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首页> 外文期刊>Cell discovery. >Identification of key factors conquering developmental arrest of somatic cell cloned embryos by combining embryo biopsy and single-cell sequencing
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Identification of key factors conquering developmental arrest of somatic cell cloned embryos by combining embryo biopsy and single-cell sequencing

机译:结合胚胎活检和单细胞测序,确定可抑制体细胞克隆胚胎发育停滞的关键因素

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摘要

Differentiated somatic cells can be reprogrammed into totipotent embryos through somatic cell nuclear transfer. However, most cloned embryos arrest at early stages and the underlying molecular mechanism remains largely unexplored. Here, we first developed a somatic cell nuclear transfer embryo biopsy system at two- or four-cell stage, which allows us to trace the developmental fate of the biopsied embryos precisely. Then, through single-cell transcriptome sequencing of somatic cell nuclear transfer embryos with different developmental fates, we identified that inactivation of Kdm4b, a histone H3 lysine 9 trimethylation demethylase, functions as a barrier for two-cell arrest of cloned embryos. Moreover, we discovered that inactivation of another histone demethylase Kdm5b accounts for the arrest of cloned embryos at the four-cell stage through single-cell analysis. Co-injection of Kdm4b and Kdm5b can restore transcriptional profiles of somatic cell nuclear transfer embryos and greatly improve the blastocyst development (over 95%) as well as the production of cloned mice. Our study therefore provides an effective approach to identify key factors responsible for the developmental arrest of somatic cell cloned embryos.
机译:分化的体细胞可以通过体细胞核转移而重新编程为全能胚胎。但是,大多数克隆的胚胎在早期就停滞了,其潜在的分子机制在很大程度上尚待探索。在这里,我们首先开发了两细胞或四细胞阶段的体细胞核移植胚胎活检系统,这使我们能够精确地追踪活检胚胎的发育命运。然后,通过具有不同发育命运的体细胞核移植胚胎的单细胞转录组测序,我们确定了组蛋白H3赖氨酸9三甲基化脱甲基酶Kdm4b的失活,成为克隆的胚胎两细胞停滞的障碍。此外,我们发现通过单细胞分析,另一组蛋白去甲基化酶Kdm5b的失活导致克隆的胚胎在四细胞阶段停滞。共注射Kdm4b和Kdm5b可以恢复体细胞核移植胚胎的转录特征,并大大改善胚泡发育(超过95%)以及克隆小鼠的生产。因此,我们的研究提供了一种有效的方法,以鉴定造成体细胞克隆胚胎发育停滞的关键因素。

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