Separation and purification of three stilbenes from the radix of Polygonum cillinerve (Nakai) Ohwl by macroporous resin column chromatography combined with high-speed counter-current chromatography

Chi, Xiaofeng; Xing, Yuxiu; Xiao, Yuancan; Dong, Qi; Hu, Fengzu

doi:10.5935/0100-4042.20140256

Abstract

An effective method for the rapid separation and purification of three stilbenes from the radix of Polygonum cillinerve (Nakai) Ohwl by macroporous resin column chromatography combined with high-speed counter-current chromatography (HSCCC) was successfully established. In the present study, a two-phase solvent system composed of chloroform-n-butanol-methanol-water (4:1:4:2, v/v/v/v) was used for HSCCC separation. A one-step separation in 4 h from 150 mg of crude extract produced 26.3 mg of trans-resveratrol-3-O-glucoside, 42.0 mg of pieceid-2"-O-gallate, and 17.9 mg of trans-resveratrol with purities of 99.1%, 97.8%, and 99.4%, respectively, as determined by high-performance liquid chromatography (HPLC). The chemical structures of these compounds were identified by nuclear magnetic resonance (NMR) spectroscopy.

Polygonum cillinerve (Nakai) Ohwl; HSCCC; stilbenes

ARTIGO

Separation and purification of three stilbenes from the radix of Polygonum cillinerve (Nakai) Ohwl by macroporous resin column chromatography combined with high-speed counter-current chromatography

Xiaofeng Chi; Yuxiu Xing; Yuancan Xiao; Qi Dong; Fengzu Hu^* * e-mail: hufz@nwipb.cas.cn

Key Laboratory of Tibetan Medicine Research, Chinese Academy of Sciences, Northwest Institute of Plateau Biology, Chinese Academy of Sciences, NO.23 Xinning Road, Xining, P. R. China

ABSTRACT

An effective method for the rapid separation and purification of three stilbenes from the radix of Polygonum cillinerve (Nakai) Ohwl by macroporous resin column chromatography combined with high-speed counter-current chromatography (HSCCC) was successfully established. In the present study, a two-phase solvent system composed of chloroform-n-butanol-methanol-water (4:1:4:2, v/v/v/v) was used for HSCCC separation. A one-step separation in 4 h from 150 mg of crude extract produced 26.3 mg of trans-resveratrol-3-O-glucoside, 42.0 mg of pieceid-2"-O-gallate, and 17.9 mg of trans-resveratrol with purities of 99.1%, 97.8%, and 99.4%, respectively, as determined by high-performance liquid chromatography (HPLC). The chemical structures of these compounds were identified by nuclear magnetic resonance (NMR) spectroscopy.

Keywords:Polygonum cillinerve (Nakai) Ohwl; HSCCC; stilbenes.

INTRODUCTION

Polygonum cillinerve (Nakai) Ohwl, a perennial herb from the Polygonum family, is distributed mainly in Qinghai, Shanxi, Gansu, and Sichuan in China. ¹ The radix of the plant is an important traditional herbal medicine that has been shown to be effective in the treatment of inflammation, rheumatism, and bacterial infections. ² Previous phytochemical studies have demonstrated that stilbenes, anthraquinones, and flavonoids are the major bioactive constituents of this plant. ^3-5

Among these constituents, stilbenes such as trans-resveratrol, trans-resveratrol-3-O-glucoside, and pieceid-2"-O-gallate have recently attracted much attention due to their pharmacological properties, which include antioxidant,^6-8 anti-influenza viral,⁹ anti-fungal,¹⁰ anti-HIV-1, and cytotoxic effects. ^11,12 In view of these biological effects, an efficient method for the separation and purification of trans-resveratrol-3-O-glucoside, pieceid-2"-O-gallate and trans-resveratrol from Polygonumcillinerve (Nakai) Ohwl is necessary.

The traditional separation methods for the isolation and purification of stilbenes are mainly silica gel column chromatography and HPLC. However, these separation methods require numerous steps and large quantities of organic solvents. High-speed counter-current chromatography (HSCCC), which was invented by Ito and Conway, provides excellent sample recovery and can be employed for semi-preparative-scale separation in a completely straight forward manner. ¹³ Therefore, it has been widely used for the separation and purification of the active components of herb plants. ^14-23 To the best of our knowledge, no reports have been published on the purification of stilbenes from Polygonum cillinerve (Nakai) Ohwl by HSCCC.

