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使用气相色谱-质谱分析法对肝微粒体和纯化的细胞色素P-450催化的氟烷氧化进行表征。

Characterization of halothane oxidation by hepatic microsomes and purified cytochromes P-450 using a gas chromatographic mass spectrometric assay.

作者信息

Gruenke L D, Konopka K, Koop D R, Waskell L A

机构信息

Department of Pharmaceutical Chemistry, University of California, San Francisco.

出版信息

J Pharmacol Exp Ther. 1988 Aug;246(2):454-9.

PMID:3404442
Abstract

A sensitive assay for trifluoroacetic acid, the major product of the oxidative metabolism of halothane, has been developed to study the biotransformation of halothane. A selected ion monitoring gas chromatographic mass spectrometric assay measured trifluoroacetic acid levels as low as 1 microM in 100 microliter of reaction mixture. This assay was used to quantitate halothane metabolism in human and rabbit microsomal systems and with purified proteins. Trifluoroacetic acid production was examined as a function of the concentration of substrate present, the amount of microsomal protein used and the length of reaction time. Halothane metabolism in microsomes was linear for at least 30 min, and up to a microsomal protein concentration of 1 mg/ml. In rabbits, phenobarbital and imidazole induced the microsomal metabolism of halothane 7.36- and 18.2-fold, respectively. Imidazole was used because it is a potent inducer of cytochrome P-450 isozyme 3a which is also induced by ethanol. The cytochrome P-450 in microsomes from a single human subject metabolized halothane at a rate comparable to that found in microsomes from phenobarbital- and imidazole-pretreated rabbits. The purified phenobarbital and imidazole inducible cytochromes P-450, isozymes 2 and 3a, catalyzed the oxidation of halothane to trifluoroacetic acid. Cytochrome b5 stimulated the isozyme 3a-catalyzed oxidation of halothane by 19-fold, whereas isozyme 2 catalyzed oxidation was increased 4.3-fold. Antibodies to cytochrome P-450 3a inhibited halothane metabolism by 90% in microsomes from imidazole-pretreated rabbits, suggesting that isozyme 3a catalyzes halothane metabolism in imidazole-pretreated rabbits. In conclusion, the oxidation of halothane to trifluoroacetic acid by cytochrome P-450 isozymes 3a and 2 is enhanced markedly by cytochrome b5.

摘要

已开发出一种用于检测三氟乙酸(氟烷氧化代谢的主要产物)的灵敏检测方法,以研究氟烷的生物转化。一种选定离子监测气相色谱 - 质谱测定法可在100微升反应混合物中测量低至1微摩尔的三氟乙酸水平。该检测方法用于定量人和兔微粒体系统以及纯化蛋白质中的氟烷代谢。将三氟乙酸的产生作为底物浓度、所用微粒体蛋白量以及反应时间长度的函数进行了研究。微粒体中的氟烷代谢在至少30分钟内呈线性,直至微粒体蛋白浓度达到1毫克/毫升。在兔中,苯巴比妥和咪唑分别使氟烷的微粒体代谢诱导了7.36倍和18.2倍。使用咪唑是因为它是细胞色素P - 450同工酶3a的强效诱导剂,乙醇也可诱导该同工酶。来自单个受试者的微粒体中的细胞色素P - 450代谢氟烷的速率与苯巴比妥和咪唑预处理兔的微粒体中发现的速率相当。纯化的苯巴比妥和咪唑诱导的细胞色素P - 450同工酶2和3a催化氟烷氧化为三氟乙酸。细胞色素b5使同工酶3a催化的氟烷氧化增加了19倍,而同工酶2催化的氧化增加了4.3倍。针对细胞色素P - 450 3a的抗体在咪唑预处理兔的微粒体中使氟烷代谢抑制了90%,这表明同工酶3a催化咪唑预处理兔中的氟烷代谢。总之,细胞色素b5显著增强了细胞色素P - 450同工酶3a和2将氟烷氧化为三氟乙酸的过程。

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