Phytochemical Profile and Free Radical Nitric Oxide (NO) Scavenging Activity of Averrhoa Bilimbi L. Fruit Extract
Phytochemical Profile and Free Radical Nitric Oxide (NO) Scavenging Activity of Averrhoa Bilimbi L. Fruit Extract
Phytochemical Profile and Free Radical Nitric Oxide (NO) Scavenging Activity of Averrhoa Bilimbi L. Fruit Extract
DOI 10.1007/s13205-017-0678-9
ORIGINAL ARTICLE
Abstract Averrhoa bilimbi L. belongs to family Oxali- study. A. bilimbi L. fruit extract is also found to have NO
daceae. Traditionally, people use this plant (root, bark, scavenging activity in our study.
leaves and fruits) for treating several illnesses include
itches, boils, syphilis, whooping cough, hypertension, fever Keywords Averrhoa bilimbi L. GC–MS Nitric oxide
and inflammation. The aim of the study was to evaluate the Phenol Phytochemical Antioxidant
nitric oxide (NO) scavenging activity and GC–MS analysis
of A. bilimbi L. fruit extract. Averrhoa bilimbi L. fruits
were collected for the preliminary phytochemical analysis, Introduction
antioxidant scavenging activity and biologically important
compounds were identified by GC–MS analysis. The pre- Everyday 50,000 premature deaths are caused due to
liminary phytochemicals, GC–MS, total phenolic content infectious diseases (Singh et al. 1992; Robin et al. 1998). In
and NO scavenging activity of the plant were analysed. In accordance with the World Health Organization (WHO)
the present investigation, the A. bilimbi L. fruit extract has 2014 diseases like malaria, dengue, leishmaniasis, Lyme
major phytochemicals. Among the 151 compounds iden- disease, tuberculosis, schistosomiasis, and yellow fever,
tified in GC–MS, 15 compounds are found to have diverse carried by mosquitoes, flies, ticks, water snails and air
biological activity. We also observed that the A. bilimbi L. infect one billion people and more than one million people
fruit extract has high level of total phenolic compounds at a will die. Pathogens and diseases become drug resistant and
concentration of 209.25 GAE mg/g. Presence of phenolic the best alternate approach are plants to eliminate diseases
compound apparently explains the antioxidant activity of and therapeutic complications (Fabricant and Farnsworth
the plant. Antioxidant activity of A. bilimbi L. fruit extract 2001). From time immemorial plants are used as medicine
is proven from its high level of NO scavenging activity of to treat diseases. Before the discovery of allopathy humans
potent IC50 value of 108.10. From the above study, it is depended on Ayurveda and homeopathy medicine which
apparent that the A. bilimbi L. fruit extract is a rich source are completely based on plants and herbs. These herbs and
of phytochemicals (natural products) with biological plant materials act as medicine to cure diseases (Nostro
activity. The GC–MS report on this fruit proves that natural et al. 2000). Tribal people depend on the rich diversity of
products have pharmacologically and biologically active forest to overcome the health care needs. Forests have
compounds. A high phenolic content is observed in our excellent vegetation (flora) with high quality of medicinal
value (Kadhirvel et al. 2010). Phytochemicals are the non-
nutrient compounds with beneficial health effects leading
& V. M. Berlin Grace to pharmacological importance and are used in medication
[email protected]; [email protected]
(Nisa et al. 2011). Fruits play major role in human diet due
Jagadish Kumar Suluvoy to their bioactive compounds, natural sugars and organic
[email protected]
acids with relatively high antioxidant activity (Rechkem-
1
Department of Biotechnology, Karunya University, Karunya mer 2001) and are a rich source of vitamins (A, B6, C, E,
Nagar, Coimbatore, Tamil Nadu, India niacin, and thiamine) dietary fibre and minerals
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(Wargovich 2000). Averrhoa bilimbi L. is a long-lived proteins and also deaminate DNA bases (Umamaheswari
green plant which gives edible fruits, belonging to the and Chatterjee 2008). Hence it is essential to reduce the
family Oxalidaceae–Oxalis and grows 16–33ft (5–10 m) in levels of NO in human body. Besides to the reactive oxy-
height, with short trunk dividing into number of upright gen species (ROS) NO was found to be elevated in
branches. It is found throughout Malaysia, Indonesia, inflammation (Baygutalp et al. 2015), colon cancer (Erd-
Myanmar, Bangladesh, Srilanka and common in Southeast man et al. 2009) and pathological conditions like gas-
