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A Versatile Method to Design Stem-Loop Primer-Based Quantitative PCR Assays for Detecting Small Regulatory RNA Molecules

机译:设计基于干循环引物的定量PCR检测小规管RNA分子的多功能方法。

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摘要

Short regulatory RNA-s have been identified as key regulators of gene expression in eukaryotes. They have been involved in the regulation of both physiological and pathological processes such as embryonal development, immunoregulation and cancer. One of their relevant characteristics is their high stability, which makes them excellent candidates for use as biomarkers. Their number is constantly increasing as next generation sequencing methods reveal more and more details of their synthesis. These novel findings aim for new detection methods for the individual short regulatory RNA-s in order to be able to confirm the primary data and characterize newly identified subtypes in different biological conditions. We have developed a flexible method to design RT-qPCR assays that are very sensitive and robust. The newly designed assays were tested extensively in samples from plant, mouse and even human formalin fixed paraffin embedded tissues. Moreover, we have shown that these assays are able to quantify endogenously generated shRNA molecules. The assay design method is freely available for anyone who wishes to use a robust and flexible system for the quantitative analysis of matured regulatory RNA-s.
机译:短调控RNA已经被鉴定为真核生物中基因表达的关键调控因子。他们参与了生理和病理过程的调控,例如胚胎发育,免疫调控和癌症。它们的相关特征之一是它们的高稳定性,这使其成为用作生物标志物的极佳候选者。随着下一代测序方法揭示了越来越多的合成细节,它们的数量正在不断增加。这些新颖的发现旨在为单个短调控RNA的新检测方法,以便能够确认主要数据并表征不同生物学条件下新近鉴定的亚型。我们已经开发出一种灵活的方法来设计非常灵敏且稳定的RT-qPCR分析。新设计的检测方法已在植物,小鼠甚至人类福尔马林固定石蜡包埋组织的样品中进行了广泛测试。此外,我们已经表明,这些测定法能够量化内源性生成的shRNA分子。任何希望使用强大而灵活的系统来定量分析成熟调节RNA的人均可免费使用该测定设计方法。

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