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线粒体转录终止因子2(MTERF2)是哺乳动物线粒体中的一种类核成分。

MTERF2 is a nucleoid component in mammalian mitochondria.

作者信息

Pellegrini Mina, Asin-Cayuela Jorge, Erdjument-Bromage Hediye, Tempst Paul, Larsson Nils-Goran, Gustafsson Claes M

机构信息

Division of Metabolic Diseases, Karolinska Institutet, SE-141 86 Stockholm, Sweden.

出版信息

Biochim Biophys Acta. 2009 May;1787(5):296-302. doi: 10.1016/j.bbabio.2009.01.018. Epub 2009 Feb 3.

DOI:10.1016/j.bbabio.2009.01.018
PMID:19366608
Abstract

The mammalian MTERF family of proteins has four members, named MTERF1 to MTERF4, which were identified in homology searches using the mitochondrial transcription termination factor, mTERF (here denoted MTERF1) as query. MTERF1 and MTERF3 are known to participate in the control of mitochondrial DNA transcription, but the function of the other two proteins is not known. We here investigate the structure and function of MTERF2. Protein import experiments using isolated organelles confirm that MTERF2 is a mitochondrial protein. Edman degradation of MTERF2 isolated from stably transfected HeLa cells demonstrates that mature MTERF2 lacks a targeting peptide (amino acids 1-35) present in the precursor form of the protein. MTERF2 is a monomer in isolation and displays a non sequence-specific DNA-binding activity. In vivo quantification experiments demonstrate that MTERF2 is relatively abundant, with one monomer present per approximately 265 bp of mtDNA. In comparison, the mtDNA packaging factor TFAM is present at a ratio of one molecule per approximately 10-12 bp of mtDNA. Using formaldehyde cross-linking we demonstrate that MTERF2 is present in nucleoids, and therefore must be located in close proximity to mtDNA. Taken together, our work provides a basic biochemical characterization of MTERF2, paving the way for future functional studies.

摘要

哺乳动物的MTERF蛋白家族有四个成员,分别命名为MTERF1至MTERF4,它们是在以线粒体转录终止因子mTERF(此处表示为MTERF1)为查询序列的同源性搜索中鉴定出来的。已知MTERF1和MTERF3参与线粒体DNA转录的调控,但其他两种蛋白的功能尚不清楚。我们在此研究MTERF2的结构与功能。使用分离细胞器进行的蛋白质导入实验证实MTERF2是一种线粒体蛋白。对从稳定转染的HeLa细胞中分离出的MTERF2进行的埃德曼降解表明,成熟的MTERF2缺乏蛋白前体形式中存在的靶向肽(氨基酸1 - 35)。MTERF2单独存在时为单体,并表现出非序列特异性的DNA结合活性。体内定量实验表明,MTERF2相对丰富,每约265 bp的线粒体DNA存在一个单体。相比之下,线粒体DNA包装因子TFAM的存在比例为每约10 - 12 bp的线粒体DNA有一个分子。使用甲醛交联我们证明MTERF2存在于类核中,因此必定定位在线粒体DNA附近。综上所述,我们的工作提供了MTERF2的基本生化特征,为未来的功能研究铺平了道路。

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