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线粒体菱形蛋白酶对 Mgm1 的跨膜水解作用对于被切割疏水区序列具有高度的混杂性。

Intramembrane proteolysis of Mgm1 by the mitochondrial rhomboid protease is highly promiscuous regarding the sequence of the cleaved hydrophobic segment.

机构信息

CEF Makromolekulare Komplexe, Mitochondriale Biologie, Fachbereich Medizin, Goethe-Universität Frankfurt am Main, Theodor-Stern-Kai 7, 60590 Frankfurt am Main, Germany.

出版信息

J Mol Biol. 2010 Aug 13;401(2):182-93. doi: 10.1016/j.jmb.2010.06.014. Epub 2010 Jun 15.

DOI:10.1016/j.jmb.2010.06.014
PMID:20558178
Abstract

Rhomboids are a family of intramembrane serine proteases that are conserved in bacteria, archaea, and eukaryotes. They are required for numerous fundamental cellular functions such as quorum sensing, cell signaling, and mitochondrial dynamics. Mitochondrial rhomboids form an evolutionarily distinct class of rhomboids. It is largely unclear how their activity is controlled and which substrate determinants are responsible for recognition and cleavage. We investigated these requirements for the mitochondrial rhomboid protease Pcp1 and its substrate Mgm1. In contrast to several other rhomboid proteases, Pcp1 does not require helix-breaking amino acids in the cleaved hydrophobic region of Mgm1, termed 'rhomboid cleavage region' (RCR). Even transmembrane segments of inner membrane proteins that are normally not processed by Pcp1 become cleavable when put in place of the authentic RCR of Mgm1. We further show that mutational alterations of a highly negatively charged region located C-terminally to the RCR led to a strong processing defect. Moreover, we show that the determinants required for Mgm1 processing by mitochondrial rhomboid protease are conserved during evolution, as PARL (the human ortholog of Pcp1) showed similar substrate requirements. These results suggest a surprising promiscuity of the mitochondrial rhomboid protease regarding the sequence requirements of the cleaved hydrophobic segment. We propose a working hypothesis on how the mitochondrial rhomboid protease can, despite this promiscuity, achieve a high specificity in recognizing Mgm1. This hypothesis relates to the exceptional biogenesis pathway of Mgm1.

摘要

菱形蛋白酶是一类跨膜丝氨酸蛋白酶,在细菌、古菌和真核生物中都有保守序列。它们参与了许多基本的细胞功能,如群体感应、细胞信号转导和线粒体动力学。线粒体菱形蛋白酶形成了一个独特的菱形蛋白酶家族。目前尚不清楚它们的活性是如何被调控的,也不清楚哪些底物决定因素负责识别和切割。我们研究了线粒体菱形蛋白酶 Pcp1 及其底物 Mgm1 的这些要求。与其他几种菱形蛋白酶不同,Pcp1 不需要 Mgm1 中被称为“菱形切割区”(RCR)的切割疏水区中的破环氨基酸。即使是通常不会被 Pcp1 加工的内膜蛋白的跨膜片段,当它们被置于 Mgm1 的真实 RCR 位置时,也变得可切割。我们进一步表明,位于 RCR 羧基末端的一个高度带负电荷区域的突变改变导致了强烈的加工缺陷。此外,我们表明,线粒体菱形蛋白酶切割 Mgm1 所需的决定因素在进化过程中是保守的,因为 PARL(Pcp1 的人类同源物)表现出类似的底物需求。这些结果表明,线粒体菱形蛋白酶对切割疏水区序列的要求具有惊人的混杂性。我们提出了一个工作假设,即线粒体菱形蛋白酶如何在这种混杂性的情况下,实现对 Mgm1 的高特异性识别。这个假设与 Mgm1 特殊的生物发生途径有关。

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