2013 Conrady Et Al
2013 Conrady Et Al
2013 Conrady Et Al
Author manuscript
Mucosal Immunol. Author manuscript; available in PMC 2013 July 01.
Author Manuscript
Abstract
Herpes simplex virus type 1 (HSV-1) is the leading cause of corneal blindness in the developed
world due to reactivation of infectious virus and the subsequent immune response. The innate
response that facilitates viral control in the cornea is currently unknown. In the present study using
a mouse chimera model, we found a bone marrow component is crucial in inhibiting viral
replication and identified inflammatory monocytes (F4/80+ GR1+) as the responsible cell. CCL2
was critical for recruiting inflammatory monocytes, and a loss of this chemokine in CCL2−/− mice
resulted in a loss of viral containment and inflammatory monocyte recruitment. To confirm these
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Introduction
Herpes simplex virus type I (HSV-1) is a double-stranded DNA virus of which 60–90% of
the adult population is seropositive.1 The pathogen is of significant clinical interest due to its
role in inducing morbidity in the central nervous system and cornea.1 HSV-1 is spread
through mucocutaneous contact in which the virus will first establish a lytic infection in
epithelial tissue and progress to invading local sensory fibers. Once the virus has gained
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access to sensory neurons, it is then transported in a retrograde fashion to the cell body
housed in local neural ganglia. In the case of initial oropharyngeal infection, HSV-1 will be
transported to the trigeminal ganglia where it can persist as a latent infection indefinitely.2
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*
Corresponding author: Daniel J.J. Carr, Ph.D., Department of Ophthalmology, DMEI #415, OUHSC, 608 Stanton L. Young Blvd.,
Oklahoma City, OK. 73104 USA; telephone: 405-271-8784; [email protected].
Disclosure: All authors have reviewed the final manuscript and have no conflicts of interest to declare.
Conrady et al. Page 2
sites innervated by divisions of the trigeminal nerve such as the cornea. Recurrent
reactivation can then initiate an inflammatory event that if perpetuated can lead to
significant corneal scaring known as herpetic keratitis (HSK).3 In individuals that have had
an viral reactivation in the cornea, the chance of subsequent reactivations drastically
increases, while cornea graft survival drops.4 Thus, identifying mechanisms to inhibit viral
replication and establishment of HSV latency could drastically reduce the incidence of HSK.
latency. Our lab as well as others have shown that type I interferon (IFN) production is
critical in preventing viral dissemination and subsequent death of the host.7, 8 Thus,
identification of other important innate mechanisms in acute control of viral replication
could be tailored to help inhibit HSV replication during the primary infection and prevent
establishment of latency in the trigeminal ganglia.
IFI-16/p204 has recently been identified as the innate sensor facilitating the acute anti-viral
state of the cornea and other epithelial tissues to HSV by induction of IFN-α production.9 A
loss of this critical protein or its downstream adaptor protein, STING, results in a significant
rise in the viral titer.9 However, the role of infiltrating innate immune cells (e.g. NK cells,
macrophages, and neutrophils) has not been evaluated relative to this sensor during acute
infection. Infiltrating leukocytes including granulocytes, monocytes/macrophages, and NK
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cells are thought to contribute in the resistance to HSV-1 infection by direct or indirect
means.10–12 Specifically, NK cells can directly target HSV-1-infected cells and target them
for cytolysis.13 In a more indirect fashion, compounds released from immune cells such as
nitric oxide (NO) have shown potent antiviral properties in cell culture.14 In the peripheral
nervous system, macrophages secreting TNF-α, NO, and IFN-γ control viral replication
during the primary infection.15
STING−/− mice.16–18 Animal treatment was consistent with the National Institutes of Health
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Guidelines on the Care and Use of Laboratory Animals. All experimental procedures were
approved by the University of Oklahoma Health Sciences Center and Dean A. McGee Eye
Institutes’ Institutional Animal and Care Use Committees. HSV-1 McKrae was passaged as
previously described.7
Plaque Assays
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The corneas of infected mice were harvested at designated times, resuspended in RPMI
1640 media supplemented with 10% FBS, antibiotic/antimycotic, and gentamicin (normal
media, Invitrogen, Gibco), and homogenized with a tissue miser for approximately 20–30
seconds as previously described.7 Supernatant was then clarified with a 10,000 × g spin for
1.5 minutes and serially diluted onto a confluent lawn of HSV-1 susceptible green monkey
kidney (Vero) cells. Plaques were allowed to develop for 24–36 hours and then counted with
the aid of an inverted Zeiss microscope.
