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复制叉结合触发 PriA 解旋酶的结构变化,从而控制大肠杆菌中的 DNA 复制起始。

Replication fork binding triggers structural changes in the PriA helicase that govern DNA replication restart in E. coli.

机构信息

Department of Biomolecular Chemistry, University of Wisconsin-Madison, Madison, WI, 53706, USA.

Department of Biochemistry, University of Wisconsin-Madison, Madison, WI, 53706, USA.

出版信息

Nat Commun. 2023 May 11;14(1):2725. doi: 10.1038/s41467-023-38144-x.

Abstract

Bacterial replisomes often dissociate from replication forks before chromosomal replication is complete. To avoid the lethal consequences of such situations, bacteria have evolved replication restart pathways that reload replisomes onto prematurely terminated replication forks. To understand how the primary replication restart pathway in E. coli (PriA-PriB) selectively acts on replication forks, we determined the cryogenic-electron microscopy structure of a PriA/PriB/replication fork complex. Replication fork specificity arises from extensive PriA interactions with each arm of the branched DNA. These interactions reshape the PriA protein to create a pore encircling single-stranded lagging-strand DNA while also exposing a surface of PriA onto which PriB docks. Together with supporting biochemical and genetic studies, the structure reveals a switch-like mechanism for replication restart initiation in which restructuring of PriA directly couples replication fork recognition to PriA/PriB complex formation to ensure robust and high-fidelity replication re-initiation.

摘要

细菌复制体在染色体复制完成之前常常从复制叉上解离。为了避免这种情况的致命后果,细菌已经进化出复制重启动途径,将复制体重新加载到过早终止的复制叉上。为了了解大肠杆菌中主要的复制重启动途径(PriA-PriB)如何选择性地作用于复制叉,我们确定了 PriA/PriB/复制叉复合物的低温电子显微镜结构。复制叉的特异性源于 PriA 与分叉 DNA 的每一条臂的广泛相互作用。这些相互作用重塑了 PriA 蛋白,在单链滞后链 DNA 周围形成一个孔,同时也暴露了 PriA 的一个表面,PriB 可以在这个表面上对接。结合支持的生化和遗传研究,该结构揭示了一种类似于开关的复制重启动起始机制,其中 PriA 的结构重排将复制叉识别与 PriA/PriB 复合物的形成直接偶联起来,以确保强大和高保真的复制重新启动。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/000d/10175261/50e3f217cc7a/41467_2023_38144_Fig1_HTML.jpg

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