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Testing for Differentially-Expressed MicroRNAs with Errors-in-Variables Nonparametric Regression

机译:测试具有差异误差非参数回归的差异表达微RNA

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摘要

MicroRNA is a set of small RNA molecules mediating gene expression at post-transcriptional/translational levels. Most of well-established high throughput discovery platforms, such as microarray, real time quantitative PCR, and sequencing, have been adapted to study microRNA in various human diseases. The total number of microRNAs in humans is approximately 1,800, which challenges some analytical methodologies requiring a large number of entries. Unlike messenger RNA, the majority of microRNA (60%) maintains relatively low abundance in the cells. When analyzed using microarray, the signals of these low-expressed microRNAs are influenced by other non-specific signals including the background noise. It is crucial to distinguish the true microRNA signals from measurement errors in microRNA array data analysis. In this study, we propose a novel measurement error model-based normalization method and differentially-expressed microRNA detection method for microRNA profiling data acquired from locked nucleic acids (LNA) microRNA array. Compared with some existing methods, the proposed method significantly improves the detection among low-expressed microRNAs when assessed by quantitative real-time PCR assay.
机译:MicroRNA是一组在转录后/翻译水平介导基因表达的小RNA分子。大多数公认的高通量发现平台,例如微阵列,实时定量PCR和测序,已被用于研究各种人类疾病中的microRNA。人类中的microRNA总数约为1800,这挑战了一些需要大量输入的分析方法。与信使RNA不同,大多数microRNA(60%)在细胞中维持相对较低的丰度。使用微阵列分析时,这些低表达微RNA的信号受其他非特异性信号(包括背景噪声)的影响。区分真正的microRNA信号与microRNA阵列数据分析中的测量误差至关重要。在这项研究中,我们提出了一种新的基于测量误差模型的归一化方法和差异表达的microRNA检测方法,用于从锁定核酸(LNA)microRNA阵列获得的microRNA分析数据。与某些现有方法相比,当通过定量实时PCR分析进行评估时,该方法显着改善了低表达microRNA的检测。

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