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rna1p的酸性C末端结构域是Ran.GTP结合和RanGAP活性所必需的。

The acidic C-terminal domain of rna1p is required for the binding of Ran.GTP and for RanGAP activity.

作者信息

Haberland J, Becker J, Gerke V

机构信息

Institute for Medical Biochemistry, University of Münster, Von-Esmarch-Strasse 56, D-48149 Münster, Federal Republic of Germany.

出版信息

J Biol Chem. 1997 Sep 26;272(39):24717-26. doi: 10.1074/jbc.272.39.24717.

DOI:10.1074/jbc.272.39.24717
PMID:9305944
Abstract

The small GTP binding protein Ran is an essential component of the nuclear protein import machinery whose GTPase cycle is regulated by the nuclear guanosine nucleotide exchange factor RCC1 and by the cytosolic GTPase activating protein RanGAP. In the yeasts Schizosaccharomyces pombe and Saccharomyces cerevisiae the RanGAP activity is encoded by the RNA1 genes which are essential for cell viability and nucleocytoplasmic transport in vivo. Although of limited sequence identity the two yeast proteins show a conserved structural organization characterized by an N-terminal domain of eight leucine-rich repeats, motifs implicated in protein-protein interactions, and a C-terminal domain rich in acidic amino acid residues. By analyzing the RanGAP activity of a series of recombinantly expressed rna1p mutant derivatives, we show that the highly acidic sequence in the C-terminal domain of both yeast proteins is indispensable for activating Ran-mediated GTP hydrolysis. Chemical cross-linking reveals that the same sequence in rna1p is required for rna1p.Ran complex formation indicating that the loss of GAP activity in the C-terminally truncated rna1p mutants results from an impaired interaction with Ran. The predominant species stabilized through the covalent cross-link is a rna1p.Ran heterodimer whose formation requires the GTP-bound conformation of Ran. As the acidic C-terminal domain of rna1p is required for establishing the interaction with Ran, the leucine-rich repeats domain in rna1p is potentially available for additional protein interactions perhaps required for directing a fraction of rna1p to the nuclear pore.

摘要

小GTP结合蛋白Ran是核蛋白输入机制的重要组成部分,其GTP酶循环由核鸟苷酸交换因子RCC1和胞质GTP酶激活蛋白RanGAP调节。在粟酒裂殖酵母和酿酒酵母中,RanGAP活性由RNA1基因编码,这些基因对于体内细胞活力和核质运输至关重要。尽管这两种酵母蛋白的序列一致性有限,但它们显示出保守的结构组织,其特征是具有八个富含亮氨酸重复序列的N端结构域、与蛋白质-蛋白质相互作用有关的基序以及富含酸性氨基酸残基的C端结构域。通过分析一系列重组表达的rna1p突变体衍生物的RanGAP活性,我们发现两种酵母蛋白C端结构域中的高酸性序列对于激活Ran介导的GTP水解是必不可少的。化学交联表明,rna1p中相同的序列是rna1p.Ran复合物形成所必需的,这表明C端截短的rna1p突变体中GAP活性的丧失是由于与Ran的相互作用受损所致。通过共价交联稳定的主要物种是rna1p.Ran异二聚体,其形成需要Ran的GTP结合构象。由于rna1p酸性C端结构域是与Ran建立相互作用所必需的,因此rna1p中富含亮氨酸的重复序列结构域可能可用于其他蛋白质相互作用,这可能是将一部分rna1p引导至核孔所必需的。

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