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Preparation of highly multiplexed small RNA sequencing libraries

机译:高度复用小RNA测序文库的制备

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MicroRNAs (miRNAs) are similar to 22-nucleotide-long small non-coding RNAs that regulate the expression of protein-coding genes by base pairing to partially complementary target sites, preferentially located in the 3' untranslated region (UTR) of target mRNAs. The expression and function of miRNAs have been extensively studied in human disease, as well as the possibility of using these molecules as biomarkers for prognostication and treatment guidance. To identify and validate miRNAs as biomarkers, their expression must be screened in large collections of patient samples. Here, we develop a scalable protocol for the rapid and economical preparation of a large number of small RNA sequencing libraries using dual indexing for multiplexing. Combined with the use of off-the-shelf reagents, more samples can be sequenced simultaneously on large-scale sequencing platforms at a considerably lower cost per sample. Sample preparation is simplified by pooling libraries prior to gel purification, which allows for the selection of a narrow size range while minimizing sample variation. A comparison with publicly available data from benchmarking of miRNA analysis platforms showed that this method captures absolute and differential expression as effectively as commercially available alternatives.
机译:microRNAs(miRNA)类似于22-核苷酸长的小非编码RNA,其通过基部配对调节蛋白质编码基因的表达,以部分互补的靶位点,优先位于靶mRNA的3'未转换区域(UTR)中。 miRNA的表达和功能在人类疾病中已经广泛研究,以及使用这些分子作为生物标志物进行预后和治疗指导的可能性。为了识别和验证miRNA作为生物标志物,必须在大量患者样品中筛选它们的表达。在这里,我们开发一种可扩展的协议,用于使用双重分度进行多路复用的大量小型RNA测序文库的快速和经济的制备。结合使用架子试剂,可以在大规模测序平台上以相当低的每种样品在大规模测序平台上同时进行测序。通过在凝胶净化之前通过汇集文库简化样品制剂,其允许选择窄尺寸范围,同时最小化样品变化。与MiRNA分析平台的基准测试的公开数据的比较表明,该方法可有效地捕获绝对和差异表达,作为商业上可用的替代品。

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