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The utility of optical detection system (qPCR) and bioinformatics methods in reference gene expression analysis

机译:光学检测系统(QPCR)和生物信息学方法在参考基因表达分析中的效用

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Real-time quantitative polymerase chain reaction is consider as the most reliable method for gene expression studies. However, the expression of target gene could be misinterpreted due to improper normalization. Therefore, the crucial step for analysing of qPCR data is selection of suitable reference genes, which should be validated experimentally. In order to choice the gene with stable expression in the designed experiment, we performed reference gene expression analysis. In this study genes described in the literature and novel genes predicted as control genes, based on the in silico analysis of transcriptome data were used. Analysis with geNorm and NormFinder algorithms allow to create the ranking of candidate genes and indicate the best reference for flower morphogenesis study. According to the results, genes CACS and CYCL were characterised the most stable expression, but the least suitable genes were TUA and EF.
机译:实时定量聚合酶链反应是作为基因表达研究中最可靠的方法。然而,由于规范化不当,靶基因的表达可能会被误解。因此,用于分析QPCR数据的关键步骤是选择合适的参考基因,应该通过实验验证。为了选择在设计实验中具有稳定表达的基因,我们进行了参考基因表达分析。在使用转录组数据的硅分析的基础上预测为对照基因的文献和新的基因中描述的该研究中,基于转录组数据的硅分析。具有Genorm和Normfinder算法的分析允许创造候选基因的排名,并表明花生育研究的最佳参考。根据结果​​,基因CACS和CAM的特征是表达最稳定的表达,但最少合适的基因是TUA和EF。

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