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Intracellular folding of the Tetrahymena group I intron depends on exon sequence and promoter choice.

机译:四膜虫群I内含子的细胞内折叠取决于外显子序列和启动子选择。

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摘要

The Tetrahymena group I intron splices 20 to 50 times faster in Tetrahymena than in vitro, implying that the intron rapidly adopts its active conformation in the cell. The importance of cotranscriptional folding and the contribution of the rRNA exons to the stability of the active pre-RNA structure were investigated by comparing the activity of minimal pre-RNAs expressed in Escherichia coli. Pre-RNAs containing exons derived from E. coli 23 S rRNA were three to four times more active than the wild-type Tetrahymena pre-RNA. E. coli transcripts of the chimeric E. coli pre-RNA were two to eight times more active than were T7 transcripts. However, the effect of cotranscriptional folding depends on exon sequences. Unexpectedly, the unspliced pre-RNA decays more slowly than predicted from the rate of splicing. This observation is best explained by partitioning of transcripts into active and inactive pools. We propose that the active pool splices within a few seconds, whereas the inactive pool is degraded without appreciable splicing.
机译:四膜虫的第I组内含子在四膜虫中的剪接速度比体外快20至50倍,这意味着该内含子在细胞中迅速采用了其活性构象。通过比较在大肠杆菌中表达的最小pre-RNA的活性,研究了共转录折叠的重要性以及rRNA外显子对活性pre-RNA结构稳定性的贡献。含有源自大肠杆菌23 S rRNA的外显子的前RNA活性比野生型四膜虫前RNA活性高三到四倍。嵌合大肠杆菌pre-RNA的大肠杆菌转录物的活性是T7转录物的2至8倍。但是,共转录折叠的效果取决于外显子序列。出乎意料的是,未剪接的pre-RNA的衰减比剪接速度所预测的要慢。通过将转录本划分为活动和非活动池,可以最好地解释此观察结果。我们建议活动池在几秒钟内进行拼接,而不活动池在没有明显拼接的情况下会降级。

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