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采用柱切换-高效液相色谱法结合荧光检测法测定大鼠、食蟹猴和人血浆中N-甲基-D-天冬氨酸受体NR2B亚基阻断剂Ro 63-1908的含量。

Determination of the N-methyl-D-aspartate receptor NR2B subunit blocker Ro 63-1908 in rat, cynomolgus monkey and human plasma by high-performance liquid chromatography with column switching and fluorescence detection.

作者信息

Wyss R, Bucheli F, Philipp W

机构信息

Pharmaceuticals Division, F. Hoffmann-La Roche Ltd., Basel, Switzerland.

出版信息

J Chromatogr A. 2000 Feb 18;870(1-2):189-98. doi: 10.1016/s0021-9673(99)01016-x.

Abstract

A HPLC method with automated column switching was developed and validated for the determination of Ro 63-1908 in rat and cynomolgus monkey plasma. Human plasma was used for calibration and was also included in the validation process. Ro 63-1908 belongs to a class of neuroprotective N-methyl-D-aspartate (NMDA) receptor blockers which were in development for the treatment of stroke and traumatic brain injury. The method involves deproteinisation of plasma samples with ethanol and direct injection of the supernatant (1.4 ml) into the HPLC column-switching system. To prevent a breakthrough of the analyte and the internal standard on the precolumn (Purospher RP-18, 75x4 mm) due to the high ethanol content, the injection solution was diluted, on-line, using an additional pump and a T-piece. 1% ammonium acetate-ethanol (100:2, v/v) was used as mobile phase for injection, as well as for on-line dilution, resulting in pre-concentration of the analyte and the internal standard on the precolumn. As Purospher RP-18 is a non-endcapped stationary phase with a special selectivity for amines, the analyte and the internal standard could then be selectively eluted with 30% acetonitrile (without any buffer in the mobile phase) and transferred to the analytical column [consisting of two coupled columns (125+250x4 mm) packed with Superspher 60 RP-select B], where they were separated by gradient elution and detected by fluorescence detection. Compared to the use of a 125 mm long precolumn and dilution of the supernatant with ammonium acetate prior to injection, the 75 mm precolumn and the on-line dilution procedure allowed about one third shorter run times (21 min) and, therefore, a higher sample throughput. The limit of quantification was 1 ng/ml using 0.4 ml plasma. The method was applied to more than 670 plasma samples from pharmacokinetic and toxicokinetic studies and is also suitable for other matrices and NMDA receptor blockers.

摘要

建立了一种具有自动柱切换功能的高效液相色谱(HPLC)方法,并对其进行了验证,用于测定大鼠和食蟹猴血浆中的Ro 63-1908。使用人血浆进行校准,并将其纳入验证过程。Ro 63-1908属于一类神经保护性N-甲基-D-天冬氨酸(NMDA)受体阻滞剂,正在开发用于治疗中风和创伤性脑损伤。该方法包括用乙醇对血浆样品进行脱蛋白处理,并将上清液(1.4 ml)直接注入HPLC柱切换系统。为防止由于乙醇含量高导致分析物和内标物在前柱(Purospher RP-18,75x4 mm)上穿透,使用额外的泵和T形管在线稀释进样溶液。1%醋酸铵-乙醇(100:2,v/v)用作进样以及在线稀释的流动相,从而使分析物和内标物在前柱上预富集。由于Purospher RP-18是一种对胺类具有特殊选择性的非封端固定相,然后可以用30%乙腈(流动相中无任何缓冲液)选择性洗脱分析物和内标物,并转移至分析柱[由两根串联的柱(125 + 250x4 mm)组成,填充有Superspher 60 RP-select B],在该柱上通过梯度洗脱进行分离,并通过荧光检测进行检测。与使用125 mm长的前柱并在进样前用醋酸铵稀释上清液相比,75 mm的前柱和在线稀释程序使运行时间缩短了约三分之一(21分钟),因此样品通量更高。使用0.4 ml血浆时定量限为1 ng/ml。该方法应用于药代动力学和毒代动力学研究的670多个血浆样品,也适用于其他基质和NMDA受体阻滞剂。

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