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作 者:谭广云[1] 谢万华[1] 周焱[1] 黄永业[1] 宋红肖[1] 李栋[1] 宋娜[1] 袁婷[1] 段新平[1] 逄大欣[1] 欧阳红生[1]
机构地区:[1]吉林大学农学部畜牧兽医学院,吉林长春130062
出 处:《现代生物医学进展》2010年第12期2230-2233,共4页Progress in Modern Biomedicine
摘 要:目的:建立绿色荧光小鼠胚胎干细胞系。方法:以ICR及GFP转基因小鼠为实验动物,冲取交配后3.5天小鼠GFP-/+囊胚,去透明带后进行完全培养,以13.5天鼠胚胎成纤维细胞(MEF)为饲养层,并对细胞克隆用亚克隆的方法分离扩大培养。结果:获得了边缘清晰,表面平滑,结构致密,隆起生长的鸟巢状克隆,碱性磷酸酶染色呈强阳性,干细胞特异性的多能因子OCT4及Nanog表达呈阳性,且能稳定表达绿色荧光的雄性干细胞系。结论:本文为小鼠ES细胞系的建立提供了一种稳定而可靠的方法。Objective:To establish a EGFP mouse ES cell line.Methods:Blastocysts which were from the female ICR mouses mated with the male GFP transgenic mouse(C57BL/6) were collected,and the zone pellucida of each blastocyst was removed by incubating in pronase solution,then the blastocysts were plated onto feeder cells of mitotically mouse embryo fibroblasts(MEFs).Result:after culturing and passaging,a cell line was got which was eage clear,surface smooth,structure compact,and nest-like,these cells showed positive alkaline phosphatase activity,expressed primate ES-special markers OCT4 and Nanog,and expressed EGFP stably.Conclusion This article provides a simple,stable and reliable method for the establishment of mouse ES cell line.
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