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Exo1 processes stalled replication forks and counteracts fork reversal in checkpoint-defective cells

机译:Exo1处理停滞的复制叉并抵消检查点缺陷单元中的叉反转

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摘要

The replication checkpoint coordinates the cell cycle with DNA replication and recombination, preventing genome instability and cancer. The budding yeast Rad53 checkpoint kinase stabilizes stalled forks and replisome-fork complexes, thus preventing the accumulation of ss-DNA regions and reversed forks at collapsed forks. We searched for factors involved in the processing of stalled forks in HU-treated rad53 cells. Using the neutral-neutral two-dimensional electrophoresis technique (2D gel) and psoralen crosslinking combined with electron microscopy (EM), we found that the Exo1 exonuclease is recruited to stalled forks and, in rad53 mutants, counteracts reversed fork accumulation by generating ss-DNA intermediates. Hence, Exo1-mediated fork processing resembles the action of E. coli RecJ nuclease at damaged forks. Fork stability and replication restart are influenced by both DNA polymerase-fork association and Exo1-mediated processing. We suggest that Exo1 counteracts fork reversal by resecting newly synthesized chains and resolving the sister chromatid junctions that cause regression of collapsed forks.
机译:复制检查点通过DNA复制和重组来协调细胞周期,从而防止基因组不稳定和癌症。出芽的酵母Rad53检查点激酶可稳定失速的叉子和复制体-叉子复合物,从而防止ss-DNA区域的积累和叉子倒塌时叉子的反向。我们搜索了HU处理过的rad53细胞中停滞叉子加工的相关因素。使用中性-中性二维电泳技术(2D凝胶)和补骨脂素交联结合电子显微镜(EM),我们发现Exo1核酸外切酶被募集到停滞的叉子中,在rad53突变体中,通过产生ss-来抵消反向的叉子积累。 DNA中间体。因此,Exo1介导的叉子加工过程类似于大肠杆菌RecJ核酸酶对受损叉子的作用。叉的稳定性和复制的重启受到DNA聚合酶叉关联和Exo1介导的处理的影响。我们建议,Exo1通过切除新合成的链并解决导致折叠前叉回归的姐妹染色单体连接来抵消前叉逆转。

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