Flow cytometry
At the appointed time pi, mice were euthanized and corneas harvested. The corneas were
then subjected to a 1 mg / ml type I collagenase digestion for 1.5–2 hours at 37°C.
Following digestion, single cell suspensions were labeled with monoclonal antibodies and
analyzed using a Coulter Epics XL flow cytometer (BD Biosciences, Beckman Coulter).
The absolute number of cells residing in the cornea was determined as previously
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described.7
iNOS inhibition
Mice were anesthetized and topically treated three times daily with 0.05 mg of iNOS
inhibitor, aminoguanidine (Sigma Aldrich), resuspended in 1X PBS.20 After two days, mice
were infected as previously described. Forty-eight hours pi, mice were euthanized and viral
loads in the cornea were evaluated by plaque assay. Mice were treated starting 2 days prior
to infection up to 48 hours pi.
recombinant EGF (Invitrogen). The cells were then transfected with 2 or 4 pmols of either
nonspecific [5′-UUCUCCGAACGUGUCA CGUTT-3′] or siRNA specific to IFI-16 [5′-
GGUGCUGAACGCAAC AGAAUCAUUU-3′] (Invitrogen, medium GC rich content
backbone) in serum free keratinocyte media. Following a four-hour incubation, serum free
media was removed and replaced with normal media. Twenty-four hours post-transfection,
cells were infected at a multiplicity of infection of .001 of HSV-1 McKrae. Media was then
replaced after 1 hour at 37°C, and the cells and supernatant harvested 24 hours pi.
Macrophage/Neutrophil Depletion
Mice were anesthetized and infected with 1,000 PFU / eye HSV-1. Thirty minutes after
infection, mice were given a 10 µl subconjunctival injection of PBS liposomes, clodronate
liposomes, IgG control antibody, or anti-Ly6G (eBioscience). For clodronate experiments,
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mice were given a second injection 24 hours later. Forty-eight hours pi, viral content was
evaluated by plaque assay. Macrophage/neutrophil depletion was determined by flow
cytometry.
RT-PCR
Corneas were harvested at the indicated time pi, and mRNA transcript was isolated as
previously described.9 iNOS primers were purchased from Origene and the other primer
sequences can be seen below.
Primer Sequence
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mβ-actinF 5'-CTTCTACAATGAGCTGCGTGTG-3'
mβ-actinR 5'-TTGAAGGTCTCAAACATGATCTGG-3'
hβ-actinF 5'-AGCCTCGCCTTTGCCGA-3'
hβ-actinR 5'-CATGTCGTCCCAGTTGGTGAC-3'
hCCL2F 5'-ATGAAAGTCTCTGCCGCCCTTCTGT-3'
hCCL2R 5'-CCTCTGCACTGAGATCTTCCTATTGGTG-3'
m, mouse; h, human
Statistical analysis
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Statistical analysis was conducted using a GBSTAT one-way analysis of variance followed
by the ad hoc Tukey’s t test in experiments with more than two groups. Significance was
defined as a p value less than 0.05 throughout the paper.
Disclosure
All authors have reviewed the final manuscript and have no conflicts of interest to declare.
