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大肠杆菌mutT基因的抑制因子:DNA复制错误的抗突变因子

Suppressors of Escherichia coli mutT: antimutators for DNA replication errors.

作者信息

Schaaper R M

机构信息

Laboratory of Molecular Genetics, National Institute of Environmental Health Sciences, Research Triangle Park, NC 27709, USA.

出版信息

Mutat Res. 1996 Feb 19;350(1):17-23. doi: 10.1016/0027-5107(95)00086-0.

DOI:10.1016/0027-5107(95)00086-0
PMID:8657178
Abstract

Previous studies in our laboratory used a papillation assay to identify a set of mutations in the E. coli dnaE gene that confer increased accuracy of DNA replication (antimutators). These antimutators were isolated as suppressors of the hugh mutability of a mismatch-repair-defective mutL strain, in which the majority of mutations represent uncorrected replication errors (mainly A.T --> G.C and G.C --> A.T transitions). In the present study, we have sought suppressors of the high mutability of a mutT mutator strain. mutT strains produce a high frequency of A.T --> C.G transversions due to their lack of the mutT-encoded 8-oxo-dGTPase, leading to a high frequency of A.(8-oxoG) mispairing errors. Following localized mutagenesis of the dnaE-dnaQ region of the chromosome, two strong suppressors of mutT mutability were obtained, both residing in the dnaE gene (dnaE940 and dnaE941). When subsequently tested in a mutL strain, these two alleles also proved antimutators in this background, dnaE941 being significantly stronger than the previously isolated antimutators. The results suggest that the DNA polymerase may use similar mechanisms to discriminate against A.(8-oxoG) transversion mispairs and A.C or T.G transition mispairs. The finding may also have significance for teh interpretation of the antimutator effect conferred by these dnaE alleles in a wild-type (mut+) background.

摘要

我们实验室之前的研究使用了一种乳头化分析方法来鉴定大肠杆菌dnaE基因中的一组突变,这些突变可提高DNA复制的准确性(抗突变体)。这些抗突变体是作为错配修复缺陷型mutL菌株高突变性的抑制子分离出来的,在该菌株中,大多数突变代表未校正的复制错误(主要是A.T→G.C和G.C→A.T转换)。在本研究中,我们寻找了mutT突变体菌株高突变性的抑制子。mutT菌株由于缺乏mutT编码的8-氧代-dGTPase,产生高频的A.T→C.G颠换,导致高频的A.(8-氧代鸟嘌呤)错配错误。对染色体的dnaE-dnaQ区域进行局部诱变后,获得了两个mutT突变性的强抑制子,它们都位于dnaE基因中(dnaE940和dnaE941)。随后在mutL菌株中进行测试时,这两个等位基因在该背景下也被证明是抗突变体,dnaE941比之前分离的抗突变体明显更强。结果表明,DNA聚合酶可能使用类似的机制来区分A.(8-氧代鸟嘌呤)颠换错配和A.C或T.G转换错配。这一发现对于解释这些dnaE等位基因在野生型(mut+)背景下赋予的抗突变体效应也可能具有重要意义。

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