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Silica-based solid-phase extraction of cross-linked nucleic acid–bound proteins

机译:基于硅胶的固相萃取交联的核酸结合蛋白

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摘要

Proteins interact with nucleic acids to regulate cellular functions. The study of these regulatory interactions is often hampered by the limited efficiency of current protocols to isolate the relevant nucleic acid–protein complexes. In this report, we describe a rapid and simple procedure to highly enrich cross-linked nucleic acid–bound proteins, referred to as “2C” for “complex capture.” This method is based on the observation that silica matrix–based columns used for nucleic acid purification also effectively retain UV cross-linked nucleic acid–protein complexes. As a proof of principle, 2C was used to isolate RNA-bound proteins from yeast and mammalian Huh7 cells. The 2C method makes RNA labelling redundant, and specific RNA–protein interactions can be observed and validated by Western blotting. RNA–protein complexes isolated by 2C can subsequently be immunoprecipitated, showing that 2C is in principle compatible with sensitive downstream applications. We suggest that 2C can dramatically simplify the study of nucleic acid–protein interactions and benefit researchers in the fields of DNA and RNA biology.
机译:蛋白质与核酸相互作用以调节细胞功能。当前规程分离相关核酸-蛋白质复合物的效率有限,常常阻碍了对这些调节相互作用的研究。在本报告中,我们描述了一种快速简单的程序来高度富集交联的核酸结合蛋白,被称为“ 2C”,用于“复杂捕获”。该方法基于以下观察结果:用于硅胶纯化的基于硅胶基质的色谱柱也有效保留了UV交联的核酸-蛋白质复合物。作为原理的证明,2C用于从酵母和哺乳动物Huh7细胞中分离RNA结合蛋白。 2C方法使RNA标记变得多余,并且可以通过Western印迹观察和验证特定的RNA-蛋白质相互作用。随后可以对2C分离出的RNA蛋白复合物进行免疫沉淀,这表明2C原则上可以与敏感的下游应用兼容。我们建议2C可以大大简化核酸-蛋白质相互作用的研究,并有益于DNA和RNA生物学领域的研究人员。

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