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大肠杆菌中氢化酶基因的克隆及H2代谢必需操纵子的精细结构分析。

Cloning of hydrogenase genes and fine structure analysis of an operon essential for H2 metabolism in Escherichia coli.

作者信息

Sankar P, Lee J H, Shanmugam K T

出版信息

J Bacteriol. 1985 Apr;162(1):353-60. doi: 10.1128/jb.162.1.353-360.1985.

DOI:10.1128/jb.162.1.353-360.1985
PMID:3884595
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC218996/
Abstract

Escherichia coli has two unlinked genes that code for hydrogenase synthesis and activity. The DNA fragments containing the two genes (hydA and hydB) were cloned into a plasmid vector, pBR322. The plasmids containing the hyd genes (pSE-290 and pSE-111 carrying the hydA and hydB genes, respectively) were used to genetically map a total of 51 mutant strains with defects in hydrogenase activity. A total of 37 mutants carried a mutation in the hydB gene, whereas the remaining 14 hyd were hydA. This complementation analysis also established the presence of two new genes, so far unidentified, one coding for formate dehydrogenase-2 (fdv) and another producing an electron transport protein (fhl) coupling formate dehydrogenase-2 to hydrogenase. Three of the four genes, hydB, fhl, and fdv, may constitute a single operon, and all three genes are carried by a 5.6-kilobase-pair chromosomal DNA insert in plasmid pSE-128. Plasmids carrying a part of this 5.6-kilobase-pair DNA (pSE-130) or fragments derived from this DNA in different orientations (pSE-126 and pSE-129) inhibited the production of active formate hydrogenlyase. This inhibition occurred even in a prototrophic E. coli, strain K-10, but only during an early induction period. These results, based on complementation analysis with cloned DNA fragments, show that both hydA and hydB genes are essential for the production of active hydrogenase. For the expression of active formate hydrogenlyase, two other gene products, fhl and fdv are also needed. All four genes map between 58 and 59 min in the E. coli chromosome.

摘要

大肠杆菌有两个不连锁的基因,负责氢化酶的合成与活性。包含这两个基因(hydA和hydB)的DNA片段被克隆到质粒载体pBR322中。含有hyd基因的质粒(分别携带hydA和hydB基因的pSE - 290和pSE - 111)被用于对总共51个氢化酶活性有缺陷的突变菌株进行遗传定位。总共有37个突变体在hydB基因中发生了突变,而其余14个hyd突变体则是hydA突变。这种互补分析还确定了两个尚未鉴定的新基因,一个编码甲酸脱氢酶 - 2(fdv),另一个产生将甲酸脱氢酶 - 2与氢化酶偶联的电子传递蛋白(fhl)。四个基因中的三个,hydB、fhl和fdv,可能构成一个单一的操纵子,并且所有这三个基因都由质粒pSE - 128中一个5.6千碱基对的染色体DNA插入片段携带。携带这个5.6千碱基对DNA一部分的质粒(pSE - 130)或从该DNA以不同方向衍生的片段(pSE - 126和pSE - 129)抑制了活性甲酸氢化酶的产生。这种抑制甚至在原养型大肠杆菌K - 10菌株中也会发生,但仅在早期诱导期。基于用克隆的DNA片段进行的互补分析,这些结果表明hydA和hydB基因对于活性氢化酶的产生都是必不可少的。对于活性甲酸氢化酶的表达,还需要另外两个基因产物fhl和fdv。所有四个基因都位于大肠杆菌染色体上58至59分钟之间。

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Cloning of hydrogenase genes and fine structure analysis of an operon essential for H2 metabolism in Escherichia coli.大肠杆菌中氢化酶基因的克隆及H2代谢必需操纵子的精细结构分析。
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