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沙门氏菌中有无重组(RecA)的多种重复形成途径。

Multiple pathways of duplication formation with and without recombination (RecA) in Salmonella enterica.

机构信息

Department of Microbiology, University of California, Davis, CA 95616, USA.

出版信息

Genetics. 2012 Oct;192(2):397-415. doi: 10.1534/genetics.112.142570. Epub 2012 Aug 3.

Abstract

Duplications are often attributed to "unequal recombination" between separated, directly repeated sequence elements (>100 bp), events that leave a recombinant element at the duplication junction. However, in the bacterial chromosome, duplications form at high rates (10(-3)-10(-5)/cell/division) even without recombination (RecA). Here we describe 1800 spontaneous lac duplications trapped nonselectively on the low-copy F'(128) plasmid, where lac is flanked by direct repeats of the transposable element IS3 (1258 bp) and by numerous quasipalindromic REP elements (30 bp). Duplications form at a high rate (10(-4)/cell/division) that is reduced only about 11-fold in the absence of RecA. With and without RecA, most duplications arise by recombination between IS3 elements (97%). Formation of these duplications is stimulated by IS3 transposase (Tnp) and plasmid transfer functions (TraI). Three duplication pathways are proposed. First, plasmid dimers form at a high rate stimulated by RecA and are then modified by deletions between IS3 elements (resolution) that leave a monomeric plasmid with an IS3-flanked lac duplication. Second, without RecA, duplications occur by single-strand annealing of DNA ends generated in different sister chromosomes after transposase nicks DNA near participating IS3 elements. The absence of RecA may stimulate annealing by allowing chromosome breaks to persist. Third, a minority of lac duplications (3%) have short (0-36 bp) junction sequences (SJ), some of which are located within REP elements. These duplication types form without RecA, Tnp, or Tra by a pathway in which the palindromic junctions of a tandem inversion duplication (TID) may stimulate deletions that leave the final duplication.

摘要

重复序列通常归因于分离的、直接重复的序列元件(>100bp)之间的“不等交换重组”,这些事件会在重复连接处留下一个重组元件。然而,在细菌染色体中,即使没有重组(RecA),重复序列也会以很高的速率形成(10(-3)-10(-5)/细胞/分裂)。在这里,我们描述了 1800 个自发的 lac 重复序列,它们非选择性地被捕获在低拷贝数的 F'(128)质粒上,lac 两侧是可移动元件 IS3(1258bp)的直接重复序列和许多准回文的 REP 元件(30bp)。在没有 RecA 的情况下,重复序列的形成速率很高(10(-4)/细胞/分裂),但只有大约 11 倍的降低。有和没有 RecA 的情况下,大多数重复序列都是由 IS3 元件之间的重组产生的(97%)。这些重复序列的形成受到 IS3 转座酶(Tnp)和质粒转移功能(TraI)的刺激。提出了三种重复途径。首先,RecA 高刺激下形成质粒二聚体,然后通过 IS3 元件之间的缺失(分辨率)进行修饰,留下一个带有侧翼 lac 重复序列的单体质粒。其次,在没有 RecA 的情况下,在转座酶在参与的 IS3 元件附近切开 DNA 后,不同姐妹染色体上的 DNA 末端通过单链退火发生复制。缺乏 RecA 可能通过允许染色体断裂持续存在来刺激退火。第三,少数 lac 重复序列(3%)具有短(0-36bp)的连接序列(SJ),其中一些位于 REP 元件内。这些重复类型在没有 RecA、Tnp 或 Tra 的情况下形成,通过串联倒位重复(TID)的回文连接可能刺激导致最终重复的缺失。

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