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ClpXP 对蛋白底物的切割谱揭示了刻意的起始和停顿。

The Cleavage Profile of Protein Substrates by ClpXP Reveals Deliberate Starts and Pauses.

机构信息

Department of Chemistry, University of Massachusetts, Amherst, Massachusetts 01003, United States.

Department of Biochemistry and Molecular Biology, University of Massachusetts, Amherst, Massachusetts 01003, United States.

出版信息

Biochemistry. 2020 Nov 10;59(44):4294-4301. doi: 10.1021/acs.biochem.0c00553. Epub 2020 Nov 2.

DOI:10.1021/acs.biochem.0c00553
PMID:33135889
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7658057/
Abstract

Cells rely on protein degradation by AAA+ proteases. A well-known example is the hexameric ClpX unfoldase, which captures ATP hydrolysis to feed substrates into the oligomeric ClpP peptidase. Recent studies show that an asymmetric ClpX spiral cycles protein translocation upon ATP hydrolysis. However, how this cycle affects peptide products is less explored in part because ClpP cleavage is thought to be solely defined by sequence constraints. Here, we comprehensively characterize peptides from ClpXP degradation of three different substrates using high-resolution mass spectrometry and find that cleavage of translocated substrates is driven by factors other than sequence. We report that defined locations in a translocated protein are especially sensitive to cleavage spaced on average every 10-13 residues. These sites are not exclusively controlled by sequence and are independent of bulk changes in catalytic peptidase sites, ATP hydrolysis, or the efficiency of initial recognition. These results fit a model in which processive translocation through ClpX starts at a specific location in a polypeptide and pauses during reset of the ClpX hexamer after a cycle of translocation. Our work suggests that defined peptides, which could be used as signaling molecules, can be generated from a given substrate by a nonspecific peptidase.

摘要

细胞依赖于 AAA+蛋白酶的蛋白质降解。一个众所周知的例子是六聚体 ClpX 解旋酶,它通过捕获 ATP 水解将底物送入寡聚 ClpP 肽酶中。最近的研究表明,不对称的 ClpX 螺旋在 ATP 水解时循环进行蛋白质易位。然而,这种循环如何影响肽产物在一定程度上还没有被探索,因为 ClpP 切割被认为仅由序列限制定义。在这里,我们使用高分辨率质谱法全面表征了 ClpXP 降解三种不同底物的肽,并发现易位底物的切割是由序列以外的因素驱动的。我们报告说,在易位蛋白中,定义的位置对平均每 10-13 个残基间隔的切割特别敏感。这些位点不仅受序列控制,而且与催化肽酶位点、ATP 水解或初始识别效率的整体变化无关。这些结果符合这样一种模型,即 ClpX 中的连续易位从多肽中的特定位置开始,并在易位循环后的 ClpX 六聚体重置期间暂停。我们的工作表明,通过非特异性肽酶可以从给定的底物产生特定的肽,这些肽可以作为信号分子。

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本文引用的文献

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Structures of the ATP-fueled ClpXP proteolytic machine bound to protein substrate.ATP 驱动的 ClpXP 蛋白水解机器与蛋白质底物结合的结构。
Elife. 2020 Feb 28;9:e52774. doi: 10.7554/eLife.52774.
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A processive rotary mechanism couples substrate unfolding and proteolysis in the ClpXP degradation machinery.一种连续旋转的机制将底物展开和蛋白水解在 ClpXP 降解机制中偶联在一起。
Elife. 2020 Jan 9;9:e52158. doi: 10.7554/eLife.52158.
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