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通过在微滴培养中同时抑制 TGF-β 和 ERK 通路,增强小鼠单细胞囊胚的发育。

Enhanced development of mouse single blastomeres into blastocysts via the simultaneous inhibition of TGF-β and ERK pathways in microdroplet culture.

机构信息

Department of Animal Biology, Faculty of Biological Sciences, Kharazmi University, Tehran, Iran.

Department of Stem Cells and Developmental Biology, Cell Science Research Center, Royan Institute for Stem Cell Biology and Technology, ACECR, Tehran, Iran.

出版信息

J Cell Biochem. 2018 Sep;119(9):7621-7630. doi: 10.1002/jcb.27106. Epub 2018 Jun 20.

Abstract

Optimization of an in vitro culture that supports blastocyst (BL) development from single blastomeres (SBs) is essential to generate additional embryos for farm animals and humans and unravel the mechanisms that underlie totipotency. In this study, we have examined BL development from SBs that were derived from 2-cell and 4-cell mouse embryos in different media. Moreover, BLs were assessed for inner cell mass (ICM) by staining with Oct4. We found that BL development was improved in a lower volume of medium (1 µL) compared with a higher volume (5 µL). Furthermore, the supplementation of medium with the inhibitors of ERK1/2 and TGFβ (R2i) signaling pathways in 1 µL droplets of T6 medium improved BL development. The co-culture of SBs with intact embryos in the presence of R2i showed more BL development and ICM to trophectoderm cell number ratio in comparison with SB culture and SB group culture. We also observed reduced total cell number, ICM, and trophectoderm cell numbers in all of the SB culture conditions versus intact embryo development. These findings might facilitate the successful generation of additional embryos for biomedical applications and elucidate the mechanisms that underlie totipotency.

摘要

优化体外培养条件,支持从单个分裂球(SBs)发育囊胚(BL),对于为农场动物和人类生成额外胚胎以及阐明全能性的基础机制至关重要。在这项研究中,我们研究了来自 2 细胞和 4 细胞期小鼠胚胎的 SBs 在不同培养基中发育 BL 的情况。此外,通过对 Oct4 进行染色评估 BL 的内细胞团(ICM)。我们发现,与高体积(5 μL)相比,在低体积(1 μL)培养基中 BL 发育得到了改善。此外,在 T6 培养基中的 1 μL 液滴中添加 ERK1/2 和 TGFβ(R2i)信号通路抑制剂,可进一步改善 BL 发育。与 SB 培养和 SB 组培养相比,在 R2i 存在的情况下,将 SB 与完整胚胎共培养显示出更多的 BL 发育和 ICM 与滋养外胚层细胞数量比。我们还观察到,与完整胚胎发育相比,在所有 SB 培养条件下,总细胞数、ICM 和滋养外胚层细胞数均减少。这些发现可能有助于成功生成更多的胚胎,用于生物医学应用,并阐明全能性的基础机制。

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