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关键DNA结合残基在复制因子C催化的夹子加载机制中充当启动/终止控制。

Linchpin DNA-binding residues serve as go/no-go controls in the replication factor C-catalyzed clamp-loading mechanism.

作者信息

Liu Juan, Zhou Yayan, Hingorani Manju M

机构信息

From the Department of Molecular Biology and Biochemistry, Wesleyan University, Middletown, Connecticut 06459.

From the Department of Molecular Biology and Biochemistry, Wesleyan University, Middletown, Connecticut 06459

出版信息

J Biol Chem. 2017 Sep 22;292(38):15892-15906. doi: 10.1074/jbc.M117.798702. Epub 2017 Aug 14.

DOI:10.1074/jbc.M117.798702
PMID:28808059
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5612119/
Abstract

DNA polymerases depend on circular sliding clamps for processive replication. Clamps must be loaded onto primer-template DNA (ptDNA) by clamp loaders that open and close clamps around ptDNA in an ATP-fueled reaction. All clamp loaders share a core structure in which five subunits form a spiral chamber that binds the clamp at its base in a twisted open form and encloses ptDNA within, while binding and hydrolyzing ATP to topologically link the clamp and ptDNA. To understand how clamp loaders perform this complex task, here we focused on conserved arginines that might play a central coordinating role in the mechanism because they can alternately contact ptDNA or Walker B glutamate in the ATPase site and lie close to the clamp loader-clamp-binding interface. We mutated Arg-84, Arg-88, and Arg-101 in the ATPase-active B, C, and D subunits of replication factor C (RFC) clamp loader, respectively, and assessed the impact on multiple transient events in the reaction: proliferating cell nuclear antigen (PCNA) clamp binding/opening/closure/release, ptDNA binding/release, and ATP hydrolysis/product release. The results show that these arginines relay critical information between the PCNA-binding, DNA-binding, and ATPase sites at all steps of the reaction, particularly at a checkpoint before RFC commits to ATP hydrolysis. Moreover, their actions are subunit-specific with RFC-C Arg-88 serving as an accelerator that enables rapid ATP hydrolysis upon contact with ptDNA and RFC-D Arg-101 serving as a brake that confers specificity for ptDNA as the correct substrate for loading PCNA.

摘要

DNA聚合酶依靠环状滑动夹进行连续复制。夹必须由夹装载器加载到引物模板DNA(ptDNA)上,夹装载器在由ATP驱动的反应中围绕ptDNA打开和关闭夹。所有夹装载器都共享一个核心结构,其中五个亚基形成一个螺旋腔,该螺旋腔以扭曲的开放形式在夹的底部结合夹,并将ptDNA封闭在其中,同时结合并水解ATP以拓扑方式连接夹和ptDNA。为了了解夹装载器如何执行这项复杂任务,我们在此聚焦于保守的精氨酸,它们可能在该机制中发挥核心协调作用,因为它们可以交替接触ptDNA或ATP酶位点中的沃克B谷氨酸,并且位于靠近夹装载器 - 夹结合界面的位置。我们分别在复制因子C(RFC)夹装载器的ATP酶活性B、C和D亚基中突变了精氨酸 - 84、精氨酸 - 88和精氨酸 - 101,并评估了对反应中多个瞬时事件的影响:增殖细胞核抗原(PCNA)夹的结合/打开/关闭/释放、ptDNA的结合/释放以及ATP水解/产物释放。结果表明,这些精氨酸在反应的所有步骤中,尤其是在RFC进行ATP水解之前的一个检查点,在PCNA结合、DNA结合和ATP酶位点之间传递关键信息。此外,它们的作用具有亚基特异性,RFC - C精氨酸 - 88作为加速器,在与ptDNA接触时能够快速进行ATP水解,而RFC - D精氨酸 - 101作为制动器,赋予ptDNA作为加载PCNA的正确底物的特异性。

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Forging Ahead through Darkness: PCNA, Still the Principal Conductor at the Replication Fork.在黑暗中奋勇前行:增殖细胞核抗原,依然是复制叉处的主要指挥者。
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The ATP sites of AAA+ clamp loaders work together as a switch to assemble clamps on DNA.AAA+ 夹钳加载器的 ATP 结合位点作为一个开关协同作用,将夹钳组装到 DNA 上。
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