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p22 头部完整包装核酸酶的结构。

Structure of p22 headful packaging nuclease.

机构信息

Department of Biochemistry and Molecular Biology, Thomas Jefferson University, Philadelphia, Pennsylvania 19107, USA.

出版信息

J Biol Chem. 2012 Aug 10;287(33):28196-205. doi: 10.1074/jbc.M112.349894. Epub 2012 Jun 19.

DOI:10.1074/jbc.M112.349894
PMID:22715098
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3431676/
Abstract

Packaging of viral genomes into preformed procapsids requires the controlled and synchronized activity of an ATPase and a genome-processing nuclease, both located in the large terminase (L-terminase) subunit. In this paper, we have characterized the structure and regulation of bacteriophage P22 L-terminase (gp2). Limited proteolysis reveals a bipartite organization consisting of an N-terminal ATPase core flexibly connected to a C-terminal nuclease domain. The 2.02 Å crystal structure of P22 headful nuclease obtained by in-drop proteolysis of full-length L-terminase (FL-L-terminase) reveals a central seven-stranded β-sheet core that harbors two magnesium ions. Modeling studies with DNA suggest that the two ions are poised for two-metal ion-dependent catalysis, but the nuclease DNA binding surface is sterically hindered by a loop-helix (L(1)-α(2)) motif, which is incompatible with catalysis. Accordingly, the isolated nuclease is completely inactive in vitro, whereas it exhibits endonucleolytic activity in the context of FL-L-terminase. Deleting the autoinhibitory L(1)-α(2) motif (or just the loop L(1)) restores nuclease activity to a level comparable with FL-L-terminase. Together, these results suggest that the activity of P22 headful nuclease is regulated by intramolecular cross-talk with the N-terminal ATPase domain. This cross-talk allows for precise and controlled cleavage of DNA that is essential for genome packaging.

摘要

将病毒基因组包装到预先形成的衣壳中需要 ATP 酶和基因组加工核酸酶的受控和同步活性,这两种酶都位于大型末端酶(L-末端酶)亚基中。在本文中,我们对噬菌体 P22 L-末端酶(gp2)的结构和调节进行了表征。有限的蛋白水解揭示了由一个 N 端 ATP 酶核心和一个灵活连接的 C 端核酸酶结构域组成的二分体组织。通过全长 L-末端酶(FL-L-末端酶)的液滴内蛋白水解获得的 P22 头部完整核酸酶的 2.02Å 晶体结构揭示了一个中央七股 β-折叠核心,其中含有两个镁离子。与 DNA 的建模研究表明,这两个离子为双金属离子依赖性催化做好了准备,但核酸酶的 DNA 结合表面被一个环-螺旋(L(1)-α(2))基序所阻碍,这与催化不相容。因此,分离的核酸酶在体外完全没有活性,而在 FL-L-末端酶的情况下,它表现出内切核酸酶活性。删除自抑制的 L(1)-α(2)基序(或仅删除环 L(1))可将核酸酶活性恢复到与 FL-L-末端酶相当的水平。这些结果表明,P22 头部完整核酸酶的活性受到与 N 端 ATP 酶结构域的分子内交叉对话的调节。这种交叉对话允许对基因组包装必不可少的 DNA 进行精确和受控的切割。

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