人血浆直接注射柱切换生物分析法测定磺脲类药物

Juliana Veloso Ferreira, G. A. Pianetti, C. Fernandes
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引用次数: 1

摘要

磺胺脲类药物被广泛用于治疗糖尿病,糖尿病是人类死亡的主要原因之一。它们的测定在药理学研究和新药开发中是必不可少的。一般来说,测定生物基质中的磺脲类是使用传统的样品制备技术进行的,这经常导致分析时间和误差的增加。在此背景下,建立并优化了人血浆直接注射同时测定磺胺脲类药物的生物分析方法。采用了一种具有限制访问介质(RAM)柱与熔芯柱耦合的高效液相色谱自动切换系统。第一维采用RAM色谱柱,流动相为pH 6.0的超纯水,流速为1.0 mL min-1。阀门切换时间为3分钟。在第二次元上,采用C18保护柱与C18熔芯柱耦合,流动相为乙腈和10 mM磷酸盐缓冲液pH 3.0 (54:46 v/v),流速为0.8 mL min-1。色谱柱切换系统在反冲洗配置下进行,分析物洗脱时间为1分钟。以氟芬那酸为内标。ram柱平均血浆蛋白排除率为104.5%。所建立和优化的方法快速简便,可将生物样品直接注入色谱系统,在12分钟内同时测定3种磺脲类化合物,包括样品处理、分离和检测。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
BIOANALYTICAL METHOD BY COLUMN-SWITCHING WITH DIRECT INJECTION OF HUMAN PLASMA FOR DETERMINATION OF SULPHONYLUREAS
Sulphonylureas are widely used in the treatment of Diabetes mellitus, one of the main causes of death in human population. Their determination is essential in pharmacological research and in the development of new drugs. Generally, determination of sulphonylureas in biological matrices is performed using conventional sample preparation techniques, which frequently leads to an increase of analysis time and errors. In this context, a bioanalytical method for the simultaneous determination of sulphonylureas by direct injection of human plasma was developed and optimized. An automated column-switching high performance liquid chromatographic system with a restricted access media (RAM) column coupled to a fused-core column was employed. At the first dimension, a RAM column with mobile phase of ultrapure water pH 6.0 at a flow-rate of 1.0 mL min-1 was used. The valve switching time was 3 minutes. At the second dimension, a C18 guard-column coupled to a C18 fused core column with mobile phase of acetonitrile and 10 mM phosphate buffer pH 3.0 (54:46 v/v) at a flow-rate of 0.8 mL min-1 were employed. The column switching system was performed in backflush configuration with an analyte elution time of 1 minute. Flufenamic acid was used as the internal standard. The mean plasma protein exclusion percentage by the RAM-column was 104.5%. The developed and optimized method showed to be fast and simple, allowing the direct injection of biological sample into the chromatographic system and the simultaneous determination of three sulphonylureas in only 12 minutes, including the sample treatment, separation and detection.
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