 22.3 shows several scenarios in
which E and O can be found to be associated. Scenario a is the case where factor
X has a causal relationship with both E and O. E and O are associated simply because
of the presence of the common risk factor X, which may or may not be measured in a
study. It should be noted that E and O share at least one common risk factor, that is,
the incessant ovulation/menstruation. Incessant ovulation or unopposed estrogen
exposure is a known major risk factor for ovarian cancer [39]. Similarly, incessant
menstruation is a known major and consistently identified risk factor for endome-
triosis [40]. Figure 22.4 shows two numerical examples, perhaps somewhat extreme
but nonetheless not unusual cases. In example a, failure to control for the
confounding factor gives rise to spurious results. It is interesting to point out that,
while the OR for the O-E association in each stratum of factor X is 1, the OR for the
association with pooled levels of the factor is 1.35 > 1. Of course, the failure to
control for confounders can also go to the other direction, in which the pooled OR
can be smaller than ORs in each stratum (example b).
In Fig. 22.3, scenario b shows the case in which both factors X and E represent
the same underlying cause for O, such as the case when X and E represent different
aspects of the same factor. Scenario c is the case where E leads to X, which, in turn,
has a causal relationship with O. In the case of E-O association, it is possible that the
diagnosis of endometriosis may result in the use of danazol, an androgenic agent,
which could increase the risk of O in light of the androgen hypothesis of ovarian
cancer [41, 42]. In other words, it could be the exposure to an androgenic agent,
once a popular therapeutic for endometriosis, that increases the risk of ovarian
cancer, not the endometriosis itself. Scenario d is the case in which E-O has a causal
relationship.
374 S.-W. Guo
Fig. 22.3 Diagrams showing 4 different scenarios in which E and O can be found associated
Fig. 22.4 Two hypothetical examples showing that failure to control for confounding can lead to
spurious results. (a) Artificially inflated OR; (b) underestimated OR
The control for shared risk (and/or protective) factors between E and O appears to
be a big challenge in sorting out the relationship between E and O association.
Besides the scenario depicted in Fig. 22.4a, it is known that E and O share
some other common risk/protective factors, for example, the use of oral
376
Table 22.3 Published case-control studies reporting ovarian cancer risk in women with endometriosis
Year of # of # of # case # controls Adjusted
ID Author publication cases controls w/ endo w/ endo OR (95%CI) Remark
N00 Ness et al. [44] 2000 764 1,364 66 85 1.7 (1.22.4)
N02 Ness et al. [45] 2002 3,678 5,268 51 39 1.73 (1.102.71) Originally considered infertility as a
possible risk factor
but also looked at patients with
infertility due to endometriosis
M04 Modugno et al. [46] 2004 2,089 2,943 177 184 1.32 (1.061.65) This study also included some data
from Ness et al. [44]
B04 Borgfeld et al. [47] 2004 27,050 81,254 81 181 1.34 (1.031.75)
M08 Merritt et al. [48] 2008 1,555 1,500 124 87 1.31 (0.971.78)
N08 Nagle et al. [49] 2008 87 1,450 13 87 3.0 (1.55.9) For endometrioid and clear cell
ovarian cancers
R08 Rossing et al. [50] 2008 585 1,293 64 94 1.6 (1.12.3) For invasive ovarian cancer
W09 Wu et al. [51] 2009 604 679 51 37 1.66 (1.012.75)
P12 Pearce et al. [5] 2012 7,911 13,226 738 818 1.46 (1.311.63) Invasive clear cell and endometrioid
ovarian cancers
M13 Merritt et al. [52] 2013 358 2,100 51 165 1.92 (1.362.71) Low-grade serous, endometrioid/
mixed, mucinous and clear cell
E13 Melin et al. [53] 2013 197 402 52 201 0.30 (0.120.74) All cases and controls had endome-
triosis. The factor of
interest was whether or not the
subject had a radical extirpation
of all visible endometriosis
OR odds ratio, SE standard error, CI confidence interval, # numbers, endo endometriosis, w/ with
S.-W. Guo
22 The Association of Endometriosis with Ovarian Cancer: A Critical Review. . . 377
Ness(2000)
Ness(2002)
Study Reference Modugno(2004)
Borgfeld(2004)
Merritt(2008)
Nagle(2008)
Rossing(2008)
Wu(2009)
Pearce(2012)
Merritt(2013)
Summary
Fig. 22.5 Forest plot summarizing the results from 10 case-control studies using data from
Table 22.3
Fig. 22.6 Funnel plot for Funnel plot for log odds ratios
the log ORs, using data
0.4
W09
represents one study N02
0.2
R08
N00M13
M08
B04
M04
0.1
P12
0.0
contraceptives (OC) and age at menarche. These factors are very likely to be
causally associated with both E and O, effectively making them confounding
factors when assessing the E-O association in case-control studies. However,
while some studies did control for OC use, few, if any, controlled for the number
of ovulations/menstrual cycles.
While the mean age at onset of ovarian cancer is about 56 years [4], the onset of
endometriosis occurs mostly and typically during womens reproductive age. This
has been taken as a support for temporality requirement in the Hills 9 criteria of
causality [4]. Indeed, the reported mean age of EAOC cases is often significantly
younger than ovarian cancer patients without endometriosis but older than women
with endometriosis alone [34].
However, the case-control studies published so far have not demonstrated a
clear, graded temporal relationship between endometriosis and ovarian cancer.
Most epithelial tumors take a latent period of at least 15 years to develop [4]. If
endometriosis is a precursor of certain types of ovarian cancer, then it should take a
certain latent period, likely to be shorter than 15 years, for ovarian cancer to
develop. Consequently, one would see that after excluding some cases with
endometriosis, say, 3 years of interval between the diagnosis of endometriosis
and of ovarian cancer, the OR would go up since this would effectively remove
many noisy cases which would dilute the association signal. Unfortunately, we
actually see the opposite from the study by Pearce et al. [5]. Figure 22.7 is a
graphical rendition of its sensitivity analysis (Table 4 in [5]). One can see that once
the cases who had at least 3, 5, or 10 years of interval between the diagnosis of
endometriosis and of ovarian cancer were removed, the OR estimate goes down
considerably.
Given the somewhat consistent but rather moderate increase in OR, some investi-
gators believe that ovarian cancer originates from endometriosis, at least for clear
cell carcinoma and endometrioid adenocarcinoma [54]; hence, screening, labora-
tory, and imaging evaluation should be recommended for early detection of
malignant disorders in women with endometriosis [55]. Some even show that
patients with EAOC actually had a more favorable prognosis [5658]. However,
other studies do not find such evidence [59, 60].
Due to the low incidence of ovarian cancer and the rather moderate increase in
risk, extreme caution needs to be exercised when conveying the message to
the public and also in the context of screening. For clear cell ovarian cancer, the
prevalence is reported to be 13 per 100,000 women (Surveillance Epidemiology
and End Results: http://seer.cancer.gov/statfacts/html/ovary.html, accessed
January 17, 2013). Assuming, perhaps too optimistically, that a screening test exists
that is 99 % sensitive and 99 % specific. Even with this rosy scenario, the
corresponding positive predictive value is a disappointing 3.7 %. In other words,
22 The Association of Endometriosis with Ovarian Cancer: A Critical Review. . . 379
3.0
C
C: Clear-cell
E: Endometrioid
C L: Low-grade serous
2.5
C
OR estimates
C
L
E
2.0
L L
L
E
E
1.5
Exclusions
Fig. 22.7 A graphical rendition of the sensitivity analysis for the association of endometriosis and
risk of invasive ovarian cancer based on timing (time interval) of diagnosis between the two
diseases, as reported by Pearce et al. [5] (their Table 4). When patients with the time interval less
than or equal to 3 years, 5 years, and 10 years are excluded, the decrease in the OR estimate is seen
out of 100 women who have tested positive, fully 96 would have a false positive
result and be likely to be subjected to invasive procedures. Therefore, given the low
incidence and also the moderate increase in OR, it is perhaps premature to talk
about screening.
22.7 Conclusion
From the funnel plots for the SIR/RRs reported from cohort studies and the ORs
from case-control studies, it seems that there may be a publication bias towards
favoring positive studies. In addition, the plots seem to suggest that the true effect
size is very moderate. Yet the vast discrepancy between RRs estimated from
prevalence of endometriosis in women with ovarian cancer and ORs reported
from published case-control studies is puzzling. Since the prevalence is likely an
underestimate, the true RR is likely to be higher, which would highlight the
discrepancy even more. It is unclear as to what factors contributed to the discrep-
ancy. Have all epidemiological studies published so far underestimated the effect
size due to failure to control for some, yet to be identified, confounders or certain
biases of unknown sources? Or have many studies reporting the prevalence of
endometriosis in ovarian cancer somehow overreported, perhaps unwittingly,
380 S.-W. Guo
Acknowledgment I would like to thank Professor Paolo Vercellini for stimulating the discussion
when preparing for this chapter. This research was supported in part by grant 81270676 from the
National Science Foundation of China and financial support from Fudan University and the
Shanghai Key Laboratory of Female Reproductive Endocrine-Related Diseases.
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Chapter 23
Surgical Management of Endometriosis
surgery for endometriomas was associated with less pain after surgery, shorter
hospital stay, and faster recovery compared with laparotomy and that the
complication rate and operative time were similar in the two approaches [5].
A meta-analysis of 27 RCTs comparing the outcome of laparoscopic surgery and
laparotomy for benign gynecologic pathologies also showed that the two
approaches exposed patients equally to complications [6]. These results suggest
that laparoscopic surgery, minimum invasive technique, is feasible and safe as well
as laparotomy and that it should be used as a first-line choice in conservative
surgery for endometriosis.
