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人类端粒酶RNA与蛋白质的相互作用。

Human telomerase RNA-protein interactions.

作者信息

Bachand F, Triki I, Autexier C

机构信息

Department of Anatomy and Cell Biology, McGill University, Montreal, Quebec H3A 2B2, Canada.

出版信息

Nucleic Acids Res. 2001 Aug 15;29(16):3385-93. doi: 10.1093/nar/29.16.3385.

Abstract

Telomere length is maintained in most eukaryotic cells by telomerase. The core components of this ribonucleoprotein (RNP) enzyme include a protein catalytic subunit, composed of motifs conserved among reverse transcriptases (RT), and an RNA subunit that contains a short template sequence essential for the synthesis of telomeric repeats. We developed an electrophoretic mobility shift assay using active telomerase partially purified from 293 cells and radiolabeled, in vitro-transcribed human telomerase RNA (hTR) to investigate the molecular interactions of the human telomerase RT (hTERT) and telomerase-associated proteins with hTR. A specific hTR-protein complex was identified and shown to contain hTERT and human Staufen by antibody supershift assays. Variants of hTR altered in distinct structural elements were analyzed for their ability to competitively inhibit complex formation. Human telomerase RNAs lacking the CR4-CR5 domain were poor inhibitors of hTR-protein complex formation, suggesting that the CR4-CR5 domain of hTR is a potential protein-binding site. Furthermore, alterations in the telomerase RNA pseudoknot's P3 helix, the CR7 domain, or the H/ACA box efficiently inhibited formation of the complex, indicating that these domains are dispensable for the assembly of a telomerase RNP in vitro. Potential telomerase-associated proteins that bind hTR were also identified using a UV cross-linking assay.

摘要

在大多数真核细胞中,端粒长度由端粒酶维持。这种核糖核蛋白(RNP)酶的核心成分包括一个蛋白质催化亚基,该亚基由逆转录酶(RT)中保守的基序组成,以及一个RNA亚基,其包含合成端粒重复序列所必需的短模板序列。我们开发了一种电泳迁移率变动分析方法,使用从293细胞中部分纯化的活性端粒酶和放射性标记的体外转录人端粒酶RNA(hTR),来研究人端粒酶逆转录酶(hTERT)和端粒酶相关蛋白与hTR的分子相互作用。通过抗体超迁移分析鉴定出一种特定的hTR-蛋白质复合物,并显示其包含hTERT和人Staufen。分析了在不同结构元件中发生改变的hTR变体竞争性抑制复合物形成的能力。缺乏CR4-CR5结构域的人端粒酶RNA对hTR-蛋白质复合物形成的抑制作用较弱,这表明hTR的CR4-CR5结构域是一个潜在的蛋白质结合位点。此外,端粒酶RNA假结的P3螺旋、CR7结构域或H/ACA框的改变有效地抑制了复合物的形成,表明这些结构域对于体外端粒酶RNP的组装并非必需。还使用紫外线交联分析鉴定了与hTR结合的潜在端粒酶相关蛋白。

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