舒胸片中人参皂苷Rg_1、人参皂苷Rb_1和三七皂苷R_1含量测定  被引量:1

Qualification and Quantification of Ginsenoside Rg_1, Rb_1 and Notoginsenoside R_1 in Shuxiong Tablet by HPLC

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作  者:漆亮 王栋 杨毅生 

机构地区:[1]江西省药品认证中心,江西南昌330046 [2]江西省食品药品检验所,江西南昌330029

出  处:《药品评价》2013年第24期24-24,26,27,共3页Drug Evaluation

基  金:国家药典委员会<中国药典>2010版一部标准研究项目;编号:ZW-208

摘  要:目的:建立舒胸片中人参皂苷Rg1、人参皂苷Rb,和三七皂苷R1含量的HPLCI]定方法。方法:采用DiamosilC18柱(4.6X250mm,5gm),流动相乙腈一水,梯度洗脱,柱温30℃,流速lmL/min,203nm波长下检测。结果:人参皂苷Rg1、人参皂苷Rb1、三七皂苷R,分别在0.442~11.050gg(r=0.9999)、0.344~8.600μg(P=0.9999)、0.208~5.200gg(r=0.9995)范围内线性关系良好,平均回收率分别为98.93%(RSD为1.7%1、98.88%(RSD为1.4%)、98.98%(RSD为1.4%)。结论:以HPLC法检测舒胸片中人参皂苷Rg1、人参皂苷Rb1和三七皂苷R1,方法简便、准确、灵敏度高、重复性好。Objective: To develop a HPLC method for the qualification and quantification of ginsenoside Rg1, Rb, and notoginsenoside R, in Shuxiong Tablet. Methods: The column was Diamosil C18 (4.6 x 250mm, 5gm). The gradient elution mixture consisted of acetonitrile and water. The flow rate was lmL/min, and the column temperature and detection wavelength were 30℃ and 203 nm, respectively. Results: Linear ranges were 0.442 11.050 μg (1=0.9999) for ginsenoside Rg,, 0.344- 8.600 μg (r=0.9999) for ginsenoside Rb1, 0.208- 5.200 gg (r=0.9995) for notoginsenoside R,. The average recovery was 98.93% with RSD 1.7% for ginsenoside Rg1, 98.88% with RSD 1.4% for ginsenoside Rbl, 98.98% with RSD 1.4% for notoginsenoside R1. Conclusion: The established HPLC method is convenient, accurate, sensitive and repeatable.

关 键 词:舒胸片 人参皂苷RG 人参皂苷RB1 三七皂苷R1 HPLC法 

分 类 号:R286.0[医药卫生—中药学]

 

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