Lumen
Epithelium of endometrioma
Fibrotic layer
Cortex
Medulla
200mM
Fig. 23.1 Normal ovarian tissue adjacent to the cyst wall of endometrioma. The tissue specimen
of the stripped cyst wall of endometrioma contains normal ovarian tissue. Arrows ovarian follicle
laparoscopy, GnRH agonist treatments, and then laser vaporization of the remains
during a second laparoscopy [47]. Ovarian reserve, determined by AMH and AFC,
was less diminished after the three-step procedure for endometrioma compared with
cystectomy [48, 49]. Donnez et al. also proposed a combined technique consisting of
excision of a large part of the endometrioma and laser vaporization of the remaining
1020 % of the cyst wall close to the hilus. AFC after the combined technique was
similar to that of women without endometriosis or contralateral normal ovaries
[50]. Use of electrosurgical coagulation to achieve hemostasis after stripping the
endometrioma may amplify damage to ovarian reserve. Why ovarian reserve declines
after cystectomy is not precisely understood, but it may relate to the methods used for
hemostasis, including suturing the ovaries and bipolar coagulation [51, 52]. Details of
the studies evaluating ovarian reserve before and after cystectomy are shown in
Table 23.1 [5357].
We know that laparoscopic cystectomy for endometrioma has a negative impact
on ovarian reserve, but we should take into account that the presence of
endometrioma per se is also associated with a decrease in ovarian reserve [58].
Celik 2012 [45] Prospective cohort 65 6 AMH 1.8 1.7 0.7 0.8 <0.001
Ercan 2010 [54] Prospective cohort 64 1 AMH 1.6 1.1 1.4 1.2 NS
Ercan 2011 [55] Prospective cohort 36 3 AMH 2.0 0.4 1.95 0.6 NS
Kitajima 2011 [44] Prospective cohort 19 3 AMH 4.3 3.0 3.0 2.5 NA
Hirokawa 2011 [45] Prospective cohort 38 1 AMH 3.9 2.5 2.1 1.6 <0.001
Hwu 2011 [56] Prospective cohort 31 3 AMH 3.9 0.4 2.01 0.2 <0.01
Lee 2010 [57] Prospective cohort 13 3 AMH 4.7 2.5 3.3 2.1 <0.05
Uncu 2013 [58] Prospective cohort 30 6 AMH 2.8 2.2 1.8 1.3 0.02
Var 2011 [46] RCT 48 6 AFC 5.6 1.1 3.67 1.3 0.001
Note: Values are mean SD. AMH levels are reported in nanograms per milliliter. P < 0.05 was statistically significant
RCT randomized controlled trial, AMH anti-Mullerian hormone, AFC antral follicle counts, NS not statistically significant, NA not available
391
392 I. Deura and T. Harada
Fig. 23.2 Laparoscopic techniques for endometriosis. (a) The adhesion surrounding the left
ovary is freed. (b) The ovarian incision obtained by cyst rupture is enlarged. (c) The cleavage
plane between the cyst wall and normal ovarian tissue is adequately identified. (d) The cyst wall
is bluntly stripped from normal ovarian tissue. (e) Laser vaporization is applied to the cyst
wall close to the left ovarian hilus. (f) The spaces outside the right uterosacral ligament are
opened and the right ureter is separated from the right uterosacral ligaments. Rt. USL the right
uterosacral ligament. (g) The space inside the right uterosacral ligament is opened and the rectum
is separated from the right uterosacral ligaments. The right uterosacral ligament. (h) Sharp
dissection using the scissors is applied between the uterus and the rectum. (i) The obliterated
cul-de-sac is opened
with atraumatic forceps and scissors applying a contralateral traction (Fig. 23.2d).
The boundary between the cyst wall and the ovarian tissue should be exposed
constantly. After removal of the cyst wall, hemostasis is achieved with the pinpoint
bipolar coagulation of bleeding sites on the ovary. The combined technique is
sometimes used for patients with bilateral or multiple endometriomas [50]
(Fig. 23.2e). The vasopressin injection technique may be useful to decrease bleed-
ing after stripping the endometrioma [72], but an inadequate cleavage plane
resulting from hydrodissection may cause the removal of normal ovarian tissue.
The procedures to open an obliterated cul-de-sac are followed. First, the bilateral
ureters are identified. The spaces outside the bilateral uterosacral ligament are
opened and the ureters are separated from the uterosacral ligaments (Fig. 23.2f).
After separation of the ureters, the spaces inside the uterosacral ligaments are
opened and the rectum is separated from the uterosacral ligaments (Fig. 23.2g).
394 I. Deura and T. Harada
The adhesion between the rectum and the uterine cervix can be dissected bluntly
with a contralateral traction when the adhesion is not dense. Sharp dissection is
needed to dissect dense adhesions with fibrotic tissue. Monopolar diathermy with
pure cutting current can dissect dense adhesions surrounding the rectum. Sharp
dissection using the scissors should be used to avoid thermal injury of the rectum
(Fig. 23.2h). After these procedures to open the obliterated cul-de-sac, it is possible
to remove the DIE lesions of the uterosacral ligaments and the rectovaginal septum
(Fig. 23.2i).
23.6 Conclusions
Surgical candidates might include the following patients with endometriosis: those
with severe pain symptoms, large ovarian endometriomas, and infertility caused by
minimal and mild endometriosis.
Surgery for endometriosis has an important role in relieving pain symptoms and
improving fertility by lysing adhesions and removing lesions. However, the optimal
procedure is as yet undetermined because of several controversial issues: the
recurrence of disease and ovarian reserve decline after conservative surgery.
Complete cure of endometriosis is not currently possible by surgery alone, partic-
ularly the conservative procedure. Surgical treatment of endometriosis should be
tailored to the individual according to clinical presentation and personal wishes,
and combined treatment with medical treatment or ART after surgery is needed.
We cannot deal with all patients with endometriosis in the same way.
References
Abstract Endometriosis has been reported as a major cause of pelvic pain. Most
notably, deep infiltrating endometriosis is a very active disease that occurs in 20 %
of women with endometriosis. We have been actively dissecting deep infiltrating
diseased areas within the sacral ligaments around the uterus in order to improve
dysmenorrhea and chronic pelvic pain caused by deep infiltrating endometriosis.
Laparoscopic surgery is an ideal option to treat deep infiltrating endometriosis
involving complete cul-de-sac obliteration due to its minimal invasiveness and
ability to achieve an appropriate depth of surgical field. It is important to prevent
pain recurrence by providing systematic surgery and removing the deep infiltrating
endometriosis safely and widely. To reduce recurrence, it is ideal to provide
postoperative education to maintain the effect of surgery.
24.1 Introduction
Endometriosis occurs in 610 % of women of reproductive age [1]. There are three
histological classifications: peritoneal endometriosis, endometrioma, and deep
infiltrating endometriosis [2]. Treatment is largely divided into either surgical or
pharmacological intervention.
24.2 Subjects
Between January 2008 and July 2012, we performed 622 laparoscopic surgical
resections of endometriosis in patients of childbearing age. Among them,
those with and without deep infiltrating endometriosis (DIE) numbered
369 and 253, respectively. Therefore, 60 % of cases had DIE (Fig. 24.1).
We divided our cohort into four groups, as follows: 372 (age: 33.91 5.75)
cases without postoperative pharmacological treatment, 123 (age: 31.60 5.70)
cases with postoperative low-dose estrogenprogestins (LEP), 35 (age:
30.94 5.97) cases with postoperative treatment with 1 mg of dienogest,
and 92 (age: 33.32 6.23) cases of postoperative treatment with 2 mg of
dienogest (Table 24.1).
41%
59%
Table 24.1 Between January 2008 and July 2012, we performed 622 laparoscopic surgical
resections of endometriosis in patients of childbearing age
Dienogest Dienogest
No postoperative COC treatment treatment
pharmacotherapy treatment 1 mg/day 2 mg/day
(n 372) (n 123) (n 35) (n 92) P-value
Age (years) 33.91 5.75 31.60 5.70 30.94 5.97 33.32 6.23 0.01
Presence of deep infiltrating endometriosis
185 48 8 12 0.01
+ 187 75 27 80
Beecham classification
Stage I 16 1 1 1 0.08
Stage II 209 65 14 26
Stage III 60 21 7 17
Stage IV 87 36 13 48
Laterality of endometriotic cysts
31 5 2 10 0.075
+
Monolateral 196 76 17 40
Bilateral 145 42 15 43
Fig. 24.2 Anatomy of cul-de-sac obliteration. The lateral pararectal space is consistent with the
outside of the uterosacral ligament. The medial pararectal space is consistent with the interstitial
space between the rectum and lateral pararectal space
Especially, adhesion occurs between the uterosacral ligament and either the urinary
tube or rectum, and the urinary tube may be unpredictably shifted; therefore, identi-
fying and separating the urinary tube first may facilitate a safe operation.
In cases of cul-de-sac obliteration, we identify the urinary tube where it crosses
the common iliac artery and trace it down as far as possible.
We locate and unfold the posterior side of the broad ligament of the uterus, and
identify the urinary tube.
Next, we open the LPRS which consists of the internal aspect of the urinary tube
and extraluminal space of the uterosacral ligament.
This leads to separation of the urinary tube from the deep infiltrating endome-
triosis centered around the uterosacral ligament (Fig. 24.3).
Fig. 24.3 LPRS lateral pararectal space. Developing on the right side of the LPRS. The ureter was
separated from the sacral ligament
This space is the MPRS described earlier. Then, we proceed to dissect the MPRS
further anterior toward the posterior part of the vagina.
This leads to complete separation of the deep infiltrating endometriosis centered
around the uterosacral ligament and rectum.
Furthermore, it has become possible to laterally identify part of the anterior
aspect of the rectum.
In this way, dissecting from the lateral side leads to gradual identification of the
rectal outline.
Approaching the right and left lateral sides leads to identification of the remaining
strongest point of adhesion between the posterior uterus and anterior rectum.
At this step, since we have clearly outlined the anterior aspect of the rectum, it is
safe to proceed with dissecting the center part of the rectum.