Asian countries (Rahman et al. 2014). In India it is avail- trointestinal disorders (Cho 2001). The traditional usage of
able mostly in Kerala regions, particularly the Kani tribal the fruits of A. bilimbi L. for anti-inflammation, anti-dia-
traditional healers in Thodu hills region (Kerala) use the betic and anti-hypertensive was highlighted in a report on
raw leaves and fruits of A. bilimbi L. plant for ailments in Malaysian medicinal plants (Harun et al. 2015). A. bilimbi
circulatory system (Xavier et al. 2014) and the local name L. is a rich source of vitamin C, A, B1 and 100 g of edible
is Irumban puli or Pulingi. The parts like bark, leaves, portion was found to have moisture, 94.2–94.7 g; fibre,
seeds, flowers, fruits, roots and the entire A. bilimbi L. plant 0.6 g; ash, 0.31–0.40; protein, 0.61 g; calcium, 3.4 g; iron,
is used as alternative medicine to treat numerous diseases 1.01 mg; riboflavin, 0.32 mg; thiamine, 0.010 mg; ascorbic
majorly as anti-diabetic agent (Kumar et al. 2013). Tradi- acid, 15.5 mg (Zakaria et al. 2007). Ascorbic acid has been
tionally it is used in medication to cure cough, cold, boils, used as standard drug for the estimation of nitric oxide
itches, syphilis, whooping cough, rheumatism and hyper- scavenging activity (singh et al. 2012). As the A. bilimbi L.
tension (Sabiha et al. 2012). A. bilimbi L. shows antimi- fruit extract has also shown a good antioxidant potential
crobial activity against gram positive and gram negative against DPPH (Chauhan and Kapfo 2013), we made an
bacteria (Karon et al. 2011), antifungal activity (Nazmul attempt to analyse its in vitro NO scavenging activity.
et al. 2011), cytotoxic activity (Das et al. 2011), anti-dia-
betic activity (Pushparaj et al. 2000) and the leaves of A.
bilimbi L. could increase the serum insulin level (Patel Materials and methods
et al. 2012) in diabetes mellitus. Administration of A. bil-
imbi L. fruit (toxicity studies) extract 1 g/kg bw did not Chemicals and reagents
affect the mice (Savithri et al. 2009). However, in spite of
having of such a great traditional medicinal use, the All the chemicals used for this experiment were analytical
knowledge on its phytochemical is limited. Few studies of grade purchased from Hi-Media, and SD Fine Chemicals.
phytochemicals on the A. bilimbi L. fruit extract have
shown contradictory data on the presence of alkaloids, Selection and authentication of fruit
tannins, glycosides, saponins and steroids (Sabiha et al.
2012). This study is therefore designed to analyse the Averrhoa bilimbi L. fruit samples were collected from
active phytochemicals present in the fruits of A. bilimbi L. Palakkad district, Kerala, during February to March (2015).
by biochemical tests and GC–MS which may be useful for The fruits of A. bilimbi L. are used as a source of food and
exploring its ethno-pharmacological significance and to medicine by tribes and settler communities of the local
validate scientifically its medicinal properties. Several people. The authentication of the fruit was done by the
previous studies have shown the free radical scavenging Botanical Survey of India (BSI) Coimbatore, Tamilnadu,
activity of A. bilimbi L. fruit extract through DPPH scav- India. The authentication number given by the BSI is BSI/
enging activity (Asna and Noriham 2014; Sabiha et al. SRC/5/23/2015/Tech.
2012). Oxidative stress has major action in human anat-
omy, physiology and diseases like cardiovascular diseases, Extraction of fruit material
diabetes, inflammatory conditions, ageing and cancer
(Joyce 1987). Nitric oxide (NO) plays a major role in The fruits of the A. bilimbi L. were collected, air dried
several in vivo diseases like neuronal signalling, smooth and made into fine powder by the mortar and pestle.
muscle relaxation, regulation of cell-mediated toxicity and Extraction from the fruits was done according to the
inhibition of platelet aggregation (Hagerman et al. 1998). method described by Singh et al. (2012). The powder
Surplus NO is reported to direct DNA fragmentation, cell (25 g) was used for the extraction with 250 ml of
damage and neuronal cell death. NO will not affect the methanol (95% v/v) in a soxhlet apparatus. The remaining
DNA and proteins directly but NO is very unstable in methanol was evaporated using rotary evaporator. The
aerobic condition and produces NO2, N3O4, N2O4 inter- obtained thick semi-solid crude extract was stored at
mediates which are genotoxic, affecting the DNA repair 2–4 °C for further use.
