琼脂糖-甲醛凝胶电泳分离长 RNA。
Separation of long RNA by agarose-formaldehyde gel electrophoresis.
机构信息
Department of Cell Biology, Rowan University, School of Osteopathic Medicine, Stratford, NJ 08084, USA.
出版信息
Anal Biochem. 2013 Oct 1;441(1):18-20. doi: 10.1016/j.ab.2013.06.008. Epub 2013 Jun 22.
Abstract
We describe a method to facilitate electrophoretic separation of high-molecular-weight RNA species, such as ribosomal RNAs and their precursors, on agarose-formaldehyde gels. Two alternative "pK-matched" buffer systems were substituted for the traditionally used Mops-based conductive medium. The key advantages include shortened run times, a 5-fold reduction in formaldehyde concentration, a significantly improved resolution of long RNAs, and consistency in separation. The new procedure has a streamlined work flow that helps to minimize errors and is broadly applicable to agarose gel electrophoresis of RNA samples and their subsequent analysis by Northern blotting.
摘要
我们描述了一种在琼脂糖-甲醛凝胶上促进高分子量 RNA 物种(如核糖体 RNA 及其前体)电泳分离的方法。两种替代的“pK 匹配”缓冲系统取代了传统使用的基于 Mops 的导电介质。其主要优点包括缩短运行时间、甲醛浓度降低 5 倍、长 RNA 的分辨率显著提高以及分离的一致性。新的程序具有简化的工作流程,有助于最大限度地减少错误,并且广泛适用于 RNA 样品的琼脂糖凝胶电泳及其随后的 Northern 印迹分析。
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