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大肠杆菌RNA聚合酶α亚基内的功能特化

Functional specialization within the alpha-subunit of Escherichia coli RNA polymerase.

作者信息

Hayward R S, Igarashi K, Ishihama A

机构信息

Department of Molecular Genetics, National Institute of Genetics, Shizuoka, Japan.

出版信息

J Mol Biol. 1991 Sep 5;221(1):23-9. doi: 10.1016/0022-2836(91)80197-3.

Abstract

The RNA polymerase core enzyme of Escherichia coli has the subunit composition alpha 2 beta beta', and when combined with one of several alternative sigma-subunits (initiation-specificity) produces holoenzyme capable of all the steps of transcription. Dimerization of the alpha-subunit and association with the beta-subunit trigger assembly of the core enzyme. Analyses of a set of deletion derivatives of rpoA (which encodes alpha) have indicated that as many as 94 carboxy-terminal amino acids (but not 153) can be removed without preventing assembly of core-like complexes in vitro. Detailed analyses of these deletion mutants have now been performed in vivo. alpha-Polypeptides truncated from the carboxy terminus to amino acid residues 235, 256 or 296 are assembled not merely into core, but also into holoenzyme-like complexes in vivo, and at least in the first two cases both of the two alpha-subunits can be replaced by the truncated versions. Nevertheless, none can complement rpoAts alleles for growth at 42 degrees C. We conclude that the domain(s) of alpha essential for the assembly of RNA polymerase (at least the major holoenzyme species) are confined to the amino-terminal 235 amino acids, while some other essential function(s) require residues close to the carboxy terminus.

摘要

大肠杆菌的RNA聚合酶核心酶具有α₂ββ'亚基组成,当与几种替代的σ亚基之一(起始特异性)结合时,会产生能够进行转录所有步骤的全酶。α亚基的二聚化以及与β亚基的结合触发了核心酶的组装。对一组rpoA(编码α)缺失衍生物的分析表明,在不阻止体外组装类核心复合物的情况下,可以去除多达94个羧基末端氨基酸(但不是153个)。现在已经在体内对这些缺失突变体进行了详细分析。从羧基末端截短至氨基酸残基235、256或296的α多肽不仅在体内组装成核心,还组装成类全酶复合物,并且至少在前两种情况下,两个α亚基都可以被截短版本替代。然而,没有一个能够在42℃下补充rpoAts等位基因以实现生长。我们得出结论,RNA聚合酶组装(至少主要的全酶种类)所必需的α结构域局限于氨基末端的235个氨基酸,而一些其他必需功能需要靠近羧基末端的残基。

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