In this paper, a convenient and efficient method has been successfully established for the separation and purification of trans-resveratrol-3-O-glucoside, pieceid-2-O-gallate, and trans-resveratrol from the extract of traditional medicinal herb Polygonum cillinerve (Nakai) Ohwl using macroporous resin column chromatography combined with HSCCC. The chemical structures of the three stilbenes are shown in Figure 1.

EXPERIMENTAL

Apparatus

HSCCC was performed on a TBE-300A instrument (Tauto Biotechnique Company, Shanghai, China) with three multilayer coil separation columns connected in series (1.6 mm, total volume = 300 mL) and a 20 mL sample loop. The revolution radius was 5 cm, and the β-values of the multilayer coil varied from 0.5 at the internal terminal to 0.8 at the external terminal. The revolution speed of the apparatus can be regulated with a speed controller in the range of 0 and 1000 rpm. An HX-1050 constant temperature circulating implement (Beijing Boyikang Lab Instrument Co. Ltd., Beijing, China) was used to control the separation temperature. An ÄKTA prime system (Amersham Pharmacia Biotechnique Group, Sweden) was used to pump the two-phase solvent and measure the UV absorbance. This system contains a switch valve and a mixer, which were used for gradient formation. The data were collected with an N-2000 chromatography workstation (Zhejiang university, Zhejiang, China). The HPLC equipment used was a Waters 515 HPLC system including a Waters Quat pump, a 2996 DAD, and an Empower HPLC workstation. Nuclear magnetic resonance (NMR) spectrometry was carried out on a Mercury Plus 400 NMR (Varian Inc., USA) with tetramethylsilane (TMS) as the internal standard.

Reagents and materials

All solvents used for the preparation of crude samples and HSCCC separation were of analytical grade (Tianjin Baishi Reagent Factory, Tianjin, China). Methanol used for HPLC was of chromatographic grade (Shandong Yuwang Chemical Factory, Shandong, China), and the water used was distilled water. Methanol-D4 was used as the solvent for NMR determination.

The radix of Polygonum cillinerve (Nakai) Ohwl was collected from Xining, Qinghai, China in 2012 and identified by Professor Shilong Cheng (Northwest Institute of Plateau Biology, Qinghai, China). A voucher specimen was deposited in the herbarium of the Northwest Institute of Plateau Biology, Xining, Qinghai, China.

Crude sample preparation

The air-dried and powered radix of Polygonum cillinerve (Nakai) Ohwl (2.5 kg) was extracted three times with 75% ethanol (each time for 2 h). After evaporation under vacuum, the extract was suspended in water and then fractionated with petroleum ether (bp. ~60-90 ºC, 2.5 L × 3 times), ethyl acetate (2.5 L × 3 times) and n-butanol (2.5 L × 3 times). The ethyl acetate solutions were evaporated to dryness under vacuum at 60 ºC to generate 180 g of ethyl acetate extract.

Macroporous resin column chromatography

In order to enrich the target components, the extract of ethyl acetate (180 g) was dissolved in deionized water, loaded into a macroporous resin column (140 × 12 cm containing 10 kg AB-8 MR), and eluted with various proportions of water/ethanol mixture (100:0, 80:20, 70:30, 60:40, 40:60, and 20:80 v/v; about 10 L for each gradient). The flow rate was controlled at approximately 20 mL min¹. The water-ethanol (60:40) fraction was concentrated to yield 8 g of crude sample for subsequent HSCCC isolation and purification.

Preparation of two-phase solvent system and sample solution

The two-phase solvent system used for HSCCC separation was composed of chloroform-n-butanol-methanol-water at a ratio of 4:1:4:2 (v/v/v/v). The solvent mixture was prepared by adding the solvents to a separation funnel according to the volume ratios and thoroughly equilibrated at room temperature. The upper and lower phases were then separated and degassed by sonication prior to use. The HSCCC sample solution was prepared by dissolving 150 mg of crude extract sample in 10 mL of the upper phase of the two-phase solvent system.

