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首页> 外文期刊>Nucleic Acids Research >Biochemical studies of the Saccharomyces cerevisiae Mph1 helicase on junction-containing DNA structures
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Biochemical studies of the Saccharomyces cerevisiae Mph1 helicase on junction-containing DNA structures

机译:酿酒酵母Mph1解旋酶对包含连接的DNA结构的生化研究

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Saccharomyces cerevisiae Mph1 is a 3-5' DNA helicase, required for the maintenance of genome integrity. In order to understand the ATPase/helicase role of Mph1 in genome stability, we characterized its helicase activity with a variety of DNA substrates, focusing on its action on junction structures containing three or four DNA strands. Consistent with its 3' to 5' directionality, Mph1 displaced 3'-flap substrates in double-fixed or equilibrating flap substrates. Surprisingly, Mph1 displaced the 5'-flap strand more efficiently than the 3' flap strand from double-flap substrates, which is not expected for a 3-5' DNA helicase. For this to occur, Mph1 required a threshold size (> 5 nt) of 5' single-stranded DNA flap. Based on the unique substrate requirements of Mph1 defined in this study, we propose that the helicase/ATPase activity of Mph1 play roles in converting multiple-stranded DNA structures into structures cleavable by processing enzymes such as Fen1. We also found that the helicase activity of Mph1 was used to cause structural alterations required for restoration of replication forks stalled due to damaged template. The helicase properties of Mph1 reported here could explain how it resolves D-loop structure, and are in keeping with a model proposed for the error-free damage avoidance pathway.
机译:酿酒酵母Mph1是3-5'DNA解旋酶,是维持基因组完整性所必需的。为了了解Mph1在基因组稳定性中的ATPase /解旋酶作用,我们用多种DNA底物表征了其解旋酶活性,重点是其对包含三或四条DNA链的连接结构的作用。与其3'至5'方向性一致,Mph1将3'-flap基底置换为双固定或平衡的瓣片基底。出人意料的是,Mph1比双瓣底物的3'瓣链更有效地置换了5'瓣链,这对于3-5'DNA解旋酶而言是无法预期的。为此,Mph1需要5'单链DNA皮瓣的阈值大小(> 5 nt)。基于本研究中定义的Mph1的独特底物要求,我们建议Mph1的解旋酶/ ATPase活性在将多链DNA结构转换为可通过加工酶(例如Fen1)切割的结构中发挥作用。我们还发现,Mph1的解旋酶活性被用于引起由于模板损坏而停滞的复制叉的修复所需的结构改变。此处报道的Mph1的解旋酶性质可以解释其如何解析D环结构,并且与为无错误破坏避免途径提出的模型保持一致。

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