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Spliceosome Assembly Pathways for Different Types of Alternative Splicing Converge during Commitment to Splice Site Pairing in the A Complex

机译:不同类型的选择性拼接的拼接体组装途径在致力于复杂复合体中的拼接位点的过程中收敛。

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摘要

Differential splice site pairing establishes alternative splicing patterns resulting in the generation of multiple mRNA isoforms. This process is carried out by the spliceosome, which is activated by a series of sequential structural rearrangements of its five core snRNPs. To determine when splice sites become functionally paired, we carried out a series of kinetic trap experiments using pre-mRNAs that undergo alternative 5′ splice site selection or alternative exon inclusion. We show that commitment to splice site pairing in both cases occurs in the A complex, which is characterized by the ATP-dependent association of the U2 snRNP with the branch point. Interestingly, the timing of splice site pairing is independent of the intron or exon definition modes of splice site recognition. Using the ATP analog ATPγS, we showed that ATP hydrolysis is required for splice site pairing independent from U2 snRNP binding to the pre-mRNA. These results identify the A complex as the spliceosomal assembly step dedicated to splice site pairing and suggest that ATP hydrolysis locks splice sites into a splicing pattern after stable U2 snRNP association to the branch point.
机译:差异剪接位点配对建立了可替代的剪接模式,从而导致产生了多个mRNA同工型。该过程由剪接体进行,该剪接体由其五个核心snRNP的一系列顺序结构重排激活。为了确定剪接位点何时在功能上配对,我们使用pre-mRNA进行了一系列动力学陷阱实验,这些mRNA经历了替代的5'剪接位点选择或替代的外显子包涵。我们表明,在两种情况下对剪接位点配对的承诺均发生在A复合物中,其特征在于U2 snRNP与分支点的ATP依赖关系。有趣的是,剪接位点配对的时间与剪接位点识别的内含子或外显子定义模式无关。使用ATP类似物ATPγS,我们证明了ATP水解是独立于U2 snRNP结合至pre-mRNA的剪接位点配对所必需的。这些结果将A复合物鉴定为专门用于剪接位点配对的剪接体组装步骤,并表明ATP水解在稳定的U2 snRNP结合至分支点后将剪接位点锁定为剪接模式。

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