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人类成体骨髓细胞可支持人类胚胎干细胞在培养中长时间扩增。

Human adult marrow cells support prolonged expansion of human embryonic stem cells in culture.

作者信息

Cheng Linzhao, Hammond Holly, Ye Zhaohui, Zhan Xiangcan, Dravid Gautam

机构信息

The Johns Hopkins University School of Medicine, Baltimore, Maryland 21231, USA.

出版信息

Stem Cells. 2003;21(2):131-42. doi: 10.1634/stemcells.21-2-131.

DOI:10.1634/stemcells.21-2-131
PMID:12634409
Abstract

Prolonged propagation of human embryonic stem (hES) cells is currently achieved by coculture with primary mouse embryonic fibroblasts (MEFs) serving as feeder cells. Unlike mouse ES cells, adding growth factors such as leukemia inhibitory factor is insufficient to maintain undifferentiated hES cells without feeder cells. The presence of uncharacterized rodent cells or crude extracts imposes a risk to the clinical applications of hES cells. While others looked for a replacement of MEFs with human fetal cells, we attempted to use easily accessible postnatal human cells such as human marrow stromal cells (hMSCs). Culture-expanded hMSCs from multiple donors were used as feeder cells to support growth of the H1 hES cell line under a serum-free culture condition. Human ES cell colonies cultured on irradiated hMSCs amplified >100-fold during the 30-day continuous culture (in five passages). The longest continuous expansion of hES cells on hMSCs tested to date is 13 passages. The expanded hES cells displayed the unique morphology and molecular markers characteristic of undifferentiated hES cells as observed when they were cultured on MEFs. They expressed the transcription factor Oct-4, a membrane alkaline phosphatase, and the stage-specific embryonic antigen (SSEA)-4, but not the SSEA-1 marker. Expanded hES cells on hMSCs retained unique differentiation potentials in culture and a normal diploid karyotype. The well-studied hMSCs (and this animal cell- and serum-free system) may provide a clinically and ethically feasible method to expand hES cells for novel cell therapies. In addition, this system may help to identify cytokines and adhesion molecules that are required for the self-renewal of hES cells.

摘要

目前,人类胚胎干细胞(hES)的长期传代培养是通过与作为饲养层细胞的原代小鼠胚胎成纤维细胞(MEF)共培养来实现的。与小鼠胚胎干细胞不同,添加白血病抑制因子等生长因子不足以在没有饲养层细胞的情况下维持未分化的hES细胞。未鉴定的啮齿动物细胞或粗提物的存在给hES细胞的临床应用带来了风险。当其他人寻求用人胎儿细胞替代MEF时,我们尝试使用易于获取的出生后人类细胞,如人类骨髓基质细胞(hMSC)。来自多个供体的培养扩增的hMSC被用作饲养层细胞,以在无血清培养条件下支持H1 hES细胞系的生长。在经辐照的hMSC上培养的人类胚胎干细胞集落在30天的连续培养(传代5次)中扩增了100倍以上。迄今为止,在hMSC上测试的hES细胞最长连续传代次数为13代。如在MEF上培养时所观察到的那样,在hMSC上扩增的hES细胞表现出未分化hES细胞特有的形态和分子标志物。它们表达转录因子Oct-4、膜碱性磷酸酶和阶段特异性胚胎抗原(SSEA)-4,但不表达SSEA-1标志物。在hMSC上扩增的hES细胞在培养中保留了独特的分化潜能和正常的二倍体核型。经过充分研究的hMSC(以及这个无动物细胞和无血清系统)可能为扩大hES细胞用于新型细胞治疗提供一种临床和伦理上可行的方法。此外,该系统可能有助于识别hES细胞自我更新所需的细胞因子和黏附分子。

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