Dissection of the remaining center part of the rectum leads to separation of the
cul-de-sac obliteration (Fig. 24.4).
Firstly, disseminate the LPRS to separate the ureter and deep infiltrating endome-
triosis centered around the uterosacral ligament. Then, by disseminating the MPRS
to separate the rectum, deep infiltrating endometriosis will be isolated, attaching to
the posterior aspect of the uterus in the shape of an upside-down U.
This isolated deep infiltrating endometriosis will be removed from the posterior
side of the uterus without injuring the deep uterine vein.
Since the urinary tube and rectum have been isolated, it is possible to further
separate the diseased area systematically (Fig. 24.5).
404 Y. Ota et al.
Fig. 24.4 MPRS medial pararectal space. Developing on the right side of the MPRS. The rectum
was separated from the side of the sacral ligament
Fig. 24.5 Isolation of DIE in the shape of a horseshoe. The LPRS and MPRS should be developed
to isolate DIE from the lateral pararectal space. It is shaped like a horseshoe
Fig. 24.6 Air leak test. To check for rectal injury, the air leak test is important. Nelatons catheter
was inserted into the anus and 50 mL of air was pumped into the rectum using a syringe
Fig. 24.7 Air leak test. Checking air leak from the rectum using a laparoscope from the inter-
abdominal side. Sometimes, pin hole rectal injury occurred in the pararectal area. If rectal injury is
overlooked, it will cause serious postoperative complications
406 Y. Ota et al.
Three hundred and seventy-two subjects who did not receive pharmacological
treatment after surgery were divided into two groups: 187 cases with surgical
resection of deep infiltrating endometriosis, and 185 cases without deep infiltrating
endometriosis. We defined recurrence of chocolate cyst of 2 cm or larger by either
ultrasound or MRI, and recurrence of pelvic pain as a VAS score equal to or greater
than the score assessed prior to the operation. The cumulative risk of recurrence was
calculated using the KaplanMeier method, and the log-rank test was performed.
The cumulative risk of recurrence in the group with deep infiltrating endome-
triosis resection was 6 % at 3 years postoperatively, while that of those who did not
require resection was 10 %. No significant difference was observed between these
two groups (Fig. 24.8).
Since these results were compared among groups without postoperative phar-
macological intervention, they indicate adequate resection of deep infiltrating
endometriosis and pain control. Therefore, these results show that our operating
method of systematic resection of deep infiltrating endometriosis is effective.
On the other hand, recurrence of chocolate cyst at 4 years postoperatively was
30 % in both groups (Fig. 24.9).
10%
6%
1.0
No DIE (n = 185)
Recurrece-free subjects (%)
0.4
0.2
Log-rank ^2 = 0.039
NS
0.0 P = 0.844
0 10 20 30 40 50 60
Time after surgery (months)
Fig. 24.8 The effect on pain of systematic DIE and endometrioma excision. Comparison of the
recurrence rate of pain in the presence/absence of deep infiltrating endometriosis (372 women
receiving no medical therapy after surgery). The recurrence rate of pain was 10 % after surgery at
4 years. There was no the significant difference between the No DIE group and Needed DIE
excision group for 4 years. Systematic DIE excision mostly controlled pain recurrence for 4 years
24 Systematic Laparoscopic Surgery for Complete Obliteration of the Cul-de-sac 407
1.0
30%
Recurrece-free subjects (%) 30%
0.8
No DIE (n = 185)
0.6 Needed DIE excision
(n = 187)
0.4
0.2
0.0
0 10 20 30 40 50 60
Time after surgery (months)
Fig. 24.9 The effect on endometrioma recurrence of systematic DIE and endometrioma excision.
Comparison of recurrence rate of endometrioma by the presence/absence of deep endometriosis
(372 women who received no medical therapy after surgery). The recurrence rate of endometrioma
was 30 % at 3 years. There was no significant difference between the No DIE group and Needed
DIE excision group for 4 years. One reason is that surgery is often incomplete to maintain the
ovarian reserve. Endometrioma will recur in 30 % after surgery within 4 years
24.5 Discussion
Treatment for endometriosis is largely divided into two types: surgical intervention
and pharmacological treatment.
Recently, it has become a trend to use pharmacological treatment with either
low-dose estrogenprogestin (LEP) or dienogest, but neither option is practical for
women who are preparing to conceive.
On the other hand, surgery provides rapid pain relief, but, among surgical
methods, the biggest setback of fertility preserving surgery has been the high
recurrence rate. It has been reported that the recurrence rate at 2 to 5 years
postoperatively of the chocolate cyst was 12 to 30 % [510], while the recurrence
rate of pain was 1049 % [5, 8, 11, 12].
Also, it has been clearly reported that deep infiltrating endometriosis has
an association with strong pelvic pain, and in those with disease around the
uterosacral ligament, the odds ratio of chronic pelvic pain was 2.1, while the odds
ratio of dyspareunia was 2.0 [2]. Therefore, we have completely removed deep
infiltrating endometriosis and optimized surgery to prevent ureteral and
rectal injury.
Specifically, in cases with complete cul-de-sac obliteration, we performed LPRS
and MPRS to systemically separate the urinary tube and rectum from deep infil-
trating endometriosis.
408 Y. Ota et al.
With this method, the 4-year postoperative pain recurrence rate was similar in
both groups, that is, almost 15 % for both patients with or without deep infiltrating
endometriosis.
These results are from the study of cases without postoperative pharmacological
intervention and, therefore, our systematic resection was considered effective for
pain control at 4 years postoperatively.
On the other hand, the cumulative risk of recurrence of ovarian chocolate cyst
was 30 % at 4 years postoperatively. Recurrence of pain was considered to be the
recurrence of deep infiltrating endometriosis, and the recurrence rate of ovarian
chocolate cyst was 3 to 5 times higher than that of deep infiltrating endometriosis.
The ovarian reserve needs to be considered in cases of ovarian chocolate cyst
surgery; however, it is possible to enucleate large fields in the case of deep
infiltrating endometriosis. The recurrence rate may be associated with differences
in both operative backgrounds. Therefore, it is important to prevent pain recurrence
by providing systematic surgery and removing the deep infiltrating endometriosis
safely and widely. On the other hand, in cases of ovarian chocolate cyst, we provide
surgery while considering the ovarian reserve. In terms of recurrence, as Vercellini
and others reported that recurrence can be reduced to 37 % at 3 years postopera-
tively by providing combined oral contraceptives (COCs), we think that it is
optimal to provide combined oral contraceptives (COCs) postoperatively [13].
24.6 Conclusion
References
25.1 Introduction
hormonal treatment. However, hormonal drugs cannot be used for those who want
to conceive since the drugs inhibit ovulation. In addition, some pain symptoms are
occasionally resistant to medical treatment. Likewise, hormonal drugs are often not
effective to eradicate developed lesions, such as endometrioma. On the other hand,
surgical treatment is appropriate for removing developed lesions and often effective
to mitigate drug-resistant pain. Widespread use of laparoscopic surgery makes it
less invasive to treat endometriosis by surgery.
Surgical treatment for endometriosis, while having relatively effective outcome
in the short term, has a problem in the long period after surgery. Hysterectomy with
bilateral oophorectomy is radical enough to cure endometriosis, but the procedure is
not acceptable for patients who want to maintain fertility. For these patients,
excision of endometriosis lesions (conservative surgery) is a method of choice.
This treatment often entails recurrence both in symptoms and in histology.
Recently, the concern is gaining traction because more and more women need
conservative surgery due to increasing tendency to childbearing in late
reproductive ages.
This problem, however, is not so new. An incipient report that examined the
recurrence after conservative surgery, while performed by open surgery in those
days, indicated several noticeable findings. The authors followed 423 patients
treated with conservative surgery and found 13.5 and 40.3 % cumulative recurrence
rates in 3 and 5 years, respectively [1]. They found that severity of disease was not
predictive of recurrence and pregnancy delayed recurrence.
There are a number of reports also in the era of laparoscopic surgery. When we
read these papers, we notice the complexity of the problems regarding recur-
rence. Some papers examine recurrence of pain, while others examine recurrence
of endometriosis lesions detected by laparoscopy or imaging. Some papers study
recurrence of endometriosis in general while others study recurrence of a specific
type of endometriosis, e.g., peritoneal lesion, ovarian endometrioma, and deep
endometriosis at the cul-de-sac. The operation methods are either not uniform,
including excision of the cyst (cystectomy) and coagulation or vaporization using
electric devises or lasers. In this chapter, we focus on the recurrence of
endometrioma, which can be easily detected by transvaginal ultrasound, after
laparoscopic excision.
while others define it by the size at least 2 cm [6, 8]. Instinctively, the time after
surgery is related to the recurrence rate. However, unless patients are regularly
followed up, as often with the case of asymptomatic patients, it is difficult to
accurately quantify the time of recurrence. It is thus not obvious in which time
period the patient is most susceptible to recurrence, or whether there is a specific
period of time after which a patient is less likely to develop recurrence. According
to Evers et al. the recurrence rate during the first 5 years gradually increases [12].
This might imply that endometriosis will eventually reappear in all patients who
underwent complete removal of the lesions. In accordance with this notion, a
longitudinal study by Liu et al. showed that the recurrence rates continued to
increase with time, 7.8, 17.7, and 32.3 % at 1, 2, and 3 years, respectively [10].
In contrast, Kikuchi et al. drew a cumulative recurrence rate curve and demon-
strated that the cumulative rate reaches a plateau at around 48 months after
surgery [6]. Further studies with longer follow-up are needed to settle the issue.
