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Effects of Gene Methylation Reprogramming in Cloned Calves Derived from In Vitro-Transfected Somatic Cells

机译:基因甲基化重编程中克隆牛的影响衍生自体积转染的体细胞

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In vitro transfection of cultured cells combined with nuclear transfer currently is the most effective procedure to produce transgenic livestock. In the present study, bovine primary fetal fibroblasts were transfected with a green fluorescent protein (GFP) reporter transgene and used as nuclear donor cells in oocyte reconstructions. To examine the role of host cytoplasm on transgene expression and developmental outcome, GFP-expressing fibroblasts were fused to oocytes reconstructed either metaphase or telophase activation, and PCR technology was also employed. The results showed that GFP became detectable at the 8-to 16-cell stage, approximately 80 h after reconstruction, and remained positive at all later stages. Embryonic development to the blastocyst stage was not significantly different among metaphase and telophase groups. Therefore, GFP transgene technology can be used to select embryoes derived from transgenic animals.
机译:体外转染培养细胞与核转移相结合目前是生产转基因牲畜的最有效的程序。在本研究中,用绿色荧光蛋白(GFP)报告转基因转染牛原胎成纤维细胞,并用作卵母细胞重建中的核供体细胞。为了检查宿主细胞质对转基因表达和发育结果的作用,将表达GFP的成纤维细胞与卵母细胞融合到卵母细胞中,重建中期或茶酶活化,并且还采用PCR技术。结果表明,GFP在重建后约80小时的8-16细胞阶段中可检测到,并且在所有后期阶段保持阳性。胚泡阶段的胚胎发育在中期和茶酶组中没有显着差异。因此,GFP转基因技术可用于选择衍生自转基因动物的胚胎。

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