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S-AKAP84的特性研究,一种新的雄性生殖细胞中受发育调控的A激酶锚定蛋白。

Characterization of S-AKAP84, a novel developmentally regulated A kinase anchor protein of male germ cells.

作者信息

Lin R Y, Moss S B, Rubin C S

机构信息

Department of Molecular Pharmacology, Atran Laboratories, Albert Einstein College of Medicine, Bronx, New York 10461, USA.

出版信息

J Biol Chem. 1995 Nov 17;270(46):27804-11. doi: 10.1074/jbc.270.46.27804.

DOI:10.1074/jbc.270.46.27804
PMID:7499250
Abstract

In mammalian spermatozoa, most of the type II alpha isoform of cAMP-dependent protein kinase (PKAII alpha) is anchored at the cytoplasmic surface of a specialized array of mitochondria in the flagellar cytoskeleton. This places the catalytic subunits of PKAII alpha in proximity with potential target substrates in the cytoskeleton. The mechanism by which PKAII alpha is anchored at the outer surface of germ cell mitochondria has not been elucidated. We now report the cloning of a cDNA that encodes a novel, germ cell A kinase anchor protein (AKAP) designated S-AKAP84. S-AKAP84 comprises 593 amino acids and contains a centrally located domain that avidly binds regulatory subunits (RII alpha and RII beta) of PKAII alpha and PKAII beta. The 3.2-kilobase S-AKAP84 mRNA and the cognate S-AKAP84 RII binding protein are expressed principally in the male germ cell lineage. Expression of S-AKAP84 is tightly regulated during development. The protein accumulates as spermatids undergo nuclear condensation and tail elongation. The timing of S-AKAP84 expression is correlated with the de novo accumulation of RII alpha and RII beta subunits and the migration of mitochondria from the cytoplasm (round spermatids) to the cytoskeleton (midpiece in elongating spermatids). Residues 1-30 at the NH2 terminus of S-AKAP84 constitute a putative signal/anchor sequence that may target the protein to the outer mitochondrial membrane. Immunofluorescence analysis demonstrated that S-AKAP84 is co-localized with mitochondria in the flagellum.

摘要

在哺乳动物精子中,大多数环磷酸腺苷依赖性蛋白激酶II型α亚型(PKAIIα)锚定在鞭毛细胞骨架中一组特殊线粒体的细胞质表面。这使得PKAIIα的催化亚基与细胞骨架中的潜在靶底物接近。PKAIIα锚定在生殖细胞线粒体外表面的机制尚未阐明。我们现在报告克隆了一种编码新型生殖细胞A激酶锚定蛋白(AKAP)的cDNA,命名为S-AKAP84。S-AKAP84由593个氨基酸组成,包含一个位于中央的结构域,该结构域能强烈结合PKAIIα和PKAIIβ的调节亚基(RIIα和RIIβ)。3.2千碱基的S-AKAP84 mRNA和同源的S-AKAP84 RII结合蛋白主要在雄性生殖细胞谱系中表达。S-AKAP84的表达在发育过程中受到严格调控。随着精子细胞经历核浓缩和尾部伸长,该蛋白会积累。S-AKAP84表达的时间与RIIα和RIIβ亚基的从头积累以及线粒体从细胞质(圆形精子细胞)向细胞骨架(伸长精子细胞的中段)的迁移相关。S-AKAP84氨基末端的1-30位残基构成一个假定的信号/锚定序列,可能将该蛋白靶向线粒体外膜。免疫荧光分析表明,S-AKAP84与鞭毛中的线粒体共定位。

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