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传感器 1 和牛乳头瘤病毒 E1 起始蛋白 Walker B 中的突变模拟核苷酸结合状态。

Mutations in Sensor 1 and Walker B in the bovine papillomavirus E1 initiator protein mimic the nucleotide-bound state.

机构信息

Cold Spring Harbor Laboratory, P.O. Box 100, 1 Bungtown Road, Cold Spring Harbor, NY 11724, USA.

出版信息

J Virol. 2010 Feb;84(4):1912-9. doi: 10.1128/JVI.01756-09. Epub 2009 Nov 25.

Abstract

Viral replication initiator proteins are multifunctional proteins that utilize ATP binding and hydrolysis by their AAA+ modules for multiple functions in the replication of their viral genomes. These proteins are therefore of particular interest for understanding how AAA+ proteins carry out multiple ATP driven functions. We have performed a comprehensive mutational analysis of the residues involved in ATP binding and hydrolysis in the papillomavirus E1 initiator protein based on the recent structural data. Ten of the eleven residues that were targeted were defective for ATP hydrolysis, and seven of these were also defective for ATP binding. The three mutants that could still bind nucleotide represent the Walker B motif (D478 and D479) and Sensor 1 (N523), three residues that are in close proximity to each other and generally are considered to be involved in ATP hydrolysis. Surprisingly, however, two of these mutants, D478A and N523A, mimicked the nucleotide bound state and were capable of binding DNA in the absence of nucleotide. However, these mutants could not form the E1 double trimer in the absence of nucleotide, demonstrating that there are two qualitatively different consequences of ATP binding by E1, one that can be mimicked by D478A and N523A and one which cannot.

摘要

病毒复制起始蛋白是多功能蛋白,它们利用 AAA+ 模块结合和水解 ATP,以实现其病毒基因组复制的多种功能。因此,这些蛋白特别适合用于理解 AAA+ 蛋白如何执行多种 ATP 驱动的功能。我们根据最近的结构数据,对乳头瘤病毒 E1 起始蛋白中参与 ATP 结合和水解的残基进行了全面的突变分析。基于最近的结构数据,我们针对 11 个目标残基中的 10 个进行了 ATP 水解缺陷分析,其中 7 个残基也存在 ATP 结合缺陷。仍能结合核苷酸的三个突变体代表 Walker B 基序(D478 和 D479)和传感器 1(N523),这三个残基彼此靠近,通常被认为参与 ATP 水解。然而,令人惊讶的是,这两个突变体 D478A 和 N523A 模拟了核苷酸结合状态,并且能够在没有核苷酸的情况下结合 DNA。然而,这些突变体在没有核苷酸的情况下不能形成 E1 双三聚体,这表明 E1 结合核苷酸有两种不同的定性后果,其中一种可以被 D478A 和 N523A 模拟,而另一种则不能。

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