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催化亚基的整合在体内激活去泛素化酶活性,这是真菌COP9信号体组装的最后一步。

Integration of the catalytic subunit activates deneddylase activity in vivo as final step in fungal COP9 signalosome assembly.

作者信息

Beckmann Elena A, Köhler Anna M, Meister Cindy, Christmann Martin, Draht Oliver W, Rakebrandt Nikolas, Valerius Oliver, Braus Gerhard H

机构信息

Institut für Mikrobiologie und Genetik, Georg-August Universität Göttingen, Grisebachstrasse 8, D-37077, Göttingen, Germany.

出版信息

Mol Microbiol. 2015 Jul;97(1):110-24. doi: 10.1111/mmi.13017. Epub 2015 Apr 23.

DOI:10.1111/mmi.13017
PMID:25846252
Abstract

The eight-subunit COP9 signalosome (CSN) is conserved from filamentous fungi to humans and functions at the interface between cellular signalling and protein half-life control. CSN consists of six PCI and two MPN domain proteins and forms a scaffold for additional interacting proteins. CSN controls protein stability in the ubiquitin-proteasome system where the MPN domain CSN5/CsnE subunit inactivates cullin-RING ligases. The CSN5/CsnE isopeptidase functions as deneddylase and removes the ubiquitin-like protein Nedd8. The six PCI domain proteins of human CSN form a horseshoe-like ring and all eight subunits are connected by a bundle of C-terminal α-helices. We show that single deletions of any csn subunit of Aspergillus nidulans resulted in the lack of deneddylase activity and identical defects in the coordination of development and secondary metabolism. The CSN1/CsnA N-terminus is dispensable for deneddylase activity but required for asexual spore formation. Complex analyses in mutant strains revealed the presence of a seven-subunit pre-CSN without catalytic activity. Reconstitution experiments with crude extracts of deletion strains and recombinant proteins allowed the integration of CSN5/CsnE into pre-CSN resulting in an active deneddylase. This supports a stable seven subunit pre-CSN intermediate where deneddylase activation in vivo can be controlled by CSN5/CsnE integration as final assembly step.

摘要

由八个亚基组成的COP9信号体(CSN)从丝状真菌到人类都保守存在,且在细胞信号传导与蛋白质半衰期控制的界面发挥作用。CSN由六个PCI结构域蛋白和两个MPN结构域蛋白组成,并为其他相互作用蛋白形成一个支架。CSN在泛素-蛋白酶体系统中控制蛋白质稳定性,其中MPN结构域的CSN5/CsnE亚基会使Cullin-RING连接酶失活。CSN5/CsnE异肽酶作为去泛素化酶发挥作用,去除类泛素蛋白Nedd8。人类CSN的六个PCI结构域蛋白形成一个马蹄形环,所有八个亚基通过一束C末端α螺旋相连。我们发现,构巢曲霉的任何一个csn亚基的单基因缺失都会导致去泛素化酶活性缺失,以及在发育和次级代谢协调方面出现相同的缺陷。CSN1/CsnA的N末端对于去泛素化酶活性是可有可无的,但对于无性孢子形成是必需的。对突变菌株的复合物分析揭示了存在一种无催化活性的七亚基前体CSN。用缺失菌株的粗提物和重组蛋白进行的重组实验使得CSN5/CsnE能够整合到前体CSN中,从而产生一种有活性的去泛素化酶。这支持了一种稳定的七亚基前体CSN中间体,其中体内去泛素化酶的激活可以通过CSN5/CsnE作为最终组装步骤的整合来控制。

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