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A viral RNA motif involved in signaling the initiation of translation on non-AUG codons

机译:涉及在非八卦密码子上发出翻译的病毒RNA基序

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Noncanonical translation, and particularly initiation on non-AUG codons, are frequently used by viral and cellular mRNAs during virus infection and disease. The Sindbis virus (SINV) subgenomic mRNA (sgRNA) constitutes a unique model system to analyze the translation of a capped viral mRNA without the participation of several initiation factors. Moreover, sgRNA can initiate translation even when the AUG initiation codon is replaced by other codons. Using SINV replicons, we examined the efficacy of different codons in place of AUG to direct the synthesis of the SINV capsid protein. The substitution of AUGby CUG was particularly efficient in promoting the incorporation of leucine or methionine in similar percentages at the amino terminus of the capsid protein. Additionally, valine could initiate translation when the AUG is replaced by GUG. The ability of sgRNA to initiate translation on non-AUG codons was dependent on the integrity of a downstream stable hairpin (DSH) structure located in the coding region. The structural requirements of this hairpin to signal the initiation site on the sgRNA were examined in detail. Of interest, a virus bearing CUG in place of AUG in the sgRNA was able to infect cells and synthesize significant amounts of capsid protein. This virus infects the human haploid cell line HAP1 and the double knockout variant that lacks eIF2A and eIF2D. Collectively, these findings indicate that leucine-tRNA or valine-tRNA can participate in the initiation of translation of sgRNA by a mechanism dependent on the DSH. This mechanism does not involve the action of eIF2, eIF2A, or eIF2D.
机译:在病毒感染和疾病期间,病毒和细胞MRNA经常使用非共同的翻译,特别是对非八卦密码子的引发。 SINDBIS病毒(SINV)亚基组学mRNA(SGRNA)构成一个独特的模型系统,用于分析封端的病毒mRNA的翻译,而不参与几种启动因子。此外,即使在八八次启动密码子被其他密码子取代时,SGRNA也可以启动翻译。使用Sinv复制子,我们检查了不同密码子代替八种八种胶囊蛋白合成的疗效。奥古比·突出的替代在促进衣壳蛋白的氨基末端的类似百分比中促进亮氨酸或蛋氨酸的掺入特别有效。此外,缬氨酸可能会在纽约州代替时启动翻译。 SGRNA在非八卦密码子上发起翻译的能力取决于位于编码区域中的下游稳定发夹(DSH)结构的完整性。详细检查了该发夹的结构要求以发出SGRNA上的起始位点。感兴趣的是,在SGRNA中代替AUG的病毒轴承座射水能够感染细胞并合成大量的衣壳蛋白。该病毒感染人单倍体细胞系HAP1和缺乏EIF2A和EIF2D的双敲除变体。总的来说,这些发现表明亮氨酸-TRNA或缬氨酸-TRNA可以通过依赖于DSH的机制参与SGRNA的翻译。该机制不涉及EIF2,EIF2A或EIF2D的动作。

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