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首页> 外文期刊>Nucleic Acids Research >Structural analysis of new local features in SECIS RNA hairpins.
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Structural analysis of new local features in SECIS RNA hairpins.

机译:SECIS RNA发夹中新的局部特征的结构分析。

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摘要

Decoding of the UGA selenocysteine codon for selenoprotein translation requires the SECIS element, a stem-loop motif in the 3'-UTR of the mRNA carrying short or large apical loops. In previous structural studies, we derived a secondary structure model for SECIS RNAs with short apical loops. Work from others proposed that intra-apical loop base pairing can occur in those SECIS that possess large apical loops, yielding form 2 SECIS versus the form 1 with short loops. In this work, SECIS elements arising from eight different selenoprotein mRNAs were assayed by enzymatic and/or chemical probing showing that seven can adopt form 2. Further, database searches led to the discovery in drosophila and zebrafish of SECIS elements in the selenophosphate synthetase 2, type 1 deiodinase and SelW mRNAs. Alignment of SECIS sequences not only highlighted the predominance of form 2 but also made it possible to classify the SECIS elements according to the type of selenoprotein mRNA they belong to. Interestingly, the alignment revealed that an unpaired adenine, previously thought to be invariant, is replaced by a guanine in four SECIS elements. Tested in vivo, neither the A to G nor the A to U changes at this position greatly affected the activity while the most detrimental effect was provided by a C. The putative contribution of the various SECIS motifs to function and ligand binding is discussed.
机译:解码UGA硒代半胱氨酸密码子以进行硒蛋白翻译需要SECIS元件,SECIS元件是带有短或大顶端环的mRNA 3'-UTR中的茎环基序。在以前的结构研究中,我们推导了具有短顶环的SECIS RNA的二级结构模型。来自其他研究者的工作提出,在那些具有较大顶环的SECIS中,可以发生顶环内碱基配对,产生的SECIS形式为2,而短环为形式1。在这项工作中,通过酶和/或化学探测分析了八种不同硒蛋白mRNA产生的SECIS元素,显示其中七种可以采用形式2。此外,数据库搜索导致果蝇和斑马鱼在硒磷酸合成酶2中发现了SECIS元素。 1型脱碘酶和SelW mRNA。 SECIS序列的比对不仅突出了形式2的优势,而且使根据其所属的硒蛋白mRNA类型对SECIS元件进行分类成为可能。有趣的是,比对揭示了以前认为是不变的未配对腺嘌呤被四个SECIS元件中的鸟嘌呤所取代。在体内进行测试,在此位置上A到G或A到U的变化都没有极大地影响活性,而C则提供了最有害的作用。讨论了各种SECIS基序对功能和配体结合的推定贡献。

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