HSCCC separation procedure

First, the multilayer coil column was entirely filled with the upper phase (stationary phase). The apparatus was then rotated at 800 rpm while the lower phase (mobile phase) was pumped into the column at a flow rate of 2.0 mL min¹. After hydrodynamic equilibrium was reached, as indicated by the emergence of the mobile phase front, the sample solution (150 mg of crude sample dissolved in 10 mL of the upper phase) was injected into the separation column through the injection valve using an ÄKTA prime system. The separation temperature was controlled at 25 ºC. The effluent from the tail end of the column was continuously monitored by a UV detector at 300 nm. Different fractions were collected manually according to the obtained chromatogram and evaporated to dryness under reduced pressure. The residuals were dissolved in methanol for subsequent HPLC analysis. The purity was obtained by HPLC peak area calculation.

HPLC analysis and identification of HSCCC peak fractions

The crude sample and each HSCCC peak fraction were analyzed by HPLC. HPLC analysis was performed on a Merck LiChrospher C₁₈ column (250 mm × 4.6 mm; dp = 5 µm) at 25 ºC. The mobile phase was methanol-water (35:75, v/v). The flow-rate and detection wavelength were set at 1.0 mL min¹ and 300 nm, respectively. The crude sample and peak fractions separated by HSCCC were analyzed by HPLC under the optimum analytical conditions, and the chromatograms are presented in Figure 2. The identification of HSCCC peak fractions was performed by ¹H and ¹³C NMR spectroscopy.

RESULTS AND DISCUSSION

Optimization of the two-phase solvent system and other HSCCC conditions

Successful HSCCC separation depends on the selection of a suitable two-phase solvent system, which provides an ideal partition coefficient range (0.2 < K < 2) for the target compounds. ²⁴ Large K values tend to produce excessive band broadening, while small K values usually result in a poor peak resolution. In the present study, different solvent systems including ethyl acetate-water, ethyl acetate-methanol-water, chloroform-methanol-water, and chloroform-n-butanol-methanol-water were tested according to the procedure described in the measurement of partition coefficient section. The K-values of the target compounds in different solvent systems were determined by HPLC, and the results are shown in Table 1. When two-phase solvent systems comprised of ethyl acetate-water (5:5, v/v) and ethyl acetate-methanol-water (5:5:5, 5:3:5, v/v/v) were employed, the K values were too large, resulting in broad peaks and long separation times. When the two-phase solvent system composed of ethyl acetate-methanol-water (3:3:5, v/v/v) was investigated, suitable K values of the target compounds were obtained; however, the separation factor was too small, which would result in poor separation. When two-phase solvent systems composed of chloroform-methanol-water (4:3:3, v/v/v) and chloroform-n-butanol-methanol-water (4:0.5:4:2, v/v/v/v) were used, the K values were large, which might lead to the poor retention of target compounds in the upper phase. Fortunately, an appropriate K value with good resolution could be obtained by using a two-phase solvent system of chloroform-n-butanol-methanol-water at the ratio of 4:1:4:2 (v/v/v/v). The K values of the three target compounds were between 0.5 and 2.0, and the separation factors were also large enough.

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The influence of the mobile phase flow rate was also investigated. The results indicated reducing the flow rate could improve the retention of the stationary phase to a certain extent, but the chromatogram peaks were extended at the same time. ²⁵ Thus, a flow rate of 2.0 mL min¹ was employed in this study. Additionally, the revolution speed can also impact stationary phase retention; a high revolution speed is likely to cause emulsification. ²⁶ Considering of this, a speed of 800 rpm was used in our isolation procedure.

HSCCC separation

Under the optimized conditions, three fractions (I, II, and III) were obtained in only one round of HSCCC separation in less than 4 h. The HSCCC chromatogram is shown in Figure 3. Three fractions were obtained from 150 mg crude sample by the one-step HSCCC separation: 26.3 mg trans-resveratrol-3-O-glucoside (peak I), 42.0 mg pieceid-2-O-gallate (peak II), and 17.9 mg trans-resveratrol (peak III). The purities of trans-resveratrol-3-O-glucoside, pieceid-2-O-gallate, and trans-resveratrol were 99.1%, 97.8%, and 99.4%, respectively (Figure 2), as determined by HPLC.