Results
Resident cells and bone marrow leukocytes contribute to HSV-1 surveillance in the cornea
A functional type I IFN pathway is absolutely required for resistance to HSV-1 replication
in the cornea as previously shown in IFN receptor A1 deficient mice, CD118−/−, in which
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these mice no longer respond to IFN signals and rapidly succumb to viral dissimination.7, 9
To dissect the contribution of resident (corneal stromal and epithelial cells) and bone
marrow (BM)-derived cells in the innate immune response to HSV-1 in the cornea, a
chimera model was chosen to evaluate resistance using WT and highly sensitive CD118−/−
mice. The 48 hour post infection (pi) time point was chosen as this period appears to be the
critical period in which HSV-1 exploits the cornea in the absence of a functional type I IFN
pathway.9 Cornea samples from WTBM>WT and CD118−/−BM>WT mice contained
significantly less virus than WTBM>CD118−/− and CD118−/−BM>CD118−/− mice
highlighting the importance of IFN-responsive corneal resident cells in HSV-1 containment
(Fig. 1). However, WTBM>WT mouse corneas possessed significantly less virus than
CD118−/−BM>WT mouse corneas implicating a role for BM-derived leukocytes in viral
surveillance of the cornea in concert with IFN-responsive resident cells (Fig. 1).
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Resident cell production of CCL2 drives inflammatory monocyte recruitment into the
cornea
To identify the innate leukocyte population(s) and thus, the BM-derived component of viral
surveillance in the cornea of mice that was implicated above, flow cytometric analysis of
select infiltrating leukocytes was performed. Previous published work reported viral
containment in toll-like receptor (TLR) adaptor protein deficient mice mirrored that of WT
controls in the cornea.9 Thus, it was hypothesized the leukocyte population required for
HSV containment would be similar in MyD88−/−, Trif−/−, and WT mice; however,
recruitment of this specific cell type would be severely reduced in CD118−/− corneas due to
their enhanced susceptibility to infection. Forty-eight hours pi, CD118−/− mice exhibited a
gross deficiency in NK cells (CD3− NK1.1+) [Fig. 2C, G] and inflammatory monocytes
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(F4/80+ Gr1+/ CD11b+ Ly6C+ Ly6G−) [Fig. 2D–F] residing in the cornea proper compared
to all other groups. In contrast, CD118−/− mice possessed similar numbers of total
leukocytes (CD45 hi) [Fig. 2A], macrophages (F4/80+ Gr1−) (data not shown), and
neutrophils (F4/80− Gr1+) [Fig. 2B] in the cornea compared to WT, MyD88−/−, and Trif−/−
mice. Taken together, these results suggested a potential role for inflammatory monocytes
and/or NK cells in viral containment in the cornea 48 hours pi, while further suggesting that
the influx of neutrophils was not responsible for HSV surveillance.
In order to identify the predominant signal for inflammatory monocyte and NK cell
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recruitment into the infected cornea, chemokine levels of CXCL1, CCL2, and CCL5, known
chemoattractants for early-responding leukocyte populations,21 were evaluated in TLR
adaptor deficient mice. In the absence of infection, CXCL1, CCL2, and CCL5 were below
the level of detection in the cornea (data not shown). Forty-eight hours pi, there were no
appreciable difference in CXCL1 production amongst all groups (Fig. 3A). Conversely,
CCL5 expression levels were diminished, while CCL2 production was severely abated in
CD118−/− mouse corneas compared to WT, MyD88−/−, and Trif−/− mice (Fig. 3A).
Furthermore, to negate TLR redundancy, DKO mouse chemokine production resembled that
of Trif−/− and MyD88−/− mice (Fig. 3A). Even though CCL2 production was significantly
elevated in TLR adaptor-deficient mice compared to CD118−/− mice, HSV-1 infected
MyD88−/−, DKO, and Trif−/− mice displayed lower levels of CCL2 compared to those of
WT mice (Fig. 3A). We interpret these results to suggest TLR activation contributes to
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CCL2 production but additional pathways play the predominant role in response to HSV-1.
By 72 hours pi, high CCL2 levels began to subside in WT mice and by 120 hours pi,
CD118−/− mice produced significantly more CCL2 in the cornea than WT controls (Fig.
3B).
