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Transcription-associated recombination is independent of XRCC2 and mechanistically separate from homology-directed DNA double-strand break repair

机译:转录相关的重组独立于XRCC2并从同源性指导的DNA双链断裂修复机制上分离

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摘要

It has previously been shown that transcription greatly enhances recombination in mammalian cells. However, the proteins involved in catalysing this process and the recombination pathways involved in transcription-associated recombination (TAR) are still unknown. It is well established that both the BRCA2 protein and the RAD51 paralog protein XRCC2 are required for homologous recombination. Here, we show that the BRCA2 protein is also required for TAR, while the XRCC2 protein is not involved. Expression of the XRCC2 gene in XRCC2 mutated irs1 cells restores the defect in homologous recombination repair of an I-SceI-induced DNA double-strand break, while TAR is unaffected. Interestingly, the XRCC2-deficient irs1 cells are also proficient in recombination induced at slowed replication forks, suggesting that TAR is mechanistically linked with this recombination pathway. In conclusion, we show that TAR depends on BRCA2 but is independent of XRCC2, and that this recombination pathway is separate from that used to repair a two-ended DNA double-strand break.
机译:先前已经表明,转录极大地增强了哺乳动物细胞中的重组。但是,催化该过程中涉及的蛋白质和转录相关重组(TAR)中涉及的重组途径仍是未知的。众所周知,同源重组需要BRCA2蛋白和RAD51旁系同源蛋白XRCC2。在这里,我们显示BRCA2蛋白也是TAR所必需的,而XRCC2蛋白则不涉及。 XRCC2突变的irs1细胞中XRCC2基因的表达恢复了I-SceI诱导的DNA双链断裂的同源重组修复中的缺陷,而TAR不受影响。有趣的是,缺乏XRCC2的irs1细胞也擅长在缓慢的复制叉诱导的重组,这表明TAR与该重组途径机械相连。总之,我们表明TAR依赖于BRCA2但独立于XRCC2,并且该重组途径与用于修复两端DNA双链断裂的途径是分开的。

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