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饥饿条件下大肠杆菌中的突变:一条导致错配修复缺陷菌株出现小缺失的新途径。

Mutation in Escherichia coli under starvation conditions: a new pathway leading to small deletions in strains defective in mismatch correction.

作者信息

Bridges B A, Timms A R

机构信息

Medical Research Council Cell Mutation Unit, University of Sussex, Falmer, Brighton, UK.

出版信息

EMBO J. 1997 Jun 2;16(11):3349-56. doi: 10.1093/emboj/16.11.3349.

DOI:10.1093/emboj/16.11.3349
PMID:9214650
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1169951/
Abstract

Strains of Escherichia coli carrying the mutY mutation lack a mismatch correction glycosylase that removes adenines from various mismatch situations. In growing bacteria, 8-oxoguanine-adenine mispairs persist and can give rise to G-->T transversions during subsequent replication cycles. We now show that when trpA23 mutY bacteria are held under tryptophan starvation conditions the tryptophan-independent mutants that arise include small in-frame deletions in addition to transversions. The trpA23 reversion system appears to be unusual in that small in-frame deletions occurring in a particular region of the gene can lead to the production of a functional protein. We suggest that this is a consequence of the deletion causing the polar group on the arginine at the trpA23 site to be pulled away from the active site of the enzyme. Such deletions are also found with starved bacteria defective in methyl-directed mismatch correction activity (mutH, mutL or mutS), and deletion mutations are also found among the much lower number of mutants that arise in bacteria wild-type for mismatch correction. There is thus a pathway, hitherto undetected, leading to deletions probably from mismatches under conditions of growth restraint. RecA, UmuC, UvrA, MutH,L,S, SbcC and SbcD proteins are not required for the operation of the deletion pathway. A possible explanation is that the deletion pathway is not dependent upon further replication and that it fails to be discernible in growing cells because it is relatively slow acting and mismatches are likely to encounter a DNA replication fork before the initial step of the deletion pathway.

摘要

携带mutY突变的大肠杆菌菌株缺乏一种错配校正糖基化酶,该酶可从各种错配情况中去除腺嘌呤。在生长的细菌中,8-氧代鸟嘌呤-腺嘌呤错配持续存在,并可能在随后的复制周期中导致G→T颠换。我们现在表明,当trpA23 mutY细菌处于色氨酸饥饿条件下时,出现的色氨酸非依赖性突变体除了颠换外还包括小的框内缺失。trpA23回复系统似乎很不寻常,因为在基因的特定区域发生的小框内缺失可导致产生功能性蛋白质。我们认为这是缺失导致trpA23位点精氨酸上的极性基团从酶的活性位点被拉开的结果。在甲基导向错配校正活性有缺陷的饥饿细菌(mutH、mutL或mutS)中也发现了这种缺失,在错配校正野生型细菌中出现的数量少得多的突变体中也发现了缺失突变。因此,存在一条迄今未被检测到的途径,可能在生长受限的条件下从不匹配导致缺失。RecA、UmuC、UvrA、MutH、L、S、SbcC和SbcD蛋白对于缺失途径的运行不是必需的。一种可能的解释是,缺失途径不依赖于进一步的复制,并且在生长细胞中无法识别,因为它作用相对较慢,错配可能在缺失途径的初始步骤之前遇到DNA复制叉。

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