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Coordination between donor cell type and cell cycle stage improves nuclear cloning efficiency in cattle

机译:供体细胞类型与细胞周期阶段之间的协调提高了牛的核克隆效率

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摘要

Several studies have shown that both quiescent and proliferating somatic donor cells can be fully reprogrammed after nuclear transfer (NT) and result in viable offspring. So far, however, no comparative study has conclusively demonstrated the relative importance of donor cell cycle stage on nuclear cloning efficiency. Here, we compare two different types of bovine fetal fibroblasts (BFFs) that were synchronized in G(0), G(1), and different phases within G(1). We show that for non-transgenic (non-TG) fibroblasts, serum starvation into G(0) results in a significantly higher percentage of viable calves at term than synchronization in early G(1) or late G(1). For transgenic fibroblasts, however, cells selected in G(1) show significantly higher development to calves at term and higher post-natal survival to weaning than cells in G(0). This suggests that it may be necessary to coordinate donor cell type and cell cycle stage to maximize overall cloning efficiency.
机译:几项研究表明,在核移植(NT)后,静止和增殖的体细胞供体细胞都可以完全重编程,并产生后代。然而,到目前为止,还没有任何比较研究能够最终证明供体细胞周期阶段对核克隆效率的相对重要性。在这里,我们比较了两种不同类型的牛胎儿成纤维细胞(BFF),它们在G(0),G(1)和G(1)内的不同阶段是同步的。我们显示对于非转基因(non-TG)成纤维细胞,血清饥饿进入G(0)会导致足月活犊牛的百分比显着高于早期G(1)或晚期G(1)的同步化。然而,对于转基因成纤维细胞,与G(0)中的细胞相比,G(1)中选择的细胞在足月发育到犊牛的发育显着更高,而断奶后的存活率也更高。这表明可能有必要协调供体细胞类型和细胞周期阶段,以使总体克隆效率最大化。

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