Pharmacognosy Magazine

ORIGINAL ARTICLE
Year
: 2015  |  Volume : 11  |  Issue : 42  |  Page : 66--72

A novel high-performance liquid chromatography-electron spray ionization-mass spectrometry method for simultaneous determination of guggulsterones, piperine and gallic acid in Triphala guggulu


Ganesh Muguli1, PR Rao Vadaparthi2, B Ramesh2, Vishakante Gowda3, Rangesh Paramesh1, Atul N Jadhav1, K Suresh Babu2,  
1 Phytochemistry, Research and Development Center, The Himalaya Drug Company, Makali, Bengaluru, India
2 Natural Products Laboratory, Division of Organic Chemistry-I, Indian Institute of Chemical Technology, Hyderabad, India
3 Department of Pharmaceutics, JSS College of Pharmacy, JSS University, Mysore, India

Correspondence Address:
Dr. K Suresh Babu
Division of Natural Products Chemistry, Indian Institute of Chemical Technology, Hyderabad, Andhra Pradesh
India

Abstract

DQTriphalaguggulu0DQ is an important Ayurvedic formulation comprising of Guggulu, that is, Commiphora wightii (Arn.) Bhandari as a base wherein powdered fruits of triphala, that is, Phyllanthus emblica L., Terminalia bellirica (Gaertn.) Roxb and Terminalia chebula Retz, along with powdered fruit of Piper longum L. are compounded. This polyherbal preparation has been strongly recommended in chronic inflammation, piles, and fistula. However, due to the complexity of compound formulation standardization of commercial products is challenging. In the present communication marker-based standardization of DQTriphalagugguluDQ preparation using gallic acid (for triphala), piperine (for P. longum L.) and guggulsterones (for guggulu) is reported. These compounds of diverse chemistry were successfully separated on a Waters HR-C18 column by isocratic elution with methanol and water (80:20 v/v) as mobile phase at the flow rate of 1.0 mL/min coupled with photodiode array detector. These optimal chromatographic conditions were used for simultaneous quantification of gallic acid, guggulsterones (E and Z) and piperine in commercial samples by high-performance liquid chromatography-electron spray ionization-mass spectrometry and method was validated as per ICH guidelines.



How to cite this article:
Muguli G, Rao Vadaparthi P R, Ramesh B, Gowda V, Paramesh R, Jadhav AN, Babu K S. A novel high-performance liquid chromatography-electron spray ionization-mass spectrometry method for simultaneous determination of guggulsterones, piperine and gallic acid in Triphala guggulu.Phcog Mag 2015;11:66-72


How to cite this URL:
Muguli G, Rao Vadaparthi P R, Ramesh B, Gowda V, Paramesh R, Jadhav AN, Babu K S. A novel high-performance liquid chromatography-electron spray ionization-mass spectrometry method for simultaneous determination of guggulsterones, piperine and gallic acid in Triphala guggulu. Phcog Mag [serial online] 2015 [cited 2021 Jun 23 ];11:66-72
Available from: http://www.phcog.com/text.asp?2015/11/42/66/157696


Full Text

 INTRODUCTION



Herbal medicine and home remedies are in practice since man recognizing their use as a cure for various ailments of the body, and currently the inclination to use herbal remedies is on increased mode. This increase in demand for herbal medicine has put pressure on the supply of natural resources. This ultimately results in use of substandard materials or substitution and adulteration. To control the adulteration and maintain the quality and the efficacy of the product analytical tool play a major role. [1]

Triphalaguggulu is a traditional Ayurvedic polyherbal preparation has been a time tested medicament for chronic inflammatory conditions such as piles and fistula. [2] It uses guggulu, that is, resin of Commiphora wightii (Arn.) Bhandari as base to carry other fruit powders. This includes fruit of Piper longum L. and triphala (i.e. fruits of Phyllanthus emblica L., Terminalia chebula Retz, and Terminalia bellirica (Gaertn.) Roxb). This preparation is made in accordance with the authorized methodology provided in Ayurvedic Formulary of India. [3] Standardization of this compound ayurvedic formulation is challenging as it is an admixture of different phytochemicals with diverse chemistry. However, in order to ensure quality and efficacy of the compound formulation, it is desired to have accurate analytical tool. Triphalaguggulu is a commercially important formulation for which standardization method is not reported.

The basic constituent of this formulation is C. wightii which is an oleo-gum-resin containing biologically active steroids viz. E and Z guggulsterones. [4] The three fruits mentioned above when combined in equal ratio constitute "Triphala", which is well-recognized preparation of Ayurveda. [5] These three fruits are rich in tannins and have gallic acid as a common marker. [6],[7] Piperine is a well-known bioavailability enhancer and is a marker for P. longum.[8] In the present communication, we are reporting the high-performance liquid chromatography-electron spray ionization-mass spectrometry (HPLC-ESI-MS) method for standardization of "Triphalaguggulu" using the above markers.

