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* Corresponding author: Chiranjib Bhattacharjee
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IJAMSCR |Volume 1 | Issue 2 | Nov - 2013
www.ijamscr.com
Research article
PHYTOCHEMICAL AND ACUTE TOXICITY STUDY OF LEAVES OF
ARTOCARPUS HETEROPHYLLUS LAM
Chiranjib Bhattacharjee1*and Amitsankar Dutta2
1
Srikrupa Institute of Pharmaceutical Sciences, Vil. Velkatta, Kondapak (Mdl), Dist. Medak,
Siddipet. AP –502 277
2
R.K.Pharmacy College, Kashipur. Surai – Sathiaon, Azamgarh. U. P. 276001
ABSTRACT
Artocarpus heterophyllus Lam commonly known as jack fruit widely distributed in north east India, West
Bengal and south Karnataka. In the present study intended with various phytochemical screening and toxicity
studies were carried out on the leaves of Artocarpus Heterophyllus. The phytochemical study shows the
presences of flavonoids, tannins, saponins and carbohydrates in methanolic and aqueous extracts. In acute
toxicity study both the extract were found safe on a dose of 2000 mg/Kg.
KEYWORDS: Artocarpus heterophyllus, Phytoconsituents, Acute toxicity.
INTRODUCTION
Since the tribal native practitioner of Manipur
claimed that the leaves of Artocarpus heterophyllus
are highly useful in many diseases and we were in
search for an alternative medicine, this claim has
attracted our attention and selected the plant for
present study. On the basis of current literature
survey leaves of Artocarpus heterophyllus Lam,
was taken for phytochemical investigation and
toxicological evaluation. The phytochemicals
present in a plant indicates the possible
pharmacological action whereas the toxicological
study indicates the possible dose to carry out the
pharmacological screening models.
MATERIAL AND METHODS
PLANT MATERIAL
Leaves of Artocarpus heterophyllus Lam were
collected from the forest of Manipur. The plant
was authenticated by Dr. Bisehwori Thongam
(IBSD/MPHRD/M/1008). The shade-dried leaves
were course powdered and this powder were
packed in soxhlet column and extracted
successively with petroleum ether, chloroform,
methanol and aqueous. The extracts were
concentrated under reduced pressure (bath
temperature 50C). The dried extracts were stored
in air tight container in refrigerator below 10C.
EXTRACTION WITH PETROLEUM ETHER
At first the finely ground leaves are placed in a
‘thimble’ made by a strong filter paper in a
chamber of soxhlet (2000ml). The powders are
extracted at 55℃ using round bottomed flask for
72 hrs. The extracting solvent in round bottomed
flask is heated and its vapour condenses in
condenser. The condensed extractant drips into the
thimble containing the crude drug and extract it by
contact. After completion of extraction petroleum
ether is filtered and concentrated to dry mass. The
extract is air dried to remove all traces of the
solvent and the percentage yield was calculated.
Petroleum ether extraction was done to defeating
the powder.
EXTRACTION WITH CHLOROFORM
The marc left after petroleum ether extraction, is
dried and subsequently extracted with 1200ml of
chloroform (61℃) in a soxhlet using round
bottomed flask for 72 hrs. Then the extract is
International Journal of Allied Medical Sciences
and Clinical Research (IJAMSCR)
Chiranjib B, al / Int. J. of Allied Med. Sci. and Clin. Research Vol-1(2) 2013 [78-81]
www.ijamscr.com
79
concentrated by using rotary evaporator and dried
to get the extract.
EXTRACTION WITH ETHANOL
The marc left is again packed in the soxhlet. The
solvent is heated using isomentle and began to
evaporate. For ethanol extraction the temperature
used is 78℃. The extraction had for 18-20 hrs and
after completion of extraction solution was
evaporated to dryness under reduced pressure and
controlled temperature by using rotary evaporator.
EXTRACTION WITH DISTILLED WATER
The marc left after ethanol extraction is placed in a
stopper container with the distilled water (1176ml)
and chloroform (24ml) and allowed to stand at
room temperature for a period of 7 days with
frequent agitation until the soluble matter has
dissolved. Then the mixture is strained, the marc is
pressed and the combined liquids are clarified by
filtration. At last the solution is dried using rotary
evaporator.
