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能够检测大肠杆菌某些DNA复制和膜突变体的信号菌株:新的单链结合蛋白等位基因ssb - 3的分离

Signal strains that can detect certain DNA replication and membrane mutants of Escherichia coli: isolation of a new ssb allele, ssb-3.

作者信息

Schmellik-Sandage C S, Tessman E S

机构信息

Department of Biological Sciences, Purdue University, West Lafayette, Indiana 47907.

出版信息

J Bacteriol. 1990 Aug;172(8):4378-85. doi: 10.1128/jb.172.8.4378-4385.1990.

Abstract

Mutations in several dna genes of Escherichia coli, when introduced into a strain with a lac fusion in the SOS gene sulA, resulted in formation of blue colonies on plates containing 5-bromo-4-chloro-3-indolyl-beta-D-galactoside (X-Gal). Unexpectedly, several lines of evidence indicated that the blue colony color was not primarily due to induction of the SOS system but rather was due to a membrane defect, along with the replication defect, making the cell X-Gal extrasensitive (phenotypically Xgx), possibly because of enhanced permeability to X-Gal or leakage of beta-galactosidase. (i) In most cases, beta-galactosidase specific activity increased only two- to threefold. (ii) Mutations conferring tolerance to colicin E1 resulted in blue colony color with no increase in beta-galactosidase specific activity. (iii) Mutations in either the dnaA, dnaB, dnaC, dnaE, dnaG, or ssb gene, when introduced into a strain containing a bioA::lac fusion, produced a blue colony color without an increase in beta-galactosidase synthesis. These lac fusion strains can serve as signal strains to detect dna mutations as well as membrane mutations. By localized mutagenesis of the 92-min region of the chromosome of the sulA::lac signal strain and picking blue colonies, we isolated a novel ssb allele that confers the same extreme UV sensitivity as a delta recA allele, which is a considerably greater sensitivity than that conferred by the two well-studied ssb alleles, ssb-1 and ssb-113. The technique also yielded dnaB mutants; fortuitously, uvrA mutants were also found.

摘要

将大肠杆菌几个dna基因的突变引入到在SOS基因sulA中带有lac融合的菌株后,在含有5-溴-4-氯-3-吲哚基-β-D-半乳糖苷(X-Gal)的平板上会形成蓝色菌落。出乎意料的是,几条证据表明蓝色菌落颜色并非主要由于SOS系统的诱导,而是由于膜缺陷以及复制缺陷,使得细胞对X-Gal格外敏感(表型为Xgx),这可能是因为对X-Gal的通透性增强或β-半乳糖苷酶泄漏。(i)在大多数情况下,β-半乳糖苷酶的比活性仅增加两到三倍。(ii)赋予对大肠杆菌素E1耐受性的突变导致蓝色菌落颜色,但β-半乳糖苷酶比活性没有增加。(iii)将dnaA、dnaB、dnaC、dnaE、dnaG或ssb基因的突变引入到含有bioA::lac融合的菌株中,会产生蓝色菌落颜色,而β-半乳糖苷酶合成没有增加。这些lac融合菌株可作为信号菌株来检测dna突变以及膜突变。通过对sulA::lac信号菌株染色体92分钟区域进行定位诱变并挑选蓝色菌落,我们分离出了一个新的ssb等位基因,它赋予的极端紫外线敏感性与δrecA等位基因相同,这比两个经过充分研究的ssb等位基因ssb-1和ssb-113赋予的敏感性要高得多。该技术还产生了dnaB突变体;幸运的是,还发现了uvrA突变体。

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