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大肠杆菌延胡索酸还原酶基因的克隆与表达

Cloning and expression of fumarate reductase gene of Escherichia coli.

作者信息

Lohmeier E, Hagen D S, Dickie P, Weiner J H

出版信息

Can J Biochem. 1981 Mar;59(3):158-64. doi: 10.1139/o81-023.

Abstract

Mutants of Escherichia coli deficient in fumarate reductase activity and therefore unable to grow anaerobically with fumarate as an electron acceptor have been isolated. By F+-mediated conjugation and complementation with the mutant host, two E. coli: Col E1 recombinant DNA plasmids have been identified from the Clarke and Carbon Colony Bank which carry the structural genes for fumarate reductase. Bacteria harboring either of these plasmids express about ten times the normal level of fumarate reductase. Enzyme purified from the two sources, plasmid-carrying and plasmidless E. coli, have identical physical and kinetic properties indicating that both the 69 000 and 25 000 dalton polypeptides are amplified. Regulation of plasmid-encoded enzyme, like the chromosomally encoded enzyme, is dependent upon the presence of fumarate and anaerobiosis.

摘要

已分离出缺乏延胡索酸还原酶活性、因此无法以延胡索酸作为电子受体进行厌氧生长的大肠杆菌突变体。通过F⁺介导的接合以及与突变宿主的互补,从克拉克和卡尔文菌落库中鉴定出了两种大肠杆菌:Col E1重组DNA质粒,它们携带延胡索酸还原酶的结构基因。携带这两种质粒之一的细菌表达的延胡索酸还原酶水平约为正常水平的十倍。从携带质粒的大肠杆菌和无质粒的大肠杆菌这两种来源纯化的酶具有相同的物理和动力学性质,表明69000道尔顿和25000道尔顿的多肽均被扩增。质粒编码酶的调节与染色体编码酶一样,取决于延胡索酸的存在和厌氧状态。

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