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抑制ColE1质粒复制缺陷突变的大肠杆菌突变体。

Escherichia coli mutants suppressing replication-defective mutations of the ColE1 plasmid.

作者信息

Naito S, Kitani T, Ogawa T, Okazaki T, Uchida H

出版信息

Proc Natl Acad Sci U S A. 1984 Jan;81(2):550-4. doi: 10.1073/pnas.81.2.550.

Abstract

Mutants of Escherichia coli K-12 have been isolated that suppress cer mutants, ColE1 mutants that are unable to replicate as the plasmid. These host suppressors were designated her, for host factor affecting ColE1 replication. Each her suppressor showed a characteristic pattern of suppression depending on the cer mutation used for selecting the mutant bacteria. One of the suppressors, named herA, that suppressed cer6, a single-base-pair alteration 160 base pairs upstream of the ColE1 replication origin, was genetically identified as an alteration of the rnh gene (RNase H). HerA was recessive to its wild-type allele. RNase H activity of herA cell extracts was defective. Conversely, rnh mutants that were isolated independently of ColE1 replication supported replication of cer6 DNA. Some rnh mutants manifested the HerA phenotype only above a certain transition temperature, and their RNase H activity was found to be temperature sensitive. Therefore, replication of cer6 DNA in vivo is sensitive to RNase H activity. Under the conditions that suppressed cer6, the wild-type colE1 replicon replicated normally. Then, ColE1 replication in vivo proceeds in the absence of RNase H activity, which has been shown to be required for in vitro replication of the DNA.

摘要

已分离出大肠杆菌K-12的突变体,这些突变体能抑制cer突变体,即无法作为质粒复制的ColE1突变体。这些宿主抑制子被命名为her,代表影响ColE1复制的宿主因子。每个her抑制子根据用于筛选突变细菌的cer突变表现出特定的抑制模式。其中一个名为herA的抑制子能抑制cer6,cer6是ColE1复制起点上游160个碱基对处的单碱基对改变,经基因鉴定,herA是rnh基因(核糖核酸酶H)的一种改变。herA对其野生型等位基因呈隐性。herA细胞提取物的核糖核酸酶H活性有缺陷。相反,独立于ColE1复制分离得到的rnh突变体支持cer6 DNA的复制。一些rnh突变体仅在特定的转变温度以上表现出HerA表型,并且发现它们的核糖核酸酶H活性对温度敏感。因此,cer6 DNA在体内的复制对核糖核酸酶H活性敏感。在抑制cer6的条件下,野生型colE1复制子正常复制。那么,ColE1在体内的复制在没有核糖核酸酶H活性的情况下进行,而核糖核酸酶H活性已被证明是DNA体外复制所必需的。

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