Structural identification

The chemical structure of each peak fraction separated by HSCCC was identified according to its ¹H-NMR and ¹³C-NMR data. In comparison with reference data, peak I, peak II, and peak III were effectively identified as trans-resveratrol-3-O-glucoside, pieceid-2-O-gallate and trans-resveratrol, respectively. The results for each peak fraction were as follows.

Peak I, white powder (methanol): ¹H NMR (CD₃OD, 400 MHz): δ = 7.35 (2H, d, J = 8.5 Hz, H-2', H-6'), 7.00 (lH, d, J = 16.3 Hz, H-8), 6.84 (lH, d, H-7), 6.78 (1H, s, H-2), 6.76 (2H, d, H-3', H-5'), 6.61 (1H, s, H-6), 6.44 (1H, s, H-4), 4.88 (1H, d, J = 7.1Hz, Glc H-1), 3.92 (1H, dd, J = 1.5 Hz, J = 12 Hz, Glc H-6a), 3.70 (1H, dd, J = 5.8 Hz, Glc H-6b), 3.48-3.38 (4H, m, Glc H-2, H-3, H-4, H-5). ¹³C NMR (400 MHz, CD₃OD): δ = 141.4 (C-1), 107.0 (C-2), 160.5 (C-3), 104.1 (C-4), 159.6 (C-5), 108.4 (C-6), 126.7 (C-7), 130.0 (C-8), 130.3 (C-1'), 128.9 (C-2'), 116.5 (C-3'), 158.5 (C-4'), 116.5 (C-5'),128.9 (C-6'), 102.4 (Glc-1), 75.0 (Glc-2), 78.1 (Glc-3), 71.5 (Glc-4),78.3 (Glc-5) and 62.6 (Glc-6). The ¹H NMR and ¹³C NMR data are in agreement with the literature data for trans-resveratrol-3-O-glucoside. ²⁷

Peak II, white powder (methanol): ¹H NMR (CD₃OD, 400 MHz): δ = 7.39 (2H, d, J =8.5 Hz, H-2', H-6'), 7.16 (2H, d, J = 8.5 Hz, H-2"', H-6"'),7.03 (lH, d, J = 16.3 Hz, H-8), 6.85 (lH, d, H-7), 6.82 (2H, d, H-3', H-5'),6.70 (1H, s, H-2), 6.65 (1H, s, H-6), 6.38 (1H, s, H-4), 5.14 (1H, d, J = 7.9Hz, Glc H-1), 4.02 (1H, dd, J = 11.4 Hz, Glc H-6a), 3.70 (1H, m, Glc H-6b), 5.14-3.45 (4H, m, Glc H-2, H-3, H-4. H-5). ¹³C NMR (400 MHz, CD₃OD): δ = 139.9 (C-1), 109.0 (C-2), 160.5 (C-3),104.1 (C-4), 159.6 (C-5), 107.4 (C-6), 126.7 (C-7), 130.0 (C-8),130.3 (C-1'), 128.9 (C-2'), 116.5 (C-3'), 158.5 (C-4'), 116.5 (C-5'),128.9 (C-6'), 102.4 (Glc-1), 78.4 (Glc-2), 76.1(Glc-3), 71.5 (Glc-4), 75.4 (Glc-5), 62.6 (Glc-6), 121.3 (C-1"'), 109.9 (C-2"'), 146.5 (C-3"'), 141.5 (C-4"'), 146.5 (C-5"'), 109.9 (C-6"') and 167.8(C-7"'). The ¹H NMR and ¹³C-NMR data are in agreement with the data for pieceid-2-O-gallate in the literature. ²⁸

Peak III, white powder (methanol): ¹H NMR (CD₃OD, 400 MHz): δ = 7.33 (2H, d, J = 8.5 Hz, H-2', H-6'), 6.96 (lH, d, J = 16.3 Hz, H-8), 6.81 (lH, d, H-7), 6.75 (2H, d, H-3', H-5') , 6.45 (2H, s, H-2, H-6), 6.17 (1H, s, H-4). ¹³C NMR (CD₃OD, 400 MHz): δ = 141.3 (C-1), 105.7 (C-2), 159.6 (C-3),102.6 (C-4), 158.3 (C-5), 105.7 (C-6), 126.9 (C-7), 129.4 (C-8), 130.4 (C-1'), 128.8 (C-2'), 116.5 (C-3'), 158.5 (C-4'), 116.5 (C-5'), 128.8 (C-6'), The ¹H NMR and ¹³C NMR data are in agreement with the data for trans-resveratrol in the literature. ²⁹

