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Two high-throughput screening assays for aberrant RNA–protein interactions in myotonic dystrophy type 1

机译:两种高通量筛选测定法用于1型肌强直性营养不良中异常RNA-蛋白质相互作用

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Myotonic dystrophy type 1 (DM1), the most prevalent form of adult muscular dystrophy, is caused by expansion of a CTG repeat in the 3′ untranslated region of the DM protein kinase (DMPK) gene. The pathogenic effects of the CTG expansion arise from the deleterious effects of the mutant transcript. RNA with expanded CUG tracts alters the activities of several RNA binding proteins, including muscleblind-like 1 (MBNL1). MBNL1 becomes sequestered in nuclear foci in complex with the expanded CUG-repeat RNA. The resulting loss of MBNL1 activity causes misregulated alternative splicing of multiple genes, leading to symptoms of DM1. The binding interaction between MBNL1 and mutant RNA could be a key step in the pathogenesis of DM1 and serves as a potential target for therapeutic intervention. We have developed two high-throughput screens suitable assays using both homogenous time-resolved fluorescence energy transfer and AlphaScreen technologies to detect the binding of a C-terminally His-tagged MBNL1 and a biotinylated (CUG)12 RNA. These assays are homogenous and successfully miniaturized to 1,536-well plate format. Both assays were validated and show robust signal-to-basal ratios and Z′ factors.
机译:成年型肌营养不良症最普遍的形式是强直性肌营养不良1型(DM1),是由DM蛋白激酶(DMPK)基因3'非翻译区CTG重复序列的扩增引起的。 CTG扩展的致病作用来自突变体转录本的有害作用。具有扩展的CUG的RNA改变了几种RNA结合蛋白的活性,包括肌盲样1(MBNL1)。 MBNL1与扩展的CUG重复RNA形成复合体,被隔离在核灶中。结果导致MBNL1活性丧失导致多个基因的可变剪接错误调节,从而导致DM1症状。 MBNL1和突变RNA之间的结合相互作用可能是DM1发病机理中的关键步骤,并可能成为治疗干预的潜在靶标。我们已经开发出两种适用于均相时间分辨荧光能量转移和AlphaScreen技术的高通量筛选合适的检测方法,用于检测C末端带有His标签的MBNL1和生物素化(CUG) 12 RNA的结合。这些测定是同质的,并且成功地小型化为1,536孔板形式。两种测定方法均得到验证,并显示出稳健的信噪比和Z'因子。

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