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Malipatil M, Chitme H. R, Chandra R, Ramesh H, Irrchaya R. Isolation and Characterization of Aromatic Amide From Methanolic Extrat of Root Ofcarissa Carandas Linn. Biosci Biotechnol Res Asia 2009;6(1)
Manuscript received on : November 26, 2008
Manuscript accepted on : December 30, 2008
Published online on:  28-06-2009
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Isolation and Characterization of Aromatic Amide From Methanolic Extrat of Root Ofcarissa Carandas Linn.

Mallikarjun Malipatil1*, H. R. Chitme2, Ramesh Chandra3, H. Ramesh4 and Raghuveer Irrchaya5

1Karnataka College of Pharmacy, Manhalli Road, Bidar - 585 403 India.

2Department of Pharmacy Azaiba, Muscat Sultanate of Oman Oman.

3Founder director, Dr.B.R.Ambedkar Center for Biomedical Research Delhi University, Delhi India.

4R.R.K. College of Pharmacy Nauabad Bidar India.

5Head and Director Institute of Pharmacy Bundelkhand University Jhansi India.

Corresponding Author E-mail: mhp1232007@rediffmail.com 

ABSTRACT: Carissa carandas Linn (Family: Apocynaceae) commonly known as Karaunda, is a large evergreen shrub with a short stem, glabrous shrub found almost through out India. All the parts of the Carissa carandas linn were reputed in indigenous medicine for various kinds of diseases and disorders. The objective of the work is to study the chemical constituents of benzene extract of root of Carissa carandas Linn. The fresh root of the plant is used internally as anthelmentics, antipyretic, stomachic and antiscorbutic. Phytochemical investigation conducted on root revealed the presence of carbohydrates, alkaloids, flavanoids, saponins, steroids and fatty acids. The aromatic amide was detected in benzene extract and methanol extract of the root. The extracts were carried out by soxhlet extractor and the yield of benzene extract was 2.5%.The TLC study of methanolic extract showed the presence of 4 spots. The three spots were identified as aromatic amides. The present study deals with isolation characterization of aromatic amide (M3) isolated from methanolic extract of root of Carissa carandas linn. The four compounds were separated by column chromatography using benzene: ethyl acetate: chloroform (4:2:1). The TLC study of separated compounds with Rf value 0.85 (M1), 0.73 (M2), 0.68 (M3) and 0.65 (M4). From UV, IR, 1HNMR and LC-Mass spectral analysis of the compound M3 .It could be characterized as aromatic amide.

KEYWORDS: Carissa carandas; methanolic extract; aromatic amide; TLC; column chromatography

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Malipatil M, Chitme H. R, Chandra R, Ramesh H, Irrchaya R. Isolation and Characterization of Aromatic Amide From Methanolic Extrat of Root Ofcarissa Carandas Linn. Biosci Biotechnol Res Asia 2009;6(1)

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Malipatil M, Chitme H. R, Chandra R, Ramesh H, Irrchaya R. Isolation and Characterization of Aromatic Amide From Methanolic Extrat of Root Ofcarissa Carandas Linn. Biosci Biotechnol Res Asia 2009;6(1). Available from: https://www.biotech-asia.org/?p=8189

Introduction

Carissa carandas Linn (Family: Apocynaceae) commonly known as Karaunda, is a large evergreen shrub with a short stem, glabrous shrub found almost through out India1. C.carandas Linn is a large evergreen shrub with  short stem and strong thorns in pairs, bark light grey,scaly;leaves simple,opposite,elliptic or obovate,shortly mucronate, glabrous shining and coriaceous;flowers white, in pubescent terminal corymbose cymes; fruit ellipsoid or globose berry, purplish black when ripe enclosing two or more seeds.2. The root has reputation of bring better stomachic. Used in the konkan, pounded with horse urine, lime juice and camphor as remedy for itching.3-5 the presence of cardio tonic activity of water soluble fraction has been attributed to the presence of glycosides of odoroside H. Presence of alkaloids is also reported in root and stem bark.4

Materials and Methods

The fresh root samples of carissa carandas linn was collected, dried and cut into pieces, crushed into powder then passed through sieve no 40 to obtain uniform particles and extracted with the solvents of increasing polarity6, Petroleum ether , benzene, chloroform, ethyl acetate and methanol for 48 hrs in fifty batches of 100gms for each batch by successive solvent extraction method. The extracts were collected to dryness in a rotary evaporator under reduced pressure and controlled temperature (50-600). After drying the extracts were weighed.

Thin Layer Chromatographic (TLC) of Methanolic Extract

The crude Methanolic extract was subjected to TLC studies using precoated silica gel GF254 Plates of 0.2 thickness7. A suitable mobile phase was developed consisting of benzene: ethyl (0.2g viewed under UV light and by spraying with dilute sulphuric acid.  TLC study of methanolic extract showed the presence of 4 spots.