Whether the recurrence of endometrioma occurs by de novo or the relapse of
residual endometrioma is poorly understood as well as the origin of endometrioma
per se. To address the issue, the recurrence rate was studied with analysis of the side
in which endometrioma recurred, supposing that recurrence in the contralateral
ovary should be de novo. Exacoustos et al. analyzed 62 patients with recurrent
endometrioma and found that 12 patients had recurrence on the counter-lateral
untreated ovary [13]. Kikuchi et al. also analyzed 26 cases with recurrence after
hemilateral surgery and found that 11 cases had recurrence on the counter-lateral
untreated ovary [6]. These findings suggest that the recurrence of endometrioma is
not totally dependent on the presence of the residual endometrioma but in part on de
novo occurrence. Of course, it cannot be denied that a lesion on the contralateral
ovary undetected by the initial laparoscopy may have progressed after surgery.
Although the difference between de novo and relapse is critical for optimal man-
agement of this disorder, it is impossible at the moment to discriminate clearly the
origin by just looking at and following up the patents and the lesions. Further
ingenious studies seem to be necessary to resolve the issue. Collectively, there is no
doubt that the recurrence of endometrioma after laparoscopic excision is a common
and serious problem, although the actual recurrence rate varies among studies.
Table 25.1 Univariate and logistic regression analysis of factors related to the recurrence of
ovarian endometrioma
Univariate
analysis Logistic regression analysis
Odds ratio
Factors P values P values (95 % confidence interval)
Age (years) NS
Infertility NS
Pain NS
Presence of uterine myoma NS
Presence of adenomyosis NS
Previous medical treatment <0.05 <0.01 2.324 (1.2324.383)
of endometriosis
Previous surgery of ovarian NS
endometrioma
Multiple cysts NS
Largest cyst diameter (cm) <0.05 <0.05 1.182 (1.0041.391)
Bilateral involvement NS
Coexistence of deep endometriosis NS NS 0.456 (0.1981.052)
Revised ASRM score NS NS 1.010 (1.0001.021)
Postoperative medical treatment NS
Postoperative pregnancy <0.05 <0.05 0.292 (0.0280.317)
ASRM American Society for Reproductive Medicine [8]
Until recently, postoperative medical treatment that prevents recurrence has not
been developed successfully. In the face of the fact that postoperative pregnancy
decreases the risk of recurrence, as described above, we came up with the idea if
postoperative oral contraceptives might decrease recurrence. We thus conducted a
before and after study on postoperative OC treatment. In 2005, our clinic introduced
the OC recommendation, that is, at the time of the operation, we provided each
patient with information about OC and the known possible benefits and risks and let
416 Y. Osuga et al.
Eligible Patients
n = 87 (20)
( ) the number
of recurrence
Initial OC take
n = 48 ( 3 )
Fig. 25.1 Recurrence after laparoscopic excision of endometrioma. Flowchart of the patients who
underwent laparoscopic excision of endometrioma after May 2005, for the retrospective cohort
study. A total of 87 patients were followed up for 24 months. Of the 87 patients, 48 started to take
OCs, but 39 did not. Of the 48 patients who had started OC, 34 continued OC for the entire study
period (24 months), whereas 14 discontinued
the patient decide whether or not to take OC. Women who chose to take OC were
given a cyclic (21 days pills/7 days no pill), monophasic OC containing ethinyl
estradiol (0.035 mg) and norethisterone (1.0 mg) (Ortho-M 21, Mochida, Tokyo,
Japan), in the first menstrual cycle after laparoscopy. We then conducted a histor-
ical study to compare the 2-year recurrence rate before and after the introduction of
the OC recommendation. The overall recurrence rate in patients who underwent
laparoscopy after the introduction of the OC recommendation was significantly
lower than that in patients who received laparoscopy before the introduction (18.6
versus 33.1 %, relative risk 0.56, 95 % CI 0.320.97, P < 0.05) [21]. Figure 25.1
depicts the recurrence rate in those who used OC which was significantly lower than
others (non-OC users plus those who quit OC) (2.9 versus 35.8 %, relative risk 0.08,
95 % CI 0.010.48, P < 0.001) [21]. This study indicated that postoperative OC use
reduces the risk of ovarian endometrioma after laparoscopic excision.
In addition to our study, there have been several studies that evaluate the role of
postoperative OC on the recurrence of endometrioma. In contrast to the classical
report showing OC had no effect on disease recurrence when used for up to
6 months [22], all studies that tested postoperative OC for 2 years or more
demonstrated protective effect of OC on recurrence [11, 21, 23]. The different
outcomes between short-term and long-term studies indicate that the duration of
treatment with OC affects recurrence. Indeed, Vercellini et al. compared cumula-
tive recurrence according to the duration of postoperative OC use and found that
women who used OC for less than 12 months were at higher risk of recurrence than
women using OC for 12 months or more [11].
GnRH analogue also has an effect to mitigate recurrence. Jee et al. analyzed the
influence of postoperative GnRH analogue according to the duration of the treat-
ment and found that a 6-month treatment had a beneficial impact compared with a
3- and 4-month treatment and expectant management, although the differences did
25 Prevention of Recurrence After Surgery 417
not reach statistical significance [24]. In another report, patients who received 3
6 months of GnRH analogue therapy alone and patients who received OC after
GnRH analogue were compared. As a result, recurrent endometrioma after
60 months was significantly lower in OC plus GnRH analogue group than in
GnRH analogue alone group (6.1 versus 43.3 %) [25]. It seems that GnRH analogue
treatment longer than 6 months reduces the recurrence, and additional OC treatment
may maintain the effect. However, the benefit of GnRH analogue should be
weighed against the risk of adverse effects associated with estrogen deprivation.
25.3 Summary
References
1. Wheeler JM, Malinak LR. Recurrent endometriosis: incidence, management, and prognosis.
Am J Obstet Gynecol. 1983;146(3):24753.
2. Busacca M, Chiaffarino F, Candiani M, Vignali M, Bertulessi C, Oggioni G, Parazzini
F. Determinants of long-term clinically detected recurrence rates of deep, ovarian, and pelvic
endometriosis. Am J Obstet Gynecol. 2006;195(2):42632.
3. Busacca M, Marana R, Caruana P, Candiani M, Muzii L, Calia C, Bianchi S. Recurrence of
ovarian endometrioma after laparoscopic excision. Am J Obstet Gynecol. 1999;180
(3):51923.
4. Ghezzi F, Beretta P, Franchi M, Parissis M, Bolis P. Recurrence of ovarian endometriosis and
anatomical location of the primary lesion. Fertil Steril. 2001;75(1):13640.
5. Alborzi S, Momtahan M, Parsanezhad ME, Dehbashi S, Zolghadri J, Alborzi S. A prospective,
randomized study comparing laparoscopic ovarian cystectomy versus fenestration and coag-
ulation in patients with endometriomas. Fertil Steril. 2004;82(6):16337.
6. Kikuchi I, Takeuchi H, Kitade M, Shimanuki H, Kumakiri J, Kinoshita K. Recurrence rate of
endometriomas following a laparoscopic cystectomy. Acta Obstet Gynecol Scand. 2006;85
(9):11204.
7. Parazzini F, Bertulessi C, Pasini A, Rosati M, Di Stefano F, Shonauer S, Vicino M,
Aguzzoli L, Trossarelli GF, Massobrio M, Bracco G, Perino A, Moroni S, Beretta
P. Determinants of short term recurrence rate of endometriosis. Eur J Obstet Gynecol Reprod
Biol. 2005;121(2):2169.
418 Y. Osuga et al.
The human ovary contains limited numbers of primordial follicles. These dormant
follicles are activated and also demised incessantly from fetus to the age of
menopause. Loss of nongrowing follicles in womens ovary is age dependent.
Age-related declining curve of ovarian reserve resembles decline of womens
fecundability along with age [1]. However, there are substantial variations in the
decline of reproductive capacity with age [2]. These variations may be defined in
part by several confounding variables. Indeed, Wallace et al. [3] showed that the
estimated number of nongrowing follicle present in the ovaries gets wider variation
after the age of 25 years, which indicates that factors other than age (e.g., smoking,
BMI, parity, stress, systemic disease, etc.) become more important in determining
the rate at which nongrowing follicles are lost through atresia.
Ovarian reserve is currently defined as the number and quality of the follicles left
in the ovary at any given time [4]. The number of remaining primordial follicles in
the ovary may define the number of follicular pool to be selected [3]. The size of
follicular pool is closely related to selectable follicular cohort in stimulation cycles.
Thus, women with decreased ovarian reserve will not be able to produce sufficient
multiple follicular growth in IVF treatment, which is a major determinant of
treatment success [5]. Response to gonadotropin may represent the size of the
cohort of FSH-sensitive follicles in the ovaries and is directly related to the
magnitude of ovarian reserve.
However, since not all the women with infertility receive ovulation induction and
as individual ovarian reserve may show wide variation, tests of ovarian reserve to
identify each reproductive potential may be valuable in particular clinical situations.
In ART settings, testing ovarian reserve before initiation of treatment cycle may be
useful in tailoring stimulation protocol. Ovarian reserve testing may also be useful to
predict womens age at menopause. On the other hand, the markers of ovarian
reserve can be used to evaluate surgical damage to normal ovarian tissue when
one attempts to perform fertility sparing surgery for several indications including
endometriosis. These tests may also be used to evaluate the effects of pharmaceu-
tical chemicals, anticancer drugs, and hormonal agents on ovarian reserve.
There are several clinical tests to estimate ovarian reserve [4]. However, it is still
unclear that these tests can measure quality and quantity of remaining primordial
follicles in ovaries precisely [4, 6]. Counting all the follicles present in serial
26 Ovarian Reserve in Patients with Endometriosis 421
Recently, serum anti-Mullerian hormone (AMH) levels had got wide popularity to
predict ovarian responsiveness in ART settings. AMH is a dimeric glycoprotein,
belongs to the transforming growth factor- family, and is produced solely by the
granulosa cells of the recruited follicles until they become sensitive to FSH [14,
15]. The serum level of AMH declines with age, is menstrual cycle independent,
and is unaffected by gonadotropin or GnRH agonist administration [16]. In
addition, it is very sensitive to changes in ovarian reserve with advancing age
and correlates well with antral follicle count [17]. Therefore, measurements of
serum AMH may be superior to other markers of ovarian reserve, given its
reliability and convenience, to indicate the number of growing follicles and
estimate ovarian follicular reserve. However, although compromised response
to controlled ovarian stimulation can be diagnosed, decreased AMH may not
always be an absolute determinant of womens fecundability. For example,
women with undetectable serum AMH value occasionally become pregnant
[18]. As these limitations may be due to threshold of the present assay system,
development of more sensitive detection method may bring about further under-
standing of the relationship between ovarian reserve testing by AMH and ovarian
functions.
