Culture on fibrin matrices maintains the colony-forming capacity and osteoblastic differentiation of mesenchymal stem cells
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作者:
Colley, Helen
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Univ Sheffield, Ctr Biomat & Tissue Engn, Kroto Res Inst, Dept Mat Engn, Sheffield S3 7HQ, S Yorkshire, EnglandUniv Sheffield, Ctr Biomat & Tissue Engn, Kroto Res Inst, Dept Mat Engn, Sheffield S3 7HQ, S Yorkshire, England
Colley, Helen
[1
]
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McArthur, Sally L.
[1
,2
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Stolzing, Alexandra
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Univ Sheffield, Ctr Biomat & Tissue Engn, Kroto Res Inst, Dept Mat Engn, Sheffield S3 7HQ, S Yorkshire, EnglandUniv Sheffield, Ctr Biomat & Tissue Engn, Kroto Res Inst, Dept Mat Engn, Sheffield S3 7HQ, S Yorkshire, England
Stolzing, Alexandra
[1
]
Scutt, Andy
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Univ Sheffield, Ctr Biomat & Tissue Engn, Kroto Res Inst, Dept Mat Engn, Sheffield S3 7HQ, S Yorkshire, England
Univ Sheffield, Fac Med Dent & Hlth, Dept Human Metab, Sheffield S10 2TN, S Yorkshire, EnglandUniv Sheffield, Ctr Biomat & Tissue Engn, Kroto Res Inst, Dept Mat Engn, Sheffield S3 7HQ, S Yorkshire, England
Scutt, Andy
[1
,3
]
机构:
[1] Univ Sheffield, Ctr Biomat & Tissue Engn, Kroto Res Inst, Dept Mat Engn, Sheffield S3 7HQ, S Yorkshire, England
[2] Swinburne Univ Technol, IRIS, Fac Engn & Ind Sci, Hawthorn, Vic 3122, Australia
[3] Univ Sheffield, Fac Med Dent & Hlth, Dept Human Metab, Sheffield S10 2TN, S Yorkshire, England
Mesenchymal stem cells (MSC) are multipotent cells capable of differentiating into a number of mesenchymal tissues including bone, cartilage, and tendon. Low numbers in vivo means exponential growth is needed in culture to enable therapeutic applications. MSC can expand rapidly in culture but usually lose their extensive capacity for differentiation that makes them therapeutically attractive. To try and maintain their capacity for differentiation and expansion in vitro, we cultured MSC on fibrin gels of different concentrations to create more physiological growth conditions for the cells. The cells were then re-plated onto tissue culture plastic and analysed. The cells that had been pre-cultured for seven days on fibrin, proliferated and maintained their differential potential to the osteogenic lineage better than tissue culture plastic expanded MSC. A concentration relationship between colony number and fibrin concentration was seen with decreasing numbers as fibrin concentration increased. These data support the concept that substrate signals significantly influence MSC growth and differentiation and that growth on a fibrin matrix could be used to maintain a stem cell phenotype during MSC expansion.
机构:
Cent South Univ, Dept Endocrinol, Xiangya Hosp 3, Changsha 410013, Hunan, Peoples R ChinaCent South Univ, Dept Endocrinol, Xiangya Hosp 3, Changsha 410013, Hunan, Peoples R China
Zhao, Liling
Liu, Xiaoyin
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Sun Yat Sen Univ, Dept Ultrasound, Affiliated Hosp 6, Guangzhou 510655, Guangdong, Peoples R ChinaCent South Univ, Dept Endocrinol, Xiangya Hosp 3, Changsha 410013, Hunan, Peoples R China
Liu, Xiaoyin
Zeng, Pingyu
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Cent South Univ, Ctr Expt Med, Xiangya Hosp 3, Changsha 410013, Hunan, Peoples R ChinaCent South Univ, Dept Endocrinol, Xiangya Hosp 3, Changsha 410013, Hunan, Peoples R China
Zeng, Pingyu
Chen, Ke
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Cent South Univ, Dept Endocrinol, Xiangya Hosp 3, Changsha 410013, Hunan, Peoples R ChinaCent South Univ, Dept Endocrinol, Xiangya Hosp 3, Changsha 410013, Hunan, Peoples R China
Chen, Ke
Mo, Zhaohui
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Cent South Univ, Dept Endocrinol, Xiangya Hosp 3, Changsha 410013, Hunan, Peoples R ChinaCent South Univ, Dept Endocrinol, Xiangya Hosp 3, Changsha 410013, Hunan, Peoples R China