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首页> 外文期刊>BMC Genomics >Transcriptional defects and reprogramming barriers in somatic cell nuclear reprogramming as revealed by single-embryo RNA sequencing
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Transcriptional defects and reprogramming barriers in somatic cell nuclear reprogramming as revealed by single-embryo RNA sequencing

机译:单胚RNA测序揭示体细胞核重编程中的转录缺陷和重编程障碍

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Nuclear reprogramming reinstates totipotency or pluripotency in somatic cells by changing their gene transcription profile. This technology is widely used in medicine, animal husbandry and other industries. However, certain deficiencies severely restrict the applications of this technology. Using single-embryo RNA-seq, our study provides complete transcriptome blueprints of embryos generated by cumulus cell (CC) donor nuclear transfer (NT), embryos generated by mouse embryonic fibroblast (MEF) donor NT and in vivo embryos at each stage (zygote, 2-cell, 4-cell, 8-cell, morula, and blastocyst). According to the results from further analyses, NT embryos exhibit RNA processing and translation initiation defects during the zygotic genome activation (ZGA) period, and protein kinase activity and protein phosphorylation are defective during blastocyst formation. Two thousand three constant genes are not able to be reprogrammed in CCs and MEFs. Among these constant genes, 136 genes are continuously mis-transcribed throughout all developmental stages. These 136 differential genes may be reprogramming barrier genes (RBGs) and more studies are needed to identify. These embryonic transcriptome blueprints provide new data for further mechanistic studies of somatic nuclear reprogramming. These findings may improve the efficiency of somatic cell nuclear transfer.
机译:核重编程通过改变体细胞的基因转录谱来恢复其全能或全能。该技术被广泛应用于医药,畜牧等行业。但是,某些缺陷严重限制了该技术的应用。使用单胚RNA-seq,我们的研究提供了卵丘细胞(CC)供体核移植(NT)产生的胚胎,小鼠成纤维细胞(MEF)供体NT产生的胚胎以及每个阶段的体内胚胎的完整转录组蓝图(合子) ,2细胞,4细胞,8细胞,桑和胚泡)。根据进一步分析的结果,NT胚胎在合子基因组激活(ZGA)期间表现出RNA加工和翻译起始缺陷,并且在胚泡形成过程中蛋白激酶活性和蛋白磷酸化缺陷。 2000个恒定基因无法在CC和MEF中重新编程。在这些恒定基因中,有136个基因在所有发育阶段都被连续错误地转录。这136个差异基因可能是重编程屏障基因(RBG),需要进行更多研究。这些胚胎转录组蓝图为体细胞核重编程的进一步机理研究提供了新数据。这些发现可能会提高体细胞核转移的效率。

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