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Dissection of the Carboxyl-Terminal Domain of the Proteasomal Subunit Rpn11 in Maintenance of Mitochondrial Structure and Function

机译:解剖甲基末端域的蛋白酶体亚基RPN11维持线粒体结构和功能

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We have previously demonstrated that the C-terminal part of Rpn11, a deubiquitinating enzyme in the lid of the proteasome, is essential for maintaining a correct cell cycle and normal mitochondrial morphology and function. The two roles are apparently unlinked as the mitochondrial role is mapped to the Carboxy-terminus, whereas the catalytic deubiquitinating activity is found within the N-terminal region. The mitochondrial defects are observed in rpn11-m1 (originally termed mpr1-1 ), a mutation that generates Rpn11 lacking the last 31 amino acids. No mitochondrial phenotypes are recorded for mutations in the MPN+/JAMM motif. In the present study, we investigated the participation of the last 31 amino acids of the Rpn11 protein by analysis of intragenic revertants and site-specific mutants. We identified a putative α-helix necessary for the maintenance of a correct cell cycle and determined that a very short region at the C-terminus of Rpn11 is essential for the maintenance of tubular mitochondrial morphology. Furthermore, we show that expression of the C-terminal part of Rpn11 is able to complement in trans all of the rpn11-m1 mitochondrial phenotypes. Finally, we investigate the mechanisms by which Rpn11 controls the mitochondrial shape and show that Rpn11 may regulate the mitochondrial fission and tubulation processes.
机译:我们之前已经证明,RPN11的C末端部分是蛋白酶盒的盖子中的脱氮酶,对于维持正确的细胞周期和正常线粒体形态和功能是必不可少的。随着线粒体的作用映射到羧基末端,两种角色显然被解释,而催化脱水活性在N-末端区域内发现。在RPN11-M1(最初称为MPR1-1)中观察到线粒体缺陷,该突变产生缺乏最后31个氨基酸的RPN11。在MPN + /堵塞主题中没有被记录线粒体表型。在本研究中,我们通过分析腺体转化剂和特异性特异性突变体来研究RPN11蛋白的最后31种氨基酸的参与。我们鉴定了维护正确细胞周期所需的推定α-螺旋,并确定RPN11的C-末端的非常短的区域对于维持管状线粒体形态是必不可少的。此外,我们表明RPN11的C末端部分的表达能够补充跨越RPN11-M1线粒体表型。最后,我们研究了RPN11控制线粒体形状的机制,并表明RPN11可以调节线粒体裂变和管道过程。

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