Development of a High-Performance Liquid Chromatography-Tandem Mass Spectrometry (HPLC-MS/MS) Method to Determine the Presence of Rivastigmine in Human Plasma in Clinical Studies of Comparative Pharmacokinetics

Antibiotics and Chemotherapy Pub Date : 2023-02-11 DOI:10.37489/0235-2990-2022-67-11-12-22-28

M. S. Dolov, L. Fishgoit, P. Sobolev, E. P. Tkach

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Abstract

The basis for conducting bioequivalence studies is the determination of the bioavailability of the active substance of the drug at its place of action by establishing the concentration of the drug in biological ﬂuids using sensitive analytical techniques. The bioanalytical technique used should provide reliable results which would lead to satisfactory level of interpretation. To investigate the bioequivalence of rivastigmine preparations, an 8 times more sensitive method (compared to the data in the available literature) for the quantitative determination of rivastigmine in human blood plasma by HPLC-MS/MS was developed. Rivastigmine is extracted from plasma by precipitation of plasma proteins with acetonitrile. Chromatographic separation of rivastigmine and the internal standard was carried out on a YMC Triart C18. 50×2.0 mm (1.9 µm) column in a gradient elution mode with a ﬂow rate of 0.5 ml/min. A 0.1% solution of ammonium hydroxide and acetonitrile were used as mobile phases. The lower limit of the quantitative determination of the method was 25 pg/ml.

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建立高效液相色谱-串联质谱(HPLC-MS/MS)测定人血浆中利瓦斯汀存在的比较药代动力学临床研究方法

进行生物等效性研究的基础是利用灵敏的分析技术确定药物在生物液中的浓度，从而确定药物的活性物质在其作用部位的生物利用度。所使用的生物分析技术应提供可靠的结果，从而导致令人满意的解释水平。为了研究利瓦斯汀制剂的生物等效性，建立了一种灵敏度比现有文献高8倍的人血浆中利瓦斯汀的HPLC-MS/MS定量测定方法。利瓦斯汀是用乙腈沉淀血浆蛋白从血浆中提取的。在YMC Triart C18上对利瓦斯汀和内标进行色谱分离。50×2.0 mm(1.9µm)柱，梯度洗脱模式，流速为0.5 ml/min。以0.1%的氢氧化铵和乙腈溶液为流动相。本方法的定量下限为25 pg/ml。

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Antibiotics and Chemotherapy

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