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真核起始因子2激酶GCN2的核糖体结合结构域促进翻译控制。

Ribosome-binding domain of eukaryotic initiation factor-2 kinase GCN2 facilitates translation control.

作者信息

Zhu S, Wek R C

机构信息

Department of Biochemistry and Molecular Biology, Indiana University School of Medicine, Indianapolis 46202-5122, USA.

出版信息

J Biol Chem. 1998 Jan 16;273(3):1808-14. doi: 10.1074/jbc.273.3.1808.

DOI:10.1074/jbc.273.3.1808
PMID:9430731
Abstract

A family of protein kinases regulate translation initiation in response to cellular stresses by phosphorylation of eukaryotic initiation factor-2 (eIF-2). One family member from yeast, GCN2, contains a region homologous to histidyl-tRNA synthetases juxtaposed to the kinase catalytic domain. It is thought that uncharged tRNA accumulating during amino acid starvation binds to the synthetase-related sequences and stimulates phosphorylation of the alpha subunit of eIF-2. In this report, we define another domain in GCN2 that functions to target the kinase to ribosomes. A truncated version of GCN2 containing only amino acid residues 1467 to 1590 can independently associate with the translational machinery. Interestingly, this region of GCN2 shares sequence similarities with the core of the double-stranded RNA-binding domain (DRBD). Substitutions of the lysine residues conserved among DRBD sequences block association of GCN2 with ribosomes and impaired the ability of the kinase to stimulate translational control in response to amino acid limitation. Additionally, as found for other DRBD sequences, recombinant protein containing GCN2 residues 1467-1590 can bind double-stranded RNA in vitro, suggesting that interaction with rRNA mediates ribosome targeting. These results indicate that appropriate ribosome localization of the kinase is an obligate step in the mechanism leading to translational control by GCN2.

摘要

一类蛋白激酶通过真核起始因子-2(eIF-2)的磷酸化来响应细胞应激,从而调节翻译起始。酵母中的一个家族成员GCN2,在其激酶催化结构域旁含有一个与组氨酰-tRNA合成酶同源的区域。据认为,在氨基酸饥饿期间积累的无电荷tRNA与合成酶相关序列结合,并刺激eIF-2α亚基的磷酸化。在本报告中,我们在GCN2中定义了另一个结构域,该结构域的功能是将激酶靶向核糖体。仅包含氨基酸残基1467至1590的GCN2截短版本可以独立地与翻译机制结合。有趣的是,GCN2的这一区域与双链RNA结合结构域(DRBD)的核心具有序列相似性。DRBD序列中保守的赖氨酸残基的替换会阻止GCN2与核糖体的结合,并损害激酶响应氨基酸限制刺激翻译控制的能力。此外,正如在其他DRBD序列中所发现的,含有GCN2残基1467 - 1590的重组蛋白在体外可以结合双链RNA,这表明与rRNA的相互作用介导了核糖体靶向。这些结果表明,激酶在核糖体上的适当定位是GCN2导致翻译控制机制中的一个必要步骤。

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