422 M. Kitajima and H. Masuzaki
Infertility is the main concern of women with endometriosis. The cause of infertility
in endometriosis is multifactorial and pathogenesis of endometriosis-associated
infertility remains uncertain [19]. The ovary is one of the frequent anatomical
locations in which endometriosis may develop. Although it is still controversial,
diminished ovarian reserve after surgical intervention to ovarian endometriosis had
been a large clinical concern in infertility care [20]. In addition, ovarian function
may be distorted by the disease itself [21]. On the other hand, some reports argued
that endometriosis is a significant confounding variable that affects the age of
menopause [22, 23]. In this view, endometriosis and its associated events through
womens reproductive life span, such as chronic inflammation, infertility, and
repeated pelvic surgery, may bring about considerable effects on ovarian functions.
Diminished ovarian reserve may be a key element of endometriosis-associated
infertility and possible confounders in health issue in women with endometriosis
at late reproductive stage. Therefore, accurate estimation of ovarian reserve in
women with endometriosis may serve an important clinical role.
Recently, several authors reported time course change in serum AMH value
postsurgery up to 1 year. Sugita et al. [40] analyzed the pattern of sequential
changes in the serum AMH levels within 1 year after cystectomy for
endometriomas. Although serum AMH levels decreased in almost all cases imme-
diately (at 1 month) after surgery, they found that 51 % of patients showed partial
recovery of AMH levels at 1 year after surgery, and in these women, the number of
follicles removed by surgery was significantly more compared to that of women
who showed persistent decrease in AMH value at 1 year after surgery. Celik
et al. [41] also reported serial change in postsurgical AMH levels and its associa-
tions with other clinicopathological factors. They found that serum AMH decreased
significantly at the sixth month (61 %) postoperatively. The FSH level increased
significantly at the sixth week but returned to normal at the sixth month. The AFC
increased significantly at the sixth week and at the sixth month. These results may
indicate that the acute decrease in the serum AMH levels caused by surgical
removal of the ovarian cortex may result in alterations of selectable follicular
cohort, which may affect the values of several ovarian reserve markers after ovarian
cystectomy.
424 M. Kitajima and H. Masuzaki
Endometriosis that develops in other anatomical sites besides the ovary, such as
pelvic peritoneal implants and rectovaginal nodules, is a common feature of
endometriosis, and their pathogenesis may be different from ovarian
endometriomas [52]. Presence of deep infiltrating endometriosis in addition to
ovarian endometriomas negatively affects ovarian reserve in terms of antral follicle
count and number of oocytes retrieved [53]. In infertile patients with minimal/mild
endometriosis, although serum FSH did not show any difference compared to
control women without endometriosis, decreased serum AMH levels were signif-
icantly lower [54]. However, other investigators reported that peritoneal endome-
triosis and ovarian endometriomas per se do not result in lower AMH levels. AMH
levels are decreased in women with previous endometrioma surgery independently
of the presence of current endometriomas [55]. Several confounding variables
affecting ovarian reserve such as severity of intrapelvic inflammation and adhesion
should be taken into account in women with and without ovarian involvement.
426 M. Kitajima and H. Masuzaki
References
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26 Ovarian Reserve in Patients with Endometriosis 429
27.1 Introduction
The fecundity rate in normal couples is in the range of 1520 % per month and
decreases with age of the female partner [1]. In contrast, in women with untreated
endometriosis, monthly fecundability is 210 % [2]. Early studies suggested that
2550 % of infertile women have endometriosis and that 3050 % of women with
endometriosis are infertile [3]. Other reports have confirmed that infertile women
are 6 to 8 times more likely to have endometriosis than fertile women [4].
Women with mid-moderate endometriosis are able to conceive without any medical
or surgical intervention, although the fecundability is significantly lower compared
with women without endometriosis. Multiple studies evaluating patients with
27 Infertility Treatment of Endometriosis Patients 433
Surgery for endometriosis can be both diagnostic and therapeutic. Surgical treat-
ment of endometriosis aims to remove macroscopic endometriosis and restore
normal pelvic anatomy, as well as normal pelvic immunological and hormonal
environment. Surgery, however, may not be able to completely reverse the chronic
inflammatory state or repair severe anatomical distortion and might even negatively
affect fertility by for instance reducing ovarian function. It is therefore important to
weigh up the benefits and the harm when measuring the effect of surgery.
There are few RCT studying the effects of surgery on fecundity in advanced-staged
diseases, and thus, there is insufficient evidence to recommended surgery for the
treatment of infertility in severe disease. Our previous study analyzed pregnancy
outcome in 186 infertile women for a follow-up period of 18 months after laparos-
copy and found that the pregnancy rate for women with minimal/mild endometri-
osis appeared to be the highest, followed by the non-endometriosis group and
the moderate/severe endometriosis group (45.1, 33.8, and 27.6 %, respectively)
[19, 20]. Accordingly, the benefit of laparoscopic surgery in increasing fecundity
seems high in mild endometriosis but limited in severe endometriosis, and alterna-
tive therapies should be considered for those with severe endometriosis.
women with stage III/IV endometriosis who have no other identifiable infertility
factors, surgery may increase fertility [22]; however, one may be aware of a
possible adverse consequence, the loss of viable ovarian cortex [23]. After the
first infertility operation, additional surgery for recurrent endometriosis has only
rarely increased fecundity, and these patients may be better treated by assisted
reproductive technology (ART) [24].
Table 27.1 Pros and cons of expectant and surgical management of endometriomas prior to ART
Expectant Surgery
Pros
Avoid surgery Exclusive malignancy
Lower FSH doses Relieve pain
Increased E2 Reduce the risk of cyst complications
(e.g., rupture)
Increased follicles Facilitate access to oocyte retrieval
Cons
Pain Risk of damage of normal ovarian tissue
No histological diagnosis Reduced number of oocytes collected
Risk of pelvic infection following oocyte retrieval Risks of surgical complication
Multiple studies have shown that prolonged GnRHa treatment before IVF may
improve fertility rates in advanced endometriosis [4244]. A Cochrane review
summarized the findings of these three RCTs, which collectively comprised
165 women with infertility and severe endometriosis. The pretreatment with
GnRHa significantly increased the clinical pregnancy and the live birth rates
compared with no pretreatment (OR 4.28, 95 % CI, 2.009.15 and OR 9.19,
95 % CI, 1.0878.22, respectively). Proposed mechanisms are via increased
retrieved oocytes, higher implantation rates, and reduced preclinical abortions
[45, 46]. Similar to GnRHa, the use of OC has been shown to improve outcomes.
De Ziegler et al. conducted a nonrandomized comparison and suggested that ART
outcomes following 68 weeks of OC in women with endometriosis are comparable
with the outcomes of age-matched controls without endometriosis [47]. Regarding
patients with endometriomas, the effectiveness of GnRHa and OC is rather contro-
versial. A Cochran review in 2010 concluded that administration of GnRHa does
not significantly affect the clinical pregnancy rate when given before ART in
patients with endometriomas, despite the pretreatment improved ovarian response
and increased the number of mature oocytes aspirated. In contrast, the study by
De Ziegler et al. showed improvement using pre-ART continuous OC therapy for
68 weeks even in those with endometriomas. Collectively, it seems that medical
treatment for endometriosis seems to benefit on ART outcomes; however, one
should also be aware that the medical treatment delays the commencement of
ART, and this may also impact the outcome of ART especially in patients with
advanced age.
27.7 Conclusions
Given the abovementioned non-RCT and RCT evidences, the Japanese Society of
Obstetrics and Gynecology (JSOG) published a guideline and recommendations for
the management of women with endometriosis (Fig. 27.1) (JSOG) [48].
27 Infertility Treatment of Endometriosis Patients 439
Fig. 27.1 Algorism for management of infertile patents with endometriosis published by the
Japanese Society of Obstetrics and Gynecology (JSOG)
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6. Koga K, Osuga Y, Taketani Y. Peritoneal environment in endometriosis. Nihon Rinsho.
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7. Schenken RS, Asch RH, Williams RF, Hodgen GD. Etiology of infertility in monkeys with
endometriosis: luteinized unruptured follicles, luteal phase defects, pelvic adhesions, and
spontaneous abortions. Fertil Steril. 1984;41(1):12230.
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integrin expression in the endometrium of women with endometriosis. J Clin Endocrinol
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442 K. Koga et al.
12. Berube S, Marcoux S, Langevin M, Maheux R. Fecundity of infertile women with minimal or
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13. Ozkan S, Murk W, Arici A. Endometriosis and infertility: epidemiology and evidence-based
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14. Hughes E, Brown J, Collins JJ, Farquhar C, Fedorkow DM, Vandekerckhove P. Ovulation
suppression for endometriosis. Cochrane Database Syst Rev. 2007;3, CD000155.
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women: a randomized trial. Gruppo Italiano per lo Studio dellEndometriosi. Hum Reprod.
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16. Jacobson TZ, Duffy JM, Barlow D, Farquhar C, Koninckx PR, Olive D. Laparoscopic surgery
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17. Jacobson TZ, Barlow DH, Koninckx PR, Olive D, Farquhar C. Laparoscopic surgery for
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20. Osuga Y, Koga K, Tsutsumi O, Yano T, Maruyama M, Kugu K, Momoeda M, Taketani
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21. Hart RJ, Hickey M, Maouris P, Buckett W. Excisional surgery versus ablative surgery for
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therapy. J Reprod Med. 1998;43(3 Suppl):26975.
