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REV1 restrains DNA polymerase ζ to ensure frame fidelity during translesion synthesis of UV photoproducts in vivo

机译:REV1抑制DNA聚合酶ζ,以确保体内跨膜合成UV光产品过程中的帧保真度

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摘要

Exposure to ultraviolet light induces a number of forms of damage in DNA, of which (6–4) photoproducts present the most formidable challenge to DNA replication. No single DNA polymerase has been shown to bypass these lesions efficiently in vitro suggesting that the coordinate use of a number of different enzymes is required in vivo. To further understand the mechanisms and control of lesion bypass in vivo, we have devised a plasmid-based system to study the replication of site-specific T–T(6–4) photoproducts in chicken DT40 cells. We show that DNA polymerase ζ is absolutely required for translesion synthesis (TLS) of this lesion, while loss of DNA polymerase η has no detectable effect. We also show that either the polymerase-binding domain of REV1 or ubiquitinated PCNA is required for the recruitment of Polζ as the catalytic TLS polymerase. Finally, we demonstrate a previously unappreciated role for REV1 in ensuring bypass synthesis remains in frame with the template. Our data therefore suggest that REV1 not only helps to coordinate the delivery of DNA polymerase ζ to a stalled primer terminus but also restrains its activity to ensure that nucleotides are incorporated in register with the template strand.
机译:暴露于紫外线下会导致DNA受到多种形式的破坏,其中(6–4)种光产物对DNA复制提出了最严峻的挑战。尚无单个DNA聚合酶在体外有效绕过这些病变,提示体内需要协调使用多种不同的酶。为了进一步了解体内病变旁路的机制和控制,我们设计了一个基于质粒的系统来研究鸡DT40细胞中特定位点的T–T(6–4)光产物的复制。我们表明,DNA聚合酶ζ是该病灶的病变合成(TLS)绝对必需的,而DNA聚合酶η的丢失则没有可检测的作用。我们还表明,REV1的聚合酶结合域或泛素化的PCNA都是招募Polζ作为催化TLS聚合酶所必需的。最后,我们证明了REV1在确保旁路合成与模板保持一致方面的前所未有的作用。因此,我们的数据表明,REV1不仅有助于协调DNA聚合酶ζ向停滞的引物末端的传递,而且还限制了其活性,以确保核苷酸与模板链结合在一起。

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