Comparative analysis of four terpenoids in root and cortex of Tripterygium wilfordii Radix by different drying methods

Background Tripterygium wilfordii Radix, a well-known traditional medicine in china which is used for treatment of inflammation, pain, tumor and immune regulation for centuries in china, accompany with the serious toxic side effects. This study was carried out for simultaneously analyzing the four main components (triptolide, triptophenolide, demethylzeylasteral and celastrol) in Tripterygium wilfordii Radix under different drying processes, which was important for reducing the toxicity and quality control of Tripterygium wilfordii Radix in future. Methods The terpenes were extracted by using ultrasonic method with ethyl acetate from root or cortex of Tripterygium wilfordii Radix, and the sensitive and rapid HPLC-PDA method was developed for simultaneous quantification of triptolide, triptophenolide, demethylzeylasteral and celastrol in root and cortex of Tripterygium wilfordii Radix for evaluation of the impacts by different drying processes. Results The four compounds in their respective determined arrange had good linearity of 0.9998≦R2≦0.9999 and the average recoveries were range from 94.69 to 100.28%, RSDs were within 0.27 to 2.42%, respectively. The contents of triptolide, triptophenolide, demethylzeylasteral and celastrol in different Tripterygium wilfordii Radix individuals were varied greatly at different drying temperatures. Under different temperatures, the contents of triptolide, triptophenolide, demethylzeylasteral, and celastrol were 37.94–70.31 mg/g, 0–1.807 mg/g, 0.3513–9.205 mg/g, 3.202–15.31 mg/g, respectively. The suitable drying temperature of terpenoids in root of wild and cultivate are 80 °C and 60 °C, the suitable drying temperature of terpenoids in cortex is 40 °C. Conclusions The method established is high sensitivity, accuracy, reliability and suitable for the simultaneous analysis of terpenoids in Tripterygium wilfordii Radix. The data provide a scientific basis and reference for the quality control of herb and preparations related to Tripterygium wilfordii Radix.


Background
Tripterygium wilfordii Hook. f. and Tripterygium hypoglaucum (Levl.) Hutch both belong to Tripterygium genus of Celastraceous, their roots were considered as Lei Gong Teng (Tripterygium wilfordii Radix) applying to clinic in China. Lei Gong Teng shows the therapeutic effects of dispel wind and eliminate dampness, activating meridians to stop pain, detoxification and insecticide, reducing swelling, and so on [1]. In China, there are three species in this genus which mainly produced in Zhejiang, Hunan, Anhui, Fujian, Taiwan, Jilin and other provinces [2], and mainly distributed in the middle and lower reaches of Yangtze River. Currently, in clinical, the preparations of Tripterygium wilfordii Radix are in the form of Tripterygium Glycosides Tablet, Tripterygium total terpenoids tablets, Tripterygium bilayer tablets, Tripterygium tablets, and triptolide ointment [3], which are of great application value. So far about 100 kinds of compounds have been isolated from plants of Tripterygium genus [4], mainly including alkaloids, diterpenes, triterpenes, etc, which exhibited anticancer, antirheumatoid arthritis, insecticide, anti-HIV activities and were used in the treatment of kidney diseases [5][6][7][8][9][10][11]. The previous studies have reported that the triptolide and triptophenolide, on behalf of diterpenoid constituents, possess anti-inflammatory, immunosuppressive [12][13][14][15], antifertility, anticyst and antitumor activities [16], and so on. The demethylzeylasteral and celastrol are the major effective ingredients of triterpenoids and have a remarkable immune inhibitory activity, anti-inflammatory, anti-tumor and other pharmacological activities [17].
It was reported that Tripterygium wilfordii Radix has serious toxicity, and the toxic side effects incidence was 58.1% [18], which has been one of the largest herbal poisoning incidents reported in nearly half a century. Triptolide, the bioactive ingredient contained in Tripterygium wilfordii Radix, is also the major toxic component [19] and has a strong toxicity [20]. The roots of Tripterygium regelii and Tripterygium hypoglaucum contain similar chemical compositions [21] and have similar clinical efficacy compared with Tripterygium wilfordii Hook.f.. The preparations of Tripterygium wilfordii Radix with therapeutic doses are close to the toxic dose. Excessive doses can easily reduce reproductive system [22], urinary system [23], digestive system, nervous system [24], cortex and mucous membranes, endocrine system [25], blood system [26,27] and other diseases, such as diarrhea, acute renal failure [28], loss of libido, vision loss, erythema, neutropenia [29], drug-induced liver injury [30], even death. So, it is important to evaluate the bioactive terpenoids and control of the quality of herbs. The multiple factors of drying processing methods, origin and breed, and different habitats for Tripterygium wilfordii Radix all determine the contents of bioactive terpenoids and influence the toxicity and efficacy. Therefore, it is significant for evaluating the effective and toxic components changes in Tripterygium wilfordii Radix during the different drying processing methods.
In this paper, a High Performance Liquid Chromatography-Photo Diode Array (HPLC-PDA) method was established to simultaneously analyze the triptolide, triptophenolide, demethylzeylasteral and celastrol and evaluate the quality of Tripterygium wilfordii Radix by different drying processes. It would be helpful for quality control, warranty of safety and efficacy of Tripterygium wilfordii Radix herb or its preparations.