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24. Deaton JL, Gibson M, Blackmer KM, Nakajima ST, Badger GJ, Brumsted JR. A randomized,
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fertnstert.2003.12.028S0015028204006119 [pii].
27 Infertility Treatment of Endometriosis Patients 443
28.1 Introduction
A clinical association between endometriosis and infertility has been suspected for
more than 60 years [1, 2] and confirmed by a large number of studies, although
mechanisms are still debated [3, 4]. Indeed, a study conducted some time ago
reported that between 30 and 50 % of women with endometriosis are infertile and
the prevalence of endometriosis in women with infertility may be between 25 and
50 % [5]. Recently, an opinion by the American Society for Reproductive Medicine
[5] confirmed such an association stating that endometriosis typically present with
pelvic pain, infertility, or an adnexal mass, and may require surgery.
Although decreased fertility in women with endometriosis is today well
established, causes seem to be multifactorial, involving mechanical, molecular,
genetic, and environmental ones [46].
In the event of severe disease causes are usually evident, since pelvic anatomy
becomes distorted and, when this happens, mechanical factors, such as pelvic
adhesions, may directly impair fertility disrupting oocyte release or pickup, altering
sperm motility, disorganizing myometrial contractions, and impairing fertilization
and tubal embryo transport [7].
In 2010, de Ziegler et al. [4] summarized possible mechanisms through which
endometriosis may impair fertility at all stages. These include:
Changes in the composition and characteristics of peritoneal fluid capable of
affecting fertilization and associated with pelvic inflammation. As a result,
sperm motility may be impaired and sperm capacitation inhibited; in addition,
oocytesperm interactions may also be hindered, sperm binding to the zona
pellucida decreased, and the acrosome reaction and spermoocyte fusion
impaired.
A direct effect of endometriosis on oocyte and embryo quality has been pro-
posed, although there is no agreement on this point.
In the presence of an ovarian endometrioma, the age-dependent decline in the
number of ovarian follicles can occur earlier in life.
The eutopic endometrium is altered in women with endometriosis and may
become less receptive because of a local production of estradiol and of proges-
terone resistance.
In conclusion, endocrine and paracrine pathways in human endometriotic
cells that are modulated by estrogens and progestogens, including chemotaxis
and apoptosis, are perturbed in women with endometriosis, contributing to
28 Pregnancy Complications Associated with Endometriosis 447
techniques (MR and ultrasonography) and the two are not both routinely
performed as complementary examinations when endometriosis or adenomyosis
is diagnosed [24]. At any rate, in reviewing obstetrical complications in association
with endometriosis, the presence of alteration in the myometrial JZ is of critical
importance. Therefore, this review will also include studies on pregnancy compli-
cations in women with adenomyosis. After reviewing the obstetrical complications
the underlying mechanisms in the endometrium and myometrial JZ will be
discussed.
28.2.2 Pathogenesis
Invasiveness of severe endometriosis has been suggested as a reason for SHiP, but
there is no apparent correlation between SHiP and stage of endometriosis. An
alternative explanation is that SHiP results from involution of decidualized ectopic
endometrium during pregnancy. In the differentiation of mesenchymal cells,
decidualization represents the point of no return; after which the cellular integrity
becomes inextricably dependent upon sustained progesterone signaling [34]. Falling
progesterone levels not only reverse the decidual phenotype, but also induce the
expression of a gene network that encodes for chemokines, proinflammatory
28 Pregnancy Complications Associated with Endometriosis 449
Table 28.1 Obstetrical complications of pregnancy after ART in women with endometriosis
In comparison with
Nature of complication Naturally conceived ART without endometriosis
Preterm birth Increased (38, 40)a
Preeclampsia Increased (38)
Antepartum hemorrhage Increased (38)
Caesarean section Increased (38)
Placenta previa Increased (50) Increased (50)
SGA birth No increase (38)
Stillbirth No increase (38)
a
Increased only if endometrioma
450 I. Brosens and G. Benagiano
study found in 3,239 women with endometriosis aged between 15 and 45 years no
evidence for an association between endometriosis and subsequent risk of either
pregnancy hypertension or preeclampsia, even after adjusting for age and gesta-
tional age [39]. A retrospective cohort study by Fernando et al. [40] found in
95 singletons ART babies from patients with ovarian endometriomas increased
rates of preterm birth and SGA in comparison with community birth records and
with other forms of endometriosis.
The association between endometriosis and preeclampsia remains controversial.
Unfortunately, the epidemiological studies were not controlled for changes in the
myometrial JZ that plays a critical role in the pathogenesis of pregnancy compli-
cations such as preeclampsia or SGA and to a lesser extent in preterm birth and
preterm premature rupture of the membranes [4143]. It should be noted that a
case-control study of preterm delivery in patients with adenomyosis by Juang
et al. [44] found an increased risk of both spontaneous preterm delivery and preterm
premature rupture of the membranes. This finding underlines the interest to evaluate
potential changes in the myometrial JZ in studies on obstetrical complications in
women with endometriosis.
ART has been suspected for some reason to increase the risk of obstetrical hemor-
rhages including placenta previa, a life-threatening complication of pregnancy. The
retrospective cohort study by Healy et al. [49] compared the prevalence of
28 Pregnancy Complications Associated with Endometriosis 451
requires full transformation of the spiral arteries in the placental bed artery from
their origin in the myometrial junction zone [55]. Recently Brosens et al. [56]
discussed the hypothesis of defective spiral artery remodeling as a cause of major
obstetrical syndromes in endometriosis and adenomyosis. The process is first
characterized by an influx of specialized uterine natural killer cells and
decidualization of the endometrial stroma and its vasculature; then, after implanta-
tion, the interstitial and endovascular trophoblast invasion begins. The final process
results in transformation of the spiral arteries into large uteroplacental arteries in the
endometrium and myometrial JZ. Kim et al. [42, 43] suggested that in the absence
of an adequate decidual effect endovascular trophoblast cell invasion is arrested at
the level of the endometrialmyometrial junction and failed to progress into the
myometrial spiral arteries. This could explain the vascular resistance in preterm
premature rupture of the membranes and preterm birth. Defective endovascular
trophoblast invasion can also be secondary to absence of natural killer cells in the
thickened myometrial JZ. It is generally accepted that natural killer cells, which are
present around spiral arteries in the basal decidua, but not deeper in the
myometrium, play a role in determining the depth of interstitial and endovascular
trophoblast [57, 58].
The question then arises whether the endometrial and myometrial JZ abnormal-
ities associated with endometriosis at the time of implantation represent a risk
factor for the vascular development of the placental bed. Unfortunately, no studies
have yet been performed on biopsies of the placental bed in women with endome-
triosis to investigate the pattern and extent of deep placentation decidualization.
Despite the lack of histopathological investigations, clinical studies have reported
an association between endometriosis and disorders such as preterm delivery that
are associated with defective deep placentation.
patients were pretreated with long-term GnRHa prior to IVF-ET. The contemporary
presence of adenomyosis had apparently no adverse effects on IVF-ET outcomes in
women with endometriosis when pretreated with long-term pituitary
downregulation. In a small case series Tremellen and Russell [62] described four
women, who previously had undergone multiple unsuccessful IVF cycles because
of failure of implantation of good quality embryos who had a coexisting uterine
adenomyosis. The inactivation of adenomyosis by an ultra-long pituitary
downregulation regime promptly resulted in successful pregnancy for all four
women. Given that the majority of fertility clinics are now moving towards the
more patient-friendly antagonist protocol, where patients are not placed in a
hypoestrogen state before commencing ovarian stimulation, the question of
whether adenomyosis has an impact on IVF success rates in GnRHa antagonist-
stimulated IVF treatment needed to be examined. In a recent retrospective cohort
study of 748 patients who underwent a screening transvaginal ultrasound to identify
possible pelvic pathology before commencing their IVF treatment, Talluri and
Tremellen [63] identified 213 patients who were eligible to be included in the
adenomyosis study as they had no obvious underlying uterine or embryonic factors
that could have interfered with successful implantation. The adenomyosis group
had a viable clinical pregnancy rate of 23.6 compared with 44.6 in the
non-adenomyosis group (P 0. 017). This is the first study to clearly describe an
implantation problem in a relatively large cohort exclusively undergoing GnRHa
antagonist cycles in women with ultrasound-diagnosed adenomyosis. Thus, avail-
able evidence supports the idea of a reversibility of myometrial JZ changes by
appropriate medication inducing a prolonged hypoestrogenic period. More studies
will be required to evaluate the beneficial effect of pituitary downregulation during
the cycle of conception on deep placentation in women with adenomyosis and the
potential of this treatment for the prevention of major obstetrical complications
associated with defective deep placentation.
28.5 Conclusions
sonographic studies of Qiu et al. [48]. Finally, the potential effect of prolonged
hypoestrogenic treatment may modify risk factors at the time of conception. It is
clear that, together with studies reporting an increased risk for preterm birth in
women with endometriosis, physicians must be aware that close antenatal follow-
up and early diagnosis of vascular complications are crucial.
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Chapter 29
Malignant Transformation of Endometriosis
Hiroshi Kobayashi
Abstract The association between endometriosis and epithelial ovarian cancer has
been supported by years of epidemiologic research. Approximately 1.0 % of women
with endometriosis may undergo malignant transformation. The malignant transfor-
mation is believed to progress in a stepwise fashion through an intermediary
endometriotic lesion, atypical endometriosis. The greatest risk is associated with
epithelial ovarian cancer of endometrioid and clear cell histology. Endometriosis
and ovarian cancer may share a common pathogenic mechanism: hyperestrogenism,
excess oxidative stress, and inflammation derived from repeated hemorrhage and
iron, contributing to ovarian tumorigenesis. The iron-induced signals can contribute
to carcinogenesis via three processes: step 1, by increasing oxidative stress, which
facilitates the accumulation of somatic mutations, contributing to endometriosis-
associated ovarian cancer initiation; step 2, by creating an estrogen-dependent micro-
environment, supporting endometrioid adenocarcinoma progression; and step 3, by
surviving stressful periods, thereby contributing to clear cell carcinoma progression.
