Bio-analytical Development and Validation of RP-HPLC Liquid Method for Quantification of Dapagliflozin Propanediol in Spiked Human Plasma

P. Subbareddy, T. Divakar
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Abstract

The purpose of the present research was to develop a suitable simple and reproducible RP-HPLC method for a quantification of dapagliflozin propanediol in spiked human plasma samples. The liquidliquid extraction plasma spiked samples of dapagliflozin propanediol were analyzed by using a ODS C18 Prontosil column under isocratic conditions. The extracted plasma spiked samples were carried using methanol, acetonitrile and pH 5.6 acetate buffer in the ratio of 50:20:10 (v/v) with a flow rate of 0.9 mL/min. The detector response was monitored at 228 nm using UV detector. The method was validated as per the ICH guidelines for bio analytical method validation and all the validation parameters were found to be within the acceptance limit The plasma spiked samples shows stability at room temperature over a period of 48 h. Thus, this method would be employed for routine quantification of dapagliflozin in human plasma samples.
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RP-HPLC液相法定量人血浆中达格列净丙二醇的生物分析方法建立与验证
本研究的目的是建立一种简便、重现性好的反相高效液相色谱法定量人血浆中达格列净丙二醇的含量。采用ODS C18型Prontosil色谱柱,在等压条件下对达格列净丙二醇的液液萃取血浆加标样品进行了分析。提取的血浆加标样品用甲醇、乙腈和pH 5.6的醋酸缓冲液以50:20:10 (v/v)的比例携带,流速为0.9 mL/min。在228 nm处用紫外检测器监测探测器的响应。该方法按照ICH生物分析方法验证指南进行了验证,所有验证参数均在可接受范围内。血浆加标样品在室温下48小时内表现出稳定性。因此,该方法可用于人血浆样品中达格列净的常规定量。
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