To localize the source of CCL2 production in the cornea, the previously described mouse
model chimera was utilized. At 48 hours pi, CCL2 levels were significantly elevated in
WTBM>WT and CD118−/−BM>WT mice compared to WTBM>CD118−/− and
CD118−/−BM>CD118−/− mice establishing resident, IFN-responsive corneal cells as the
primary source of CCL2 (Fig. 3C). There was no significant difference between CD118−/−
mouse recipients of WT or CD118−/−BM cells or between WT mouse recipients of WT or
CD118−/−BM cells further emphasizing the importance of the resident population in CCL2
production (Fig. 3C).
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Previously, CCL2 had been shown to mediate NK cell trafficking and activity as well as
macrophage recruitment to sites of infection and inflammation.22–24 However, its role in the
cornea is poorly understood in relation to these cell types. Thus, we sought to elucidate the
contribution of CCL2 production in viral surveillance of the cornea utilizing WT and CCL2
deficient (CCL2−/−) mice. Consistent with our previous results, CCL2−/− mice suffered from
a significant rise in infectious virus in the cornea compared to WT animals at 48 hr pi but
viral levels returned to those of WT controls 120 hrs pi whereas more virus was recovered in
the TG 5 days pi (Fig. 4A, B). Changes in replicating virus levels occurred despite similar
numbers of NK cells (Fig. 4C), neutrophils (Fig. 4E), and total leukocytes in the cornea
proper (data not shown). CCL2 levels were readily detectable in the cornea of WT mice
compared to CCL2−/− mice at this time point (Fig. 4F). Furthermore, the activation status of
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NK cells (expression of NK cell activation marker, CD9425, 26) was similar in CCL2−/− and
WT mice as well as mean fluorescent intensity (Fig. 4D, data not shown). We interpreted
these results to suggest NK cells were not the cell type responsible for immune surveillance
of the cornea 48 hrs pi. Thus, the sensitivity of CCL2−/− mice to HSV-1 infection of the
cornea was assigned exclusively to a gross deficiency in the recruitment of inflammatory
monocytes (F4/80+ Gr1+) to the cornea (Fig. 4E, G). To solidify the critical role of
inflammatory monocytes, subconjunctival injections of clodronate liposomes were used to
show a significant drop in viral containment associated with a loss of inflammatory
monocytes in the cornea proper compared to those of PBS-liposome controls (Fig. 5A–B).
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While the clodronate liposome treatment resulted in a decrease in total neutrophils as well,
previous data shown herein negated their contribution to ocular HSV immunity (Fig. 2).
Additionally, depletion of neutrophils did not result in an enhanced corneal susceptibility to
HSV-1 infection consistent with previous findings in an HSV-1 flank infection model (Fig.
6).27
in the cornea of both infected CD118−/− and CCL2−/− mice were indistinguishable from
uninfected controls (Fig. 5C). In stark contrast, iNOS expression was elevated two-fold in
the cornea of WT animals. Furthermore, gel electrophoresis of RT-PCR products confirmed
a reduction or absence of iNOS in uninfected CD118−/− and mouse corneas (Fig. 5C–D). To
determine the significance of NO production in viral containment, HSV-1 levels were
determined following iNOS inhibition with aminoguanidine.20 Viral titers were significantly
elevated in aminoguanidine-treated mice compared to vehicle-treated WT controls 48 hr pi
(Fig. 5E). Taken together, these results suggested a reduction of inflammatory monocyte
migration into the corneas of CD118−/− and CCL2−/− mice results in the loss of the primary
source of NO production and consequential rise in virus output.
We previously identified the innate sensor, p204/IFI-16, as the crucial regulator of IFN-α in
response to HSV infection of the cornea and thus, hypothesized that signals such as CCL2
were induced by the sensor to recruit the BM arm of innate immunity. To first identify a
potential role of IFI-16/p204 in CCL2 production, CCL2 transcript expression was evaluated
24 hours pi in human corneal epithelial cells (THCE) transfected with nonspecific siRNA or
that directed to IFI-16. A loss of IFI-16 (~70% reduction)9 resulted in a significant reduction
in CCL2 mRNA transcript solidifying a role of the innate sensor in CCL2 production (Fig.
