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参与前体mRNA剪接的裂殖酵母Prp4蛋白激酶的功能分析及一种假定的哺乳动物同源物的分离。

Functional analysis of the fission yeast Prp4 protein kinase involved in pre-mRNA splicing and isolation of a putative mammalian homologue.

作者信息

Gross T, Lützelberger M, Weigmann H, Klingenhoff A, Shenoy S, Käufer N F

机构信息

Institüt für Genetik-Biozentrum, Technische Universität Braunschweig, Spielmannstrasse 7, D-38106 Braunschweig, Germany.

出版信息

Nucleic Acids Res. 1997 Mar 1;25(5):1028-35. doi: 10.1093/nar/25.5.1028.

Abstract

The prp4 gene of Schizosaccharomyces pombe encodes a protein kinase. A physiological substrate is not yet known. A mutational analysis of prp4 revealed that the protein consists of a short N-terminal domain, containing several essential motifs, which is followed by the kinase catalytic domain comprising the C-terminus of the protein. Overexpression of N-terminal mutations disturbs mitosis and produces elongated cells, Using a PCR approach, we isolated a putative homologue of Prp4 from human and mouse cells. The mammalian kinase domain is 53% identical to the kinase domain of Prp4. The short N-terminal domains share <20% identical amino acids, but contain conserved motifs. A fusion protein consisting of the N-terminal region from S. pombe followed by the mammalian kinase domain complements a temperature-sensitive prp4 mutation of S. pombe. Prp4 and the recombinant yeast/mouse protein kinase phosphorylate the human SR splicing factor ASF/SF2 in vitro in its RS domain.

摘要

粟酒裂殖酵母的prp4基因编码一种蛋白激酶。其生理底物尚不清楚。对prp4的突变分析表明,该蛋白由一个短的N端结构域组成,包含几个必需基序,随后是包含蛋白C端的激酶催化结构域。N端突变的过表达会干扰有丝分裂并产生细长细胞。利用PCR方法,我们从人和小鼠细胞中分离出了一个假定的Prp4同源物。哺乳动物的激酶结构域与Prp4的激酶结构域有53%的同一性。短的N端结构域的氨基酸同一性小于20%,但含有保守基序。由粟酒裂殖酵母的N端区域和哺乳动物激酶结构域组成的融合蛋白可互补粟酒裂殖酵母的温度敏感型prp4突变。Prp4和重组酵母/小鼠蛋白激酶在体外可使其RS结构域中的人SR剪接因子ASF/SF2磷酸化。

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