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Selection of Osteoprogenitors from the Jaw Periosteum by a Specific Animal-Free Culture Medium
被引:13
作者:
Alexander, Dorothea
[1
]
Rieger, Melanie
[1
]
Klein, Christian
[2
,3
]
Ardjomandi, Nina
[1
]
Reinert, Siegmar
[1
]
机构:
[1] Univ Tubingen Hosp, Dept Oral & Maxillofacial Surg, Tubingen, Germany
[2] Univ Tubingen Hosp, Dept Conservat Dent, Tubingen, Germany
[3] Dent Practice Zahngesundheit Waiblingen, Waiblingen, Germany
来源:
PLOS ONE
|
2013年
/
8卷
/
12期
关键词:
MESENCHYMAL STEM-CELLS;
T-CELLS;
DIFFERENTIATION;
PROLIFERATION;
INHIBIT;
OSTEOGENESIS;
INVOLVEMENT;
CAPACITY;
INDUCE;
NICHES;
D O I:
10.1371/journal.pone.0081674
中图分类号:
O [数理科学和化学];
P [天文学、地球科学];
Q [生物科学];
N [自然科学总论];
学科分类号:
07 ;
0710 ;
09 ;
摘要:
The goal of our research work is to establish mesenchymal osteoprogenitors derived from human jaw periosteum for tissue engineering applications in oral and maxillofacial surgery. For future autologous and/or allogeneic transplantations, some issues must be addressed. On the one hand, animal-free culture conditions have yet to be established. On the other hand, attempts should be undertaken to shorten the in vitro culturing process efficiently. The aim of the present study is to compare and analyze the phenotype of osteoprogenitors from the jaw periosteum under normal FCS-containing and animal-free culture conditions. Therefore, we analyzed the proliferation rates of MesenCult-XF medium (MC-) in comparison to DMEM-cultured JPCs. Whereas jaw periosteal cells (JPCs) show relatively slow proliferation rates and a fibroblastoid shape under DMEM culture conditions, MC-cultured JPCs diminished their cell size significantly and proliferated rapidly. By live-monitoring measurements of adhesion and proliferation, we made an interesting observation: whereas the proliferation of the MSCA-1(+) subpopulation and the unseparated cell fraction were favored by the animal-free culture medium, the proliferation of the MSCA-1(-) subpopulation seemed to be repressed under these conditions. The alkaline phosphatase expression pattern showed similar results under both culture conditions. Comparison of the mineralization capacity revealed an earlier formation of calcium-phosphate precipitates under MC culture conditions; however, the mineralization capacity of the DMEM-cultured cells seemed to be higher. We conclude that the tested animal-free medium is suitable for the in vitro expansion and even for the specific selection of osteoprogenitor cells derived from the jaw periosteum.
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