7A). This was confirmed in vivo with mice deficient in the adaptor protein for IFI-16,
STING, in which CCL2 levels mirrored those of CD118−/− mice and were severely
diminished compared to those of WT controls (Fig. 7B). We interpret these results suggested
that signals emanating from p204/IFI-16 were responsible for regulating CCL2 production.
IFI-16 has been shown to activate both NF-κB and IRF-3/IFN cascades, and CCL2 is a
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48 hours pi (Fig. 7D). To then evaluate the role of IFN, THCE cells were treated with
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recombinant IFN-α and CCL2 mRNA was evaluated. CCL2 transcript levels rose 10-fold 6
hours post treatment but returned to near baseline 6 hours later suggesting that IFN alone
could drive CCL2 production (Fig. 7E). To further solidify this point, WT mice topically
treated with rIFN-α had significantly higher levels of CCL2 24 hrs post-treatement than
PBS-treated controls and CD118−/− mice treated with PBS or IFN (Fig. 7F).
Discussion
We have previously shown IFI-16 was responsible for the recognition of HSV in epithelial
tissue and once activated, the sensor drove IRF-3-dependent IFN production critical in
containing viral replication.9 However, we did not explore the contribution of infiltrating
leukocytes.9 In the study described herein, we have identified inflammatory monocytes
(F4/80+ Gr1+) as the BM component of innate immunity within the cornea proper that
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The chemokine CCL2 is widely studied due to its up-regulation in autoimmune diseases,
tumors, and infections.22, 32, 33 CCL2 attributes can be favorable or unfavorable to the host.
From a negative aspect, the chemokine facilitates tumor metastasis and HIV entry into the
CNS.34, 35 However, CCL2 is also needed in muscle repair36 and as we have found, is
required in the cornea to recruit inflammatory monocytes to contain HSV-1 replication.
Additionally, CCL2 production has been shown to be regulated by both TNF-α and STAT-2
signals.37, 38 However, we show the CCL2 upstream promoter contains an IFN-responsive
element, and cells treated with recombinant IFN alone up-regulate CCL2 mRNA. Such
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results imply multiple host signals elicit CCL2 expression dependent upon the initiating
stimulus. We hypothesize the timing of CCL2 production is facilitated by different signals
and is likely tissue-specific. This notion is best observed in CD118−/− mice that lack
downstream IFN signals. Forty-eight hours pi, CD118−/− mice produce very low levels of
CCL2 in the cornea; however, by 5 days pi, CCL2 concentrations are significantly higher in
CD118−/− mice than WT controls. Furthermore, we have previously shown in peripheral
nervous system tissue such as the trigeminal ganglia that there were no identified differences
in CCL2 production comparing HSV-1 infected WT to CD118−/− mice.7 This was in stark
contrast to the brain stem where the only difference in levels of the chemokine was detected
5 days pi when CD118−/− mouse brain stem possessed significantly more CCL2.7 Thus, the
regulation of CCL2 is complex and warrants further inspection. Furthermore, while we
found no precedent for enhanced p65 nuclear translocation in uninfected CD118−/− mice, an
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immediate early gene of HSV-1, ICP0, has been shown to inhibit NF-κB signaling by
reducing specific TLR adaptor protein levels possibly explaining the loss of nuclear p65 in
infected CD118−/− corneas in which viral levels are much higher than WT controls.39
However, we show in mice that recruit inflammatory monocytes with far less efficiency
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(CD118−/− and CCL2−/− mice) than WT animals, such mice suffer from significantly more
virus in the cornea which correlates with a reduction in NO levels. Although NO is likely
only one of several viral replication inhibitors secreted by infiltrating monocytes (e.g. TNF-
α),45 its ability to antagonize viral replication has been previously noted.14, 20, 46 To further
substantiate the role of inflammatory monocytes in innate immunity of the cornea, localized
clodronate depletion was performed and resulted in significantly higher HSV-1 titers. The
one caveat to these results is that the treatment resulted in a loss of neutrophils (F4/80−
Gr1+) as well. However, CD118−/− and CCL2−/− mice have similar numbers of neutrophils
despite significantly more infectious virus in the cornea than those of WT controls.
