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The positioning of Chi sites allows the RecBCD pathway to suppress some genomic rearrangements

机译:CHI位点的定位允许RECBCD途径抑制一些基因组重排

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Bacterial recombinational repair of double-strand breaks often begins with creation of initiating 3 single-stranded DNA (ssDNA) tails on each side of a double-strand break (DSB). Importantly, if the RecBCD pathway is followed, RecBCD creates a gap between the sequences at 3 ends of the initiating strands. The gap flanks the DSB and extends at least to the nearest Chi site on each strand. Once the initiating strands form ssDNA-RecA filaments, each ssDNA-RecA filament searches for homologous double-stranded DNA (dsDNA) to use as a template for the DNA synthesis needed to fill the gap created by RecBCD. Our experimental results show that the DNA synthesis requires formation of a heteroduplex dsDNA that pairs >20 contiguous bases in the initiating strand with sequence matched bases in a strand from the original dsDNA. To trigger synthesis, the heteroduplex must be near the 3 end of the initiating strand. Those experimentally determined requirements for synthesis combined with the Chi site dependence of the function of RecBCD and the distribution of Chi sites in bacterial genomes could allow the RecBCD pathway to avoid some genomic rearrangements arising from directly induced DSBs; however, the same three factors could promote other rearrangements.
机译:双链断裂的细菌重组修复通常始于在双链断裂(DSB)的每一侧上启动3个单链DNA(SSDNA)尾部的创造。重要的是,如果遵循RecBCD途径,则RecBCD在引发股的3末端产生序列之间的间隙。间隙侧翼DSB并至少延伸到每条股线上的最近的CHI位点。一旦发起链形成SSDNA-RECA长丝,每个SSDNA-RECA灯丝搜索同源的双链DNA(DSDNA)用作填充RecBCD产生的间隙所需的DNA合成的模板。我们的实验结果表明,DNA合成需要形成在从原始DSDNA的股线中的序列匹配碱中对> 20邻接碱的异络DSDNA。为了触发合成,异水上复合必须靠近启动股的3末端。这些实验确定的合成要求与CHI位点依赖性的RECBCD功能和细菌基因组中的CHI位点的分布可以允许RECBCD途径避免直接诱导的DSB产生的一些基因组重排;但是,相同的三个因素可以促进其他重排。

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