Chemicals, reagents and materials
The reference standards of tiptophenolide (20120425) and demethylzeylasteral (ZJ0619BC13) were purchased from the Shanghai yuanye Bio-Technology Co., Ltd (Shanghai, China). The reference standards of trtiptolide (LGT-B-20131121) and celastrol (LGT-H-20121211) were purchased from the Nanjing Spring & Autumn Biological Engineering Co., Ltd (Nanjing, China). The chemical structures of them are shown in Fig. 1.
Acetonitrile and methanol were of HPLC grade and obtained from Tedia (Fairfield, USA). Formic acid and ethyl acetate were of analytical grade and from Merck (Darmstadt, Germany). Deionized water was purified by the Millipore water purification system (Millipore, Milford, MA, USA) and filtered with 0.22 μm membranes. All other reagents used were of analytical grade.
The 13 batches of Tripterygium wilfordii Radix were collected from different origins of the whole country. Their detailed information was listed in Table 1. The corresponding author authenticated all the raw materials, and the herbal drugs were verified according to the Chinese pharmacopoeia (Chinese pharmacopoeia, 2010). The voucher specimens were deposited at the Herbarium in Nanjing University of Chinese Medicine.

Preparation of the test solution
The Tripterygium wilfordii Radix fresh herbs were selected randomly and separated into cortex and root under its season, 40, 60, 80, 100°C drying and ground into powder with 40 meshes, respectively. An aliquot (1 g) was weighed precisely and ultrasound with 40 mL ethyl acetate solution for 60 min at room temperature using an ultrasonic water bath (100 kHz), and finally made to a volume of 40 mL using ethyl acetate solution. Three replicates of the extraction process were carried out on the independent samples. The solution was centrifuged 10 min at 13,000 r/min and filtered through 0.22 μm membrane prior to use. Then the 10 μL aliquot was injected into the HPLC system for analysis, calculate the sample content of triptolide, triptophenolide, demethylzeylasteral and celastrol.

Chromatographic conditions
The analyses were performed on a Waters 2695 Alliance HPLC system (Waters Corp., Milford, MA, USA), equipped with a quaternary pump solvent management system, an auto-sampler, and an on-line degasser. The separation was carried out on a Dimonsiol C 18 column (250 mm × 4.6 mm, 5 μm) at a column temperature of 25°C. The mobile phase was composed of A (acetonitrile) and B (0.1% formic acid, v/v) with a gradient elution at the flow rate of 1.0 mL/min: 0~5 min, 40% A, 5~40 min, 40~90% A, 40~42 min, 90~40% A; detection wavelength was 250 nm (Diterpenoids triptolide maximum UV absorption at 222 nm, triptophenolide at maximum UV absorption at 223 nm, triterpenoids maximum absorption wavelength varied, celastrol maximum absorption at 430 nm, demethylzeylasteral maximum UV absorption at 268 nm. Considering the wavelength of maximum absorption of the compounds, the final choice was measured at 250 nm. Equilibration duration was 10 min between individual runs. A Waters 2996 photo diode array (PDA) was connected to the liquid chromatography for detection of the raw data.
The HPLC chromatograms of reference substance and samples were stated in Fig. 2.

The linear range of inspection
Take appropriate triptolide, triptophenolide, demethylzeylasteral, and celastrol reference substance to injection and record peak area values with described chromatographic conditions. A peak area values for the vertical axis, sample concentration C as abscissa. The standard stock and working solutions were all stored at 4°C until  analysis and filtered through a 0.22 μm membrane prior to injection.