PRELIMINARY PHYTOCHEMICALS
SCREENING
The preliminary phytochemical Screening was
carried out on petroleum ether, chloroform,
Ethanolic and aqueous extracts of Artocarpus
heterophyllus for qualitative identification of type
of phytoconstituents present.
DETECTION OF ALKALOIDS
Extracts were dissolved individually in dilute
Hydrochloric acid and filtered.
MAYER’S TEST
Filtrates were treated with Mayer’s reagent
(Potassium Mercuric Iodide). Formation of a
yellow coloured precipitate indicates the presence
of alkaloids.
WAGNER’S TEST
Filtrates were treated with Wagner’s reagent
(Iodine in Potassium Iodide). Formation of
brown/reddish precipitate indicates the presence of
alkaloids.
DRAGENDROFF’S TEST
Filtrates were treated with Dragendroff’s reagent
(solution of Potassium Bismuth Iodide). Formation
of red precipitate indicates the presence of
alkaloids.
HAGER’S TEST
Filtrates were treated with Hager’s reagent
(saturated picric acid solution). Presences of
alkaloids are confirmed by the formation of yellow
coloured precipitate.
DETECTION OF FLAVONOIDS
ALKALINE REAGENT TEST
Extracts were treated with few drops of sodium
hydroxide solution. Formation of intense yellow
colour, which becomes colourless on addition of
dilute acid, indicates the presence of flavonoids.
LEAD ACETATE TEST
Extracts were treated with few drops of lead acetate
solution. Formation of yellow colour precipitate
indicates the presence of flavonoids.
DETECTION OF PHYTOSTEROLS
SALKOWSKI’S TEST
Extracts were treated with chloroform and filtered.
The filtrates were treated with few drops of Conc.
Sulphuric acid, shaken and allowed to stand.
Appearance of golden yellow colour indicates the
presence of triterpenes.
LIBERMANN BURCHARD’S TEST
Extracts were treated with chloroform and filtered.
The filtrates were treated with few drops of acetic
anhydride, boiled and cooled. Conc. Sulphuric acid
was added. Formation of brown ring at the junction
indicates the presence of phytosterols.
DETECTION OF TANNINS
GELATIN TEST
 To the extract, 1% gelatin solution containing
sodium chloride was added. Formation of
white precipitate indicates the presence of
tannins.
 About 0.5 g of the individual extract was
boiled in 10 ml of water in a test tube and then
filtered. A few drops of 0.1% ferric chloride
(FeCl3) was added and observed for brownish
green or a blue-black coloration.
 The alcoholic or aqueous extract is treated with
lead acetate (10%) solution. White precipitate
is formed.
DETECTION OF SAPONINS
FROTH TEST
Extracts were diluted with distilled water to 20ml
and this was shaken in a graduated cylinder for 15
minutes. Formation of 1 cm layer of foam indicates
the presence of saponins.
FOAM TEST
Chiranjib B, al / Int. J. of Allied Med. Sci. and Clin. Research Vol-1(2) 2013 [78-81]
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80
0.5 gm of extract was shaken with 2 ml of water. If
foam produced persists for ten minutes it indicates
the presence of saponins.
DETECTION OF PROTEINS AND
AMINOACIDS
XANTHOPROTEIC TEST
The extracts were treated with few drops of conc.
Nitric acid. Formation of yellow colour indicates
the presence of proteins.
NINHYDRIN TEST
To the extract, 0.25% w/v ninhydrin reagent was
added and boiled for few minutes. Formation of
blue colour indicates the presence of amino acid.
DETECTION OF CARBOHYDRATES
Extracts were dissolved individually in 5 ml
distilled water and filtered. The filtrates were used
to test for the presence of carbohydrates.
MOLISCH’S TEST
Filtrates were treated with 2 drops of alcoholic α-
naphthol solution in a test tube. Formation of the
violet ring at the junction indicates the presence of
Carbohydrates.
BENEDICT’S TEST
Filtrates were treated with Benedict’s reagent and
heated gently. Orange red precipitate indicates the
presence of reducing sugars.
FEHLING’S TEST
Filtrates were hydrolysed with dil. HCl, neutralized
with alkali and heated with Fehling’s A & B
solutions. Formation of red precipitate indicates the
presence of reducing sugars.
