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大鼠肝脏微粒体中存在的酶活性将类视黄醇醚转化为醇。

Conversion of retinoid ethers to alcohols by enzymatic activity present in rat liver microsomes.

作者信息

Shih T W, Shealy Y F, Hill D L

机构信息

Southern Research Institute, Birmingham, AL 35255-5305.

出版信息

Drug Metab Dispos. 1991 Mar-Apr;19(2):336-9.

PMID:1676633
Abstract

An enzyme present in rat liver microsomes catalyzes the conversion of retinyl methyl ether (RME) to retinol; NADPH is required for activity. The optimum pH for the reaction is 7.4; the KM and Vmax values are 120 microM RME and 14.3 nmol of retinol/mg protein/hr, respectively. As a substrate, the 2,3,6-trimethyl-4-methoxyphenyl analog of RME is as effective as RME. There is, however, no measurable activity for dealkylation of retinyl ethyl ether or retinyl butyl ether. Hepatic enzyme activity for the metabolism of RME is induced by 3-methylcholanthrene but not by phenobarbital or RME itself. The induced activity also requires NADPH as a cofactor. The optimum pH for the induced enzyme is 8.4; the KM and Vmax values are 50 microM RME and 111 nmol of retinol/mg protein/hr, respectively. For this enzyme, RME is a better substrate than the 2,3,6-trimethyl-4-methoxyphenyl analog of RME; retinyl ethyl ether is less effective; and again, there is no measurable activity with retinyl butyl ether as a substrate. Neither constitutive nor induced activity is detectable in microsomes from lung, spleen, stomach, kidney, small intestine, or large intestine. The enzyme activity that cleaves retinoid ethers appears to be similar to other microsomal NADPH-requiring O-dealkylases and different from a reported tetrahydropteridine-requiring dealkylase.

摘要

大鼠肝脏微粒体中存在的一种酶催化视黄基甲基醚(RME)转化为视黄醇;该活性需要NADPH。反应的最佳pH值为7.4;KM和Vmax值分别为120μM RME和14.3 nmol视黄醇/毫克蛋白/小时。作为底物,RME的2,3,6-三甲基-4-甲氧基苯基类似物与RME一样有效。然而,视黄基乙醚或视黄基丁醚的脱烷基化没有可测量的活性。RME代谢的肝脏酶活性由3-甲基胆蒽诱导,但不由苯巴比妥或RME本身诱导。诱导活性也需要NADPH作为辅因子。诱导酶的最佳pH值为8.4;KM和Vmax值分别为50μM RME和111 nmol视黄醇/毫克蛋白/小时。对于这种酶,RME是比RME的2,3,6-三甲基-4-甲氧基苯基类似物更好的底物;视黄基乙醚效果较差;同样,以视黄基丁醚为底物时没有可测量的活性。在肺、脾、胃、肾、小肠或大肠的微粒体中均未检测到组成型或诱导型活性。裂解类视黄醇醚的酶活性似乎与其他需要微粒体NADPH的O-脱烷基酶相似,并且与报道的需要四氢蝶啶的脱烷基酶不同。

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