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Analysis of variance normal quantile-quantile correlation and effective expression support of pooled expression ratio of reference genes for defining expression stability

机译:分析方差正常分位数-分位数相关性和参考基因的总表达比例的有效表达支持以定义表达稳定性

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摘要

Identification of a reference gene unaffected by the experimental conditions is obligatory for accurate measurement of gene expression through relative quantification. Most existing methods directly analyze variability in crossing point (Cp) values of reference genes and fail to account for template-independent factors that affect Cp values in their estimates. We describe the use of three simple statistical methods namely analysis of variance (ANOVA), normal quantile-quantile correlation (NQQC) and effective expression support (EES), on pooled expression ratios of reference genes in a panel to overcome this issue. The pooling of expression ratios across the genes in the panel nullify the sample specific effects uniformly affecting all genes that are falsely reflected as instability. Our methods also offer the flexibility to include sample specific PCR efficiencies in estimations, when available, for improved accuracy. Additionally, we describe a correction factor from the ANOVA method to correct the relative fold change of a target gene if no truly stable reference gene could be found in the analyzed panel. The analysis is described on a synthetic data set to simplify the explanation of the statistical treatment of data.
机译:为了通过相对定量准确测量基因表达,必须鉴定不受实验条件影响的参考基因。大多数现有方法直接分析参考基因的交叉点(Cp)值的变异性,并且无法在估计中考虑影响模板Cp值的独立于模板的因素。我们描述了三种简单的统计方法,即方差分析(ANOVA),正常分位数-分位数相关性(NQQC)和有效表达支持(EES),在小组中参考基因的合并表达比上克服了这个问题。面板中各基因之间的表达比的合并使均匀影响所有被错误地反映为不稳定的所有基因的样品特异性作用无效。我们的方法还提供了灵活性,可以在估计时将样品特定的PCR效率包括在内,以提高准确性。另外,如果在分析的面板中找不到真正稳定的参考基因,我们将描述一种来自ANOVA方法的校正因子,以校正目标基因的相对倍数变化。在综合数据集上描述该分析,以简化对数据的统计处理的说明。

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