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Specific RNP capture with antisense LNA /DNA mixmers

机译:用反义LNA捕获特异性RNP / DNA混合器

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摘要

RNA-binding proteins (RBPs) play essential roles in RNA biology, responding to cellular and environmental stimuli to regulate gene expression. Important advances have helped to determine the (near) complete repertoires of cellular RBPs. However, identification of RBPs associated with specific transcripts remains a challenge. Here, we describe “specific ribonucleoprotein (RNP) capture”, a versatile method for the determination of the proteins bound to specific transcripts in vitro and in cellular systems. Specific RNP capture employs UV irradiation to covalently stabilize protein-RNA interactions taking place at “zero distance”. Proteins bound to the target RNA are captured by hybridization with antisense Locked Nucleic Acid (LNA)/DNA oligonucleotides covalently coupled to a magnetic resin. After stringent washing, interacting proteins are identified by quantitative mass spectrometry. Applied to in vitro extracts, specific RNP capture identifies the RBPs bound to a reporter mRNA containing the sex-lethal (Sxl) binding motifs, revealing that the Sxl homologue Sister of Sex lethal (Ssx) displays similar binding preferences. This method also revealed the repertoire of RBPs binding to 18S or 28S rRNAs in HeLa cells, including previously unknown rRNA-binding proteins.
机译:RNA结合蛋白(RBP)在RNA生物学中起着至关重要的作用,对细胞和环境刺激作出反应以调节基因表达。重要的进步有助于确定(几乎)完整的细胞RBP组成。然而,鉴定与特定转录本相关的RBP仍然是一个挑战。在这里,我们描述了“特异性核糖核蛋白(RNP)捕获”,这是一种用于确定在体外和在细胞系统中与特定转录本结合的蛋白质的通用方法。特定的RNP捕获使用紫外线辐射来共价稳定发生在“零距离”处的蛋白质-RNA相互作用。通过与与磁性树脂共价偶联的反义锁核酸(LNA)/ DNA寡核苷酸杂交来捕获与靶RNA结合的蛋白质。严格洗涤后,通过定量质谱鉴定相互作用的蛋白质。应用于体外提取物时,特定的RNP捕获可识别与包含性致死(Sxl)结合基序的报告基因mRNA结合的RBP,这表明Sxl致死性同胞姐妹(Ssx)显示出相似的结合偏好。该方法还揭示了与HeLa细胞中18S或28S rRNA结合的RBP的组成,包括以前未知的rRNA结合蛋白。

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