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用于测定番泻叶片中番泻苷A和B的经过验证的高效液相色谱法。

Validated HPLC method for determination of sennosides A and B in senna tablets.

作者信息

Sun Shao Wen, Su Hsiu Ting

机构信息

School of Pharmacy, National Taiwan University, 1 Jen-Ai Road Sec. 1, Taipei, Taiwan, ROC.

出版信息

J Pharm Biomed Anal. 2002 Jul 31;29(5):881-94. doi: 10.1016/s0731-7085(02)00208-x.

DOI:10.1016/s0731-7085(02)00208-x
PMID:12093522
Abstract

This study developed an efficient and reliable ion-pair liquid chromatographic method for quantitation of sennosides A and B in commercial senna tablets. Separation was conducted on a Hypersil C 18 column (250 x 4.6 mm, 5 microm) at a temperature of 40 degrees C, using a mixture of 0.1 M acetate buffer (pH 6.0) and acetonitrile (70:30, v/v) containing 5 mM tetrahexylammonium bromide as mobile phase. Sennosides A and B were completely separated from other constituents within 14 min. The developed method was validated. Both run-to-run repeatability (n=10) and day-to-day reproducibility (n=3) of peak area were below 0.4% RSD. Linearity of peak area was tested in the range 30-70 microg/ml (r>0.9997). Accuracy was assessed with recovery and the recoveries for sennosides A and B were 101.73+/-1.30% and 101.81+/-2.18% (n=3 x 6), respectively. Robustness of the analytical method was tested using a three-leveled Plackett-Burman design in which 11 factors were assessed with 23 experiments. Eight factors (column, concentration of ion pair reagent, % of organic modifier (acetonitrile), buffer pH, column temperature, flow rate, time constant and detection wavelength) were investigated in a specified range above and below the nominal method conditions. It was found that: (1) column and % acetonitrile affected significantly resolution and retention time, (2) column, % acetonitrile, column temperature, flow rate and time constant affected significantly the plate number of sennoside A, and (3) column and time constant affected significantly the tailing factor.

摘要

本研究建立了一种高效可靠的离子对液相色谱法,用于定量测定市售番泻叶片中的番泻苷A和番泻苷B。采用Hypersil C 18柱(250×4.6 mm,5μm),在40℃下进行分离,以含5 mM溴化四己基铵的0.1 M醋酸盐缓冲液(pH 6.0)和乙腈(70:30,v/v)的混合物为流动相。番泻苷A和番泻苷B在14分钟内与其他成分完全分离。所建立的方法经过了验证。峰面积的批内重复性(n = 10)和日间重现性(n = 3)的相对标准偏差均低于0.4%。在30 - 70μg/ml范围内测试了峰面积的线性(r>0.9997)。通过回收率评估准确度,番泻苷A和番泻苷B的回收率分别为101.73±1.30%和101.81±2.18%(n = 3×6)。使用三级Plackett - Burman设计测试了分析方法的稳健性,其中通过23次实验评估了11个因素。在标称方法条件的上下指定范围内研究了8个因素(柱、离子对试剂浓度、有机改性剂(乙腈)百分比、缓冲液pH、柱温、流速、时间常数和检测波长)。结果发现:(1)柱和乙腈百分比对分离度和保留时间有显著影响;(2)柱、乙腈百分比、柱温、流速和时间常数对番泻苷A的塔板数有显著影响;(3)柱和时间常数对拖尾因子有显著影响。

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