EXPERIMENTAL ANIMALS
Albino mice (20-30gm) of either sex were
procured from Sri Venkateshwara
enterprises, Bangalore. After procuring the
animals were acclimatized for 10 day’s
under standard husbandry conditions as
follows;
Room temperature - 27  3C
Relative humidity - 65  10 %
12 hours light / dark cycle -
The animals were fed with feed gold mohr,
Lipton India Ltd., Bangalore and water was
given ad libitum under strict hygienic
conditions. This project was approved by
Institutional Animal Ethical Committee
(IAE/SKIPS/2011/MAY15/I/12/RATS-
96/MICE-36).
ACUTE TOXICITY
The acute toxicity for methanolic and aqueous
extracts of leaves of Artocarpus heterophyllus was
determined in albino mice, maintained under
standard conditions. The animals were fasted
overnight prior to the experiment. Fixed dose
(OCED Guideline No. 420) method of CPCSEA
was adopted for toxicity studies.
RESULTS AND DISCUSSION
PREPARATION OF EXTRACTS
The yield, colour and consistency of extracts of
leaves of Artocarpus heterophyllus, were shown in
the table no 1.
Table No. 1: Colour, Consistency and Percentage yield of extracts of leaves of Artocarpus heterophyllus
Sl. No. Solvent Colour and Consistency Percentage yield
1 Pet. Ether Dark Brown Sticky 5.40%
2 Chloroform Dark Brown Solid 2.67%
3 Methanol Very Dark Brown Sticky 7.50%
4 Aqueous Brown Solid 10.83%
PRELIMINARY PHYTOCHEMICAL
STUDIES OF DIFFERENT EXTRACT
Preliminary phytochemical studies revealed that
leaves of different extracts contain flavonoids,
tannins, saponins and carbohydrates in ethanolic
and aqueous extracts where as steroids are found to
be present in pet. ether and extract of leaves. The
results are compiled in table no 2.
Chiranjib B, al / Int. J. of Allied Med. Sci. and Clin. Research Vol-1(2) 2013 [78-81]
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81
Table No.2: Preliminary phytochemical studies of different extract of leaves of Artocarpus heterophyllus
Chemical constituents Solvent Used
Pet. Ether Chloroform Methanol Aqueous
Alkaloids    
Flavonoids   + +
Steroids +   
Tannins + + + +
Saponin   + +
Proteins    
Carbohydrate _ _ + +
+ Present
- Absent
ACUTE TOXICITY
The acute toxicity for methanolic and aqueous
extracts of leaves of Artocarpus heterophyllus was
determined in albino mice, maintained under
standard conditions. The animals were fasted
overnight prior to the experiment. Fixed dose
(OCED Guideline No. 420) method of CPCSEA
was adopted for toxicity studies. There were no
sign of toxicity for first 48 hours and no animal
died on 14 day of study at a dose of 2000 mg/Kg.
REFERENCES
[1]. Vaidyaratnam PS. Indian medicinal plants a compendium of 500 species. Orient Longman Ltd, 1993(1):
208.
[2]. Asima Chatterjee, Satyesh Chandra Pakrashi. Vol 2. The treatise on Indian Medicinal Plants, New Delhi:
Publications and Information Directorate, 1995 (1): 37
[3]. Mei-Ing Chung, Chai-Ming Lu, Pao-Lin Huang, Chun-Nan Lin. Prenylflavonoids of Artocarpus
heterophyllus. Phytochem 1995; 40(4): 1279-82
[4]. Chai-Ming Lu, Chun-Nan Lin. Two 2',4',6'-trioxygenated flvonones from Artocarpus heterophyllus.
Phytochem 1993; 33(4): 909-11
[5]. Feng N Ko, Zhi J Cheng, Chun N Lin, Che M Teng. Scavenger and antioxidant properties of prenylflavones
isolated from Artocarpus heterophyllus. Free Radl Biol Med. 1998; 25(2): 160-68
[6]. Jayaraman J. “Laboratory Manual in Biotechemistry. Published by birla publication New Delhi (I): 50-53,
1995
[7]. Kokate CK, Ed. Practical Pharmacognosy. 4th
ed. New Delhi: Vallabha Prakashan; 1999: 149-56.
