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食蟹猴胚胎干细胞的电穿孔法

Electroporation of cynomolgus monkey embryonic stem cells.

作者信息

Furuya Masataka, Yasuchika Kentaro, Mizutani Ken-Ichi, Yoshimura Yasunori, Nakatsuji Norio, Suemori Hirofumi

机构信息

Department of Development and Differentiation, Institute for Frontier Medical Sciences, Kyoto University, Japan.

出版信息

Genesis. 2003 Dec;37(4):180-7. doi: 10.1002/gene.10246.

Abstract

Efficient genetic modification of primate embryonic stem (ES) cells is essential for the application for both basic and preclinical research. The transfection efficiency of primate ES cells is reportedly lower than that of mouse ES cells. Cynomolgus monkey ES cells provide a powerful model for understanding human development and disease. We evaluated electroporation as a method to introduce foreign genes into cynomolgus monkey ES cells. Our examination has allowed us to establish a protocol producing about 100 stably transfected clones from 10(7) cynomolgus monkey ES cells. Differences in efficiency, however, were observed for other ES cell lines. We compared the transcriptional activities of the PGK-1, CMV, and SV40 promoters in cynomolgus monkey ES cells generating efficient G418 selection. Although the PGK-1 and SV40 promoters efficiently drove neo gene expression, the CMV promoter was significantly less transcriptionally active in cynomolgus monkey ES cells. Using this electroporation method, we established fluorescent cynomolgus monkey ES cell lines. These cells may be useful tools for tracing grafted cells in transplantation studies using a variety of functional cells derived from cynomolgus monkey ES cells.

摘要

灵长类胚胎干细胞(ES细胞)的高效基因改造对于基础研究和临床前研究的应用至关重要。据报道,灵长类ES细胞的转染效率低于小鼠ES细胞。食蟹猴ES细胞为理解人类发育和疾病提供了一个强大的模型。我们评估了电穿孔作为将外源基因导入食蟹猴ES细胞的一种方法。我们的研究使我们能够建立一种方案,从10^7个食蟹猴ES细胞中产生约100个稳定转染的克隆。然而,在其他ES细胞系中观察到了效率差异。我们比较了在产生高效G418选择的食蟹猴ES细胞中PGK-1、CMV和SV40启动子的转录活性。尽管PGK-1和SV40启动子有效地驱动了新霉素基因的表达,但CMV启动子在食蟹猴ES细胞中的转录活性明显较低。使用这种电穿孔方法,我们建立了荧光食蟹猴ES细胞系。这些细胞可能是在使用源自食蟹猴ES细胞的各种功能细胞进行移植研究中追踪移植细胞的有用工具。

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