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首页> 外文期刊>Nucleic acids research >Two-step model of stop codon recognition by eukaryotic release factor eRF1
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Two-step model of stop codon recognition by eukaryotic release factor eRF1

机译:真核释放因子eRF1识别终止密码子的两步模型

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摘要

Release factor eRF1 plays a key role in the termination of protein synthesis in eukaryotes. The eRF1 consists of three domains (N, M and C) that perform unique roles in termination. Previous studies of eRF1 point mutants and standard/variant code eRF1 chimeras unequivocally demonstrated a direct involvement of the highly conserved N-domain motifs (NIKS, YxCxxxF and GTx) in stop codon recognition. In the current study, we extend this work by investigating the role of the 41 invariant and conserved N-domain residues in stop codon decoding by human eRF1. Using a combination of the conservative and non-conservative amino acid substitutions, we measured the functional activity of 80 mutant eRF1s in an in vitro reconstituted eukaryotic translation system and selected 15 amino acid residues essential for recognition of different stop codon nucleotides. Furthermore, toe-print analyses provide evidence of a conformational rearrangement of ribosomal complexes that occurs during binding of eRF1 to messenger RNA and reflects stop codon decoding activity of eRF1. Based on our experimental data and molecular modelling of the N-domain at the ribosomal A site, we propose a two-step model of stop codon decoding in the eukaryotic ribosome.
机译:释放因子eRF1在终止真核生物蛋白质合成中起关键作用。 eRF1由三个域(N,M和C)组成,它们在终结处理中发挥独特的作用。先前对eRF1点突变体和标准/变异代码eRF1嵌合体的研究明确表明,高度保守的N域基序(NIKS,YxCxxxF和GTx)直接参与了终止密码子的识别。在当前的研究中,我们通过研究41个不变和保守的N域残基在人类eRF1终止密码子解码中的作用来扩展这项工作。使用保守和非保守氨基酸取代的组合,我们在体外重构的真核翻译系统中测量了> 80个突变eRF1的功能活性,并选择了15个对不同终止密码子核苷酸的识别必不可少的氨基酸残基。此外,脚印分析提供了核糖体复合物构象重排的证据,该构象重排发生在eRF1与信使RNA结合期间,并反映了eRF1的终止密码子解码活性。基于我们的实验数据和核糖体A位点N域的分子模型,我们提出了一个两步模型,用于真核生物核糖体中的终止密码子解码。

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