Anti Inflammatory Activity of Ormosia Calavensis Azola Bahai Leaf Extract
Anti Inflammatory Activity of Ormosia Calavensis Azola Bahai Leaf Extract
Anti Inflammatory Activity of Ormosia Calavensis Azola Bahai Leaf Extract
Volume: 3 | Issue: 4 | May-Jun 2019 Available Online: www.ijtsrd.com e-ISSN: 2456 - 6470
Anti-Inflammatory Activity of
Ormosia Calavensis Azola (Bahai) Leaf Extract
Jellian B. Pedong1, Melinda C. Getalado1,2
1Department of Physical Sciences, College of Science,
2University Research and Development Services,
1,2University of Eastern, Northern Samar, Philippines
@ IJTSRD | Unique Paper ID – IJTSRD25223 | Volume – 3 | Issue – 4 | May-Jun 2019 Page: 1687
International Journal of Trend in Scientific Research and Development (IJTSRD) @ www.ijtsrd.com eISSN: 2456-6470
METHODOLOGY Test for Alkaloid
A total of two hundred (200) grams of Bahai leaf samples About 5 g of the Bahai leaf was extracted with 25 mL diluted
was collected and used in the entire study. The leaf of the hydrochloric acid. The acidic filtrate was rendered alkaline
Bahai plant were washed and pruned from its shoots using a with ammonium hydroxide and extracted with three
scissor and collected into a beaker. successive portions (each mL of chloroform). The
chloroform extracts was evaporated until incipient dryness
The leaf of the plant was weighed and finely cut. For the and the residues have been dissolved in 2 mL of dilute
extraction procedure, about 200 g of finely cut leaf as soaked hydrochloric acid and tested with Mayer’s and modified
in pure methanol. The flask was covered and the leaf was Dragendorff’s reagent.
soaked overnight. After soaking, the mixture was filtered
through clean cheesecloth to separate the leaf followed by Mayer’s reagent: when added to the residue solution, turbid
filtration using a Buchner funnel. The filtrate was distilled by or white precipitate will be formed; this indicates the
heating to the boiling point of methanol. The solvent-free presence of alkaloids.
leaf extract of Bahai was stored in clean labelled airtight
bottle inside the refrigerator ready for use. The crude leaf Dragendorff’s reagent: when added to the residue solution
extract was measured and transferred into clean bottle. The an orange precipitate was confirmed; this indicates the
extract was ready for testing of secondary metabolites and presence of alkaloids.
anti-inflammatory agent.
Test for Anthraquinones
Test for Physical Properties Leaf extract of about 5 mL was prepared and evaporated to
Color determination was tested on the extract of Bahai leaf incipient dryness over a stem bath. 10 mL of distilled water
using the sense of sight of a total of five respondents. About was added to the residue and was filtered separately with 5
two (2) mL of Bahai leaf extract was measured and put in a mL ammonia solution and shaken, and then it was compared
clear test tube. Then, using the sense of sight, the to the control tube.
respondents described the color of the extract contained in
the test tube. The obtained perceptions of the color from the The Borntrager’s test detects presence of anthraquinones. A
respondents were gathered for proper color determination. red colorization in the lower ammoniacal layer indicates the
presence of anthraquinones.
Odor determination was tested on the Bahai leaf extract
using the olfactory sense of a total of five respondents. About Test for Flavonoids
two (2) mL of Bahai leaf extract was measured in a clear test About 0.5 g of Bahai leaf extract was dissolved in ethanol,
tube. Then, using the sense of smell, the respondents warmed and then filtered. Three pieces of Magnesium chips
described the odor of the leaf extract contained in the Petri was added to the filtrate followed by a few drops of
dish. The obtained perceptions for the odor of the extract concentrated hydrochloric acid. A pink, orange or red to
from the respondents were gathered for proper odor purple is the evidence for the presence of flavonoids.
determination.