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3 Biotech (2017)7:85 Page 3 of 11 85
The A. bilimbi L. fruit (methanol) extract was analysed for 0.1gm of crude extract of A. bilimbi L. fruit was mixed in
the presence of alkaloid, carbohydrate, glycosides, phenols, distilled water and filtered. Few drops of ferric chloride
flavonoids, saponins, steroids and tannins using the solution were added to the filtrate. The green or blue-green
respective biochemical tests as follows. precipitate indicated the presence of tannins (Trease and
Evans 2002).
Test for alkaloids
Two millilitre of 1% HCl was mixed with 0.1 gm of crude GC–MS analysis on A. bilimbi L. fruit extract
extract and heated slightly. After cooling Wagner’s reagent
and Mayer’s reagent were added to it. The presence of Averrhoa bilimbi L. methanolic fruit extract was sub-
buff-coloured precipitate indicated the presence of alka- jected to gas chromatography–mass spectroscopy (GC–
loids (Sofowora 1993). MS) analysis. The Thermo GC-Trace Ultra VER: 5.0
(Bremen, Germany) and Mass Spectroscopy (MS) MS
DSQ II electron ionization mode with ionization energy
Test for carbohydrates
of 70 eV were used. The temperature of the column was
set to 80–250 °C at 8 °C/min rate. Temperature of 280
Benedict’s reagents was mixed with the 0.1 gm of crude
and 290 °C were set for the GC injector and MS transfer,
extract and slightly boiled, appearance of reddish brown
respectively. Helium was used as a carrier gas at a flow
precipitate indicated the presence of the carbohydrates
rate of 1.0 ml/min. The sample volume of 1 ll was used
(Harborne 1973).
for analysis. By the retention time and mass fragmenta-
tion patterns, the major compounds present in the fruit
Test for flavonoids extract were analysed. The National Institute of Standards
and Technology (NIST) and Wiley 9.0 library was used
The appearance of pink scarlet colour when 0.1 gm of (Sakthivel and Guruvayoorappan 2013) for the detection
crude extract was mixed with few drops of concentrated of compounds.
HCl and Mg pellets indicated the presence of flavonoids
(Odebiyi and Sofowora 1978).
Estimation of phenols in A. bilimbi L. fruit extract
Test for phenols
The total phenolic compounds were estimated using the
Two millilitre of 2% ferric chloride was mixed with the Folin–Ciocalteu reagent (Slinkard and Singleton 1977).
0.1 gm of crude extract and the presence of blue-green or Briefly 0.1 ml of A. bilimbi L. fruit extract of different
black coloration indicated the presence of phenols (Yadav concentrations (50, 100, 150, 200, and 250 lg/ml) were
and Agarwala 2011). mixed with 2 ml of 10% Folin–Ciocalteu reagent and
3 ml of 7% Na2 CO3 was added. This was incubated for
Test for saponins 30 min at room temperature and the absorbance was
measured using UV-spectrophotometer at 760 nm.
Saponin presence was detected by the frothing test. Briefly Gallic acid was used as standard and all the results were
0.1 gm of crude extract was mixed well in water and performed in triplicates. The total phenol concentration
shaken, the appearance of foam indicated the preliminary is expressed in mg gallic acid equivalent (GAE).
evidence for the presence of saponins (Kumar et al. 2009).
