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介导真核生物硒蛋白中硒代半胱氨酸共翻译插入的RNA。

RNAs mediating cotranslational insertion of selenocysteine in eukaryotic selenoproteins.

作者信息

Hubert N, Walczak R, Sturchler C, Myslinski E, Schuster C, Westhof E, Carbon P, Krol A

机构信息

UPR 9002 du CNRS, Structure des Macromolécules Biologiques et Mécanismes de Reconnaissance, IBMC, Strasbourg, France.

出版信息

Biochimie. 1996;78(7):590-6. doi: 10.1016/s0300-9084(96)80005-8.

DOI:10.1016/s0300-9084(96)80005-8
PMID:8955902
Abstract

Selenocysteine, a selenium-containing analog of cysteine, is found in the prokaryotic and eukaryotic kingdoms in active sites of enzymes involved in oxidation-reduction reactions. Its biosynthesis and cotranslational insertion into selenoproteins is performed by an outstanding mechanism, implying the participation of several gene products. The tRNA(Sec) is one of these. In eukaryotes, its transcription mode by RNA polymerase III differs from that of classical tRNA genes, both at the level of the promoter elements and transcription factors involved. In addition, enhanced transcription is afforded by a newly characterized zinc finger activator. Not only transcription of the gene, but also the tRNA(Sec) itself is atypical since its 2D and 3D structures exhibit features which set it apart from classical tRNAs. Decoding of eukaryotic selenocysteine UGA codons requires a stem-loop structure in the 3'UTR of mRNAs, the selenocysteine insertion sequence (SECIS) element. Structure probing and sequence comparisons led us to propose a 2D structure model for the SECIS element, containing a novel RNA motif composed of four consecutive non-Watson-Crick base-pairs. A 3D model, rationalizing the accessibility data, was elaborated by computer modeling. It yields indicative or suggestive evidence for the role that could play some conserved residues and/or structural features in SECIS function. These might act as signals for interaction with SBP, the SECIS binding protein that we have characterized.

摘要

硒代半胱氨酸是半胱氨酸的含硒类似物,存在于原核生物和真核生物界中参与氧化还原反应的酶的活性位点。它的生物合成以及共翻译插入硒蛋白是通过一种卓越的机制完成的,这意味着有几种基因产物参与其中。tRNA(Sec)就是其中之一。在真核生物中,它由RNA聚合酶III转录的模式在启动子元件和所涉及的转录因子层面都与经典tRNA基因不同。此外,一种新鉴定的锌指激活剂可增强转录。不仅该基因的转录,而且tRNA(Sec)本身也不典型,因为其二维和三维结构呈现出使其有别于经典tRNA的特征。真核生物硒代半胱氨酸UGA密码子的解码需要mRNA 3'UTR中的一个茎环结构,即硒代半胱氨酸插入序列(SECIS)元件。结构探测和序列比较使我们提出了SECIS元件的二维结构模型,其中包含一个由四个连续的非沃森-克里克碱基对组成的新型RNA基序。通过计算机建模构建了一个三维模型,该模型使可及性数据合理化。它为SECIS功能中一些保守残基和/或结构特征可能发挥的作用提供了指示性或暗示性证据。这些可能作为与我们已鉴定的SECIS结合蛋白SBP相互作用的信号。

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RNAs mediating cotranslational insertion of selenocysteine in eukaryotic selenoproteins.介导真核生物硒蛋白中硒代半胱氨酸共翻译插入的RNA。
Biochimie. 1996;78(7):590-6. doi: 10.1016/s0300-9084(96)80005-8.
2
Solution structure of SECIS, the mRNA element required for eukaryotic selenocysteine insertion--interaction studies with the SECIS-binding protein SBP.真核生物硒代半胱氨酸插入所需的mRNA元件SECIS的溶液结构——与SECIS结合蛋白SBP的相互作用研究
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A novel RNA structural motif in the selenocysteine insertion element of eukaryotic selenoprotein mRNAs.真核生物硒蛋白mRNA的硒代半胱氨酸插入元件中的一种新型RNA结构基序。
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An essential non-Watson-Crick base pair motif in 3'UTR to mediate selenoprotein translation.3'非翻译区中一个介导硒蛋白翻译的重要非沃森-克里克碱基对基序。
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Decoding apparatus for eukaryotic selenocysteine insertion.真核生物硒代半胱氨酸插入的解码装置。
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Characterization of the UGA-recoding and SECIS-binding activities of SECIS-binding protein 2.硒代半胱氨酸插入序列结合蛋白2的UGA重编码及硒代半胱氨酸插入序列结合活性的表征
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