Several analytical methods, available in the literature include liquid chromatography (LC)-MS/MS, HPLC and high-performance thin layer chromatography methods for the quantification of the above mentioned markers. [9],[10],[11],[12],[13],[14],[18] However, in our survey we did not find any report on the simultaneous determination of gallic acid, piperine and guggulsterones (E and Z) in Triphala guggulu. In the present work, we have developed a new, simple, rapid and specific reversed-phase HPLC-ESI-MS method with simultaneous quantification of these four markers. This method successfully determines the compounds of diverse polarities and chemical nature, which is phenolic acid or derivative (gallic acid, ellagic acid), alkaloid (piperine) and phytosterols (guggulsterones). [15] Further, this method is used successfully to determine these compounds in a complex matrix of five different Ayurvedic herbs. [3] This method can be used for the standardization of Triphalaguggulu commercial preparations and also for standardization of these herbs and their extracts for respective markers.

 EXPERIMENTAL



Plant material and preparation of the formulation

The materials C. wightii (Arn.) Bhandari (ole-gum-resin) were purchased from Gujarat Medicinal Plant Grower's Society. Other plant materials that is T. chebula Retz. (fruit rind), T. bellirica (Gaertn.) Roxb. (fruit), P. emblica L.(fruit) and Piper longum L. (fruit), (voucher specimens NPD/499/12, NPD/531/12, NPD/59/12 and NPD/119/12 resp.) were obtained locally and were authenticated by Dr. Kannan of The Himalaya Drug Company, Bangalore, India.

Chromatographic conditions

The chromatographic separation was achieved on Waters HR-C18 (300 mm × 3.9 mm, 6 μm) column using methanol and water (80:20 v/v) as mobile phase at the flow rate of 1.0 mL/min coupled with photodiode array detector. HPLC-MS studies were performed using an Agilent 1100 series online ion trap mass selective detector mass spectrometer with ESI source equipped with a degasser (G1379A), binary pump (G1312A), autosampler (G1329A), autosampler thermostat (G1329B) and diode array detector (G1315B) (Agilent Technologies, Waldbronn, Germany). The data were acquired and processed using Chemstation software 4.2 (Bruker, Waldbronn, Germany). An isocratic elution with methanol and water (80:20 v/v) as mobile phase was pumped at a flow rate of 1.0 mL/min; the sample injection volume was 20 μL with column temperature maintained at ambient conditions. The MS detection was set to electrospray (ESI) in positive ionization mode. Nitrogen was employed as the nebulizer gas. The ion source conditions were set as follows: Temperature, 335°C; nebulizer gas, 35 psi; dry gas, 10.0 L/min; skimmer 40.0V; capillary exit 128.0V; trap drive 44.5; max accu time 200 ms; Icc target 20000.

Standard solution preparation

Gallic acid (98%) and piperine (97%) were obtained from Sigma-Aldrich. Guggulsterones (E and Z, 99.6%) were obtained from Sami Labs Ltd. with E: Z ratio of 44:56. Accurately weighed 10 mg of each standard (piperine, gallic acid and guggulsterones (E and Z)) and dissolved in 10 mL methanol in volumetric flask, by vigorous shaking and then volume was made-up to mark with methanol to obtain a final concentration of 1 mg/mL of each compound.

Preparation of formulation

Triphalaguggulu samples marketed by different Ayurvedic medicine manufacturers (Shree Dhootapapeshwar Ltd., Baidyanath Ayurved Bhawan) were purchased locally at Bangalore.

In-house preparation of Triphalaguggulu

In order to ascertain the utility of the newly developed method Triphalaguggulu was made in-house in accordance with The Ayurvedic Formulary of India. [3] This was also intended to compare with market samples in case they differ widely from each other.

Preparation of sample

Approximately 50 mg of the formulation was weighed and transferred to 10 mL volumetric flask 5 mL of methanol was transferred and sonicated for 30 min, then transferred to a centrifuge vial and centrifuged for 20 min at a 4000 rpm, the supernatant liquid was decanted, the same cycle was repeated three times, the resultant solution was dried under vacuum and 10 mg/mL solution was prepared. The sample was injected to LC-MS system.