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of A. bilimbi L. fruit extract at different concentrations (25, analysis reported the presence of various phenol, flavonoid,
50, 75, 100, 125, and 150 lg/ml) and incubated at 25 °C lipid, alkaloid and acid compounds which were shown in
for 150 min. Then 0.5 ml of the reaction mixture was basic phytochemical screening test.
removed and 1 ml of sulfanilic acid reagent (0.33% in 20%
glacial acetic acid) was added and again incubated for Total phenolic content
5 min at 25 °C. After adding 1 ml of naphthyl ethylene
diamine dichloride (0.1 w/v), the entire reaction mixture The total phenolic content of the A. bilimbi L. fruit extract
was allowed to stand for 30 min at room temperature. The was expressed as gallic acid equivalent in milligram per
absorbance was measured at 540 nm. Similar procedure gram (GAE mg/g) of methanolic fruit extract. The optical
was repeated for the standard ascorbic acid at different density values and its straight line equation (y = mx ? c)
concentrations (25, 50, 75, 100, 125, 150 lg/ml). The same of standard gallic acid is shown in Fig. 2. The total phe-
reaction mixture with the methanol served as control nolic content for 250 lg/ml is found to be 209.25 GAE
(without extract and standard) mg/g.
%Inhibition ¼ ðA0 A1 Þ=A0 100;
Nitric oxide (NO) scavenging activity
where A0 is the absorbance of the control and A1 is the
absorbance of the sample. The A. bilimbi L. fruit extract showed an increased nitric
oxide scavenging activity with increase of concentration of
the extract. Ascorbic acid is used as a standard for deter-
Results mining the IC50 value. Decreased OD values were observed
when the concentration of fruit extract increased. The
Phytochemical analysis percentage of inhibition is shown in Table 4 and the
regression curve for the standard ascorbic acid and A.
Preliminary phytochemical tests revealed the presence of bilimbi L. extract is shown in Fig. 3, respectively. The
alkaloids, carbohydrates, phenols, flavonoids, saponins and IC50 value of A. bilimbi L. fruit extract and standard
tannins (Table 1). The presence of more phenols was ascorbic acid was found to be 108.10 and 85.01 which is
observed in the preliminary screening. The test for sterols shown in Table 4.
answered negative in our study.
Discussion
Phytochemical compounds identified by GC–MS
analysis Traditionally 6000 plants are used in Indian folk and herbal
medication and 3000 plants are in documented medicine
By comparing with the National Institute of Standards and used against diseases (Rajshekharan 2002). Their medici-
Technology (NIST) and Wiley 9.0 library, the major nal value is due to the presence of phytochemicals. Phy-
compounds are identified and listed in Table 2. The GC– tochemicals are also called as natural products, plant
MS chromatogram is shown in Fig. 1. Among the 151 constituents, and secondary metabolites which have
compounds identified, 15 compounds are found to have medicinal properties to which they belong and the mech-
various biological activity which were reported from other anism of action was not known up to the extent. These
studies as mentioned in Table 3. Furthermore, the GC–MS phytochemicals have great potentialities in drug discovery
for various diseases (Justin et al. 2014). The phytochemi-
Table 1 The phytochemicals present in A. bilimbi L. fruit extract. It cals like alkaloid, carbohydrate, glycosides, phenols, fla-
reveals the presence of alkaloids, carbohydrates, phenols, flavonoids, vonoids, saponins, steroids, and tannins compounds are
saponins, tannins. (?? indicates more amount) and the absence of
remedy to cure diseases and fight against different kinds of
steroids (-)
pathogens, as medicine (Hassan et al. 2004). In the current
S. no Test Results investigation, we have revealed the presence of phyto-
1 Alkaloids ? chemicals (alkaloids, carbohydrate, phenols, flavonoids,
2 Carbohydrates ? saponins and tannins) in the A. bilimbi L. fruit extract. Our
3 Phenols ?? result on phytochemical presence is consistent with an
4 Flavonoids ? earlier study (Hasanuzzaman et al. 2013). Moreover, there
5 Saponins ?
may be a region-wise difference in the presence of phy-
6 Steroids -
tochemicals in any plant. Gas chromatographic–mass
spectrometry (GC–MS) is a ubiquitous analytical technique
7 Tannins ?
of choice in toxicology, environmental research, food
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Table 2 continued
S. Compound Empirical Empirical Probability Area
no formula weight %
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3 Biotech (2017)7:85 Page 7 of 11 85
Table 2 continued
S. Compound Empirical Empirical Probability Area
no formula weight %
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Table 2 continued
S. Compound Empirical Empirical Probability Area
no formula weight %
science and forensic research. A. bilimbi L. fruit extract level of total phenolic compounds in the A. bilimbi L. fruit
was separated by GC and the compounds were identified extract at a concentration of 209.25 GAE mg/g. Presence of
by the MS by the NIST and Wiley 9.0 libraries. GC–MS phenolic compound apparently explains the antioxidant
analysis revealed the presence of major biologically active nature of the plant (Awika et al. 2003) due to its hydroxyl
compounds (4H-pyran-4-one, 2,3-dihydro3,5-dihydroxy-6- group which have the scavenging activity (Hatano et al.
methyl, hexadecanoic acid, squalene, erucic acid, oleic 1989). More and more phenolic compounds are used in
acid, chimanine D, boronic acid, 5-hydroxymethyl furfural, foods to improve the nutritional quality (Kahkonen et al.