Test leucoanthocyanin
pH determination was tested on the Bahai leaf extract using About 5 mL of Bahai leaf extract was deffated by taking up
a pH paper. About 5 mL of the extract were poured in a 10 the residue with 3 mL hexane and 2 mL water or with
mL beaker. Then, a pH paper was dipped into the extracts. petroleum ether. The hexane was discarded or the
After a period of one (1) minute, the pH value was compared petroleum ether extract. Aqueous extract ws diluted with 10
and recorded. The procedure was repeated thrice. Average mL 80% ethanol and were filtered. The filtrate was divided
pH was also computed. into two test tubes, one portion as a control, and then one
portion of the alcohol filtrate was treated with 0.5 mL HCL. A
About Ten (10) mL of the Bahai leaf extract was measured positive result is indicated by the formation of a strong violet
omn an analytical balance, the weight of the leaf extract used color.
(in mL). The procedure was repeated thrice. Average density
was also computed. The equation used is shown below: Test for Saponin
Density = The capillary test was used to determine the presence of
saponins. If the level of the plant extract in the capillary tube
For testing the miscibility of the Bahai leaf extract, three (3) is half or less than in the other tube containing water. The
solvents were used, namely; Hexane, water and acetone. presence of the saponins may be inferred. Load the capillary
About 2 mL of the Bahai extract were put into nine (9) clear tube with plant extract by immersing the tube to a height of
test tubes. Then, two (2) mL each of hexane was poured 10 mm in the plant extract.
intro three test tubes, same goes to another three test tubes, Test for Tannin
but it was poured with two (@) mL each of water, and lastly,
About 5 mL of Bahai leaf extract as added with 3 mL gelatine
the remaining three test tubes with the leaf extracts of Bahai
salt reagent. The formation of the jelly-precipitate indicates
extract was poured with two (2) nL each of acetone solvent.
the presence of tannin.
For one (1) full hour, the nine test tubes were observed to
determine the miscibility of the extract in three () different Test for Terpenoids
solvents. After the given hour, the researcher recorded the About 2 mL of Bahai leaf extract was added 2 mL of acetic
result whether it is (1) miscible or (2) slightly miscible and anhydride and concentrated sulphuric acid. The formation of
(3) not miscible. blue or orange rings indicates the presence of terpenoids.
Secondary Metabolites Screening Test for triterpenes
Test for the secondary metabolites of the Bahai alcoholic The Lieberman-Burchard test was used to test for the
extracts was done. The following procedures were used in presence of triterpene. A range of colors from blue to green,
the tests with three replications:
@ IJTSRD | Unique Paper ID – IJTSRD25223 | Volume – 3 | Issue – 4 | May-Jun 2019 Page: 1688
International Journal of Trend in Scientific Research and Development (IJTSRD) @ www.ijtsrd.com eISSN: 2456-6470
red, pink, purple or violet indicates the presence of the saponins, tannin, terpernoids, triterpene and the ant-
triterpene. inflammatory activity.
Equivalent of 3 g of plant extract was evaporated to incipient The physical properties of Bahai leaf extract were
dryness over a steam bath. Then, cooled to room determined in terms of color, pH, density and solubility. The
temperature. The material was deffated by taking up the color of the Bahai leaf extract was observed and recorded by
residue 6 mL of hexane and 3 mL of water. Partition by the five respondents. The odor was obtained by wafting the
gently shaking the mixture in the test tube. The upper air above the extract. The color of Bahai leaf extract was
hexane layer was pipetted. The treatment was repeated with brownish while the odor of the Bahai leaf extract was
hexane until most of the color pigments has been removed unpleasant. The pH results of Bahai leaf extract was
and discard all the hexane properly. The aqueous layers was determined using the pH paper indicator. The average pH of
treated with 5 mL chloroform and gently shake. Te mixture the Bahai leaf extract is 4.7 which mean that the extract was
was allowed to stand and chloroform extract was dried by acidic. The density was obtained by dividing the mass of the
filtering through about 100 mg anhydrous sodium sulphate extract by volume of the extract. It was done three trials.
