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表皮生长因子和三维支架为小鼠胚胎干细胞向卵母细胞样细胞的分化提供了有利的环境。

Epidermal growth factor and three-dimensional scaffolds provide conducive environment for differentiation of mouse embryonic stem cells into oocyte-like cells.

机构信息

Stem Cell Research Laboratory, Department of Anatomical Sciences, School of Medicine, Shiraz University of Medical Sciences, Shiraz, Iran.

出版信息

Cell Biol Int. 2020 Sep;44(9):1850-1859. doi: 10.1002/cbin.11391. Epub 2020 May 31.

DOI:10.1002/cbin.11391
PMID:32437076
Abstract

Three-dimensional (3D) culture provides a biomimicry of the naive microenvironment that can support cell proliferation, differentiation, and regeneration. Some growth factors, such as epidermal growth factor (EGF), facilitate normal meiosis during oocyte maturation in vivo. In this study, a scaffold-based 3D coculture system using purified alginate was applied to induce oocyte differentiation from mouse embryonic stem cells (mESCs). mESCs were induced to differentiate into oocyte-like cells using embryoid body protocol in the two-dimensional or 3D microenvironment in vitro. To increase the efficiency of the oocyte-like cell differentiation from mESCs, we employed a coculture system using ovarian granulosa cells in the presence or absence of epidermal growth factor (+EGF or -EGF) for 14 days and then the cells were assessed for germ cell differentiation, meiotic progression, and oocyte maturation markers. The cultures exposed to EGF in the alginate-based 3D microenvironment showed the highest level of premeiotic (Oct4 and Mvh), meiotic (Scp1, Scp3, Stra8, and Rec8), and oocyte maturation (Gdf9, Cx37, and Zp2) marker genes (p < .05) in comparison to other groups. According to the gene-expression patterns, we can conclude that alginate-based 3D coculture system provided a highly efficient protocol for oocyte-like cell differentiation from mESCs. The data showed that this culture system along with EGF improved the rate of in vitro oocyte-like cell differentiation.

摘要

三维(3D)培养提供了一种类似于原始微环境的仿生环境,可以支持细胞增殖、分化和再生。一些生长因子,如表皮生长因子(EGF),在体内卵母细胞成熟过程中促进正常减数分裂。在这项研究中,应用了基于支架的 3D 共培养系统,该系统使用纯化的藻酸盐来诱导来自小鼠胚胎干细胞(mESCs)的卵母细胞分化。mESCs 通过体外用胚体方案在二维或 3D 微环境中被诱导分化为卵母细胞样细胞。为了提高 mESCs 向卵母细胞样细胞分化的效率,我们采用了一种共培养系统,在存在或不存在表皮生长因子(+EGF 或 -EGF)的情况下,用卵巢颗粒细胞培养 14 天,然后评估细胞的生殖细胞分化、减数分裂进程和卵母细胞成熟标志物。暴露于藻酸盐基 3D 微环境中的 EGF 的培养物显示出最高水平的前减数分裂(Oct4 和 Mvh)、减数分裂(Scp1、Scp3、Stra8 和 Rec8)和卵母细胞成熟(Gdf9、Cx37 和 Zp2)标志物基因(p<.05)与其他组相比。根据基因表达模式,我们可以得出结论,藻酸盐基 3D 共培养系统为 mESCs 向卵母细胞样细胞分化提供了一种高效的方案。数据表明,该培养系统与 EGF 一起提高了体外卵母细胞样细胞分化的效率。

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