Validation of the method
A series of concentrations of standard solution were prepared for the establishment of calibration curves. The peak areas were plotted against the corresponding concentrations to obtain the calibration curves. LODs and LOQs were determined using diluted standard solution when the signal-to-noise ratios (S/N) of analytes were about 3 and 10, respectively. The S/N was calculated as the peak height divided by the background noise value. Intra-day and inter-day variations were chosen to determine the precision of the developed method. In intraday variability test, the mixed standards solutions were analyzed for six replicates within a day; while in interday variability test, the solutions were examined in duplicates for consecutive three days. Repeatability was confirmed with six independent analytical sample solutions prepared from the same batch of sample. One of the sample solutions was stored at 20°C and analyzed at 0, 2, 4, 8, 12, and 24 h, respectively, to evaluate their stability. All these variations were expressed by relative standard deviation (RSD).
A recovery test was used to evaluate the accuracy of this method. The test was performed by adding known amounts of the standards at low (80% of the known amounts), medium (the same as the known amounts) and high (120% of the known amounts) levels. The spiked samples were then extracted, processed, and quantified in accordance with the aforementioned methods. The average recovery percentage was calculated by the formula: Recovery (%) = (observed amountoriginal amount)/spiked amount × 100%.

Optimization of experimental conditions
The tripterines containing carboxylic acid groups, so using a mobile phase system of aqueous acid can reduce tailing. By comparing with the acetonitrile-acid elution, both acetonitrile-0.2% phosphoric acid and acetonitrile-0.1% formic acid water solution can achieve a better separation, but phosphoric acid has some damage to column, and could easily lead to blockage of the valve, so we choose acetonitrile-0.1% formic acid as the mobile phase.
This experiment compared the ultrasonic-methanol (U1), ultrasonic-ethanol (U2), ultrasonic-ethyl acetate (U3), reflux-methanol (R1), reflux-ethanol (R2), refluxethyl acetate (R3) solvent extraction efficiency of terpenoids in Tripterygium wilfordii Radix. The results showed that there was a lower dissolution rate of terpenoids obtained by methanol, ethanol solvent extraction, but the acetate extraction rate is higher than that of methanol and ethanol. Besides, the dissolution rate of triptolide, demethylzeylasteral and celastrol had no significant difference between ultrasonic and reflux extraction, while the dissolution rate of triptophenolide with ultrasonic extraction was higher than reflux. Therefore, we selected the ultrasonic-ethyl acetate as the extraction solvent. The results were shown in Fig. 3.

Methodological data results
Linear regression data, precision, repeatability, stability and recovery of 4 analytes were shown in Table 2. The results showed that the RSDs of precision test for triptolide, triptophenolide, demethylzeylasteral and celastrol were 2.95, 3.55, 0.350 and 0.270%, respectively, which indicated a good precision of the experimental method. The RSDs of stability test were 2.53, 3.04, 0.521 and 0.861%, respectively, and the absorbance of the sample solution showed stable within 24 h. The RSDs of repeatability test were 2.83, 3.40, 0.693 and 0.752%, respectively, which indicated a good reproducibility of the samples.

Determination of terpenoids contents
The contents of terpenoids in samples were shown in Tables 3, 4, 5 and 6. The contents of triptolide, triptophenolide, demethylzeylasteral and celastrol, obtained from the Tripterygium wilfordii Radix samples derived from different producing areas and by different drying process temperatures, exhibited obviously different. Among which the contents of triptophenolide are obvious difference at different drying temperatures. There is trace quantity of triptophenolide in some samples of Tripterygium wilfordii Radix. The content of tripterine has nearly two times difference and the demethylzeylasteral about 3 times.