Column chromatography of methanolic extract

The methanolic extract was chromatographed in a column with a aluminium oxide neutral built in petroleum ether and eluted with benzene: ethyl acetate: chloroform (4:2:1), four fractions were collected and concentrated.Fraction-1 upon concentration yielded reddish semisolid mass (0.2g) and named them as M1.Similarly fractions 2, 3, and 4 are concentrated and yielded, 0.25 g, 0.3 g and 0.35 g respectively ).They were labeled as M2, M3,and M4 respectively . The collected fractions are subjected to thin layer chromatography using the solvent system benzene: ethyl acetate: chloroform (3:2:1), spraying the developed plates with dilute sulphuric acid yellow color spots were observed. The Rf value of four compounds were calculated as M1 Rf value =0.85, M2 Rf value = 0.73, M3 Rf value= 0.68, and M4 Rf value = 0.65 All the four compounds were subjected for anti fungal activity the compound M3 was showed the moderate anti fungal activity hence the compound M3 was subjected for spectral analysis for further studies to know the chemical constituent responsible for the activity.

Chemical and Spectroscopic Analysis of Compound M3

The compound M3 was examined for there colour, odour, nature, melting point and solubility. The melting point was   determined by open capillaries of glass and they are uncorrected. The UV spectrum of the compound was recorded by using UV spectrophotometer. The IR spectrum was recorded in KBr pellet using FTIR spectrophotometer. The 1HNMR of the compound was recorded in CDCl3 using Bruker NMR spectrophotometer. The data obtained are given in Table no I.

Table 1: Spectroscopic Analysis of Compound M3.

Compound Spectrum Characteristics Peaks
M3

 

 

 

 

 

 

 

 

UV Spectrum

IR Spectrum (KBr) Cm-1

 

 

1HNMR(CDcl3 )

 

 

LC-Mass

 

λmax=310nm

3460( NH2 group), 3000-3100 (aromatic stretching ),

2300-2919 (C-H stretching of the CH2  and CH3   groups)

1706C=O group), 1652 (N-H bending and C=N), 1608 (C= C).

0.6– 4.3 δppm( presence of CH2 and CH3groups)

5.5  δppm (NH2 group)

7.2–7.7 δppm( presence of aromatic ring)

m/z 413.5 (the basic peak)

 

Antifungal activity of Aromatic Amide of Root of Carissa Carandas

The crude aromatic amide isolated from benzene extract were tested for antifungal activity by cup plate method8 at 1% and 2% concentration in dimethyl sulphoxide and fluconazole was used as standard drug. The photo agar media was used for this work8. The test organisms used were (A. Niger and, A Fumigatus).The zone of inhibition was measured in mm Table II

Table 2: Antifungal Activity of compound M3  .

 Microorganism

 

 

Zone of inhibition in mm.

B5(compound)       (Fluconazole)

1%W/W      2%W/W          1%W/W

 

 

2%W/W

 A. Niger

 A Fumigatus s

 

16                 17                     16

17                 18                    18

 

18

19

 

Results and Discussion

From benzene extract of root of carissa carandas linn aromatic amide was separated by column choromatography.The table I and II shows the results of spectral analysis and anti-fungal activity of M3 compound.

TLC studies of methanolic extract showed four spots and developed yellow colour with dilute sulphuric acid. The aromatic amide with Rf value of M3 (0.68) was isolated by preparative TLC.

In the spectroscopic analysis of M3 compound showed an absorption bands. In  IR spectrum KBr) cm-1 .Table I suggested presence of 3460 cm-1  ( hydrogen bonded NH2 group), the weak band around 3000-3100 cm-1 ( aromatic stretching), 2300-2919  cm-1 ( C-H stretching of the CH2 and CH3   groups), 1706 cm-1  (C=O group),1652 cm-1  (N-H bending and C=N) and 1608 cm-1 (due to C= C) .

The 1HNMR of the compound M3 showed the characteristics signals as below The major peaks observed in the 1HNMR spectrum at δ  0.6– 4.3  indicates the presence of CH2 and CH3 groups.  The peak at 5.5 may be due to NH2 group and the peak at δ 7.2–7.7 may be due to aromatic proton indicating the presence of aromatic ring. The IR and 1HNMR spectral studies of component M3 suggests the presence of aromatic ring, amino group, carbonyl group, and methylene and methyl group.  Hence, the compound M3 may contain an aromatic with aside chain having CH2 and CH3 groups and containing amide group.  Hence the compound M3 is an aromatic amide. In contrary, the mechanism of   amides will not depend on chain length and number of double or triple bonds. It has been hypothesized to produce its effects through conjugation with peptides and proteins of surface membranes thereby increase the permeability of the membrane and effective against all types of microbes. This could be the reason behind the antifungal activity of M3 compound. The phytochemical investigation and spectral analysis of compound M3 has shown the presence of aromatic amide in Methanolic extract. The aromatic amide could be the reason for its effectiveness as antifungal activity.

The LC-Mass spectrum of compound B5 showed the base peak at m/z 803.6.The molecular peak not recorded. The antifungal activity of the compound B5  because of aromatic amide.

Acknowledgement

Authors are greatly thankful to Dr.R.H.Udapi Professor in department of chemistry N.E.T.College of Pharmacy Raichur for his help in interpretation spectra.

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