在雄性大鼠饮食铁缺乏症模型中评估用于实时定量 PCR 分析的候选参考基因。

Joanna L Fiddler, Stephen L Clarke
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引用次数: 0

摘要

背景:实时定量聚合酶链反应(qPCR)是一种可靠、高效的基因表达定量方法。由于 qPCR 越来越多地用于研究养分与基因之间的相互作用,因此研究、开发和利用标准化方法进行数据分析和解释非常重要。表达数据标准化的常用方法包括使用参考基因 (RG) 来确定相对 mRNA 丰度。在计算相对丰度时,参考基因的选择会影响实验结果,并有可能使数据解读出现偏差。虽然常用的 RG 可用于归一化,但通常很少考虑 RG 的选择是否适合实验条件或不同组织或细胞类型。在本研究中,我们使用 BestKeeper、比较 delta 定量循环、NormFinder 和 RefFinder 对缺铁大鼠和配对喂养铁完全大鼠的各种组织中的基因表达稳定性进行了检测,以确定在 10 个候选 RG 中的最佳选择:结果:我们的研究结果表明,与其他候选 RG(如 Rpl19 和 Rps29)相比,几种常用的 RG(如 Actb 和 Gapdh)在缺铁和铁完全配对喂养条件下都表现出较低的稳定性。对于所有评估的 RG,与铁完全配对喂养对照组相比,缺铁动物肝脏中的 Tfrc 表达量显著增加;然而,最适合的 RG(Rpl19)和最不适合的 RG(Gapdh)之间的相对诱导量相差近 4 倍:这些结果表明,RG 的选择和使用应根据经验来确定,不同的实验条件和生物组织对 RG 的选择可能不同。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Evaluation of candidate reference genes for quantitative real-time PCR analysis in a male rat model of dietary iron deficiency.

Evaluation of candidate reference genes for quantitative real-time PCR analysis in a male rat model of dietary iron deficiency.

Evaluation of candidate reference genes for quantitative real-time PCR analysis in a male rat model of dietary iron deficiency.

Evaluation of candidate reference genes for quantitative real-time PCR analysis in a male rat model of dietary iron deficiency.

Background: Quantitative real-time polymerase chain reaction (qPCR) is a reliable and efficient method for quantitation of gene expression. Due to the increased use of qPCR in examining nutrient-gene interactions, it is important to examine, develop, and utilize standardized approaches for data analyses and interpretation. A common method used to normalize expression data involves the use of reference genes (RG) to determine relative mRNA abundance. When calculating the relative abundance, the selection of RG can influence experimental results and has the potential to skew data interpretation. Although common RG may be used for normalization, often little consideration is given to the suitability of RG selection for an experimental condition or between various tissue or cell types. In the current study, we examined the stability of gene expression using BestKeeper, comparative delta quantitation cycle, NormFinder, and RefFinder in a variety of tissues obtained from iron-deficient and pair-fed iron-replete rats to determine the optimal selection among ten candidate RG.

Results: Our results suggest that several commonly used RG (e.g., Actb and Gapdh) exhibit less stability compared to other candidate RG (e.g., Rpl19 and Rps29) in both iron-deficient and iron-replete pair-fed conditions. For all evaluated RG, Tfrc expression significantly increased in iron-deficient animal livers compared to the iron-replete pair-fed controls; however, the relative induction varied nearly 4-fold between the most suitable (Rpl19) and least suitable (Gapdh) RG.

Conclusion: These results indicate the selection and use of RG should be empirically determined and RG selection may vary across experimental conditions and biological tissues.

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