Additionally, specific depletion of neutrophils in WT mice did not result in an increase in
viral titers recovered from the cornea following HSV-1 infection. This would suggest and be
supported by previous work with herpetic lesions in the skin showing that depletion of
Ly6G+ cells (neutrophils) did not compromise the anti-viral response.27 However, this study
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did suggest the loss of Gr1+ cells (includes both neutrophils and inflammatory monocytes)
resulted in a deficiency in viral containment.27 Thus, the role of neutrophils in HSV
surveillance of the cornea is likely only minimal at best with a notable contribution to ocular
pathology.47 Additionally, viral resistance mediated by NK cells during acute HSV infection
of the cornea is likely minimal compared to that of inflammatory monocytes and a later
response than that of monocytes. This is evident in CCL2−/− mice that are compromised in
viral surveillance 48 hours pi but activity (CD94 expression25) and total numbers of NK
cells does not differ from those of WT controls. Studies implicating NK cells in ocular
surveillance have used depletion techniques to confirm their role within the first ninety-six
hours;44 however, the antibody targeting NK cells (anti-ASGM-1) has also been reported to
reduce inflammatory monocyte recruitment into the cornea proper.44, 48 Furthermore, we
identified that the major contribution of inflammatory monocytes occurs within the first
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forty-eight hours after infection. Thus, it is unclear what role, if any, NK cells contribute to
the earliest phases of the inflammatory monocyte-driven innate immunity within the cornea
and how these responses are orchestrated.
establishment of latency.52 Furthermore, the widely used adjuvant, alum, is known to excite
IRF-3-dependent cascades due to the release of host DNA from dying cells.53 We
hypothesize that this could be due at least in part to IFI-16 activity as a result of the ability
of the protein to respond to both host and viral DNA54 and thus, boost the overall immune
response to the vaccine. Consequently, activating the IFI-16 pathway may be more fruitful
in preventing early viral replication and establishment of latency due to its significant role in
initiating the innate immune response to HSV-1 and HSV-2 in epithelial tissue.9
In conclusion, we propose that IFI-16 activates IFN production and NF-κB signaling
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Acknowledgements
We would like to thank Julie Tran, Sara Moore, Linh Sramek, and Gabby Nguyen for technical support and Drs.
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Helen Rosenberg, Russell Vance, and Shizuro Akira for the CD118−/−, STING−/−, and MyD88−/− mice
respectively. The authors would also like to thank Roche Diagnostics GmbH for clodronate liposomes. Principal
support for the study was from NIH AI053108 to DJJC. Additional support includes an OUHSC Presbyterian
Health Foundation Presidential Professorship award to DJJC, NIH/NCRR P20 RR017703, and a senior investigator
award (to DJJC) from Research to Prevent Blindness.
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Figure 2. CD118−/− mice exhibit gross deficiencies in inflammatory monocyte and NK cell
recruitment into the cornea
Forty-eight hr pi, corneas from HSV-1-infected mice (n = 6–10 corneas / group) were
harvested and subsequently digested in type I collagenase. Single cell suspensions were then
stained with specific monoclonal antibodies to phenotypically identify infiltrating CD45hi
total leukocytes (A), F4/80− Gr1+ neutrophils (B), CD3− NK1.1+ NK cells (C), and F4/80+
Gr1+/CD11b+ Ly6C+ Ly6G− inflammatory monocytes (D–E) by flow cytometry. Results
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Corneas (4–10 corneas / group) were harvested from infected TLR adaptor protein deficient
48 hrs pi (A), WT and CD118−/− mice 72 and 120 hrs pi (B) and chimeric mice (C) 48 hrs pi
and evaluated for specific chemokine production by suspension arrays. Results represent 2–
3 independent experiments and are summarized as the mean pg / mg ± SEM. **, p < .01; *,
p < 0.05 when compared to CD118−/−, WTBM>CD118−/− or CD118−/−BM>CD118−/−.
NSD, no significant difference.
