School of Pharmacy, Anhui Medical University, Hefei, Anhui 230032, P.R. China.
Department of Pharmacology, The Second Hospital of Anhui Medical University, Hefei, Anhui 230601, P.R. China.
Int J Mol Med. 2018 Jun;41(6):3527-3536. doi: 10.3892/ijmm.2018.3527. Epub 2018 Mar 1.
Investigations of hepatic gene expression are crucial for determining the molecular factors involved in acute alcoholic liver injury. The results of liver molecular investigations may reveal etiologically important genomic alterations. Therefore, it is necessary to normalize gene expression data to identify stable genes, which may be used as a reference under different experimental conditions. The aim of the present study was to apply reverse transcription‑quantitative polymerase chain reaction analysis and use analysis software to investigate the expression stability of candidate reference genes in hepatic tissues from mice with acute alcoholic liver injury. The acute alcoholic liver injury models were established by the intragastric administration of alcohol (5 mg/kg) in Imprinting Control Region mice. Total RNA was isolated from the mouse livers, following which the expression levels of seven reference genes, β-actin, glyceraldehyde 3-phosphate dehydrogenase (Gadph), glucuronidase β, hypoxanthine phosphoribosyltransferase 1 (Hprt1), 18S ribosomal RNA, TATA binding protein and β‑2 microglobulin, were examined, and gene expression stability was assessed using the geNorm, NormFinder and BestKeeper tools. The geNorm analysis revealed that the gene with the lowest variability was Hprt1. Hprt1 and Gapdh were validated as the optimal reference gene pair in all samples from all groups. The NormFinder and BestKeeper results showed that Hprt1 was the most stable gene in all samples. Alcohol induces endoplasmic reticulum (ER) stress, causing changes in the expression levels of ER stress‑associated genes. The stability of Hprt1 was verified by the expression analysis of ER stress‑associated genes, and gene expression levels in the ethanol groups were upregulated, with a significant difference in expression, compared with those in the control group. Therefore, Hprt1 was selected as the most stable gene, and Hprt1 and Gapdh were determined to be the optimum gene pair in mouse models of acute alcoholic liver injury. The reliability of the Hprt1 gene was confirmed by expression analysis of ER stress‑associated genes.
肝基因表达研究对于确定急性酒精性肝损伤相关的分子因素至关重要。肝分子研究的结果可能揭示病因学上重要的基因组改变。因此,有必要对基因表达数据进行归一化,以鉴定稳定的基因,这些基因可在不同的实验条件下作为参考。本研究旨在应用逆转录定量聚合酶链反应分析,并使用分析软件,研究急性酒精性肝损伤小鼠肝组织中候选参考基因的表达稳定性。通过灌胃给予酒精(5mg/kg)建立急性酒精性肝损伤模型。从小鼠肝脏中提取总 RNA,检测 7 个候选参考基因(β-肌动蛋白、甘油醛 3-磷酸脱氢酶(Gadph)、β-葡糖苷酸酶、次黄嘌呤磷酸核糖基转移酶 1(Hprt1)、18S 核糖体 RNA、TATA 结合蛋白和β-2 微球蛋白)的表达水平,并使用 geNorm、NormFinder 和 BestKeeper 工具评估基因表达稳定性。geNorm 分析显示,变异最小的基因是 Hprt1。Hprt1 和 Gapdh 在所有组别的所有样本中均被验证为最佳参考基因对。NormFinder 和 BestKeeper 结果表明,Hprt1 是所有样本中最稳定的基因。酒精诱导内质网(ER)应激,导致 ER 应激相关基因表达水平的变化。通过对 ER 应激相关基因的表达分析验证了 Hprt1 的稳定性,与对照组相比,乙醇组的基因表达水平上调,差异有统计学意义。因此,Hprt1 被选为最稳定的基因,Hprt1 和 Gapdh 被确定为急性酒精性肝损伤小鼠模型的最佳基因对。通过对 ER 应激相关基因的表达分析验证了 Hprt1 基因的可靠性。
