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Stable plasmid-based siRNA silencing of gene expression in human embryonic stem cells.

机译:人类胚胎干细胞中基因表达的基于质粒的稳定siRNA沉默。

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RNA interference (RNAi) using short inhibitory RNAs (siRNAs) has been widely explored for the suppression of cellular mRNA levels to investigate the function of specific genes, including gene function in differentiation and development. The establishment of human embryonic stem cell (hESC) models for differentiation of selected lineages is an area of intense interest and activity. On the basis of our previous work with stable overexpression of enhanced green fluorescent protein (EGFP) in hESC, we used plasmid vector-based siRNA expression to silence EGFP expression in stably-transfected hESC. After hygromycin selection, we derived several cell lines in which EGFP expression was significantly reduced. At the genomic DNA level, there was no difference between the two cell lines and the parental H1EGFP cell line when analyzed with quantitative PCR; however, there were significant differences among the three cell lines at the RNA and protein levels as analyzed with real-time RT-PCR and Western blotting. From these data, we conclude that the decrease in EGFP expression was caused by RNAi, not by genomic DNA loss. Down-regulation of EGFP expression was sustained through multiple passages of both siEGFP cell lines. This simple silencing system will allow novel investigations of target gene function in hESC self-renewal or differentiation, as well as differentiated function in other cell types.
机译:已经广泛探索了使用短抑制性RNA(siRNA)的RNA干扰(RNAi)来抑制细胞mRNA水平,以研究特定基因的功能,包括分化和发育中的基因功能。建立人类胚胎干细胞(hESC)模型以分化选定的谱系是一个引起人们极大兴趣和活动的领域。基于我们先前在hESC中稳定增强绿色荧光蛋白(EGFP)过表达的工作,我们使用了基于质粒载体的siRNA表达来沉默稳定转染的hESC中EGFP的表达。选择潮霉素后,我们获得了其中EGFP表达明显降低的几种细胞系。在基因组DNA水平上,用定量PCR分析时,两种细胞系与亲本H1EGFP细胞系之间没有差异。但是,通过实时RT-PCR和Western印迹分析,三种细胞系在RNA和蛋白质水平上存在显着差异。从这些数据,我们得出结论,EGFP表达的下降是由RNAi引起的,而不是基因组DNA的丢失。 EGFP表达的下调通过两种siEGFP细胞系的多次传代得以维持。这个简单的沉默系统将允许对hESC自我更新或分化中靶基因功能以及其他细胞类型中的分化功能进行新颖的研究。

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