Characterization of Human Fetal Cartilage Progenitor Cells During Long-Term Expansion in a Xeno-Free Medium

被引:11
|
作者
Kim, Hwal Ran [1 ,2 ]
Kim, Jiyoung [3 ]
Park, So Ra [3 ]
Min, Byoung-Hyun [1 ,2 ,4 ]
Choi, Byung Hyune [5 ]
机构
[1] Ajou Univ, Dept Mol Sci & Technol, 206 World Cup Ro, Suwon 16499, South Korea
[2] Ajou Univ, Med Ctr, Cell Therapy Ctr, 206 World Cup Ro, Suwon 16499, South Korea
[3] Inha Univ, Dept Physiol & Biophys, Coll Med, 100 Inha Ro, Incheon 22212, South Korea
[4] Ajou Univ, Sch Med, Dept Orthoped Surg, 164 World Cup Ro, Suwon 16499, South Korea
[5] Inha Univ, Coll Med, Dept Biomed Sci, 100 Inha Ro, Incheon 22212, South Korea
关键词
Human fetal cartilage progenitor cells; Serum-free medium; Cell therapy; Pluripotency; MESENCHYMAL STEM-CELLS; NANOG; OCT4;
D O I
10.1007/s13770-018-0132-z
中图分类号
Q813 [细胞工程];
学科分类号
摘要
BACKGROUND: Stem cell therapy requires a serum-free and/or chemically-defined medium for commercialization, but it is difficult to find one that supports long-term expansion of cells without compromising their stemness, particularly for novel stem cells. METHODS: In this study, we tested the efficiency of StemPro (R) MSC SFM Xeno Free (SFM-XF), a serum-free medium, for the long-term expansion of human fetal cartilage-derived progenitor cells (hFCPCs) from three donors in comparison to that of the conventional alpha-Modified Eagle's Medium (alpha-MEM) supplemented with 10% fetal bovine serum (FBS). RESULTS: We found that SFM-XF supported the expansion of hFCPCs for up to 28-30 passages without significant changes in the doubling time, while alpha-MEM with 10% FBS showed a rapid increase in doubling time at 10-18 passages depending on the donor. Senescence of hFCPCs was not observed until passage 10 in both media but was induced in approximately 15 and 25% of cells at passage 20 in SFM-XF and alpha-MEM with 10% FBS, respectively. The colony forming ability of hFCPCs in SFX-XF was also comparable to that in alpha-MEM with 10% FBS. hFCPCs expressed pluripotency genes like Oct-4, Sox-2, Nanog, SCF, and SSEA4 at passage 20 and 31 in SFM-XF; however, this was not observed when cells were cultured in alpha-MEM with 10% FBS. The ability of hFCPCs to differentiate into three mesodermal lineages decreased gradually in both media but it was less significant in SFM-XF. Finally we found no chromosomal abnormality after long-term culture of hFCPCs until passage 17 by karyotype analysis. CONCLUSION: These results suggest that SFM-XF supports the long-term expansion of hFCPCs without significant phenotypic and chromosomal changes. This study have also shown that hFCPCs can be mass-produced in vitro, proving their commercial value as a novel source for developing cell therapies.
引用
收藏
页码:649 / 659
页数:11
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