首页> 外文OA文献 >The Direct Binding of Mrc1, a Checkpoint Mediator, to Mcm6, a Replication Helicase, Is Essential for the Replication Checkpoint against Methyl Methanesulfonate-Induced Stress▿
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The Direct Binding of Mrc1, a Checkpoint Mediator, to Mcm6, a Replication Helicase, Is Essential for the Replication Checkpoint against Methyl Methanesulfonate-Induced Stress▿

机译:Mrc1(检查点介体)与Mcm6(复制解旋酶)的直接结合对于抵抗甲基磺酸甲酯诱导的应激的复制检查点至关重要。

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摘要

Mrc1 plays a role in mediating the DNA replication checkpoint. We surveyed replication elongation proteins that interact directly with Mrc1 and identified a replicative helicase, Mcm6, as a specific Mrc1-binding protein. The central portion of Mrc1, containing a conserved coiled-coil region, was found to be essential for interaction with the 168-amino-acid C-terminal region of Mcm6, and introduction of two amino acid substitutions in this C-terminal region abolished the interaction with Mrc1 in vivo. An mcm6 mutant bearing these substitutions showed a severe defect in DNA replication checkpoint activation in response to stress caused by methyl methanesulfonate. Interestingly, the mutant did not show any defect in DNA replication checkpoint activation in response to hydroxyurea treatment. The phenotype of the mcm6 mutant was suppressed when the mutant protein was physically fused with Mrc1. These results strongly suggest for the first time that an Mcm helicase acts as a checkpoint sensor for methyl methanesulfonate-induced DNA damage through direct binding to the replication checkpoint mediator Mrc1.
机译:Mrc1在介导DNA复制检查点中发挥作用。我们调查了直接与Mrc1相互作用的复制延伸蛋白,并确定了复制解旋酶Mcm6作为特定的Mrc1结合蛋白。已发现Mrc1的中央部分包含一个保守的卷曲螺旋区域,对于与Mcm6的168个氨基酸的C末端区域相互作用是必不可少的,并且在该C末端区域引入了两个氨基酸取代,从而消除了在体内与Mrc1相互作用。带有这些取代的mcm6突变体显示出响应由甲磺酸甲酯引起的应激而在DNA复制检查点激活中存在严重缺陷。有趣的是,该突变体在响应羟基脲处理的DNA复制检查点激活中未显示任何缺陷。当突变体蛋白与Mrc1物理融合时,mcm6突变体的表型被抑制。这些结果首次强烈表明,Mcm解旋酶通过直接与复制检查点介体Mrc1结合而充当甲烷磺酸甲酯诱导的DNA损伤的检查点传感器。

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