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指导NADH-细胞色素b5还原酶定位于酵母线粒体内两个位置的分选信号分析。

Analysis of the sorting signals directing NADH-cytochrome b5 reductase to two locations within yeast mitochondria.

作者信息

Haucke V, Ocana C S, Hönlinger A, Tokatlidis K, Pfanner N, Schatz G

机构信息

Biozentrum, Department of Biochemistry, University of Basel, Switzerland.

出版信息

Mol Cell Biol. 1997 Jul;17(7):4024-32. doi: 10.1128/MCB.17.7.4024.

Abstract

Mitochondrial NADH-cytochrome b5 reductase (Mcr1p) is encoded by a single nuclear gene and imported into two different submitochondrial compartments: the outer membrane and the intermembrane space. We now show that the amino-terminal 47 amino acids suffice to target the Mcr1 protein to both destinations. The first 12 residues of this sequence function as a weak matrix-targeting signal; the remaining residues are mostly hydrophobic and serve as an intramitochondrial sorting signal for the outer membrane and the intermembrane space. A double point mutation within the hydrophobic region of the targeting sequence virtually abolishes the ability of the precursor to be inserted into the outer membrane but increases the efficiency of transport into the intermembrane space. Import of Mcr1p into the intermembrane space requires an electrochemical potential across the inner membrane, as well as ATP in the matrix, and is strongly impaired in mitochondria lacking Tom7p or Tim11p, two components of the translocation machineries in the outer and inner mitochondrial membranes, respectively. These results indicate that intramitochondrial sorting of the Mcr1 protein is mediated by specific interactions between the bipartite targeting sequence and components of both mitochondrial translocation systems.

摘要

线粒体NADH-细胞色素b5还原酶(Mcr1p)由单个核基因编码,并被导入两个不同的亚线粒体区室:外膜和膜间隙。我们现在表明,氨基末端的47个氨基酸足以将Mcr1蛋白靶向这两个目的地。该序列的前12个残基作为一个较弱的基质靶向信号;其余残基大多是疏水的,并作为外膜和膜间隙的线粒体内分选信号。靶向序列疏水区域内的双点突变几乎消除了前体插入外膜的能力,但提高了转运到膜间隙的效率。Mcr1p导入膜间隙需要跨内膜的电化学势以及基质中的ATP,并且在缺乏Tom7p或Tim11p的线粒体中严重受损,Tom7p和Tim11p分别是线粒体外膜和内膜转运机制的两个组分。这些结果表明,Mcr1蛋白的线粒体内分选是由二分靶向序列与两个线粒体转运系统的组分之间的特异性相互作用介导的。

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