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一种采用柱前衍生化和荧光检测法测定血浆中6-巯基嘌呤的灵敏高效液相色谱法。

A sensitive high-performance liquid chromatographic method for the determination of 6-mercaptopurine in plasma using precolumn derivatization and fluorescence detection.

作者信息

Warren D J, Slørdal L

机构信息

Department of Clinical Pharmacology, Norwegian Radium Hospital, Oslo.

出版信息

Ther Drug Monit. 1993 Feb;15(1):25-30. doi: 10.1097/00007691-199302000-00004.

Abstract

A sensitive high-performance liquid chromatographic (HPLC) method for measuring plasma concentrations of 6-mercaptopurine (6-MP) is described. After protein precipitation with 5-sulfosalicylic acid, samples are subjected to precolumn derivatization using the thiol-reactive fluorophore monobromobimane (mBrB). The drug-mBrB adduct is then resolved by isocratic elution from a C18 reversed-phase support and quantified by fluorescence detection. Recovery of 6-MP after protein precipitation was consistently > 85% and the drug-mBrB adduct was found to be stable for at least 2 weeks at room temperature. With plasma samples containing 30 nM 6-MP, the assay displayed within-run (n = 6) and between-day (n = 6) coefficients of variation of 2.2 and 10.6%, respectively. The limit of detection for 6-MP in plasma was 3 nM (500 pg/ml) and the standard curve was linear up to 3 microM. Using this method, we have observed that 6-MP is stable in heparinized whole blood for at least 24 h provided samples are maintained on ice. Since this method requires few manipulations during sample preparation and is readily adaptable to automated techniques, it may prove useful in the routine clinical laboratory setting.

摘要

本文描述了一种用于测定血浆中6-巯基嘌呤(6-MP)浓度的灵敏高效液相色谱(HPLC)方法。用5-磺基水杨酸进行蛋白质沉淀后,样品使用硫醇反应性荧光团单溴代双马来酰亚胺(mBrB)进行柱前衍生化。然后,药物-mBrB加合物通过从C18反相载体上进行等度洗脱来分离,并通过荧光检测进行定量。蛋白质沉淀后6-MP的回收率始终>85%,并且发现药物-mBrB加合物在室温下至少稳定2周。对于含有30 nM 6-MP的血浆样品,该测定法的批内(n = 6)和批间(n = 6)变异系数分别为2.2%和10.6%。血浆中6-MP的检测限为3 nM(500 pg/ml),标准曲线在高达3 microM范围内呈线性。使用该方法,我们观察到,只要样品保持在冰上,6-MP在肝素化全血中至少稳定24小时。由于该方法在样品制备过程中所需操作较少,并且易于适应自动化技术,因此在常规临床实验室环境中可能证明是有用的。

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