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小鼠胚胎以及分化中的人源和小鼠胚胎干细胞中内参基因的选择。

Selection of reference genes in mouse embryos and in differentiating human and mouse ES cells.

作者信息

Willems Erik, Mateizel Ileana, Kemp Caroline, Cauffman Greet, Sermon Karen, Leyns Luc

机构信息

Lab for Cell Genetics, Vrije Universiteit Brussel (VUB), Brussels, Belgium.

出版信息

Int J Dev Biol. 2006;50(7):627-35. doi: 10.1387/ijdb.052130ew.

Abstract

Embryonic Stem (ES) cells have the potential to form every cell of the body and thus are of great promise for tissue transplantation. One of the rising techniques that allows studying the differentiation state of ES cells is quantitative RT-PCR (qRT-PCR). When relative quantification by qRT-PCR is applied, accurate normalization is necessary, since differentiated embryonic stem cells and developing embryos contain heterogeneous cell populations. Corrections for variations in the qRT-PCR reaction are needed to allow comparisons between different samples. We applied the normalization tools geNorm and Normfinder to ten reference genes identifying the most stable ones for relative quantification of gene expression during differentiation of human ES cells, as well as in differentiated mouse ES cells and in the developing mouse embryo. For relative quantification by qRT-PCR in these systems, we advise to use normalization factors based on multiple stable reference genes. However, when the use of several reference genes would be unpractical, a single reference gene in each experimental setup could be sufficient. When looking for single stable reference genes, beta-actin works best in both mouse embryo and ES cell experiments and glyceraldehyde-3-phosphate-dehydrogenase can be applied in both mouse and human ES cell experiments.

摘要

胚胎干细胞(ES细胞)有潜力分化为机体的每一种细胞,因此在组织移植方面极具前景。定量逆转录聚合酶链反应(qRT-PCR)是一种新兴的用于研究ES细胞分化状态的技术。当应用qRT-PCR进行相对定量时,准确的标准化是必要的,因为分化的胚胎干细胞和发育中的胚胎包含异质性细胞群体。为了能够对不同样本进行比较分析,需要对qRT-PCR反应中的变化进行校正。我们将标准化工具geNorm和Normfinder应用于十个参考基因,以确定在人类ES细胞分化过程中,以及在分化的小鼠ES细胞和发育中的小鼠胚胎中,用于基因表达相对定量的最稳定的参考基因。对于这些体系中通过qRT-PCR进行相对定量分析,我们建议使用基于多个稳定参考基因的标准化因子。然而,当使用多个参考基因不切实际时,每个实验设置中使用单一参考基因可能就足够了。在寻找单一稳定参考基因时,β-肌动蛋白在小鼠胚胎和ES细胞实验中效果最佳,而甘油醛-3-磷酸脱氢酶可应用于小鼠和人类ES细胞实验。

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