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古菌中复制 DNA 聚合酶的进化及其对真核复制机制的贡献。

Evolution of replicative DNA polymerases in archaea and their contributions to the eukaryotic replication machinery.

机构信息

National Center for Biotechnology Information, National Library of Medicine, National Institutes of Health Bethesda, MD, USA.

Unité Biologie Moléculaire du Gène chez les Extrêmophiles, Institut Pasteur Paris, France.

出版信息

Front Microbiol. 2014 Jul 21;5:354. doi: 10.3389/fmicb.2014.00354. eCollection 2014.

Abstract

The elaborate eukaryotic DNA replication machinery evolved from the archaeal ancestors that themselves show considerable complexity. Here we discuss the comparative genomic and phylogenetic analysis of the core replication enzymes, the DNA polymerases, in archaea and their relationships with the eukaryotic polymerases. In archaea, there are three groups of family B DNA polymerases, historically known as PolB1, PolB2 and PolB3. All three groups appear to descend from the last common ancestors of the extant archaea but their subsequent evolutionary trajectories seem to have been widely different. Although PolB3 is present in all archaea, with the exception of Thaumarchaeota, and appears to be directly involved in lagging strand replication, the evolution of this gene does not follow the archaeal phylogeny, conceivably due to multiple horizontal transfers and/or dramatic differences in evolutionary rates. In contrast, PolB1 is missing in Euryarchaeota but otherwise seems to have evolved vertically. The third archaeal group of family B polymerases, PolB2, includes primarily proteins in which the catalytic centers of the polymerase and exonuclease domains are disrupted and accordingly the enzymes appear to be inactivated. The members of the PolB2 group are scattered across archaea and might be involved in repair or regulation of replication along with inactivated members of the RadA family ATPases and an additional, uncharacterized protein that are encoded within the same predicted operon. In addition to the family B polymerases, all archaea, with the exception of the Crenarchaeota, encode enzymes of a distinct family D the origin of which is unclear. We examine multiple considerations that appear compatible with the possibility that family D polymerases are highly derived homologs of family B. The eukaryotic DNA polymerases show a highly complex relationship with their archaeal ancestors including contributions of proteins and domains from both the family B and the family D archaeal polymerases.

摘要

真核生物 DNA 复制机制非常复杂,它由古菌祖先进化而来,而古菌本身就相当复杂。在这里,我们讨论了古菌核心复制酶(即 DNA 聚合酶)的比较基因组学和系统发育分析,以及它们与真核聚合酶的关系。在古菌中,有三组 B 家族 DNA 聚合酶,历史上被称为 PolB1、PolB2 和 PolB3。这三组聚合酶似乎都起源于现存古菌的最后共同祖先,但它们随后的进化轨迹似乎大相径庭。虽然 PolB3 存在于除 Thaumarchaeota 以外的所有古菌中,并且似乎直接参与滞后链复制,但该基因的进化并不遵循古菌的系统发育,这可能是由于多次水平转移和/或进化速度的巨大差异所致。相比之下,PolB1 在广古菌中缺失,但其他方面似乎是垂直进化的。B 家族的第三组古菌聚合酶 PolB2 主要包括其聚合酶和外切酶结构域的催化中心被破坏的蛋白质,因此这些酶似乎失活了。PolB2 组的成员分散在古菌中,可能与修复或调节复制有关,还与失活的 RadA 家族 ATP 酶以及编码在同一预测操纵子中的另一个未鉴定的蛋白质有关。除了 B 家族聚合酶外,除了泉古菌以外的所有古菌都编码一种独特的 D 家族酶,其起源尚不清楚。我们考察了多种因素,这些因素似乎都支持 D 家族聚合酶是 B 家族高度衍生的同源物的可能性。真核生物 DNA 聚合酶与古菌祖先之间的关系非常复杂,包括来自 B 家族和 D 家族古菌聚合酶的蛋白质和结构域的贡献。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/141c/4104785/a56a74c441d2/fmicb-05-00354-g0001.jpg

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