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猪肾醛还原酶的动力学及作用机制

Kinetics and mechanism of action of aldehyde reductase from pig kidney.

作者信息

Davidson W S, Flynn T G

出版信息

Biochem J. 1979 Feb 1;177(2):595-601. doi: 10.1042/bj1770595.

Abstract

An improved procedure for purifying aldehyde reductase is described. Utilization of Blue Dextran--Sepharose 4B and elimination of hydroxyapatite chromatography greatly improves the yield and ease of purification. Starting with 340 g of kidney tissue (two pig kidneys) approx. 50 mg of purified reductase may be routinely and reproducibly obtained. The purified reductase was used to establish the kinetic reaction mechanism of the enzyme. Initial-velocity analysis and product-inhibition data revealed that pig kidney aldehyde reductase follows an Ordered Bi Bi reaction mechanism in which NADPH binds first before D-glyceraldehyde. The limiting Michaelis constants for D-glyceraldehyde and NADPH were 4.8 +/- 0.7 mM and 9.1 +/- 2.1 micrometer respectively. The mechanism is similar to that of another monomeric oxidoreductase, octopine dehydrogenase, towards which aldehyde reductase exhibits several similarities, but differs from that of other aldehyde reductases. Phenobarbital is a potent inhibitor of aldehyde reductase, inhibiting both substrate and cofactor non-competitively (Ki = 80.4 +/- 10.5 micrometer and 66.9 +/- 1.6 micrometer respectively). Barbiturate inhibition seems to be a common property of NADPH-dependent aldehyde reductases.

摘要

本文描述了一种改进的醛还原酶纯化方法。使用蓝色葡聚糖-琼脂糖4B并省去羟基磷灰石层析,可大大提高产量并简化纯化过程。以340克肾组织(两个猪肾)为起始材料,通常可重复获得约50毫克纯化的还原酶。纯化的还原酶用于确定该酶的动力学反应机制。初速度分析和产物抑制数据表明,猪肾醛还原酶遵循有序双双反应机制,其中NADPH在D-甘油醛之前首先结合。D-甘油醛和NADPH的极限米氏常数分别为4.8±0.7毫摩尔和9.1±2.1微摩尔。该机制与另一种单体氧化还原酶章鱼碱脱氢酶的机制相似,醛还原酶与章鱼碱脱氢酶有几个相似之处,但与其他醛还原酶的机制不同。苯巴比妥是醛还原酶的有效抑制剂,对底物和辅因子均有非竞争性抑制作用(Ki分别为80.4±10.5微摩尔和66.9±1.6微摩尔)。巴比妥类药物的抑制作用似乎是NADPH依赖性醛还原酶的共同特性。

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