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普遍保守的依赖 ATP 的蛋白酶 FtsH 介导的膜蛋白的折叠-降解关系。

Folding-Degradation Relationship of a Membrane Protein Mediated by the Universally Conserved ATP-Dependent Protease FtsH.

机构信息

Department of Bioengineering , University of Illinois at Chicago , Chicago , Illinois 60607 , United States.

出版信息

J Am Chem Soc. 2018 Apr 4;140(13):4656-4665. doi: 10.1021/jacs.8b00832. Epub 2018 Mar 21.

DOI:10.1021/jacs.8b00832
PMID:29528632
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5892824/
Abstract

ATP-dependent protein degradation mediated by AAA+ proteases is one of the major cellular pathways for protein quality control and regulation of functional networks. While a majority of studies of protein degradation have focused on water-soluble proteins, it is not well understood how membrane proteins with abnormal conformation are selectively degraded. The knowledge gap stems from the lack of an in vitro system in which detailed molecular mechanisms can be studied as well as difficulties in studying membrane protein folding in lipid bilayers. To quantitatively define the folding-degradation relationship of membrane proteins, we reconstituted the degradation using the conserved membrane-integrated AAA+ protease FtsH as a model degradation machine and the stable helical-bundle membrane protein GlpG as a model substrate in the lipid bilayer environment. We demonstrate that FtsH possesses a substantial ability to actively unfold GlpG, and the degradation significantly depends on the stability and hydrophobicity near the degradation marker. We find that FtsH hydrolyzes 380-550 ATP molecules to degrade one copy of GlpG. Remarkably, FtsH overcomes the dual-energetic burden of substrate unfolding and membrane dislocation with the ATP cost comparable to that for water-soluble substrates by robust ClpAP/XP proteases. The physical principles elucidated in this study provide general insights into membrane protein degradation mediated by ATP-dependent proteolytic systems.

摘要

ATP 依赖性蛋白降解途径由 AAA+ 蛋白酶介导,是细胞内蛋白质质量控制和功能网络调控的主要途径之一。尽管大多数蛋白质降解研究都集中在水溶性蛋白质上,但对于具有异常构象的膜蛋白如何被选择性降解,人们的了解还很有限。这一知识空白源于缺乏一个能够深入研究详细分子机制的体外系统,以及在研究脂质双层中膜蛋白折叠时所面临的困难。为了定量定义膜蛋白的折叠-降解关系,我们以保守的膜整合 AAA+ 蛋白酶 FtsH 为模型降解机器,以稳定的螺旋束膜蛋白 GlpG 为模型底物,在脂质双层环境中重新构建了降解过程。我们证明 FtsH 具有主动展开 GlpG 的强大能力,并且降解过程显著依赖于降解标记附近的稳定性和疏水性。我们发现 FtsH 水解 380-550 个 ATP 分子来降解一个 GlpG 分子。值得注意的是,FtsH 通过 ClpAP/XP 蛋白酶的强大作用,克服了底物展开和膜移位的双重能量负担,其 ATP 成本与水溶性底物相当。本研究中阐明的物理原理为 ATP 依赖性蛋白水解系统介导的膜蛋白降解提供了普遍的见解。

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