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Impact of reference gene selection for type 2 cannabinoid receptor gene expression studies in human spermatozoa

机译:参考基因选择对人类精子中2型大麻素受体基因表达研究的影响

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Quantitative real-time polymerase chain reaction (qRT-PCR) has been employed to study the gene expression profiles in human spermatozoa, but accurate analysis is dependent upon normalisation of data against an endogenous control. β-Actin (ACTB) and glyceraldehyde-3-phosphate dehydrogenase (GAPDH) are the most commonly used reference genes for normalisation of gene expression in human spermatozoa, but the expression of these genes in many tissues has considerable variation under different physiological, pathological and experimental conditions which limits their effectiveness in normalisation. The expression stability of a panel of 12 reference genes was studied in normal and pathological human spermatozoa using geNorm and NormFinder software. Although there were some discrepancies in the ranking of reference gene stability, each software program ranked B2M, ACTB, CYC1 and 18S RNA within the top 5 and recommended the combined use of at least two reference genes. Normalisation of qRT-PCR data for the cannabinoid receptor type 2 in spermatozoa using the different housekeeping genes demonstrated how, without validation, conflicting results are obtained. We recommend that the arbitrary use of reference genes should be avoided and the validation of reference gene stability should be undertaken prior to every study. For normalisation of CB2 expression, we would recommend using the geometric mean of B2M and ACTB.
机译:实时定量聚合酶链反应(qRT-PCR)已用于研究人类精子中的基因表达谱,但准确的分析取决于相对于内源性对照的数据标准化。 β-肌动蛋白(ACTB)和3-磷酸甘油醛脱氢酶(GAPDH)是使人类精子中基因表达正常化的最常用参考基因​​,但是这些基因在许多组织中的表达在不同的生理,病理和生理条件下都有相当大的差异。实验条件限制了其标准化的有效性。使用geNorm和NormFinder软件在正常和病理性人类精子中研究了12个参考基因组的表达稳定性。尽管参考基因稳定性的排名存在差异,但每个软件程序均将B2M,ACTB,CYC1和18S RNA排在前5位,并建议组合使用至少两个参考基因。使用不同管家基因对精子中2型大麻素受体的qRT-PCR数据进行归一化表明,如何在未经验证的情况下获得矛盾的结果。我们建议应避免随意使用参考基因​​,并应在每次研究之前进行参考基因稳定性的验证。为了标准化CB2表达,我们建议使用B2M和ACTB的几何平均值。

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