ABSTRACT
The surge of interest in naturally occurring phytochemicals with high therapeutic potential has led to the discovery of many molecules, out of which naturally occuring coumarins such as marmelosin, umbelliferone and scopoletin present in Aegle marmelos (Bael) fruit shows good therapeutic potential. The aim of the present work is to develop and validate Reverse Phase-High Performance Liquid Chromatography (RP-HPLC) method for simultaneous determination of marmelosin, umbelliferone and scopoletin in A. marmelos fruit extracts. The chromatographic separation was performed with isocratic elution of 55:45 (%, v/v) methanol-water containing 0.1 % acetic acid as mobile phase. The method used to analyse the extract of A. marmelos showed good resolution with retention time within 12 min. The relative concentrations of above phytoconstituent were determined in A. marmelos fruits. The method was found to give compact peaks for scopoletin, umbelliferone and marmelosin (Rt of 4.6, 6.5 and 11.3 min respectively) and were linear over the range 5-30 µg ml(-1) (R(2) = 0.9655), 2-10 µg ml(-1) (R(2) = 0.9964) and 2-10 µg ml(-1) (R(2) = 0.9862) respectively. The mean recoveries for marmelosin, umbelliferone and scopoletin at three concentrations were in the range of 98.8-102.9, 98.8-101.1 and 94.2-98.3 % respectively. The relative standard deviation of accuracy, precision and repeatability were within 2 %, indicating the method produced highly reproducible results. Therefore this simple, precise and accurate method enables simultaneous separation of this phytoconstituent and hence can be successfully applied in analysis and routine quality control of herbal material and formulation containing A. marmelos.
ABSTRACT
The aim of the present work was to develop and validate a reversed-phase high-performance liquid chromatography method for the simultaneous estimation of picroside I, plumbagin, and Z-guggulsterone in a polyherbal formulation containing Picrorhiza kurroa, Plumbago zeylanica, and Commiphora wightii extracts. The analysis was performed on a C18 column using the mobile phase consisting of solvent A (acetonitrile) and solvent B (0.1% orthophosphoric acid in water) with the following gradient: 0-12 min, 25% A; 12-17 min, 25-80% A; 17-32 min, 80% A; and 32-37 min, 80-25% A at a flow rate of 1 ml/min. Ultraviolet detection was at 255 nm. The method was validated for accuracy, precision, linearity, specificity, and sensitivity as per the norms of the International Conference on Harmonization. From the validation study, it was found that the method is specific, accurate, precise, reliable, and reproducible. Good linear correlation coefficients (r(2)>0.900) were obtained for calibration plots in the ranges tested. Limits of detection were 2.700, 0.090 and 0.099 µg/ml and limits of quantification were 9.003, 0.310, and 0.330 µg/ml for picroside I, plumbagin, and Z-guggulsterone, respectively. Intra and interday relative standard deviation (RSD) of retention times and peak areas was less than 3.0%. Recovery was found to be 100.21% for picroside I, 102.5% for plumbagin, and 103.84% for Z-guggulsterone. The established method was appropriate and the three markers were well resolved, enabling efficient quantitative analysis of picroside I, plumbagin and Z-guggulsterone. The method is a rapid and cost-effective quality control tool for routine quantitative analysis of picroside I, plumbagin, and Z-guggulsterone in tablet dosage form.
ABSTRACT
Embelin, a naturally occurring benzoquinone, is obtained from fruits of Embelia ribes, which plays a vital role in the Ayurvedic system of medicine. The benzoquinone has diverse pharmacological and therapeutic properties and now constitutes a part of modern medicine. The aim of our study was to observe the effect of various stress conditions on this potential drug candidate. Embelin was subjected to stress conditions of acid and alkaline hydrolysis, oxidation, photolysis and thermal degradation. A significant degradation was found to occur by acid hydrolysis, oxidation and to a lesser extent under thermal stress and alkaline hydrolysis; the compound was found to be stable to photolytic stress. Further, the degradation product resulting from the acid hydrolysis was isolated and its structure was elucidated using spectroscopic techniques. Stress degradation studies on embelin provide an insight for its stability and storage considering the formulation aspects of modern medicine.
ABSTRACT
A rapid, simple and specific reversed-phase HPLC method has been developed for analysis of karanjin in Pongamia pinnata Linn. leaves. HPLC analysis was performed on a C(18) column using an 85:13.5:1.5 (v/v) mixtures of methanol, water and acetic acid as isocratic mobile phase at a flow rate of 1 ml/min. UV detection was at 300 nm. The method was validated for accuracy, precision, linearity, specificity. Validation revealed the method is specific, accurate, precise, reliable and reproducible. Good linear correlation coefficients (r(2)>0.997) were obtained for calibration plots in the ranges tested. Limit of detection was 4.35 µg and limit of quantification was 16.56 µg. Intra and inter-day RSD of retention times and peak areas was less than 1.24% and recovery was between 95.05 and 101.05%. The established HPLC method is appropriate enabling efficient quantitative analysis of karanjin in Pongamia pinnata leaves.
ABSTRACT
A simple and efficient method for the isolation of rhein from Cassia angustifolia (senna) leaves is described in which the hydrolysis of the sennosides and extraction of the hydrolysis products (free anthraquinones) is carried out in one step. Further isolation of rhein is achieved from the anthraquinone mixture. This method reduces the number of steps required for isolation of rhein as compared to conventional methods.
ABSTRACT
The phyto-constituents of Gymnema sylvestre are used in the treatment of diabetes and obesity. The present work reports on the extraction of gymnemic acid through gymnemagenin from callus cultures of G. sylvestre. Components were separated on pre-coated silica gel 60 GF254 plates with chloroform:methanol (8:2) and scanned using a densitometric scanner at 205 nm in the near-UV region. Linearity of determination of gymnemagenin was observed in the range 2-10 microg. The average percentage recovery of gymnemagenin from leaf callus extracts was 98.9+/-0.3.
Subject(s)
Alkaloids/chemistry , Gymnema sylvestre/chemistry , Saponins/analysis , Triterpenes/analysis , Chromatography, Thin Layer , Plant Leaves/chemistry , Plant Stems/chemistry , Seeds/chemistry , Tissue Culture TechniquesABSTRACT
The size of the phytoecdysteroids family is rapidly growing. Recent data shows over 250 ecdysteroid analogs have been identified so far in plants. It is theorized that there are over 1000 possible structures, which might occur in nature, but it is a fact that ecdysteroids usually occur in plants as a complex cocktail of structurally different compounds. Among these compounds, the major component is usually the common ecdysteroid-like 20-hydroxyecdysone. Ecdysteroids are polar steroids, almost sugar-like in their solubility properties. Extraction and purification of ecdysteroids (polyhydroxy steroids) is complicated by their polar nature and poor crystallizing properties. These properties make them difficult to separate from other polar plant constituents. Besides, this plant extract is very often processed by multistep procedures to isolate the major and minor ecdysteroids from the new or existing sources. A simplified scheme consisting of a few extraction steps for the purification of ecdysteroid from plants is in great demand. A quantitative approach through high-performance liquid chromatography has been initiated for developing an easy method for the extraction of ecdysteroids from Ipomoea hederacea (kaladana) seeds.
