首页> 美国卫生研究院文献>Journal of Virology >The signal for translational readthrough of a UGA codon in Sindbis virus RNA involves a single cytidine residue immediately downstream of the termination codon.
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The signal for translational readthrough of a UGA codon in Sindbis virus RNA involves a single cytidine residue immediately downstream of the termination codon.

机译:Sindbis病毒RNA中UGA密码子的翻译通读信号涉及紧邻终止密码子下游的一个胞苷残基。

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摘要

The nucleotide sequences surrounding termination codons influence the efficiency of translational readthrough. In this report, we examined the sequence requirement for efficient readthrough of the UGA codon in the Sindbis virus genomic RNA which regulates production of the putative viral RNA polymerase, nsP4. The UGA codon and its neighboring nucleotide sequences were subcloned into a heterologous coding context, and readthrough efficiency was measured by cell-free translation of RNA transcripts in rabbit reticulocyte lysates. The CUA codon immediately downstream of the UGA codon was found to be sufficient for efficient translational readthrough. Further mutagenesis of residues in the CUA triplet demonstrated that mutations at the second or third residues following the UGA codon (U and A, respectively) had little effect on readthrough efficiency. In contrast, replacement of the cytidine residue immediately downstream of the UGA codon with any of the other three nucleotides (U, A, or G) dramatically reduced the readthrough efficiency from approximately 10% to less than 1%. These results show that a simple sequence context can allow efficient readthrough of UGA codons in a mammalian translation system. Interestingly, compilation studies of nucleotide sequences surrounding eukaryotic termination codons indicate a strong bias against cytidine residues immediately 3' to UGA termination codons. Taken together with our results, this bias may reflect a selective pressure for efficient translation termination for most eukaryotic gene products.
机译:终止密码子周围的核苷酸序列影响翻译通读的效率。在本报告中,我们研究了在信德比斯病毒基因组RNA中有效阅读UGA密码子的序列要求,该基因调控假定的病毒RNA聚合酶nsP4的产生。将UGA密码子及其邻近核苷酸序列亚克隆到异源编码环境中,并通过兔网织红细胞裂解物中RNA转录物的无细胞翻译来测量通读效率。发现紧邻UGA密码子下游的CUA密码子足以进行有效的翻译通读。 CUA三联体中残基的进一步诱变表明,UGA密码子之后的第二个或第三个残基处的突变(分别为U和A)对通读效率影响很小。相反,用其他三个核苷酸(U,A或G)中的任何一个替换UGA密码子下游紧邻的胞苷残基,会使通读效率从大约10%降低到不足1%。这些结果表明,简单的序列背景可以使哺乳动物翻译系统中的UGA密码子有效地通读。有趣的是,围绕真核终止密码子的核苷酸序列的汇编研究表明,紧靠UGA终止密码子3'端的胞苷残基存在强烈的偏向。结合我们的结果,这种偏见可能反映了大多数真核基因产物有效终止翻译的选择性压力。

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