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作 者:郭志林[1] 王新庄 张涌[1] 王木[2] 王轶敏[1] 胡文举[1]
机构地区:[1]西北农林科技大学动物科技学院,杨凌712100 [2]河南省肉牛工程技术研究中心,郑州450003
出 处:《农业生物技术学报》2006年第5期688-691,共4页Journal of Agricultural Biotechnology
基 金:河南省杰出人才创新基金项目(No.0421002100)资助
摘 要:为提高昆明小鼠胚胎生殖细胞(embryonicgermcells,EGcells)建系效率,以怀孕8.5~12.5d小鼠胎儿为材料,比较了胎儿后1/3部位的组织共培养、生殖嵴共培养、差速贴壁和穿刺生殖嵴4种分离胚胎原始生殖细胞(primordialgermcells,PGCs)的方法以及不同传代方式对EG细胞克隆的影响。结果表明:生殖嵴共培养和差速贴壁方式获得了较好分离EG细胞的效果,与其它两组比较差异显著;手工传代方式与连同成纤维细胞一起消化的传代方式相比获得了较高传代比率。对所分离EG细胞经形态观察、AKP染色和体外分化能力检测,证实其符合小鼠EG细胞的集落状生长、细胞未分化特性及细胞多能性等特征。Four isolation methods: co-culture back 1/3 position of embryonic tissue, co-culture genital ridges, different speed attaching and puncture the genital ridges were compared to improve the efficiency for establishing the embryonic germ cells (EG cells) line from Kunming mice. Two passage ways, hand and digestion together with fibroblast, were used to clone EG cells. Results showed that co-culture the genital ridges and different speed attaching were more effective methods than that of the others. And passage by hand could improved passage efficiency of EG cells compared with digestion together with fibroblast. When isolated EG cells were examined by morphology observation, AKP strain and in vitro differentiation ability, they were convinced to have a series of characters of mice EG cells including cloning grow way, undifferentiation state and pluripotency of cells.
关 键 词:昆明小鼠 原始生殖细胞 胚胎生殖细胞 胚胎干细胞 生殖嵴
分 类 号:S185[农业科学—农业基础科学]
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