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大鼠肝脏微粒体将14C-甲苯激活为共价结合代谢物。

Activation of 14C-toluene to covalently binding metabolites by rat liver microsomes.

作者信息

Pathiratne A, Puyear R L, Brammer J D

出版信息

Drug Metab Dispos. 1986 Jul-Aug;14(4):386-91.

PMID:2873983
Abstract

14C-Toluene was incubated with rat liver microsomes in the presence of an NADPH-generating system and metabolites were concentrated on cyclohexyl cartridges. The metabolites were separated by reverse phase HPLC and identified by comparing the retention time to standards. 14C-Toluene was converted to 14C-benzylalcohol, 14C-cresols, and an unidentified 14C-metabolite. Some of the radioactivity was found to bind covalently to microsomal macromolecules, preferentially to proteins. The binding was proportional to incubation time and microsomal protein concentration and required NADPH and molecular oxygen. The binding was greatly diminished when microsomes were heat denatured. The binding process was partially inhibited by carbon monoxide and SKF 525-A. When microsomes from phenobarbital- and 3-methylcholanthrene-treated rats were employed, binding was enhanced by 8- and 4-fold, respectively. The binding process was effectively diminished by the presence of reduced glutathione or cysteine in the incubation mixture and was not affected by lysine. Styrene oxide greatly enhanced binding. UDP-glucuronic acid, superoxide dismutase, and ascorbic acid also diminished the binding to some degree. It was concluded that toluene undergoes a hepatic microsomal monooxygenase-mediated activation, and the resultant reactive metabolites binds covalently to microsomal proteins.

摘要

将14C-甲苯与大鼠肝微粒体在NADPH生成系统存在的情况下进行温育,代谢产物浓缩于环己基柱上。通过反相高效液相色谱法分离代谢产物,并通过与标准品比较保留时间来进行鉴定。14C-甲苯被转化为14C-苄醇、14C-甲酚以及一种未鉴定的14C-代谢产物。发现部分放射性与微粒体大分子共价结合,优先与蛋白质结合。这种结合与温育时间和微粒体蛋白浓度成正比,且需要NADPH和分子氧。当微粒体热变性时,结合显著减少。结合过程被一氧化碳和SKF 525-A部分抑制。当使用苯巴比妥和3-甲基胆蒽处理过的大鼠的微粒体时,结合分别增强了8倍和4倍。温育混合物中存在还原型谷胱甘肽或半胱氨酸时,结合过程有效减弱,且不受赖氨酸影响。环氧苯乙烷极大地增强了结合。尿苷二磷酸葡萄糖醛酸、超氧化物歧化酶和抗坏血酸也在一定程度上减弱了结合。得出的结论是,甲苯经历肝微粒体单加氧酶介导的活化,产生的活性代谢产物与微粒体蛋白共价结合。

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