 Results and Discussion



Optimization of chromatographic conditions

Optimization of chromatographic conditions is equally critical for their adequate retention and separation. In the present work, the chromatography was performed on several reversed-phase columns such as Agilent Eclipse XDB-C18 (150 mm × 4.6 mm, 5 μm), Atlantis dC18 (150 mm × 4.6 mm, 5 μm), Waters HR-C18 (300 mm × 3.9 mm, 6 μm) and Xterra RP C18 (250 mm × 4.6 mm, 5 μm) to achieve a short run time, symmetric peak shapes, minimum matrix interference and solvent consumption. This was investigated by appropriate changes to the mobile phase composition (aqueous and organic part), and flow rate. The four compounds guggulsterones (E and Z stereoisomer) are mid polar, piperine-an alkaloid and gallic acid-a phenolic acid are polar in nature. Hence, a suitable combination of aqueous and organic solvent (methanol and water) was optimized with methanol 80% in water as the suitable mobile phase. The mobile phase was operated at a flow rate of 1.0 mL/min. The elution order and retention times were: Gallic acid (1.85 min), piperine (4.05 min) and guggulsterones (E and Z) were (6.12 and 7.06 min). This method was considered further analysis [Figure 1]. To achieve good sensitivity and accuracy for quantification, the different ultraviolet (UV) max values of four analytes were considered carefully. Thus, the PDA detection wavelengths were set at 273 nm for gallic acid, at 340 nm for piperine and 245 nm for guggulsterones according to the maximum absorption wavelength of each compound.{Figure 1}

Validation

The validation process was carried out according to the ICH guidelines (ICH, 2005). [16]

Calibration curve and limit of detection and limit of quantification

Calibration standards were prepared by diluting the appropriate volume of stock solution with methanol to attain the concentration levels of 10, 20, 40, 100, 200 μg/mL for piperine and guggulsterones and 10, 20, 40, 100, 200,5 00 and 800 μg/mL for gallic acid. The data of peak area versus drug concentrations were treated by linear least-square regression. The response was linear (r 2 =0.997 for gallic acid, 0.999 piperine and 0.998, 0.997 for guggulsterones) over the concentration range between 10 μg/mL and 200 μg/mL for piperine and guggulsterones, 10-800 μg/mL for gallic acid. The limit of detection was found to be 0.32 μg/mL for gallic acid, 0.40 μg/mL for piperine, 0.64 μg/mL, 0.59 μg/mL for guggulsterones. Limit of quantitation for gallic acid, piperine and guggulsterones (E and Z) were found to be 0.89 μg/mL, 1.05 μg/mL, 1.13 μg/mL, 1.25 μg/mL, respectively, as depicted in [Table 1].{Table 1}

Precision

The Precision of the method was examined by performing the intra- and inter-day assays of six replicate injections of the mixture of standard solution at three concentration levels. The intra-day assay precision was performed with the interval of 4 h in 1 day while the inter-day assay precision was performed over 6 days.

The results of the intra-day and inter-day precision experiments are shown in [Table 2]. The developed method was found to be precise as the relative standard deviation (RSD) values for repeatability and intermediate precision studies, respectively, were around <2%.{Table 2}

Specificity

The specificity of the method was determined by analyzing the standard and test samples. The peaks for gallic acid, piperine and guggulsterones test samples were confirmed by comparing the room temperature value and the UV-spectrum of the peak with that of the standard. Furthermore, the adequate selectivity and separation power was given by MS. The mass spectrum acquired in the m/z range from 0 to 600 showed [M-H]- ion at m/z 168.8 for gallic acid [Figure 2]a and [M+H]+ ions at m/z 286.1 [Figure 2]b and 313.2 [Figure 2]c and d for piperine and guggulsterones respectively. Thus, the identity of the peaks and an adequate chromatographic selectivity were confirmed.{Figure 2}

Accuracy

The accuracy of the method was confirmed by the recovery studies. The standard addition method was used for determining the recoveries of standards understudy. The recovery experiments of these compounds were performed by adding gallic acid, piperine and guggulsterones in different concentrations to the preanalyzed sample solutions. The results of the recovery study ranged from 98% to 102% with RSD ranging 1.83-4.48. Results of recovery studies are reported in [Table 3].{Table 3}

Application of the method

The newly developed and validated RP-HPLC method was applied for the analysis of studied marker compounds in different Triphalaguggulu samples. The peak areas of triplicate samples were analyzed by the regression equation obtained from the calibration plot to determine the content of these markers in samples. No interference was found at the retention time of the studied analytes in samples [Figure 3]. The analytical results for each component identified are summarized in [Table 4]. Therefore, the simultaneous determination of these active components in herbal preparations could be successfully applied to improve the safety and quality control of the formulations available in the market.{Figure 3}{Table 4}

 CONCLUSIONS



Traditional medicines are easily available to masses but are complex mixtures of natural substances and are prone for variation and adulteration. Triphala guggulu is one of the well-known Ayurvedic polyherbal preparation, which contains guggulu as one of the ingredient, which is in high demand and also listed as an endangered medicinal plant by IUCN. [17] In the present communication, we are reporting successful development and validation of RP-HPLC-PDA method for simultaneous determination of four biologically active markers representing the majority of the constitution of this polyherbal formulation. In the present study simultaneous quantification of gallic acid, piperine and guggulsterones has been achieved using RP-HPLC with multiple wavelength monitoring.

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