In conclusion, some endometriosis lesions may predispose to ovarian cancer, but
future studies are needed to know the exact mechanisms of endometriosis-associated
ovarian cancer.
29.1 Introduction
Epithelial ovarian cancers have been classified into four major histologic subtypes:
serous (60 %), endometrioid (1020 %), clear cell (<10 %), and mucinous
(<5 %). Serous, endometrioid, clear cell, and mucinous ovarian tumors histologi-
cally resemble the phenotypes of the fallopian tube, proliferative endometrium,
gestational endometrium, and endocervix/gastrointestinal tract, respectively.
29 Malignant Transformation of Endometriosis 459
Comparing the profile of epithelial ovarian cancer between Japanese and Cauca-
sians, clear cell carcinomas (27.6 vs. <10 %) are more common in Japan, possibly
with fewer serous adenocarcinomas (40.7 vs. 60 %). One possibility is that the
Japanese may exhibit a lower proportion of serous adenocarcinoma compared to the
United States population. This may reflect a proportional change.
The investigators have focused on latest knowledge of the genetic and environ-
mental factors affecting the development of epithelial ovarian cancer and outline
future challenges in its pathogenesis research [18]. The time trend analyses of
incidence between 1973 and 2005 in the United States exhibited a decline by
27 % in epithelial ovarian cancer incidence [19, 20]. The incidence trend of ovarian
cancer in the United States is similar to the trends observed in most of the European
countries. In contrast, an increase in epithelial ovarian cancer rates has been
reported in Japan. It is generally accepted that oral contraceptive (OC) use reduces
the risk of ovarian cancer and endometrial cancer. Although the exact reasons for
the higher ovarian cancer incidence rates in Japan are unknown, the trends may be
due to changes in risk factors, such as diet and environmental factors and the low
prevalence of OC use (23 %) in Japan. Although some part of the pathogenesis has
been unveiled, the complete events of genetic and epigenetic changes associated
with epithelial ovarian cancer remain to be identified.
The association between endometriosis and malignant transformation has often
been described in the medical literature. A literature search of MEDLINE (online
PubMed database) was conducted for published articles from 1966 to October 2010
using the keywords endometriosis combined with malignant transformation [21].
The search revealed an increase in reports describing endometriosis-associated
malignant transformation. Overall, more than 400 articles were included following
a process of independent review of each article and six were graded as good
quality [2227]. Numerous epidemiologic studies have shown an association
between endometriosis and ovarian cancer [28, 29]. Epidemiologic studies have
shown an increased risk of epithelial ovarian cancer, especially endometrioid and
clear cell histologies, among women with endometriosis. Brinton et al. examined
the records of 20,686 women hospitalized with endometriosis between 1969 and
1983 [22]. Standardized incidence ratios (SIRs) of cancers were calculated to
compare the cancer incidence of the study cohort with that of the general popula-
tion. After adjustment for age, period, and comorbidities, the hazards ratio was 1.9
for the endometriosis group compared with the control group, indicating that this
cohort had an increased overall risk of ovarian cancer. They also found further
increases in ovarian cancer risk among women with long-standing histories of
ovarian endometrioma (SIR, 4.2) [22]. The same group reported that patients
with endometriosis had the risk (4.19-fold) compared with the general population
if they presented with primary infertility [24].
There is one unique epidemiologic study in Japan, supporting the hypothesis
that ovarian endometrioma increases the subsequent risk of developing ovarian
cancer [30]. A cohort of 6,398 women with a clinically documented ovarian
endometrioma enrolled between 1985 and 1995 in the prefecture-wide Shizuoka
Cohort Study on Endometriosis and Ovarian Cancer Programme has prospectively
460 H. Kobayashi
Although the etiology and the ovarian carcinogenesis still need clarification, the link
between ovarian carcinogenesis and (epi)genetic mutations is well established [18].
The investigators have utilized genome-wide gene expression analysis and associ-
ation studies to identify a specific gene signature distinguishing ovarian cancer from
controls and which served as a molecular signature for complicated histologies.
Recent high-throughput whole genome or targeted sequencing studies have also
identified numerous somatic mutations across the whole exome in a variety of
neoplasms.
High-grade serous ovarian carcinomas develop rapidly without a definite
precursor lesion. Multiple genetic and epigenetic changes are involved in the
molecular pathogenesis of serous adenocarcinoma, for example, high-grade serous
carcinomas are characterized by the tumor suppressor gene TP53 mutations. They
also have germline or somatic loss-of-function mutations in BRCA1 or BRCA2 or
promoter methylation of BRCA1. Mucinous adenocarcinoma most probably arises
via an adenoma-borderline tumor-carcinoma sequence. KRAS mutation (up to
75 %) and lack of TP53 mutations are common in mucinous tumors. Mutations
of Wnt/CTNNB1 (beta-catenin) are common in endometrioid adenocarcinoma.
Loss-of-function mutations of PIK3CA (phosphatidylinositol-4,5-bisphosphate
3-kinase, catalytic subunit alpha)/PTEN (phosphatase and tensin homolog) are
29 Malignant Transformation of Endometriosis 461
Epidemiologic studies account for the fact that endometriosis has been associated
with an increased risk of epithelial ovarian cancer. Genome-wide studies demon-
strate that endometriosis shares several genetic characteristics with ovarian cancer.
The same pathophysiology (immune alterations, excess oxidative stress and inflam-
mation, estrogen excess, and steroid hormone interaction) orchestrates the progres-
sion of endometriosis and its transformation to ovarian cancer. These facts show
that some endometriosis has been shown to undergo malignant transformation.
Ovarian cancer precursor lesions are known to be atypical endometriosis, which
was identified in ~50 % of these histologic subtypes. Many investigators agree that
the potential of invasive epithelial malignancies arises in atypical endometriosis
[3638]. Malignant transformation of endometriosis is not a single entity; rather it
462 H. Kobayashi
29.7 Estrogen
29.8 Conclusion
Step 1
Endometriosis Atypical Endo.
Endometrioid
KRAS, BRAF, ERBB2, CTNNB1, PTEN
PIK3CA, ARID1A, and PPPR1A mutations HNF-1beta-negative Ov. Ca. Mutations of
ER-positive ARID1A
CTNNB1
hyperestrogenism PTEN
PIK3CA
Genetic mutation PPP2R1A
Fig. 29.1 The carcinogenic pathways. Endometriosis may contribute to carcinogenesis via three
processes: step 1, by increasing oxidative stress, which facilitates the accumulation of somatic
mutations, contributing to endometriosis-associated ovarian cancer initiation; step 2, by creating
an estrogen-dependent microenvironment, supporting endometrioid adenocarcinoma progression;
and step 3, by surviving stressful periods via temporarily HNF-1beta overexpression, thereby
contributing to clear cell carcinoma progression
Acknowledgments Grant support: Supported by Grant-in-Aid for Scientific Research from the
Ministry of Education, Science, and Culture of Japan to the Department of Obstetrics and
Gynecology, Nara Medical University (H. Kobayashi).