CONCLUSION

In the present study, A convenient and efficient method for the preparative separation and purification of three active components (trans-resveratrol-3-O-glucoside, pieceid-2-O-gallate and trans-resveratrol) from the Chinese traditional herb Polygonum cillinerve (Nakai) Ohwl was successfully developed using macroporous resin column chromatography combined with high-speed counter-current chromatography. The compounds obtained may be used as reference substances for chromatographic purposes as well as for further pharmaceutical studies. The method might also be successfully applied to the separation of various other stilbenes from natural products.

ACKNOWLEDGMENTS

This work was supported by the Equipment Function Development Innovation Programs of the Chinese Academy of Sciences (Grant No. yg2012086) and the National Natural Science Foundation of China (Grant No. 41203018)

Recebido em 26/03/2014

aceito em 08/07/2014

publicado na web em 22/09/2014

1. Gang, A. S.; Cai, X.; J. Syst. Evol. 2008, 46, 742.
2. Editorial Committee of Chinese Bencao of State Administration of Chinese Materia Medica of State Administration of Traditional Chinese Medicine; Chinese Bencao; Shanghai Science and Technology Publishing House: Shanghai, 2000.
3. Yoshizaki, M.; Fujino, H.; Arise, A.; Ohmura, K.; Arisawa, M.; Morita, N.; Planta Med. 1987, 273.
4. Iliya, I.; Tanaka, T.; Iinuma, M.; Ali, Z.; Furasawa, M.; Nakaya, K.; Shirataki, Y.; Murata, J.; Darnaedi, D.; Chem. Pharm. Bull. 2002, 50, 796.
5. Chu, X.; Sun, A. L.; Liu, R. M.; J. Chromatogr. A 2005, 1097, 33.
6. Teguo, P. W.; Fauconneau, B.; Deffieux, G.; Huguet, F.; Vercauteren, J.; Merillon, J.M.; J. Nat. Prod. 1998, 61, 655.
7. Merillon, J. M.; Fauconneau, B.; Teguo, P. W.; Barrier, L.; Vercauteren, J.; Huguet, F.; Clin. Chem. 1997, 43, 1092.
8. Fauconneau, B.; WaffoTeguo, P.; Huguet, F.; Barrier, L.; Decendit, A.; Merillon, J. M.; Life Sci. 1997, 61, 2103.
9. Liu, A.L.; Yang, F.; Zhu, M. A.; Zhou, D.; Lin, M.; Lee, S. M. Y.; Wang, T.; Du, G. H.; Planta Med. 2010, 76, 1874.
10. Pacher, T.; Seger, C.; Engelmeier, D.; Vajrodaya, S.; Hofer, O.; Greger, H.; J. Nat. Prod. 2002, 65, 820.
11. Pflieger, A.; Teguo, P. W.; Papastamoulis, Y.; Chaignepain, S.; Subra, F.; Munir, S.; Delelis, O.; Lesbats, P.; Calmels, C.; Andreola, M. L.; Merillon, J. M.; Auge-Gouillou, C.; Parissi, V.; PLoS One 2013, 8, e81184.
12. Dai, J. R.; Hallock, Y. F.; Cardellina, J. H.; Boyd, M. R.; J. Nat. Prod. 1998, 61, 351.
13. Ito, Y; Conway, W. D.; Anal. Chem. 1984, 56, A534.
14. Fang, L.; Liu, Y. Q.; Yang, B.; Wang, X.; Huang, L. Q.; J. Sep. Sci. 2011, 34, 2545.
15. Sun, Y. S.; Lin, H. M.; Wang, J. H.; Hu, J. N.; Liu, Z. B; Gao, A. D.; Phytochem. Anal. 2011, 22, 526.
16. Lu, H. T.; Liu, J.; Deng, R.; Song, J. Y.; Phytochem. Anal. 2012, 23, 637.
17. Wang, D. J.; Lin, Y. L.; Lin, X. J.; Geng, Y. L.; Wang, X.; Zhang, J. J.; Qiu, J. Y.; Quim. Nova 2012, 35, 337.
18. Xu, P. P.; Guan, S. H.; Feng, R. H.; Tang, R. N.; Guo, D. A.; Phytochem. Anal. 2012, 23, 228.
19. Chu, C.; Zhang, S. D.; Tong, S. Q.; Li, X. N.; Yan, J. Z.; J. Sep. Sci. 2013, 36, 3958.
20. Li, J. L.; Zhang, Y. Q.; Lin, Y. L.; Wang, X.; Fang, L.; Geng, Y. L.; Zhang, Q. D.; Quim. Nova 2013, 36, 686.
21. Liang, J. R.; Ito, Y.; Zhang, X. X.; He, J.; Sun, W. J.; J. Sep. Sci. 2013, 36, 3934.
22. Shu, X. K.; Wang, M.; Liu, D. C.; Wang, D. J.; Lin, X. J.; Liu, J. H.; Wang, X.; Huang, L.Q.; Quim. Nova 2013, 36, 836.
23. Liu, F.; Xi, X. J.; Wang, M.; Fan, L.; Geng, Y. L.; Wang, X.; J. Sep. Sci. 2014, 37, 376.
24. Oka, F.; Oka, H.; Ito, Y.; J. Chromatogr. 1991, 538, 99.
25. Yue, H. L.; Zhao, X. H.; Mei, L. J.; Shao, Y.; J. Sep. Sci. 2013, 36, 3123.
26. Wang, P.; Liu, Y. L.; Chen, T.; Xu, W. H.; You, J. M.; Liu, Y. J.; Li, Y. L.; Phytochem. Anal. 2013, 24, 603.
27. Teguo, P. W.; Decendit, A.; Vercauteren, J.; Deffieux, G.; Merillon, J. M.; Phytochemistry 1996, 42, 1591.
28. Lee, J. P.; Min, B. S.; An, R. B.; Na, M. K.; Lee, S. M.; Lee, H. K.; Kim, J. G.; Bae, K. H.; Kang, S. S.; Phytochemistry 2003, 64, 759.
29. Chen, L.; Han, Y. S.; Yang, F. Q.; Zhang, T. Y.; J. Chromatogr. A 2001, 907, 343.

