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从粗提细胞裂解液中快速且特异性地纯化 Argonaute-小 RNA 复合物。

Rapid and specific purification of Argonaute-small RNA complexes from crude cell lysates.

机构信息

Howard Hughes Medical Institute and Department of Biochemistry and Molecular Pharmacology, University of Massachusetts Medical School, Worcester, Massachusetts 01605, USA.

出版信息

RNA. 2013 Feb;19(2):271-9. doi: 10.1261/rna.036921.112. Epub 2012 Dec 18.

Abstract

Small interfering RNAs (siRNAs) direct Argonaute proteins, the core components of the RNA-induced silencing complex (RISC), to cleave complementary target RNAs. Here, we describe a method to purify active RISC containing a single, unique small RNA guide sequence. We begin by capturing RISC using a complementary 2'-O-methyl oligonucleotide tethered to beads. Unlike other methods that capture RISC but do not allow its recovery, our strategy purifies active, soluble RISC in good yield. The method takes advantage of the finding that RISC partially paired to a target through its siRNA guide dissociates more than 300 times faster than a fully paired siRNA in RISC. We use this strategy to purify fly Ago1- and Ago2-RISC, as well as mouse AGO2-RISC. The method can discriminate among RISCs programmed with different guide strands, making it possible to deplete and recover specific RISC populations. Endogenous microRNA:Argonaute complexes can also be purified from cell lysates. Our method scales readily and takes less than a day to complete.

摘要

小干扰 RNA(siRNA)指导 Argonaute 蛋白,即 RNA 诱导沉默复合物(RISC)的核心成分,切割互补的靶 RNA。在这里,我们描述了一种纯化含有单一独特小 RNA 指导序列的活性 RISC 的方法。我们首先使用与珠粒相连的互补 2'-O-甲基寡核苷酸捕获 RISC。与其他捕获 RISC 但不允许其回收的方法不同,我们的策略以良好的产率纯化活性、可溶性 RISC。该方法利用了这样一个发现,即通过其 siRNA 指导部分与靶标配对的 RISC 比完全配对的 siRNA 在 RISC 中解离快 300 多倍。我们使用这种策略来纯化果蝇 Ago1 和 Ago2-RISC ,以及小鼠 AGO2-RISC。该方法可以区分不同指导链编程的 RISCs,从而有可能耗尽和回收特定的 RISC 群体。内源性 microRNA:Argonaute 复合物也可以从细胞裂解物中纯化。我们的方法易于扩展,不到一天即可完成。

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