CCL2−/− and WT mice were infected with 1,000 PFU HSV-1 / eye and 48 or 120 hrs pi
corneas (6–8 corneas / group) were harvested and evaluated for viral content in the cornea
(A) and TG (B), leukocyte influx (C–E), and chemokine production (F). Representative
histograms depicted in (G). Values summarize 2 independent experiments and are
represented as the mean ± SEM. **, p < 0.01; *, p < 0.05 when WT and CCL2−/− groups
were compared. Dotted line, limit of detection.
sample can be seen above gel (C) and mean normalized intensity ± SEM of the entire
experiment is expressed in (D). (E) Forty-eight hours pi (1,000 PFU HSV-1 / eye), mRNA
was isolated from whole corneas of WT, CD118−/−, and CCL2−/− mice (n = 3–10) and RT-
PCR was performed to determine the presence of iNOS. The results were normalized to
uninfected (UI) controls and the housekeeping gene β-actin. (D) WT mice were topically
treated with aminoguanidine (0.05 mg) or vehicle three times daily starting 48 hr prior to
infection with HSV-1 (1,000 PFU / eye). Viral titers in the cornea were evaluated 48 hr pi
and compared to vehicle-treated WT mice (n = 6–8 corneas / group). Data is presented as the
mean ± SEM. **, p < 0.01.
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Figure 6. Loss of neutrophils does not enhance corneal susceptibility to HSV infection
WT mice were infected with HSV-1 (1,000 PFU/eye) and then given a subconjunctival
injection of either IgG control or anti-Ly6G antibody. Forty-eight hours pi, viral content (A)
was evaluated by plaque assay and presented as the Log PFU / cornea ± SEM (n = 7 / group,
2 experiments). To confirm depletion, flow cytometry was used to evaluate total neutrophils
(B) residing within the cornea and is representative of 2 independent experiments. Values
are presented as the total neutrophils ± SEM.
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(A) THCE cells were transfected with control or siRNA specific to IFI-16 and infected with
HSV-1. Twenty-four hours pi, mRNA transcript expression was evaluated for CCL2 and
normalized to uninfected controls and the housekeeping gene β-actin. Results are expressed
as the mean ± SEM. (B) STING−/−, CD118−/−, and WT mice (n = 4–8) were infected with
1,000 PFU / eye. Forty-eight hours pi chemokine content was evaluated by suspension array
and is presented as the mean pg / mg ± SEM. (C) Evaluation of the upstream promoter of
CCL2 identified IFN (red) and NF-κB (green) responsive elements. (D) WT, MyD88−/−,
Trif−/−, and CD118−/− mice were infected and NF-κB nuclear translocation was assessed 44
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hours pi by Western blot and compared to uninfected (UI) controls. Image is representative
of 2 independent experiments. (E) THCE cells (n = 9) were treated with rIFN-α and CCL2
mRNA transcript assessed at 6 or 12 hours post-treatment. Results were normalized to
ddH20 controls and the housekeeping gene β-actin. Tx, treatment; IU, units; Values are
expressed as the mean ± SEM of 2–3 independent experiments. (F) To confirm IFN was
responsible for driving CCL2, WT and CD118−/− mice were treated with PBS or 30,0000 U
rIFN-α. Twenty-four hrs later, chemokine levels were assessed and are presented as the
mean ± SEM of 3 independent experiments of 2–3 corneas / group. **, p < 0.01; *, p < 0.05
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IFI-16/p204 binds HSV-1 and subsequently activates IFN production through an IRF-3-
STING-dependent mechanism and NF-κB signaling to induce antiviral proteins such as
protein kinase R and RNAse L as well as CCL2. The localized CCL2 gradient chemoattracts
circulating inflammatory monocytes (iMon) from the blood to the site of infection in the
cornea, where the monocytes secrete NO to further block HSV-1 spread. These finely-tuned
responses (BM and resident) work in concert to orchestrate acute resistance to HSV-1 in the
cornea and are first initiated by p204. iMon, inflammatory monocyte; iNOS+, iNOS
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