held over the dry filter paper. The filtrate was divided in two
portions, use one for control. Other portion was treated with The solubility of Bahai leaf extract was determined using
3 drops of acetic anhydride then1 drop of concentrated three solvents (water, hexane and acetone). The solubility of
sulphuric acid. Observation was done for any immediate Bahai leaf extracts on three different solvents. leaf extracts
color change. were soluble to both water and acetone but insoluble to
hexane. This implies that the extract is polar. All were
Anti-inflammatory test insoluble in hexane, hexane being a non polar solvent.
A total of twenty (20) albino mice were used to determine
the anti-inflammatory activity of the Bahai leaf extract using Table1. Summary results of the physical properties of
carrageenan induced paw edema. Mefenamic acid was used Bahai leaf extract.
as positive control, while water a used as the negative PHYSICAL PROPERTIES RESULTS
control. Miscibility Polar
Color Brownish
Preparation of the Test Animals using Carrageenan Density 0.96 g/mL
Induced Paw Edema Odor Unpleasant
Each albino mice were weighed according to the body and pH 4.7
the mass of mice preferably 25-30g. To the right paw of each
mice 0.05 mL stock solution of carrageenan/ gelatin was Secondary metabolites. The test for alkaloid was done
injected extradermally. Dosage was 2 mL/ gbw of mice, time using Dragendorff’s reagent and Mayer’s reagent. In the test
treatment was recorded for each mice. The researcher used of the leaf extract starting from trials 1 to 3 same results
gelatine powder as alternative for carrageenan, since it is were obtained. There was orange precipitate formed when it
also a product of sewage same as the carrageenan. A 3.25g of was treated with Dragendorff’s and Mayer’s reagent. This
mefenamic acid (Positive control) was dissolved in saline means that alkaloid is present in the Bahai leaf extract.
solution drop by drop until the mefenamic acid was
dissolved. Carrageenan of about 0.25g was dissolved in The modified Bontrager’s test was used to determine the
saline solution. Prepared 50 mL of negative control and 30 presence of Anthraquinone. A red color indicates a positive
ml of pure extract. Nine (9) mice per trial, 27 mice in all and result of Anthraquinone. The results starting from trials 1 to
all identified will be put a tape. 3 show the same results. The leaf extract gives negative
results when it was treated with ammonia. It reveals that the
Testing of the Extract, Positive and Negative control leaf of Bahai do not contain Anthraquinone.
The mice was grouped into three and treated them as
follows: treat 1 (negative control) – inject intradermaly to In the test for flavonoids, three pieces of magnesium chips
the right hind paw 0.05 mL of distilled water per 25g mouse; was added to filtrate followed by a few drops of
treatment 2 (Positive control)- inject intradermaly to the concentrated hydrochloric acid. A pink, orange or red to
right hind paw 0.05 mL of the stock solution of mefenamic purple coloration is the evidence for the presence of
acid per 25g mouse; treatment 3 (plant extract)- administer flavonoids. There was a red colored formed when it was
orally using dropper 0.25 mL of extract per 25g of mice, time added of Mg chips and drops of conc. HCL. This means that
treatment was recorded for each mice, the volume of the flavonoids are present in the Bahai leaf extract.
right paw was measured for every mice using vernier
caliper. One hour after the above treatment, to the right paw Bate-Smith and Metcalf method was used to determine the
of each mice 0.05 mL stock solution of carrageenan / presence of leucoanthocynin. A strong red or violet color
gelatine was injected extradermaly. The researcher used indicates a positive result. Bahai leaf extract treated with 0.5
gelatin powder as alternative for carrageenan, since it is also mL conc. HCL, within minutes there is a change in color
a product of sewage same as the carrageenan. happened, which indicates a positive result.
