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发动蛋白样GTP酶Dnm1与线粒体动力学蛋白Fis1的直接结合受到Fis1 N端臂的负调控。

Direct binding of the dynamin-like GTPase, Dnm1, to mitochondrial dynamics protein Fis1 is negatively regulated by the Fis1 N-terminal arm.

作者信息

Wells Robert C, Picton Lora K, Williams Sarah C P, Tan Frederick J, Hill R Blake

机构信息

Department of Biology, The Johns Hopkins University, Baltimore, Maryland, 21218.

Department of Biology, The Johns Hopkins University, Baltimore, Maryland, 21218; Department of Chemistry, The Johns Hopkins University, Baltimore, Maryland 21218.

出版信息

J Biol Chem. 2007 Nov 16;282(46):33769-33775. doi: 10.1074/jbc.M700807200. Epub 2007 Sep 20.

Abstract

Recruitment of a dynamin-like GTPase (Drp1/Dlp1/Dnm1) to membranes requires the mitochondrial dynamics protein Fis1. Mdv1 has been proposed to act as an adaptor between Fis1 and Dnm1 in Saccharomyces cerevisiae. We show that S. cerevisiae Fis1 binds directly to Dnm1 and to Mdv1. Two Fis1 regions have been previously implicated in Mdv1 recruitment: an N-terminal "arm" and a concave surface formed by evolutionarily conserved residues in the tetratricopeptide repeat domain. Perturbing either Fis1 region does not affect Mdv1 binding, but both regions influence Dnm1 binding. Fis1 lacking its N-terminal arm binds tightly to Dnm1, and binding is abolished by mutations to the Fis1 concave surface. The Fis1-Dnm1 interaction decreases more than 100-fold in the presence of the Fis1 arm, suggesting that the arm acts in an autoinhibitory manner to restrict access to the Dnm1 binding site on Fis1. Our data indicate that the concave surface of the Fis1 tetratricopeptide repeat-like domain is evolutionarily conserved to bind the dynamin-like GTPase Dnm1 and not Mdv1 as previously predicted.

摘要

一种类似发动蛋白的GTP酶(Drp1/Dlp1/Dnm1)定位于膜上需要线粒体动力蛋白Fis1。在酿酒酵母中,Mdv1被认为是Fis1和Dnm1之间的衔接蛋白。我们发现酿酒酵母Fis1直接与Dnm1和Mdv1结合。先前有两个Fis1区域与Mdv1募集有关:一个N端“臂”和由四肽重复结构域中进化保守残基形成的凹面。干扰这两个Fis1区域中的任何一个都不会影响Mdv1结合,但两个区域都会影响Dnm1结合。缺失N端臂的Fis1与Dnm1紧密结合,而Fis1凹面的突变会消除这种结合。在存在Fis1臂的情况下,Fis1-Dnm1相互作用降低了100多倍,这表明该臂以自抑制方式作用,限制对Fis1上Dnm1结合位点的访问。我们的数据表明,Fis1四肽重复样结构域的凹面在进化上保守,用于结合类似发动蛋白的GTP酶Dnm1,而不是如先前预测的Mdv1。

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