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Circulating Messenger RNA Profiling with Microarray and Next-generation Sequencing: Cross-platform Comparison

机译:循环信使RNA分析与微阵列和下一代测序:跨平台比较

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Background: Circulating mRNA is a less invasive and more easily accessed source of samples for biomedical research and clinical applications. However, it is of poor quality. We explored and compared the ability of two high-throughput platforms for the profiling of circulating mRNA regarding their ability to retrieve useful information out of this type of samples. Materials and Methods: Circulating mRNAs from three non-small cell lung cancer patients and three healthy controls were analyzed by the cDNA-mediated annealing, selection, extension, and ligation (DASL) assay and high-throughput RNA sequencing (RSEQ). Twelve genes were selected for further confirmation by reverse transcription-quantitative polymerase chain reaction (RT-qPCR). Results: The overall expression profiles derived from the two platforms showed modest-to-moderate correlation. Genes with higher expression levels had higher cross-platform concordance than those of medium- and low-expression levels. In addition, the pathway signatures identified by gene set enrichment analysis from both platforms were in agreement. The RT-q PCR results for the selected genes correlated well with that of RSEQ. Conclusion: Genes with higher expression levels have cross-platform concordance and can be potential biomarkers. Furthermore, RSEQ is a better tool for profiling circulating mRNAs.
机译:背景:循环mRNA是用于生物医学研究和临床应用的侵入性较小且更易于获取的样品来源。但是,它的质量很差。我们探索并比较了两个高通量平台对循环mRNA进行谱分析的能力,这涉及它们从此类样品中检索有用信息的能力。材料和方法:通过cDNA介导的退火,选择,延伸和连接(DASL)分析和高通量RNA测序(RSEQ)分析了三名非小细胞肺癌患者和三名健康对照者的循环mRNA。通过逆转录定量聚合酶链反应(RT-qPCR)选择了十二个基因以进一步确认。结果:来自两个平台的总体表达谱显示出中等至中等的相关性。具有较高表达水平的基因比具有中等表达水平和低表达水平的基因具有更高的跨平台一致性。此外,通过基因富集分析从两个平台鉴定的途径签名是一致的。所选基因的RT-q PCR结果与RSEQ的相关性很好。结论:高表达水平的基因具有跨平台一致性,并且可能是潜在的生物标记。此外,RSEQ是用于分析循环mRNA的更好工具。

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