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通过外源表达鱼精蛋白 1 重塑体细胞核,以创建精子细胞样结构用于体细胞核移植。

Remodeling somatic nuclei via exogenous expression of protamine 1 to create spermatid-like structures for somatic nuclear transfer.

机构信息

Faculty of Veterinary Medicine, University of Teramo, Teramo, Italy.

INSERM, U823, Institut Albert Bonniot, Université Grenoble Alpes, Grenoble, France.

出版信息

Nat Protoc. 2016 Nov;11(11):2170-2188. doi: 10.1038/nprot.2016.130. Epub 2016 Oct 6.

DOI:10.1038/nprot.2016.130
PMID:27711052
Abstract

This protocol describes how to convert the chromatin structure of sheep and mouse somatic cells into spermatid-like nuclei through the heterologous expression of the protamine 1 gene (Prm1). Furthermore, we also provide step-by-step instructions for somatic cell nuclear transfer (SCNT) of Prm1-remodeled somatic nuclei in sheep oocytes. There is evidence that changing the organization of a somatic cell nucleus with that which mirrors the spermatozoon nucleus leads to better nuclear reprogramming. The protocol may have further potential application in determining the protamine and histone footprints of the whole genome; obtaining 'gametes' from somatic cells; and furthering understanding of the molecular mechanisms regulating the maintenance of DNA methylation in imprinted control regions during male gametogenesis. The protocol is straightforward, and it requires 4 weeks from the establishment of the cell lines to their transfection and the production of cloned blastocysts. It is necessary for researchers to have experience in cell biology and embryology, with basic skills in molecular biology, to carry out the protocol.

摘要

本方案描述了如何通过精蛋白 1 基因(Prm1)的异源表达,将绵羊和小鼠体细胞的染色质结构转化为精子细胞样核。此外,我们还提供了在绵羊卵母细胞中进行 Prm1 重构体细胞核体细胞核移植(SCNT)的分步说明。有证据表明,用类似于精子核的方式改变体细胞核的组织会导致更好的核重编程。该方案在确定整个基因组的精蛋白和组蛋白足迹、从体细胞获得“配子”以及进一步了解调节印迹控制区域中 DNA 甲基化在雄性配子发生过程中的维持的分子机制方面可能具有进一步的潜在应用。该方案简单直接,从细胞系的建立到转染和克隆囊胚的产生,需要 4 周时间。研究人员需要有细胞生物学和胚胎学方面的经验,以及分子生物学方面的基本技能,才能进行该方案。

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