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A rank-based algorithm of differential expression analysis for small cell line data with statistical control

机译:统计控制的基于秩的小细胞系数据差异表达分析算法

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摘要

To detect differentially expressed genes (DEGs) in small-scale cell line experiments, usually with only two or three technical replicates for each state, the commonly used statistical methods such as significance analysis of microarrays (SAM), limma and RankProd (RP) lack statistical power, while the fold change method lacks any statistical control. In this study, we demonstrated that the within-sample relative expression orderings (REOs) of gene pairs were highly stable among technical replicates of a cell line but often widely disrupted after certain treatments such like gene knockdown, gene transfection and drug treatment. Based on this finding, we customized the RankComp algorithm, previously designed for individualized differential expression analysis through REO comparison, to identify DEGs with certain statistical control for small-scale cell line data. In both simulated and real data, the new algorithm, named CellComp, exhibited high precision with much higher sensitivity than the original RankComp, SAM, limma and RP methods. Therefore, CellComp provides an efficient tool for analyzing small-scale cell line data.
机译:为了在小规模细胞系实验中检测差异表达基因(DEG),通常每个状态只有两个或三个技术重复,缺少常用的统计方法,例如微阵列(SAM),limma和RankProd(RP)的显着性分析统计能力,而倍数变化方法缺乏任何统计控制。在这项研究中,我们证明了基因对的样品内相对表达顺序(REO)在细胞系的技术复制品中高度稳定,但在某些处理(如基因敲除,基因转染和药物处理)后经常被广泛破坏。基于此发现,我们定制了RankComp算法,该算法先前设计用于通过REO比较进行个性化差异表达分析,以通过小规模细胞系数据的某些统计控制来识别DEG。在模拟数据和实际数据中,名为CellComp的新算法都具有很高的精度,并且比原始的RankComp,SAM,limma和RP方法具有更高的灵敏度。因此,CellComp提供了一种用于分析小规模细胞系数据的有效工具。

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