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首页> 外文期刊>Molecular biotechnology >Validation of reference genes for normalizing gene expression in real-time quantitative reverse transcription pcr in human thyroid cells in primary culture treated with progesterone and estradiol
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Validation of reference genes for normalizing gene expression in real-time quantitative reverse transcription pcr in human thyroid cells in primary culture treated with progesterone and estradiol

机译:验证参考基因以使经孕酮和雌二醇处理的原代培养人甲状腺细胞中实时定量逆转录pcr中的基因表达正常化

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摘要

The use of appropriately chosen reference genes for normalizing gene expression in real-time quantitative reverse transcription polymerase chain reaction is an important step in the analysis of gene expression, compensating for several technical factors. As female sex hormones have been shown to influence growth and differentiation of thyroid follicular cells, the establishment of normalizer genes in human thyroid cells in primary culture, treated with progesterone, and estradiol, is important to evaluate their effect on gene expression in these cells, so candidate reference genes were studied. β-Actin, glyceraldehyde-3-phosphate dehydrogenase (GAPDH), β2-microglobulin (B2M), and TATA box binding protein (TBP) were evaluated in thyroid cells treated with estradiol, progesterone, and their inhibitors. Normfinder software was used to assess the stability of the genes and identified β-actin as the gene with adequate stability and lower inter-group variations, when compared to TBP, B2M, and GAPDH.
机译:在实时定量逆转录聚合酶链反应中,使用适当选择的参考基因对基因表达进行标准化是分析基因表达的重要步骤,可以弥补一些技术因素。由于已经显示出女性性激素会影响甲状腺滤泡细胞的生长和分化,因此在经过孕酮和雌二醇处理的原代培养的人甲状腺细胞中建立正常化基因对于评估其对这些细胞中基因表达的影响非常重要,因此研究了候选参考基因。在用雌二醇,孕酮及其抑制剂治疗的甲状腺细胞中,评估了β-肌动蛋白,3-磷酸甘油醛脱氢酶(GAPDH),β2-微球蛋白(B2M)和TATA盒结合蛋白(TBP)。与TBP,B2M和GAPDH相比,使用Normfinder软件评估基因的稳定性,并将β-肌动蛋白鉴定为具有足够稳定性且组间变异较低的基因。

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