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不同饲养状态下鸡下丘脑逆转录定量聚合酶链反应的内参基因选择

Reference gene selection for reverse transcription quantitative polymerase chain reaction in chicken hypothalamus under different feeding status.

作者信息

Simon Á, Jávor A, Bai P, Oláh J, Czeglédi L

机构信息

Department of Animal Science, Faculty of Agricultural and Food Sciences and Environmental Management, University of Debrecen, Debrecen, Hungary.

Department of Medical Chemistry, Faculty of Medicine, University of Debrecen, Debrecen, Hungary.

出版信息

J Anim Physiol Anim Nutr (Berl). 2018 Feb;102(1):286-296. doi: 10.1111/jpn.12690. Epub 2017 Mar 15.

Abstract

This study was designed to investigate the stability of 10 candidate reference genes, namely ACTB, B2M, GAPDH, HMBS, LBR, POLR2B, RN18S, RPS17, TBP, and YWHAZ for the normalization of gene expression data obtained by quantitative real-time polymerase chain reaction (qPCR) in studies related to feed intake of chicken. Samples were isolated from hypothalamus under three different nutritional status (ad libitum, fasted for 24 hr, fasted for 24 hr then refed for 2 hr). Five different algorithms were applied for the analysis of reference gene stability: BestKeeper, geNorm, NormFinder, the comparative ΔCt method, and a novel approach using multivariate linear mixed-effects modelling for stable reference gene selection. TBP and POLR2B were identified as the two most suitable and B2M and RN18S as the two least stable reference genes for normalization. Despite our review, the current literature showing that RN18S is one of the most commonly used reference gene in chicken gene expression studies, its applicability for normalization should be evaluated before each qPCR experiment.

摘要

本研究旨在调查10个候选参考基因(即ACTB、B2M、GAPDH、HMBS、LBR、POLR2B、RN18S、RPS17、TBP和YWHAZ)的稳定性,以便在与鸡采食量相关的研究中,对通过定量实时聚合酶链反应(qPCR)获得的基因表达数据进行标准化。样本取自处于三种不同营养状态(自由采食、禁食24小时、禁食24小时后再喂食2小时)的下丘脑。应用了五种不同的算法来分析参考基因的稳定性:BestKeeper、geNorm、NormFinder、比较ΔCt法以及一种使用多变量线性混合效应模型进行稳定参考基因选择的新方法。TBP和POLR2B被确定为标准化最适合的两个参考基因,而B2M和RN18S则是最不稳定的两个参考基因。尽管我们查阅了相关文献,目前的文献表明RN18S是鸡基因表达研究中最常用的参考基因之一,但在每次qPCR实验之前,都应评估其用于标准化的适用性。

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