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离子(K⁺/Na⁺)及pH对GTPase活性和FtsZ(微管蛋白的原核直系同源物)聚合作用影响的结构与功能模型

Structural and functional model for ionic (K(+)/Na(+)) and pH dependence of GTPase activity and polymerization of FtsZ, the prokaryotic ortholog of tubulin.

作者信息

Mendieta Jesús, Rico Ana Isabel, López-Viñas Eduardo, Vicente Miguel, Mingorance Jesús, Gómez-Puertas Paulino

机构信息

Centro de Biología Molecular "Severo Ochoa", Madrid, Spain.

出版信息

J Mol Biol. 2009 Jul 3;390(1):17-25. doi: 10.1016/j.jmb.2009.05.018. Epub 2009 May 15.

DOI:10.1016/j.jmb.2009.05.018
PMID:19447111
Abstract

Bacterial cell division occurs through the formation of a protein ring (division ring) at the site of division, with FtsZ being its main component in most bacteria. FtsZ is the prokaryotic ortholog of eukaryotic tubulin; it shares GTPase activity properties and the ability to polymerize in vitro. To study the mechanism of action of FtsZ, we used molecular dynamics simulations of the behavior of the FtsZ dimer in the presence of GTP-Mg(2+) and monovalent cations. The presence of a K(+) ion at the GTP binding site allows the positioning of one water molecule that interacts with catalytic residues Asp235 and Asp238, which are also involved in the coordination sphere of K(+). This arrangement might favor dimer stability and GTP hydrolysis. Contrary to this, Na(+) destabilizes the dimer and does not allow the positioning of the catalytic water molecule. Protonation of the GTP gamma-phosphate, simulating low pH, excludes both monovalent cations and the catalytic water molecule from the GTP binding site and stabilizes the dimer. These molecular dynamics predictions were contrasted experimentally by analyzing the GTPase and polymerization activities of purified Methanococcus jannaschii and Escherichia coli FtsZ proteins in vitro.

摘要

细菌细胞分裂通过在分裂位点形成蛋白质环(分裂环)来进行,在大多数细菌中,FtsZ是其主要成分。FtsZ是真核微管蛋白的原核直系同源物;它具有GTPase活性特性以及在体外聚合的能力。为了研究FtsZ的作用机制,我们对FtsZ二聚体在GTP-Mg(2+)和单价阳离子存在下的行为进行了分子动力学模拟。GTP结合位点处K(+)离子的存在允许一个水分子定位,该水分子与催化残基Asp235和Asp238相互作用,这两个残基也参与K(+)的配位球。这种排列可能有利于二聚体稳定性和GTP水解。与此相反,Na(+)会使二聚体不稳定,并且不允许催化水分子定位。模拟低pH时GTPγ-磷酸的质子化将单价阳离子和催化水分子都排除在GTP结合位点之外,并使二聚体稳定。通过分析纯化的詹氏甲烷球菌和大肠杆菌FtsZ蛋白在体外的GTPase和聚合活性,将这些分子动力学预测与实验结果进行了对比。

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