RESULTS AND DISCUSSION Capillary tubes were used to determine the presence of
The Bahai leaf extract was collected from Scout city, saponins. If the height of the extract is half or less than in the
University of Eastern Philippines, Catarman N. Samar. other tube containing distilled water, then the presence of
Results of the study are herein presented. The physical saponin may be inferred. The results for the saponins test of
characterization in terms of color and odor, pH, density and the Bahai leaf extract revealed that it is positive.
solubility. The secondary metabolites are in terms of
alkaloid, Anthraquinone, flavonoids, leucoanthocyanin, The 10% gelatine salt reagent was used to determine the
presence of tannin. The leaf extracts has a positive result
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International Journal of Trend in Scientific Research and Development (IJTSRD) @ www.ijtsrd.com eISSN: 2456-6470
when it was treated with 10% gelatine salt reagent which In Anti-inflammatory activity the negative control rapidly
indicate a positive result in tannin. increases the thickness of paw with reddish color of
inflammation after treated with carrageenan. Both the
Terpenoid was determined using acetic anhydride and positive control and the plant extract had significant
conc. . In all the results starting from trial 1 to 3 there reduction effect on the inflammation. These results implied
is a formation of blue or orange rings which indicates the that Bahai leaf extract is an effective anti-inflammatory
presence of terpenoid. substitute.
The liberman-Burchard test was used to test for the Table3. Average reading of inflammations thickness over
presence of triterpene. A range of colors from blue to green, a period of 5 hours
red, purple or violet indicates the presence of the Average thickness (mm)
Treatment
triterpene.The results of the triterpene test in Bahai leaf Trial 1 Trial 2 Trial 3
extract from trails 1 to 3 has no color appearance, which (-)control 0.62 0.66 0.66
indicate a negative result. Bahai leaf extract treated with 0.5 (+)control 0.60 0.60 0.53
ml conc. HCl, within minutes there is no change in color Plant sample 0.51 0.46 0.45
happened, which indicates a negative result.
CONCLUSIONS
Table2. Summary results of the secondary metabolite of The Bahai leaf extract has a pH of 4.7, density of 0.96 g/mL.
Bahai leaf extract. Extract is polar. Its color was brownish with unpleasant
SECONDARY odor. The alkaloid, flavonoids, leucoanthocyanin, saponins,
RESULTS INTERPRETATION tannin and terpenoids they are the secondary metabolites
METABOLITES
have present in Bahai extract. Bahai leaf extract is an
Alkaloid White effective anti-inflammatory substitute. Bahai leaf extract was
Mayer’s reagent precipitate comparable with the commercial drug.
Positive
Dragendorff’s Orange
Positive
reagent precipitate References
Clear [1] Bhatt SV, Verma Y. 1993. Antimicrobial of Ormosia
Anthraquinone Negative calavensis extract. An experimentel and clinical
solution
evaluation. Phytother Res; The World Book
Red Encyclopedia, Vol 1: 353.
Flavonoids Positive
coloration
[2] Consolacion Y. Ragasa, Angel Lyn Kristin C. CoJohn A.
Strong Rideout. 2005. Antifungal metabolites from Ormosia
violet calavensis. Natural Product Research, 19(3): 231-237.
Leucoanthocyanin Positive
colored
solution [3] Guevara Q. 2005. A guide book to plant phytochemical
screening. UST Publishing House, Espana, Manila.
Higher than
Saponins Positive
the extract [4] Mahesh PG, Velasco RN, Demigillo JM, Rivera WL. 2010.
Antimicrobial Activity of some medicinal plant against
White jelly plant and human pathogen. World Journal of
Tannin Positive
precipitate Agricultural Science, 4(5): 839-843.
Orange ring Positive [5] Saadabi and Abuzaid. 2011. Antimicrobial Effect of
Terpenoids
precipitate Ormosia calavensis extract in preadipocytes and
adipocytes. National Center for Biotechnology
Clear
Triterpene Negative Information, US National Library of Medicine 8600
solution
Rockville Pike, Bethesda MD.
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