2-deoxy-D-galactose, mannitol, desulphosinigrin, methyl 1999). The presence of benzenoid ring (hydrophobic) and
pyroglutamate) having medicinal important as given in hydrogen bonding in phenolic hydroxyl groups will help in
Table 3. We have not identified any steroid compounds in interacting with the proteins, accounting for its potent
GC–MS report which correlates well with the results of nature to act as antioxidants (Parr and Bolwel 2002). Free
phytochemical screening. Total phenolic compounds pre- radicals possess high reactive nature; they attack nearest
sent in the A. bilimbi L. fruit extract were determined by stable molecules like lipids, proteins, DNA and carbohy-
Folin–Ciocalteu method. We have also observed a high drates by sneaking their electrons (Patil et al. 2013).
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3 Biotech (2017)7:85 Page 9 of 11 85
Table 4 Percentage inhibition S. no Concentration (lg) Ascorbic acid % inhibition A. bilimbi L. fruit extract %
of A. bilimbi L. fruit extract on on nitric oxide inhibition on nitric oxide
nitric oxide and its comparison
with that of standard ascorbic 1 25 21.10 ± 0.84 2.95 ± 0.88
acid. The IC50 of ascorbic acid
2 50 33.67 ± 0.87 22.9 ± 1.90
is 85.01 and IC50 of A. bilimbi
L. extract is 108.10 3 75 47.15 ± 1.89 32.70 ± 1.60
4 100 56.74 ± 1.22 46.23 ± 1.56
5 125 63.55 ± 4.67 58.84 ± 1.84
6 150 85.14 ± 1.17 71.09 ± 2.67
IC50 85.01 108.10
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85 Page 10 of 11 3 Biotech (2017)7:85
Conclusion Erdmana SE, Rao VP, Poutahidisa T, Rogersa AB, Taylora CL,
Jackson EA, Ge Z, Lee CW, Schauera DB, Wogan GN,
Tannenbaumc SR, Foxa JG (2009) Nitric oxide and TNF-a
From the above study, it is apparent that the A. bilimbi L. trigger colonic inflammation and carcinogenesis in Helicobacter
fruit extract is a rich source of phytochemicals (natural hepaticus-infected, Rag2-deficient mice. PNAS
products) with biological activity. The GC–MS report on 106(4):1027–1032
Fabricant DS, Farnsworth NR (2001) The value of plants used in
this fruit proves that natural products have pharmacologi-
traditional medicine for drug discovery. Environ Health Perspect
cally and biologically active compounds. A high phenolic 1(109):69–75
content is observed in our study. A. bilimbi L. fruit extract Firenzuoli F, Gori L (2001) Herbal medicine today: clinical and
is also found to have NO scavenging activity in our study. research issues. eCAM 4(S1):37–40
Fournet A, Barrios AA, Victoria M, Reynald H, Andre C, Jean B
(1993) 2-Substituted quinoline alkaloids as potential antileish-
Acknowledgements The authors are thankful to the Department of
manial drugs. Antimicrob Agents Chemother 37:859–863
Biosciences and Technology, Karunya University and The South
Hagerman AE, RiedK M, Jones GA, Sovik KN, Ritchard NT,
Indian Textile Research Association (SITRA), Coimbatore.
Hartzfeld PW (1998) High molecular weight plant polyphenolics
(tannins) as biological antioxidants. J. Agric. And Food Chem.
Compliance with ethical standards
46:1887–1892
Harborne JB (1973) Phytochemical methods: a guide to modern
Conflict of interest The author declares that there is no conflict of
technique of plant analysis. Chapman & Hall, London
interest.
Harun NH, Septama AW, Jantan I (2015) Immunomodulatory effects
of selected Malaysian plants on the CD18/11a expression and
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