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通过后染色法对聚丙烯酰胺凝胶中芒果标记的RNA进行荧光可视化

Fluorescent Visualization of Mango-tagged RNA in Polyacrylamide Gels via a Poststaining Method.

作者信息

Yaseen Iqra M, Ang Quiana R, Unrau Peter J

机构信息

Department of Molecular Biology and Biochemistry, Simon Fraser University.

Department of Molecular Biology and Biochemistry, Simon Fraser University;

出版信息

J Vis Exp. 2019 Jun 21(148). doi: 10.3791/59112.

Abstract

Native and denaturing polyacrylamide gels are routinely used to characterize ribonucleoprotein (RNP) complex mobility and to measure RNA size, respectively. As many gel-imaging techniques use nonspecific stains or expensive fluorophore probes, sensitive, discriminating, and economical gel-imaging methodologies are highly desirable. RNA Mango core sequences are small (19-22 nt) sequence motifs that, when closed by an arbitrary RNA stem, can be simply and inexpensively appended to an RNA of interest. These Mango tags bind with high affinity and specificity to a thiazole-orange fluorophore ligand called TO1-Biotin, which becomes thousands of times more fluorescent upon binding. Here we show that Mango I, II, III, and IV can be used to specifically image RNA in gels with high sensitivity. As little as 62.5 fmol of RNA in native gels and 125 fmol of RNA in denaturing gels can be detected by soaking gels in an imaging buffer containing potassium and 20 nM TO1-Biotin for 30 min. We demonstrate the specificity of the Mango-tagged system by imaging a Mango-tagged 6S bacterial RNA in the context of a complex mixture of total bacterial RNA.

摘要

天然聚丙烯酰胺凝胶和变性聚丙烯酰胺凝胶通常分别用于表征核糖核蛋白(RNP)复合物的迁移率和测量RNA大小。由于许多凝胶成像技术使用非特异性染色剂或昂贵的荧光团探针,因此非常需要灵敏、有区分性且经济的凝胶成像方法。RNA芒果核心序列是小的(19 - 22个核苷酸)序列基序,当被任意RNA茎封闭时,可以简单且廉价地附加到感兴趣的RNA上。这些芒果标签与一种名为TO1 - 生物素的噻唑橙荧光团配体具有高亲和力和特异性结合,结合后荧光增强数千倍。在这里,我们表明芒果I、II、III和IV可用于在凝胶中以高灵敏度特异性成像RNA。通过将凝胶浸泡在含有钾和20 nM TO1 - 生物素的成像缓冲液中30分钟,可检测到天然凝胶中低至62.5 fmol的RNA和变性凝胶中低至125 fmol的RNA。我们通过在总细菌RNA的复杂混合物背景下对标记有芒果的6S细菌RNA进行成像,证明了芒果标记系统的特异性。

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