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Trans-complementation of the second step of pre-mRNA splicing by exogenous 5' exons.

机译:前mRNA剪接的第二步通过外源5'外显子进行反式互补。

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摘要

During splicing of nuclear pre-mRNAs, the first step liberates the 5' exon (exon 1) and yields a lariat intron-3'exon (intron-exon 2) intermediate. The second step results in exon ligation. Previous results indicated that severe truncations of the 5' exon of the actin pre-mRNA result in a block to the second splicing step in vitro in yeast extracts, leading to an accumulation of intron-exon 2 lariat intermediates. We show that exogenous exon 1 RNA oligonucleotides can chase these stalled intermediates into lariat intron and spliced exons. This reaction requires some of the cis elements and trans-acting factors that are required for a normal second step. There is no strong sequence requirement for the exon 1 added in trans, but oligonucleotides with complementarity to the U5 snRNA conserved loop perform the chase more efficiently. Using a dominant negative mutant of the DEAH-box ATPase Prp16p and ATP depletion, we show that the stalled intermediate is blocked after the Prp16p-dependent step. These results show that exogenous RNAs with various sequences but containing no splicing signals can be incorporated into spliceosomes and undergo RNA recombination and exon shuffling during the second step of pre-mRNA splicing.
机译:在核前mRNA的剪接过程中,第一步是释放5'外显子(外显子1)并产生套索内含子3'外显子(内含子外显子2)中间体。第二步导致外显子结扎。先前的结果表明,肌动蛋白前mRNA的5'外显子的严重截断导致酵母提取物中体外第二个剪接步骤受阻,从而导致内含子-外显子2套索中间体的积累。我们显示外源外显子1 RNA寡核苷酸可以追逐这些停滞的中间体成套索内含子和剪接的外显子。该反应需要正常第二步所需的一些顺式元素和反式作用因子。反式添加的外显子1不需要很强的序列要求,但是与U5 snRNA保守环互补的寡核苷酸可以更有效地执行追踪。使用DEAH框ATPase Prp16p和ATP耗竭的显性负突变体,我们表明,失速的中间体在Prp16p依赖性步骤后被阻断。这些结果表明,具有各种序列但不包含剪接信号的外源RNA可以掺入剪接体中,并在mRNA预剪接的第二步中进行RNA重组和外显子改组。

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