*

e-mail:

hufz@nwipb.cas.cn

Publication Dates

Publication in this collection
24 Oct 2014
Date of issue
2014

History

Accepted
08 July 2014
Received
26 Mar 2014

This work is licensed under a Creative Commons Attribution-NonCommercial 4.0 International License.

[1] 1. Gang, A. S.; Cai, X.; J. Syst. Evol. 2008, 46, 742.

[2] 2. Editorial Committee of Chinese Bencao of State Administration of Chinese Materia Medica of State Administration of Traditional Chinese Medicine; Chinese Bencao; Shanghai Science and Technology Publishing House: Shanghai, 2000.

[3] 3. Yoshizaki, M.; Fujino, H.; Arise, A.; Ohmura, K.; Arisawa, M.; Morita, N.; Planta Med. 1987, 273.

[4] 4. Iliya, I.; Tanaka, T.; Iinuma, M.; Ali, Z.; Furasawa, M.; Nakaya, K.; Shirataki, Y.; Murata, J.; Darnaedi, D.; Chem. Pharm. Bull. 2002, 50, 796.

[5] 5. Chu, X.; Sun, A. L.; Liu, R. M.; J. Chromatogr. A 2005, 1097, 33.

[6] 6. Teguo, P. W.; Fauconneau, B.; Deffieux, G.; Huguet, F.; Vercauteren, J.; Merillon, J.M.; J. Nat. Prod. 1998, 61, 655.

[7] 7. Merillon, J. M.; Fauconneau, B.; Teguo, P. W.; Barrier, L.; Vercauteren, J.; Huguet, F.; Clin. Chem. 1997, 43, 1092.

[8] 8. Fauconneau, B.; WaffoTeguo, P.; Huguet, F.; Barrier, L.; Decendit, A.; Merillon, J. M.; Life Sci. 1997, 61, 2103.

