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低生理氧条件下的培养可提高诱导多能干细胞的干性和质量。

Culture under low physiological oxygen conditions improves the stemness and quality of induced pluripotent stem cells.

机构信息

Department of Stem Cell Biology, Nagasaki University Graduate School of Biomedical Sciences, Nagasaki, Japan.

出版信息

J Cell Physiol. 2013 Nov;228(11):2159-66. doi: 10.1002/jcp.24389.

DOI:10.1002/jcp.24389
PMID:23589166
Abstract

The ex vivo expansion of stem cells under low physiological oxygen (O2 ) conditions has been demonstrated to improve the stemness and genomic stability of the cells. We investigated whether low-oxygen culture would be beneficial for the culture of induced pluripotent stem (iPS) cells. Two human iPS cell lines (201B7 and 253G1) were used for the experiments. Cells expanded from a single colony of each cell line were initiated for culture in 2.5% O2 , 5% O2 , or 20% O2 and maintained for 2 months in parallel. The levels of intracellular and mitochondrial reactive oxygen species did not differ between the cells cultured under different conditions. More colonies of uniformly smaller size were observed at 2.5% and 5% O2 than at 20% O2 . All of these iPS colonies that expanded under the various oxygen conditions stained positively for Oct3/4, Nanog, SSEA-4, and ALP. However, Western blot analysis showed that the iPS cells cultured at 2.5% and 5% O2 expressed significantly more Nanog but less 53BP1 than those cultured at 20% O2 . Data from an array CGH showed no significant chromosomal abnormalities, although some genes involved in cellular and metabolic processes were amplified in the low oxygen culture, particularly at 2.5% O2 . Our data suggest that low physiological oxygen culture could improve the stemness and quality of iPS cells, a result that might be associated with the amplification of genes involved in metabolic and cellular processes. Long-term culture will be necessary to confirm whether low physiological oxygen levels also improve genomic stability.

摘要

在低生理氧 (O2) 条件下对干细胞进行体外扩增已被证明可以提高细胞的干性和基因组稳定性。我们研究了低氧培养是否有益于诱导多能干细胞 (iPS) 细胞的培养。使用了两种人类 iPS 细胞系 (201B7 和 253G1) 进行实验。从每个细胞系的单个菌落中扩增的细胞开始在 2.5% O2、5% O2 或 20% O2 下培养,并在平行条件下维持 2 个月。在不同条件下培养的细胞之间细胞内和线粒体活性氧的水平没有差异。在 2.5% 和 5% O2 下观察到的均匀较小大小的菌落比在 20% O2 下更多。在各种氧气条件下扩增的所有这些 iPS 集落均对 Oct3/4、Nanog、SSEA-4 和 ALP 呈阳性染色。然而,Western blot 分析表明,在 2.5% 和 5% O2 下培养的 iPS 细胞表达的 Nanog 显著更多,但 53BP1 明显少于在 20% O2 下培养的细胞。阵列 CGH 的数据显示没有明显的染色体异常,尽管在低氧培养中,特别是在 2.5% O2 下,一些参与细胞和代谢过程的基因被扩增。长期培养将是必要的,以确认低生理氧水平是否也能提高基因组稳定性。

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