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哈维氏弧菌中半胱氨酸289参与NADP(+)特异性脂肪醛脱氢酶的催化活性

Involvement of cysteine 289 in the catalytic activity of an NADP(+)-specific fatty aldehyde dehydrogenase from Vibrio harveyi.

作者信息

Vedadi M, Szittner R, Smillie L, Meighen E

机构信息

Department of Biochemistry, McGill University, Montreal, Canada.

出版信息

Biochemistry. 1995 Dec 26;34(51):16725-32. doi: 10.1021/bi00051a022.

Abstract

Fatty aldehyde dehydrogenase (Vh.ALDH) from the luminescent bacterium, Vibrio harveyi, may be implicated in controlling luminescence as it catalyzes the oxidation of the fatty aldehyde substrate for the light-emitting reaction. On the basis of the amino-terminal sequence of Vh.ALDH, a degenerate probe was used to screen a genomic library of V harveyi in pBR322, a positive clone was selected containing the Vh.ALDH gene and expressed in Escherichia coli, and the enzyme was purified to homogeneity. Although the sequence of the V. harveyi ALDH significantly diverged from other aldehyde dehydrogenases, mutation of a conserved cysteine implicated in catalysis completely inactivated the enzyme without loss of its ability to bind nucleotides, consistent with a catalytic role for this residue. Using absorption and fluorescence assays for NAD(P)H, it was shown that NAD+ and NADP+ bound to the same site and that saturation of Vh.ALDH with NADP+ occurred with a Michaelis constant (Km = 1.4 microM) over 40 times lower than that reported for other aldehyde dehydrogenases. Although V. harveyi aldehyde dehydrogenase is unique in terms of its high specificity for NADP+, the identification of a catalytic conserved cysteine in Vh.ALDH clearly indicates that a highly related mechanism and structure have been retained among even the most diverged aldehyde dehydrogenases.

摘要

来自发光细菌哈维弧菌的脂肪醛脱氢酶(Vh.ALDH)可能参与控制发光,因为它催化发光反应中脂肪醛底物的氧化。根据Vh.ALDH的氨基末端序列,使用简并探针筛选pBR322载体中的哈维弧菌基因组文库,选择了一个含有Vh.ALDH基因的阳性克隆并在大肠杆菌中表达,然后将该酶纯化至同质。尽管哈维弧菌ALDH的序列与其他醛脱氢酶有显著差异,但参与催化的保守半胱氨酸发生突变会使该酶完全失活,而不影响其结合核苷酸的能力,这与该残基的催化作用一致。通过对NAD(P)H进行吸收和荧光测定,结果表明NAD+和NADP+结合到同一位点,并且Vh.ALDH被NADP+饱和时的米氏常数(Km = 1.4 microM)比其他醛脱氢酶报道的值低40多倍。尽管哈维弧菌醛脱氢酶对NADP+具有高度特异性,但在Vh.ALDH中鉴定出催化保守半胱氨酸清楚地表明,即使是差异最大的醛脱氢酶之间也保留了高度相关的机制和结构。

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