Compare the terpenoids in cortex of Tripterygium wilfordii Radix
As for the cortex of Tripterygium wilfordii Radix, the content of triptolide in sample from Guizhou (wild) is the highest (70.31 mg/g), Fujian (wild, 66.92 mg/g), Yueyang (wild, 49.82 mg/g) followed; the content of triptophenolide from Hubei (wild) is the highest (1.807 mg/ g), Fujian (cultivate, 1.164 mg/g), Fujian (wild, 0.9746 mg/g) followed; the content of demethylzeylasteral from Hubei (wild) is the highest (9.205 mg/g), Zhejiang (cultivate, 9.112 mg/g), Guizhou (cultivate, 8.520 mg/g) followed; the content of celastrol from Hubei Shaoyang (wild) is the highest (15.32 mg/g), Hubei Yuncheng (wild, 14.50 mg/g) and Guizhou (wild, 14.25 mg/g), followed. During the different drying temperature, the suitable drying temperature for cortex of Tripterygium wilfordii Radix was shown in Fig. 5. It was found that the highest content of triptolide in wild samples such as sample 1, 2, 6 and 10 were at 100°C by comparing different temperatures. It was occupied more than half in all wild samples. The highest content of triptolide in cultivate samples such as samples 4,8,9,12 and 13 were at 100°C by comparing different temperatures. These samples are far more than in all cultivate samples in half. So it was considered that the suitable drying temperature were both 100°C, respectively. The highest content of triptophenolide in wild samples such as sample 1, 2, 7 and 10 were at 40°C by comparing different temperatures. The highest content of triptophenolide in cultivate samples such as samples 4, 5, 8 and 13 were at 80°C by comparing different temperatures and they account for more than half in all wild and cultivate samples. So it was considered the suitable drying temperature were 40 and 80°C. The highest content of demethylzeylasteral in wild samples such as sample 1, 6, 7 and 10 were at 40°C by comparing different temperatures. It was occupied more than half in all wild samples. The highest content of demethylzeylasteral in cultivate samples such as sample 4, 5, 9, 12 and 13 were at 40°C by comparing different temperatures. These samples are far more than in all cultivate samples in half. So it was considered the suitable drying temperature were both 40°C. The highest content of celastrol in wild samples such as sample 1, 2, 6 and 10 were at 80°C by comparing different temperatures. It was occupied more than half in all wild samples. The highest content of celastrol in cultivate samples such as sample 4, 5, 9, 12 and 13 were at 60°C by comparing different temperatures. These samples are far more than in all cultivate samples in half. So it was considered the suitable drying temperature were 80 and 60°C.
From the above conclusion, the different contents of Tripterygium wilfordii Radix drying temperature are different. Therefore, choose a suitable drying temperature in order to make the medicinal full and effective use is imperative. Generally speaking, the terpenoids in cortex of Tripterygium wilfordii Radix suitable drying temperature is 40°C, because it could get most types of ingredients. On the contrary, it is considered the suitable drying temperature is 80°C as for a maximum contents of total terpenoids obtained.  Compare the terpenoids in root of Tripterygium wilfordii Radix As for the root of Tripterygium wilfordii Radix, the content of triptolide in sample from Fujian (wild) is the highest (55.91 mg/g), Guizhou (wild, 53.30 mg/g), Jiangxi Suizhou (cultivate, 47.66 mg/g) followed. The content of triptophenolide in sample from Fujian (wild) is the highest (1.245 mg/g), Hubei Shaoyang City (wild, 0.9867 mg/g) and Jiangxi (cultivate, 0.9061 mg/g) were followed. The content of demethylzeylasteral in sample from Guizhou (cultivated) is the highest (7.214 mg/g), Fujian (cultivate, 7.046 mg/g), and Zhejiang (cultivate, 5.452 mg/g) were followed. And the content of celastrol in sample from Guizhou (wild, 12.97 mg/g) is the highest, Hubei Shaoyang (wild, 12.80 mg/g), and Hubei Yuncheng (wild, 9.067 mg/g) were followed. During the different drying processes, the feasible drying temperature for root of Tripterygium wilfordii Radix was shown in Fig. 6. It was found that the highest content of triptolide in wild samples such as sample 2, 3, 6 and 7 was at 80°C by comparing different temperatures. The highest content of triptolide in cultivate samples such as sample 4, 8, 9 and 13 was at 100°C by comparing different temperatures. The highest content of triptophenolide in wild samples such as sample 2, 6, 7 and 10 was at 40°C by comparing different temperatures. The highest content of triptophenolide in cultivate samples such as sample 4,5,8,11 and 12 was at 80°C by comparing

Conclusion
In this study, the HPLC-PDA assay method was established for simultaneously determination of the triptolide, triptophenolide, demethylzeylasteral and celastrol in root and cortex of Tripterygium wilfordii Radix by different  Fig. 4 The contents of four terpenoids in cortex and root of Tripterygium wilfordii Radix Fig. 5 The contents of four terpenoids in wild and cultivate cortex of Tripterygium wilfordii Radix at different drying temperature Fig. 6 The contents of four terpenoids in wild and cultivate root of Tripterygium wilfordii Radix at different drying temperature drying processes. Compared with the previously reported methods, the present method employed a simple and rapid extraction procedure for sample preparation, and offered higher sensitivity analyzed method. The method was successfully applied to the analysis of four terpenoids in Tripterygium wilfordii Radix samples derived from different producing areas and different drying processes. These results would be provide an useful information for the further quality control of Tripterygium wilfordii Radix and its preparations and to master the dosage and indications for herbs and formulations product.