[8]. Khandelwal KR. Practical Pharmacognosy techniques and experiments. 2nd
ed. Pune: Nirali Prakashan;
2000: 149-56
[9]. Mrs. Prema Veeraraghavan. Expert consultant, CPCSEA, OECD guideline No. 420.

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Phytochemical and acute toxicity study of leaves of artocarpus heterophyllus lam

  • 1. * Corresponding author: Chiranjib Bhattacharjee ~ 78 ~ IJAMSCR |Volume 1 | Issue 2 | Nov - 2013 www.ijamscr.com Research article PHYTOCHEMICAL AND ACUTE TOXICITY STUDY OF LEAVES OF ARTOCARPUS HETEROPHYLLUS LAM Chiranjib Bhattacharjee1*and Amitsankar Dutta2 1 Srikrupa Institute of Pharmaceutical Sciences, Vil. Velkatta, Kondapak (Mdl), Dist. Medak, Siddipet. AP –502 277 2 R.K.Pharmacy College, Kashipur. Surai – Sathiaon, Azamgarh. U. P. 276001 ABSTRACT Artocarpus heterophyllus Lam commonly known as jack fruit widely distributed in north east India, West Bengal and south Karnataka. In the present study intended with various phytochemical screening and toxicity studies were carried out on the leaves of Artocarpus Heterophyllus. The phytochemical study shows the presences of flavonoids, tannins, saponins and carbohydrates in methanolic and aqueous extracts. In acute toxicity study both the extract were found safe on a dose of 2000 mg/Kg. KEYWORDS: Artocarpus heterophyllus, Phytoconsituents, Acute toxicity. INTRODUCTION Since the tribal native practitioner of Manipur claimed that the leaves of Artocarpus heterophyllus are highly useful in many diseases and we were in search for an alternative medicine, this claim has attracted our attention and selected the plant for present study. On the basis of current literature survey leaves of Artocarpus heterophyllus Lam, was taken for phytochemical investigation and toxicological evaluation. The phytochemicals present in a plant indicates the possible pharmacological action whereas the toxicological study indicates the possible dose to carry out the pharmacological screening models. MATERIAL AND METHODS PLANT MATERIAL Leaves of Artocarpus heterophyllus Lam were collected from the forest of Manipur. The plant was authenticated by Dr. Bisehwori Thongam (IBSD/MPHRD/M/1008). The shade-dried leaves were course powdered and this powder were packed in soxhlet column and extracted successively with petroleum ether, chloroform, methanol and aqueous. The extracts were concentrated under reduced pressure (bath temperature 50C). The dried extracts were stored in air tight container in refrigerator below 10C. EXTRACTION WITH PETROLEUM ETHER At first the finely ground leaves are placed in a ‘thimble’ made by a strong filter paper in a chamber of soxhlet (2000ml). The powders are extracted at 55℃ using round bottomed flask for 72 hrs. The extracting solvent in round bottomed flask is heated and its vapour condenses in condenser. The condensed extractant drips into the thimble containing the crude drug and extract it by contact. After completion of extraction petroleum ether is filtered and concentrated to dry mass. The extract is air dried to remove all traces of the solvent and the percentage yield was calculated. Petroleum ether extraction was done to defeating the powder. EXTRACTION WITH CHLOROFORM The marc left after petroleum ether extraction, is dried and subsequently extracted with 1200ml of chloroform (61℃) in a soxhlet using round bottomed flask for 72 hrs. Then the extract is International Journal of Allied Medical Sciences and Clinical Research (IJAMSCR)