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Index
CYR61. See Cysteine-rich angiogenic EFI. See Endometriosis fertility index (EFI)
inducer 61 (CYR61) EGF. See Epidermal growth factor (EGF)
Cystectomy, 388, 412 Endocrine-disrupting, 278
of endometrioma, 413 Endocrine-disrupting chemicals
Cysteine-rich angiogenic inducer (EDCs), 280
61 (CYR61), 136 Endocrine-disrupting compounds
Cytokeratin, 217 (EDCs), 297
Cytokines, 50, 68, 88, 90, 278, 432 Endometrial biopsy, 326
Endometrial cancer, 159
Endometrial curettage, 326
D Endometrial-myometrial junction, 452
DAD-1. See Defender against cell Endometriomas, 385, 388, 412417,
death 1(DAD-1) 437, 447, 462
Danazol, 238, 433 Endometriosis, 180
DDT. See Dichlorodiphenyltrichloroethane Endometriosis-associated ovarian cancer
(DDT) (EAOC), 224
Death signal, 180 Endometriosis fertility index (EFI), 349
Decidual changes, 317 Endometriotic cells, 92
Decidualization, 448 Endometriotic cysts, 311, 317319
Deep endometriosis, 435 Endometriotic stromal cells, 128
Deep infiltrating endometriosis (DIE), 198, Endometrium, 252
313, 352, 353, 386, 400, 438 Endotoxin, 88, 89
Deep placentation, 452 Environmental factors, 115
Defender against cell death 1(DAD-1), 259 Enzian, 352
Delta method, 369 Enzian classification, 352
Dendritic cells, 64 Epidermal growth factor (EGF), 131, 253
Density of nerve fibres, 197 receptors, 253
Dental sealants, 298 Epigenetic aberrations, 365
DES. See Diethylstilbestrol (DES) Epigenetic change, 5, 159
Diagnostic laparoscopy, 434 Epigenetics, 107
Diagnostic test, 323 Epigenetics refers, 241
Dichlorodiphenyltrichloroethane (DDT), 281 EP2 receptor, 131
DIE. See Deep infiltrating EP receptors, 132
endometriosis (DIE) Escherichia coli (E. coli), 24
Diethylstilbestrol (DES), 280, 295, 298 Estradiol (E2), 182, 262, 421
Dioxin, 281 Estrogen, 137, 156, 163, 231, 466
DL--amino-3-hydroxy-5-methylisoxazole-4- production, 108
propionic acid receptor (AMPA), 192 Estrogen receptor 1 (ESR1), 150
DNA methylation, 108, 466 Estrogen receptor 2 (ESR2), 150
DNA methyltransferases (DNMTs), 115 Estrogen receptor (ER), 28, 111,
Dorsal root ganglia (DRG), 191 148, 157, 466
Douglas, 10 Estrogen receptor alpha (ER), 111,
Drainage, 388 148, 150, 165, 201, 252, 262
Dual-specificity phosphatase-2 Estrogen receptor beta (ER), 111, 148, 150,
(DUSP2), 129, 137 165, 201, 252, 262
Dyschezia, 386 Estromedin, 132
Dysmenorrhea, 279, 322, 386 Etiology, 126
Dyspareunia, 322, 386 Eutopic endometrium, 55, 92, 128, 180
Excision, 388, 434
Expectant management, 433
E Exposure-disease relationship, 373
E-cadherin, 113 Extracellular signal-regulated
Ectopic endometrium, 4 kinase (ERK1/2), 259
472 Index
F Hemoglobin, 21
Family history, 279 Hemosiderin, 21
Far adenomyosis (FA), 355 Heparin, 240
Far bladder (FB), 355 Hepatocyte growth factor (HGF), 96, 202
Farnesyl pyrophosphate (FPP), 240 Hepatocyte nuclear factor-1 (HNF-1beta),
Far ureter (FU), 356 227, 465
Fas, 184 HIFs. See Hypoxia-inducible factors (HIFs)
Fas ligand (FasL), 183 Hills 9 criteria, 378
Fasudil, 186 Histamine, 193
Fat cells, 298 Histone acetyltransferases, 116
Fat-suppressed T1-weighted imaging, 313 Histone deacetylases (HDACs), 116, 241
Fc receptor, 50 Histone deacetylases inhibitors
Fibroblast growth factor-2 (FGF2), 131 (HDACIs), 116
Fibroblast growth factor-9 (FGF9), 132, 202 Histone H3, 162
Fibromuscular hyperplasia, 314 Histone H4, 162
Fibromyalgia, 283 Histone modifications, 116, 162
Fibrotic plaque, 313 Histopathological criteria, 366
Follicle-stimulating hormone (FSH), 421 Historical score, 349
Follicular pool, 420 HOX10, 330
Food, 298 HOXA10, 5, 113, 115, 237
Functionalis, 252 HSPs. See Heat shock proteins (HSPs)
Funnel plots, 365, 371 Human heat shock protein 70 (HSP70), 25
Human leukocyte antigen (HLA), 54
Human leukocyte antigen G
G (HLA-G), 55, 56
GABA. See Gamma-aminobutyric acid 3-Hydroxy-3-methylglutaryl coenzyme A
(GABA) (HMG-CoA), 239
Gamma-aminobutyric acid (GABA), 192 17-Hydroxysteroid dehydrogenase
Genome-wide (GW), 108 (17-HSD), 15
Genome-wide association study 17--Hydroxysteroid dehydrogenase type
(GWAS), 108 1 (HSD17B1), 149, 164
Genome-wide DNA methylation, 114 17--Hydroxysteroid dehydrogenase type
Geranylgeranyl pyrophosphate (GGPP), 240 2 (HSD17B2), 149, 164, 263
Glutathione peroxidase (GPx), 229 Hypermethylation, 5, 108
Gonadotropin-releasing hormone Hypomethylation, 108
(GnRH), 238 Hypoxia, 95
analogs, 424 Hypoxia-inducible factors (HIFs), 129
Gonadotropin-releasing hormone agonist HIF-, 129
(GnRHa), 185, 433, 438, 453 HIF-1, 129, 137, 230
Gravidity, 293 Hypoxia-inducible transcription
Green tea, 291292 factor-1alpha (HIF1), 95
Growth factors, 88, 278 Hypoxic stress, 128
Guanosine triphosphate (GTPase), 239
I
H IAP. See Inhibitors of apoptosis family (IAP)
Haptoglobin, 16 ICAMs. See Intercellular adhesion molecules
Hazard rate (HR), 370 (ICAMs)
Heat shock element (HSE), 56 IGF-1. See Insulin-like growth factor-1 (IGF-1)
Heat shock factor 1 (HSF1), 56 IME. See Invisible microscopic
Heat shock protein 27 (HSP 27), 202 endometriosis (IME)
Heat shock proteins (HSPs), 25 Immune cells, 64
Heme, 21 Immune clearance, 5
Index 473
Immune surveillance, 67 K
Immunoglobulin-like transcript (ILT), 53 Ki-67, 28, 218
Implantation, 20 Killer-cell immunoglobulin-like
Implantation theory, 4, 218 receptors (KIRs), 52
Incessant menstruation, 373 KIR2DL1, 52
Incidence, 370 KIR2DL4, 52, 55
Incidence rate, 370 Kistner, 342
Inclusion criteria, 371 Knockout, 214
Infertility, 96, 278, 387, 422, 431, 446 KRAS, 225, 462
Inhibin-B, 421, 423
Inhibitors of apoptosis family (IAP), 237
Inhibitors of NF- (NF-) activity, 186 L
Inhibitory killer cell immunoglobulin-like Laparoscopic ablation, 434
receptors (KIRs), 52 Laparoscopic cystectomy, 422
Insulin-like growth factor-1 (IGF-1), Laparoscopy, 322, 385
131, 201, 253 Lateral pararectal space (LPRS), 401, 403
Intercellular adhesion molecule-1 Lauchlan, 10
(ICAM-1), 67, 93 L1 cell adhesion molecule
Intercellular adhesion molecules (L1CAM), 261
(ICAMs), 21 Leak test, 404
Interferon (INF), 50, 90 Letrozole, 169, 170, 171
Interleukin-1 (IL-1), 90 Lipopolysaccharide (LPS), 23
Interleukin-2 (IL-2), 185 Logistic regression, 371
Interleukin-2 (ILT-2), 55 Loss of heterozygosity (LOH), 226227
Interleukin-4 (IL-4), 90 Lovastatin, 240
Interleukin-4 (ILT-4), 55 Low birth weight (LBW), 297
Interleukin-5 (IL-5), 90 Low-dose estrogen-progestin (LEP), 407
Interleukin-6 (IL-6), 4, 90, 230, 288 Luteinized unruptured follicle
Interleukin-8 (IL-8), 4, 90, 93, 95, syndrome, 432
182, 185
Interleukin-10 (IL-10), 9092
Interleukin-12 (IL-12), 90, 93 M
Interleukin-13 (IL-13), 90 Macrophage chemotactic factor-1
Interleukin-17 (IL-17), 90 (MCP-1), 288
Interleukin-23 (IL-23), 90 Macrophage chemotactic protein
Interleukin-33(IL-33), 90 (MCP)-1, 65
Interleukin-1 (IL-1), 68, 128, 137 Macrophage colony stimulating factor
Interstitial cystitis, 283 (MCSF), 90
Intestinal tethering, 313 Macrophage migration inhibitory
Intrauterine devices (IUD), 285 factor (MIF), 165, 289
Intrauterine insemination (IUI), 435436 Macrophages, 62, 90, 91
Invisible (occult) endometriosis, 2629 Magnetic resonance imaging (MRI), 356
Invisible microscopic endometriosis Major histocompatibility complex
(IME), 26 (MHC), 50
In vitro fertilization (IVF), 388, 436 Malignant transformation, 317, 364, 463
Irritable bowel syndrome, 283 MAPK. See Mitogen-activated protein
Ischemia, 95 kinase (MAPK)
IUD. See Intrauterine devices (IUD) Mass spectrometry, 257
IVF. See In vitro fertilization (IVF) Matrix metalloproteinases
(MMPs), 133, 259
MBD1, 110, 162
J MCP-1. See Macrophage chemotactic
Junction zone (JZ), 447, 450452 factor-1 (MCP-1)
474 Index
S T
SAHA. See Suberoylanilide TAK1, 100
bishydroxamine (SAHA) 2,3,7,8-Tetrachlorodibenzo-p-dioxin
Sample size, 369 (TCDD), 281, 295
Sampson, 10, 20, 214 TGF. See Transforming growth
Sampsons retrograde menstruation, 254 factor (TGF)
Sampsons theory, 28 Thalidomide, 238
SCID mice, 214 T-helper cells, 91
Secondary Mullerian system, 10 T-helper cells 1(Th1), 91
Secretoneurin (SN), 195 T-helper cells 2(Th2), 91
Selection biases, 371 Tissue inhibitors of MMPs (TIMPs), 65
Sensory C, 326 TLR4. See Toll-like receptor 4 (TLR4)
Serotonin, 192, 193 3.0 T MR imaging, 312
Serous ovarian carcinomas, 462 TNFRSF1B, 200
SF-1. See Steroidogenic factor-1 (SF-1) Toll-like receptor 4 (TLR4), 24, 25
Siagnostic test, 333 Toll-like receptors (TLRs), 464
Signal-regulated kinase (ERK), 98 TP53, 462
Simvastatin, 240 TPCK. See N-tosyl-L-phenylalanine
Single nucleotide polymorphisms chloromethyl ketone (TPCK)
(SNPs), 159 Transforming growth factor 1
SIR. See Standardized incidence (TGF1), 197
ratios (SIRs) Transforming growth factor
Small for gestational age (TGF), 90, 253
(SGA), 449450 Transgenic mice, 214
Small nerve fibres, 196 Transient receptor potential vanilloid
Smooth muscle actin (SMA), 238 1 (TRPV1), 193, 198
SN-50, 238 Translational activators, 332
SOD2, 230 Translational repression, 330
Soluble FasL, 184 Transplantation, 11, 214
Sorafenib, 290 Tricostatin A (TSA), 109, 242
Sperm, 97 Tubal motility, 96
Spiral artery remodeling, 452 Tumor necrosis factor- (TNF-), 50, 90,
Spontaneous hemoperitoneum, 448 95, 128, 198
Standardized incidence ratios Tumour growth factor, 65
(SIRs), 370, 461 Tyrosine kinase A receptor
Statins, 239, 290 (TrkA), 199, 200
Index 477