A quantitative method to evaluate mesenchymal stem cell lipofection using real‐time PCR

流式细胞术 转染 质粒 间充质干细胞 生物 实时聚合酶链反应 分子生物学 背景(考古学) 报告基因 DNA 基因传递 溶解 电穿孔 细胞 细胞内 干细胞 遗传增强 基因 细胞生物学 基因表达 遗传学 古生物学
作者
Sérgio Conti Ribeiro,Rui D. Mendes,Catarina Madeira,Gabriel A. Monteiro,Cláudia L. da Silva,Joaquim M. S. Cabral
出处
期刊:Biotechnology Progress [Wiley]
卷期号:26 (5): 1501-1504 被引量:10
标识
DOI:10.1002/btpr.451
摘要

Genetic modification of human mesenchymal stem cells (MSC) is a powerful tool to improve the therapeutic utility of these cells and to increase the knowledge on their regulation mechanisms. In this context, strong efforts have been made recently to develop efficient nonviral gene delivery systems. Although several studies addressed this question most of them use the end product of a reporter gene instead of the DNA uptake quantification to test the transfection efficiency. In this study, we established a method based on quantitative real-time PCR (RT-PCR) to determine the intracellular plasmid DNA copy number in human MSC after lipofection. The procedure requires neither specific cell lysis nor DNA purification. The influence of cell number on the RT-PCR sensitivity was evaluated. The method showed good reproducibility, high sensitivity, and a wide linear range of 75-2.5 x 10⁶ plasmid DNA copies per cell. RT-PCR results were then compared with the percentage of transfected cells assessed by flow cytometry analysis, which showed that flow cytometry-based results are not always proportional to plasmid cellular uptake determined by RT-PCR. This work contributed for the establishment of a rapid quantitative assay to determine intracellular plasmid DNA in stem cells, which will be extremely beneficial for the optimization of gene delivery strategies.

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