  • 2. Chiranjib B, al / Int. J. of Allied Med. Sci. and Clin. Research Vol-1(2) 2013 [78-81] www.ijamscr.com 79 concentrated by using rotary evaporator and dried to get the extract. EXTRACTION WITH ETHANOL The marc left is again packed in the soxhlet. The solvent is heated using isomentle and began to evaporate. For ethanol extraction the temperature used is 78℃. The extraction had for 18-20 hrs and after completion of extraction solution was evaporated to dryness under reduced pressure and controlled temperature by using rotary evaporator. EXTRACTION WITH DISTILLED WATER The marc left after ethanol extraction is placed in a stopper container with the distilled water (1176ml) and chloroform (24ml) and allowed to stand at room temperature for a period of 7 days with frequent agitation until the soluble matter has dissolved. Then the mixture is strained, the marc is pressed and the combined liquids are clarified by filtration. At last the solution is dried using rotary evaporator. PRELIMINARY PHYTOCHEMICALS SCREENING The preliminary phytochemical Screening was carried out on petroleum ether, chloroform, Ethanolic and aqueous extracts of Artocarpus heterophyllus for qualitative identification of type of phytoconstituents present. DETECTION OF ALKALOIDS Extracts were dissolved individually in dilute Hydrochloric acid and filtered. MAYER’S TEST Filtrates were treated with Mayer’s reagent (Potassium Mercuric Iodide). Formation of a yellow coloured precipitate indicates the presence of alkaloids. WAGNER’S TEST Filtrates were treated with Wagner’s reagent (Iodine in Potassium Iodide). Formation of brown/reddish precipitate indicates the presence of alkaloids. DRAGENDROFF’S TEST Filtrates were treated with Dragendroff’s reagent (solution of Potassium Bismuth Iodide). Formation of red precipitate indicates the presence of alkaloids. HAGER’S TEST Filtrates were treated with Hager’s reagent (saturated picric acid solution). Presences of alkaloids are confirmed by the formation of yellow coloured precipitate. DETECTION OF FLAVONOIDS ALKALINE REAGENT TEST Extracts were treated with few drops of sodium hydroxide solution. Formation of intense yellow colour, which becomes colourless on addition of dilute acid, indicates the presence of flavonoids. LEAD ACETATE TEST Extracts were treated with few drops of lead acetate solution. Formation of yellow colour precipitate indicates the presence of flavonoids. DETECTION OF PHYTOSTEROLS SALKOWSKI’S TEST Extracts were treated with chloroform and filtered. The filtrates were treated with few drops of Conc. Sulphuric acid, shaken and allowed to stand. Appearance of golden yellow colour indicates the presence of triterpenes. LIBERMANN BURCHARD’S TEST Extracts were treated with chloroform and filtered. The filtrates were treated with few drops of acetic anhydride, boiled and cooled. Conc. Sulphuric acid was added. Formation of brown ring at the junction indicates the presence of phytosterols. DETECTION OF TANNINS GELATIN TEST  To the extract, 1% gelatin solution containing sodium chloride was added. Formation of white precipitate indicates the presence of tannins.  About 0.5 g of the individual extract was boiled in 10 ml of water in a test tube and then filtered. A few drops of 0.1% ferric chloride (FeCl3) was added and observed for brownish green or a blue-black coloration.  The alcoholic or aqueous extract is treated with lead acetate (10%) solution. White precipitate is formed. DETECTION OF SAPONINS FROTH TEST Extracts were diluted with distilled water to 20ml and this was shaken in a graduated cylinder for 15 minutes. Formation of 1 cm layer of foam indicates the presence of saponins. FOAM TEST
  • 3. Chiranjib B, al / Int. J. of Allied Med. Sci. and Clin. Research Vol-1(2) 2013 [78-81] www.ijamscr.com 80 0.5 gm of extract was shaken with 2 ml of water. If foam produced persists for ten minutes it indicates the presence of saponins. DETECTION OF PROTEINS AND AMINOACIDS XANTHOPROTEIC TEST The extracts were treated with few drops of conc. Nitric acid. Formation of yellow colour indicates the presence of proteins. NINHYDRIN TEST To the extract, 0.25% w/v ninhydrin reagent was added and boiled for few minutes. Formation of blue colour indicates the presence of amino acid. DETECTION OF CARBOHYDRATES Extracts were dissolved individually in 5 ml distilled water and filtered. The filtrates were used to test for the presence of carbohydrates. MOLISCH’S TEST Filtrates were treated with 2 drops of alcoholic α- naphthol solution in a test tube. Formation of the violet ring at the junction indicates the presence of