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Deep-Sequencing Protocols Influence the Results Obtained in Small-RNA Sequencing

机译:深度测序协议会影响在小RNA测序中获得的结果

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摘要

Second-generation sequencing is a powerful method for identifying and quantifying small-RNA components of cells. However, little attention has been paid to the effects of the choice of sequencing platform and library preparation protocol on the results obtained. We present a thorough comparison of small-RNA sequencing libraries generated from the same embryonic stem cell lines, using different sequencing platforms, which represent the three major second-generation sequencing technologies, and protocols. We have analysed and compared the expression of microRNAs, as well as populations of small RNAs derived from repetitive elements. Despite the fact that different libraries display a good correlation between sequencing platforms, qualitative and quantitative variations in the results were found, depending on the protocol used. Thus, when comparing libraries from different biological samples, it is strongly recommended to use the same sequencing platform and protocol in order to ensure the biological relevance of the comparisons.
机译:第二代测序是鉴定和定量细胞小RNA成分的有力方法。但是,很少关注测序平台和文库制备方案的选择对所得结果的影响。我们提供了使用不同的测序平台,从相同的胚胎干细胞系生成的小RNA测序文库的全面比较,代表了三种主要的第二代测序技术和方案。我们已经分析并比较了microRNA的表达以及源自重复元件的小RNA的数量。尽管不同的文库在测序平台之间显示出良好的相关性,但根据所使用的方案,发现了结果的定性和定量变化。因此,当比较来自不同生物样品的文库时,强烈建议使用相同的测序平台和方案,以确保比较的生物学相关性。

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