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大肠杆菌中异常DNA复制导致的增强型缺失形成

Enhanced deletion formation by aberrant DNA replication in Escherichia coli.

作者信息

Saveson C J, Lovett S T

机构信息

Department of Biology, Brandeis University, Waltham, Massachusetts 02254-9110, USA.

出版信息

Genetics. 1997 Jun;146(2):457-70. doi: 10.1093/genetics/146.2.457.

Abstract

Repeated genes and sequences are prone to genetic rearrangements including deletions. We have investigated deletion formation in Escherichia coli strains mutant for various replication functions. Deletion was selected between 787 base pair tandem repeats carried either on a ColE1-derived plasmid or on the E. coli chromosome. Only mutations in functions associated with DNA Polymerase III elevated deletion rates in our assays. Especially large increases were observed in strains mutant in dnaQ the epsilon editing subunit of Pol III, and dnaB, the replication fork helicase. Mutations in several other functions also altered deletion formation: the alpha polymerase (dnal;), the gamma clamp loader complex (holC, dnaX), and the beta clamp (dnaN) subunits of Pol III and the primosomal proteins, dnaC and priA. Aberrant replication stimulated deletions through several pathways. Whereas the elevation in dnaB strains was mostly recA- and lexA-dependent, that in dnaQ strains was mostly recA- and lexA-independent. Deletion product analysis suggested that slipped mispairing, producing monomeric replicon products, may be preferentially increased in a dnaQ mutant and sister-strand exchange, producing dimeric replicon products, may be elevated in dnaE mutants. We conclude that aberrant Polymerase III replication can stimulate deletion events through several mechanisms of deletion and via both recA-dependent and independent pathways.

摘要

重复基因和序列易于发生包括缺失在内的基因重排。我们研究了大肠杆菌中各种复制功能突变菌株的缺失形成情况。在源自ColE1的质粒或大肠杆菌染色体上携带的787个碱基对的串联重复序列之间选择缺失。在我们的实验中,只有与DNA聚合酶III相关的功能突变会提高缺失率。在Pol III的ε编辑亚基dnaQ和复制叉解旋酶dnaB突变的菌株中观察到特别大的增加。其他几种功能的突变也改变了缺失形成:Pol III的α聚合酶(dnal;)、γ钳加载复合物(holC、dnaX)和β钳(dnaN)亚基以及引发体蛋白dnaC和priA。异常复制通过多种途径刺激缺失。虽然dnaB菌株中的增加大多依赖recA和lexA,但dnaQ菌株中的增加大多不依赖recA和lexA。缺失产物分析表明,产生单体复制子产物的滑动错配在dnaQ突变体中可能优先增加,而产生二聚体复制子产物的姐妹链交换在dnaE突变体中可能增加。我们得出结论,异常的聚合酶III复制可以通过几种缺失机制以及recA依赖和独立途径刺激缺失事件。

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