Carbohydrates. BENEDICT’S TEST Filtrates were treated with Benedict’s reagent and heated gently. Orange red precipitate indicates the presence of reducing sugars. FEHLING’S TEST Filtrates were hydrolysed with dil. HCl, neutralized with alkali and heated with Fehling’s A & B solutions. Formation of red precipitate indicates the presence of reducing sugars. EXPERIMENTAL ANIMALS Albino mice (20-30gm) of either sex were procured from Sri Venkateshwara enterprises, Bangalore. After procuring the animals were acclimatized for 10 day’s under standard husbandry conditions as follows; Room temperature - 27  3C Relative humidity - 65  10 % 12 hours light / dark cycle - The animals were fed with feed gold mohr, Lipton India Ltd., Bangalore and water was given ad libitum under strict hygienic conditions. This project was approved by Institutional Animal Ethical Committee (IAE/SKIPS/2011/MAY15/I/12/RATS- 96/MICE-36). ACUTE TOXICITY The acute toxicity for methanolic and aqueous extracts of leaves of Artocarpus heterophyllus was determined in albino mice, maintained under standard conditions. The animals were fasted overnight prior to the experiment. Fixed dose (OCED Guideline No. 420) method of CPCSEA was adopted for toxicity studies. RESULTS AND DISCUSSION PREPARATION OF EXTRACTS The yield, colour and consistency of extracts of leaves of Artocarpus heterophyllus, were shown in the table no 1. Table No. 1: Colour, Consistency and Percentage yield of extracts of leaves of Artocarpus heterophyllus Sl. No. Solvent Colour and Consistency Percentage yield 1 Pet. Ether Dark Brown Sticky 5.40% 2 Chloroform Dark Brown Solid 2.67% 3 Methanol Very Dark Brown Sticky 7.50% 4 Aqueous Brown Solid 10.83% PRELIMINARY PHYTOCHEMICAL STUDIES OF DIFFERENT EXTRACT Preliminary phytochemical studies revealed that leaves of different extracts contain flavonoids, tannins, saponins and carbohydrates in ethanolic and aqueous extracts where as steroids are found to be present in pet. ether and extract of leaves. The results are compiled in table no 2.
  • 4. Chiranjib B, al / Int. J. of Allied Med. Sci. and Clin. Research Vol-1(2) 2013 [78-81] www.ijamscr.com 81 Table No.2: Preliminary phytochemical studies of different extract of leaves of Artocarpus heterophyllus Chemical constituents Solvent Used Pet. Ether Chloroform Methanol Aqueous Alkaloids     Flavonoids   + + Steroids +    Tannins + + + + Saponin   + + Proteins     Carbohydrate _ _ + + + Present - Absent ACUTE TOXICITY The acute toxicity for methanolic and aqueous extracts of leaves of Artocarpus heterophyllus was determined in albino mice, maintained under standard conditions. The animals were fasted overnight prior to the experiment. Fixed dose (OCED Guideline No. 420) method of CPCSEA was adopted for toxicity studies. There were no sign of toxicity for first 48 hours and no animal died on 14 day of study at a dose of 2000 mg/Kg. REFERENCES [1]. Vaidyaratnam PS. Indian medicinal plants a compendium of 500 species. Orient Longman Ltd, 1993(1): 208. [2]. Asima Chatterjee, Satyesh Chandra Pakrashi. Vol 2. The treatise on Indian Medicinal Plants, New Delhi: Publications and Information Directorate, 1995 (1): 37 [3]. Mei-Ing Chung, Chai-Ming Lu, Pao-Lin Huang, Chun-Nan Lin. Prenylflavonoids of Artocarpus heterophyllus. Phytochem 1995; 40(4): 1279-82 [4]. Chai-Ming Lu, Chun-Nan Lin. Two 2',4',6'-trioxygenated flvonones from Artocarpus heterophyllus. Phytochem 1993; 33(4): 909-11 [5]. Feng N Ko, Zhi J Cheng, Chun N Lin, Che M Teng. Scavenger and antioxidant properties of prenylflavones isolated from Artocarpus heterophyllus. Free Radl Biol Med. 1998; 25(2): 160-68 [6]. Jayaraman J. “Laboratory Manual in Biotechemistry. Published by birla publication New Delhi (I): 50-53, 1995 [7]. Kokate CK, Ed. Practical Pharmacognosy. 4th ed. New Delhi: Vallabha Prakashan; 1999: 149-56. [8]. Khandelwal KR. Practical Pharmacognosy techniques and experiments. 2nd ed. Pune: Nirali Prakashan; 2000: 149-56 [9]. Mrs. Prema Veeraraghavan. Expert consultant, CPCSEA, OECD guideline No. 420.