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Development of a chemiluminescence-based ribonuclease protection assay

机译:基于化学发光的核糖核酸酶保护性检测方法的开发

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摘要

The ribonuclease protection assay (RPA) is a widely used method for the detection and quantification of specific mRNA transcripts in a complex mixture of total RNA or mRNA molecules. While exhibiting many advantages over other RNA detection methods, RPAs are traditionally performed using radiolabeled probes that often require gel purification steps and lengthy exposure times to visualize results. Moreover these probes can only be used for 1-2 weeks because of their short isotopic half-life and radiolysis. We report a method that improves the traditional RPA by replacing radiolabeled probes with biotinylated probes and lengthy exposure times with quick, streptavidin/HRP-based chemiluminescent detection technology. Biotinylated probes can be used without gel purification and are stable for years, as opposed to weeks. Most importantly, our streptavidin/HRP-based chemiluminescent technology enables us to achieve sensitivity results similar to radioactive RPAs and to detect multiple transcripts in a single sample more efficiently. Furthermore, this new protocol addresses and eliminates the one major drawback unique to using biotinylated probes in chemiluminescent RPAs: a confounding artifact, not seen when running radioactive RPAs but commonly detected when using certain biotinylated rare message probes.
机译:核糖核酸酶保护分析(RPA)是一种用于检测和定量总RNA或mRNA分子的复杂混合物中特定mRNA转录物的方法。尽管与其他RNA检测方法相比具有许多优势,但是RPA传统上是使用放射性标记的探针进行的,通常需要凝胶纯化步骤和较长的暴露时间才能显现结果。此外,由于它们的同位素半衰期短和放射分解短,这些探针只能使用1-2周。我们报告了一种方法,该方法通过使用生物素标记的探针代替放射性标记的探针并通过快速,基于链霉亲和素/ HRP的化学发光检测技术来延长放射时间来改善传统的RPA。生物素化探针无需凝胶纯化即可使用,并且可以稳定使用数年而不是数周。最重要的是,我们基于链霉亲和素/ HRP的化学发光技术使我们能够获得与放射性RPA相似的灵敏度结果,并能更高效地检测单个样品中的多个转录本。此外,该新协议解决并消除了在化学发光RPA中使用生物素化探针所独有的一个主要缺点:一个混杂的伪像,在运行放射性RPA时看不到,但是在使用某些生物素化的稀有信息探针时通常可以检测到。

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