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剪接失调是亨廷顿病中 RNA 诱导毒性的主要机制。

Deregulated Splicing Is a Major Mechanism of RNA-Induced Toxicity in Huntington's Disease.

机构信息

German Center for Neurodegenerative Diseases (DZNE), 53127, Bonn, North Rhine-Westphalia, Germany.

Max Planck Institute for Biology of Ageing, 50931 Cologne, North Rhine-Westphalia, Germany.

出版信息

J Mol Biol. 2019 Apr 19;431(9):1869-1877. doi: 10.1016/j.jmb.2019.01.034. Epub 2019 Jan 31.

Abstract

Huntington's disease (HD) is caused by an expanded CAG repeat in the huntingtin (HTT) gene, translating into an elongated polyglutamine stretch. In addition to the neurotoxic mutant HTT protein, the mutant CAG repeat RNA can exert toxic functions by trapping RNA-binding proteins. While few examples of proteins that aberrantly bind to mutant HTT RNA and execute abnormal function in conjunction with the CAG repeat RNA have been described, an unbiased approach to identify the interactome of mutant HTT RNA is missing. Here, we describe the analysis of proteins that preferentially bind mutant HTT RNA using a mass spectrometry approach. We show that (I) the majority of proteins captured by mutant HTT RNA belong to the spliceosome pathway, (II) expression of mutant CAG repeat RNA induces mis-splicing in a HD cell model, (III) overexpression of one of the splice factors trapped by mutant HTT ameliorates the HD phenotype in a fly model and (VI) deregulated splicing occurs in human HD brain. Our data suggest that deregulated splicing is a prominent mechanism of RNA-induced toxicity in HD.

摘要

亨廷顿病(HD)是由亨廷顿(HTT)基因中 CAG 重复序列的扩展引起的,导致多聚谷氨酰胺延伸。除了神经毒性突变 HTT 蛋白外,突变的 CAG 重复 RNA 还可以通过捕获 RNA 结合蛋白来发挥毒性作用。虽然已经描述了少数与 CAG 重复 RNA 异常结合并执行异常功能的异常结合突变 HTT RNA 的蛋白质的例子,但识别突变 HTT RNA 相互作用组的无偏方法仍然缺失。在这里,我们描述了使用质谱方法分析优先结合突变 HTT RNA 的蛋白质的分析。我们表明:(I)突变 HTT RNA 捕获的大多数蛋白质都属于剪接体途径,(II)突变 CAG 重复 RNA 的表达在 HD 细胞模型中诱导了错误剪接,(III)突变 HTT 捕获的剪接因子之一的过表达改善了在蝇模型中的 HD 表型,以及(VI)人类 HD 大脑中存在失调的剪接。我们的数据表明,剪接失调是 HD 中 RNA 诱导毒性的主要机制。

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