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Mouse Rev1 protein interacts with multiple DNA polymerases involved in translesion DNA synthesis

机译:小鼠Rev1蛋白与参与跨病变DNA合成的多种DNA聚合酶相互作用

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摘要

Polκ and Rev1 are members of the Y family of DNA polymerases involved in tolerance to DNA damage by replicative bypass [translesion DNA synthesis (TLS)]. We demonstrate that mouse Rev1 protein physically associates with Polκ. We show too that Rev1 interacts independently with Rev7 (a subunit of a TLS polymerase, Polζ) and with two other Y-family polymerases, Polι and Polη. Mouse Polκ, Rev7, Polι and Polη each bind to the same ∼100 amino acid C-terminal region of Rev1. Furthermore, Rev7 competes directly with Polκ for binding to the Rev1 C-terminus. Notwith standing the physical interaction between Rev1 and Polκ, the DNA polymerase activity of each measured by primer extension in vitro is unaffected by the complex, either when extending normal primer-termini, when bypassing a single thymine glycol lesion, or when extending certain mismatched primer termini. Our observations suggest that Rev1 plays a role(s) in mediating protein–protein interactions among DNA polymerases required for TLS. The precise function(s) of these interactions during TLS remains to be determined.
机译:Polκ和Rev1是DNA聚合酶Y家族的成员,该家族参与通过复制性旁路[DNA转移(TLS)]对DNA损伤的耐受性。我们证明小鼠Rev1蛋白与Polκ物理关联。我们还表明,Rev1与Rev7(TLS聚合酶的一个亚基,Polζ)以及其他两个Y家族聚合酶,PolI和Polη相互作用。小鼠Polκ,Rev7,PolI和Polη分别与Rev1的约100个氨基酸的C末端区域结合。此外,Rev7与Polκ直接竞争与Rev1 C末端的结合。尽管具有Rev1和Polκ之间的物理相互作用,但在体外延伸引物末端,绕过单个胸腺嘧啶二醇病变时或在延伸某些错配引物时,通过体外引物延伸测量的每种DNA聚合酶活性均不受复合物的影响。总站。我们的观察结果表明,Rev1在介导TLS所需的DNA聚合酶之间的蛋白质间相互作用中发挥了作用。 TLS期间这些交互的确切功能还有待确定。

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