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The Major Roles of DNA Polymerases Epsilon and Delta at the Eukaryotic Replication Fork Are Evolutionarily Conserved

机译:DNA聚合酶Epsilon和Delta在真核复制叉中的主要作用是进化保守的。

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摘要

Coordinated replication of eukaryotic genomes is intrinsically asymmetric, with continuous leading strand synthesis preceding discontinuous lagging strand synthesis. Here we provide two types of evidence indicating that, in fission yeast, these two biosynthetic tasks are performed by two different replicases. First, in Schizosaccharomyces pombe strains encoding a polδ-L591M mutator allele, base substitutions in reporter genes placed in opposite orientations relative to a well-characterized replication origin are strand-specific and distributed in patterns implying that Polδ is primarily involved in lagging strand replication. Second, in strains encoding a polε-M630F allele and lacking the ability to repair rNMPs in DNA due to a defect in RNase H2, rNMPs are selectively observed in nascent leading strand DNA. The latter observation demonstrates that abundant rNMP incorporation during replication can be tolerated and that they are normally removed in an RNase H2-dependent manner. This provides strong physical evidence that Polε is the primary leading strand replicase. Collectively, these data and earlier results in budding yeast indicate that the major roles of Polδ and Polε at the eukaryotic replication fork are evolutionarily conserved.
机译:真核基因组的协调复制本质上是不对称的,连续的前导链合成先于不连续的滞后链合成。在这里,我们提供了两种类型的证据,表明在裂变酵母中,这两个生物合成任务是由两个不同的复制品执行的。首先,在编码polδ-L591M突变体等位基因的粟酒裂殖酵母菌株中,相对于充分表征的复制起点而言,位于相反方向的报告基因中的碱基取代是链特异性的,并且分布的方式表明Polδ主要参与滞后链的复制。其次,在编码polε-M630F等位基因且由于RNase H2缺陷而缺乏修复DNA中rNMPs能力的菌株中,在新生的前导链DNA中选择性地观察到rNMPs。后一个观察结果表明,复制过程中大量rNMP的掺入是可以容忍的,并且通常以RNase H2依赖的方式将其清除。这提供了有力的物理证据,证明Polε是主要的前导链复制酶。总的来说,这些数据和早期萌芽结果表明,Polδ和Polε在真核复制叉中的主要作用在进化上是保守的。

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