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Fen-1 Facilitates Homologous Recombination by Removing Divergent Sequences at DNA Break Ends

机译:Fen-1通过去除DNA断裂末端的不同序列来促进同源重组

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摘要

Homologous recombination (HR) requires nuclease activities at multiple steps, but the contribution of individual nucleases to the processing of double-strand DNA ends at different stages of HR has not been clearly defined. We used chicken DT40 cells to investigate the role of flap endonuclease 1 (Fen-1) in HR. FEN-1-deficient cells exhibited a significant decrease in the efficiency of immunoglobulin gene conversion while being proficient in recombination between sister chromatids, suggesting that Fen-1 may play a role in HR between sequences of considerable divergence. To clarify whether sequence divergence at DNA ends is truly the reason for the observed HR defect in FEN-1−/− cells we inserted a unique I-SceI restriction site in the genome and tested various donor and recipient HR substrates. We found that the efficiency of HR-mediated DNA repair was indeed greatly diminished when divergent sequences were present at the DNA break site. We conclude that Fen-1 eliminates heterologous sequences at DNA damage site and facilitates DNA repair by HR.
机译:同源重组(HR)需要在多个步骤中进行核酸酶活性,但是在HR的不同阶段,单个核酸酶对双链DNA末端加工的贡献尚未明确。我们使用鸡DT40细胞来研究皮瓣内切核酸酶1(Fen-1)在HR中的作用。缺乏FEN-1的细胞表现出免疫球蛋白基因转化效率的显着降低,同时精通姐妹染色单体之间的重组,这表明Fen-1可能在相当不同的序列之间的HR中发挥作用。为了弄清楚DNA末端的序列差异是否确实是FEN-1 -/-细胞中观察到的HR缺陷的原因,我们在基因组中插入了一个独特的I-SceI限制性酶切位点,并测试了各种供体和受体HR底材。我们发现,当DNA断裂位点处存在分歧序列时,HR介导的DNA修复的效率确实大大降低了。我们得出的结论是Fen-1消除了DNA损伤位点的异源序列,并促进了HR修复DNA。

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