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Co-expression of RNA–protein complexes in Escherichia coli and applications to RNA biology

机译:大肠杆菌中RNA-蛋白质复合物的共表达及其在RNA生物学中的应用

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摘要

RNA has emerged as a major player in many cellular processes. Understanding these processes at the molecular level requires homogeneous RNA samples for structural, biochemical and pharmacological studies. We previously devised a generic approach that allows efficient in vivo expression of recombinant RNA in Escherichia coli. In this work, we have extended this method to RNA/protein co-expression. We have engineered several plasmids that allow overexpression of RNA–protein complexes in E. coli. We have investigated the potential of these tools in many applications, including the production of nuclease-sensitive RNAs encapsulated in viral protein pseudo-particles, the co-production of non-coding RNAs with chaperone proteins, the incorporation of a post-transcriptional RNA modification by co-production with the appropriate modifying enzyme and finally the production and purification of an RNA–His-tagged protein complex by nickel affinity chromatography. We show that this last application easily provides pure material for crystallographic studies. The new tools we report will pave the way to large-scale structural and molecular investigations of RNA function and interactions with proteins.
机译:RNA已成为许多细胞过程中的主要参与者。在分子水平上理解这些过程需要用于结构,生化和药理学研究的均质RNA样品。我们之前设计了一种通用方法,可在大肠杆菌中高效表达重组RNA。在这项工作中,我们已经将该方法扩展到RNA /蛋白质共表达。我们设计了几种质粒,可在大肠杆菌中过量表达RNA蛋白复合物。我们已经研究了这些工具在许多应用中的潜力,包括包裹在病毒蛋白假颗粒中的核酸酶敏感RNA的生产,非编码RNA与伴侣蛋白的共同生产,转录后RNA修饰的整合通过与适当的修饰酶共同生产,最后通过镍亲和色谱法生产和纯化RNA–His标记的蛋白复合物。我们证明了该最后的应用很容易为晶体学研究提供纯净的材料。我们报告的新工具将为RNA功能及其与蛋白质相互作用的大规模结构和分子研究铺平道路。

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