[9] 9. Liu, A.L.; Yang, F.; Zhu, M. A.; Zhou, D.; Lin, M.; Lee, S. M. Y.; Wang, T.; Du, G. H.; Planta Med. 2010, 76, 1874.

[10] 10. Pacher, T.; Seger, C.; Engelmeier, D.; Vajrodaya, S.; Hofer, O.; Greger, H.; J. Nat. Prod. 2002, 65, 820.

[11] 11. Pflieger, A.; Teguo, P. W.; Papastamoulis, Y.; Chaignepain, S.; Subra, F.; Munir, S.; Delelis, O.; Lesbats, P.; Calmels, C.; Andreola, M. L.; Merillon, J. M.; Auge-Gouillou, C.; Parissi, V.; PLoS One 2013, 8, e81184.

[12] 12. Dai, J. R.; Hallock, Y. F.; Cardellina, J. H.; Boyd, M. R.; J. Nat. Prod. 1998, 61, 351.

[13] 13. Ito, Y; Conway, W. D.; Anal. Chem. 1984, 56, A534.

[14] 14. Fang, L.; Liu, Y. Q.; Yang, B.; Wang, X.; Huang, L. Q.; J. Sep. Sci. 2011, 34, 2545.

[15] 15. Sun, Y. S.; Lin, H. M.; Wang, J. H.; Hu, J. N.; Liu, Z. B; Gao, A. D.; Phytochem. Anal. 2011, 22, 526.

[16] 16. Lu, H. T.; Liu, J.; Deng, R.; Song, J. Y.; Phytochem. Anal. 2012, 23, 637.

[17] 17. Wang, D. J.; Lin, Y. L.; Lin, X. J.; Geng, Y. L.; Wang, X.; Zhang, J. J.; Qiu, J. Y.; Quim. Nova 2012, 35, 337.

[18] 18. Xu, P. P.; Guan, S. H.; Feng, R. H.; Tang, R. N.; Guo, D. A.; Phytochem. Anal. 2012, 23, 228.

[19] 19. Chu, C.; Zhang, S. D.; Tong, S. Q.; Li, X. N.; Yan, J. Z.; J. Sep. Sci. 2013, 36, 3958.

[20] 20. Li, J. L.; Zhang, Y. Q.; Lin, Y. L.; Wang, X.; Fang, L.; Geng, Y. L.; Zhang, Q. D.; Quim. Nova 2013, 36, 686.

[21] 21. Liang, J. R.; Ito, Y.; Zhang, X. X.; He, J.; Sun, W. J.; J. Sep. Sci. 2013, 36, 3934.

[22] 22. Shu, X. K.; Wang, M.; Liu, D. C.; Wang, D. J.; Lin, X. J.; Liu, J. H.; Wang, X.; Huang, L.Q.; Quim. Nova 2013, 36, 836.

[23] 23. Liu, F.; Xi, X. J.; Wang, M.; Fan, L.; Geng, Y. L.; Wang, X.; J. Sep. Sci. 2014, 37, 376.

[24] 24. Oka, F.; Oka, H.; Ito, Y.; J. Chromatogr. 1991, 538, 99.

[25] 25. Yue, H. L.; Zhao, X. H.; Mei, L. J.; Shao, Y.; J. Sep. Sci. 2013, 36, 3123.

[26] 26. Wang, P.; Liu, Y. L.; Chen, T.; Xu, W. H.; You, J. M.; Liu, Y. J.; Li, Y. L.; Phytochem. Anal. 2013, 24, 603.

[27] 27. Teguo, P. W.; Decendit, A.; Vercauteren, J.; Deffieux, G.; Merillon, J. M.; Phytochemistry 1996, 42, 1591.

[28] 28. Lee, J. P.; Min, B. S.; An, R. B.; Na, M. K.; Lee, S. M.; Lee, H. K.; Kim, J. G.; Bae, K. H.; Kang, S. S.; Phytochemistry 2003, 64, 759.

[29] 29. Chen, L.; Han, Y. S.; Yang, F. Q.; Zhang, T. Y.; J. Chromatogr. A 2001, 907, 343.

Brasil

Brasil

Separation and purification of three stilbenes from the radix of Polygonum cillinerve (Nakai) Ohwl by macroporous resin column chromatography combined with high-speed counter-current chromatography

Abstract

Publication Dates

History