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An Alu-derived intronic splicing enhancer facilitates intronic processing and modulates aberrant splicing in ATM

机译:源自Alu的内含子拼接增强剂有助于内含子处理并调节ATM中的异常拼接

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摘要

We have previously reported a natural GTAA deletion within an intronic splicing processing element (ISPE) of the ataxia telangiectasia mutated (ATM) gene that disrupts a non-canonical U1 snRNP interaction and activates the excision of the upstream portion of the intron. The resulting pre-mRNA splicing intermediate is then processed to a cryptic exon, whose aberrant inclusion in the final mRNA is responsible for ataxia telangiectasia. We show here that the last 40 bases of a downstream intronic antisense Alu repeat are required for the activation of the cryptic exon by the ISPE deletion. Evaluation of the pre-mRNA splicing intermediate by a hybrid minigene assay indicates that the identified intronic splicing enhancer represents a novel class of enhancers that facilitates processing of splicing intermediates possibly by recruiting U1 snRNP to defective donor sites. In the absence of this element, the splicing intermediate accumulates and is not further processed to generate the cryptic exon. Our results indicate that Alu-derived sequences can provide intronic splicing regulatory elements that facilitate pre-mRNA processing and potentially affect the severity of disease-causing splicing mutations.
机译:我们以前已经报告了共济失调毛细血管扩张突变(ATM)基因的内含子剪接加工元件(ISPE)中的自然GTAA缺失,该基因破坏了非典型的U1 snRNP相互作用并激活了内含子上游部分的切除。然后将所得的前mRNA剪接中间体加工成隐性外显子,其最终mRNA中的异常内含导致毛细血管扩张性共济失调。我们在这里显示,下游内含子反义Alu重复序列的最后40个碱基是通过ISPE缺失激活外显子所必需的。通过杂交小基因测定对前mRNA剪接中间体的评估表明,鉴定出的内含子剪接增强子代表了一类新型的增强子,可能通过将U1 snRNP募集到有缺陷的供体位点来促进剪接中间体的加工。在缺少该元素的情况下,剪接中间体会积累,不会进一步处理以生成隐秘外显子。我们的结果表明,Alu衍生的序列可以提供内含子剪接调控元件,从而促进mRNA预处理,并可能影响致病性剪接突变的严重性。

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