Vera Grotheer, D. Eckhardt, J. Schulz, Olga Messel, J. Windolf, C. Suschek
{"title":"衰老和培养衰老对成纤维细胞增殖和成骨分化的影响","authors":"Vera Grotheer, D. Eckhardt, J. Schulz, Olga Messel, J. Windolf, C. Suschek","doi":"10.37421/jtse.2019.10.222","DOIUrl":null,"url":null,"abstract":"Objective: The use of autologous cortical and cancellous bone remains the gold standard of bone-grafting. However, donor side morbidity, limited availability, and the risk of infections lead surgeons and researchers to seek suitable alternatives. Human fibroblasts are potent immunoregulatory cells with multipotent differentiation potential, which are easy to harvest and proliferate in vitro, which makes them attractive tools for bone tissue engineering. But for an autologous application in cell-based therapies, attention should be paid to the effect of donor age on differentiation potential. Culture senescence must also be considered, as some proliferation steps are necessary to obtain a sufficient cell number for therapeutic use. Methods: The results of this study reveal that an additional supplementation of insulin-like growth factor 1 is more suitable for osteogenic differentiation of foreskin fibroblasts, evaluated with an alkaline phosphatase assay, and quantification of calcium deposition in the extracellular matrix. Results: Our findings demonstrate that increasing donor age and culture senescence negatively affect the proliferation and osteogenic differentiation capacity of foreskin fibroblasts. These results suggest that the best approach to increase cell numbers is to optimize the seeding density, while additional growth factor application has no beneficial effect on the proliferation in early passages, analysed with a cell viability assay. Furthermore, commonly used osteogenic differentiation strategies consist of an application of ascorbate2-phosphate, dexamethasone, and β-glycerophosphate. However, phenotypic and differentiation potential discrepancies exist between multipotent mesenchymal stromal cells from different tissue origins as well as among fibroblasts from different dermal origins. Conclusion: This work illustrates, that human fibroblasts, provided by young donors and in early cell culture passages, are a viable cell source for bone tissue engineering. Differentiation. J Tissue Sci Eng 10: 222. doi: 10.37421/jtse.2019.10.222 DOI: 10.37421/jtse.2019.10.222 Citation: Grotheer V, Eckhardt D, Schulz J, Messel O, Windolf J, et al. (2019) The Effect of Aging and Culture Senescence on Fibroblast Proliferation","PeriodicalId":89595,"journal":{"name":"Journal of tissue science & engineering","volume":"41 1","pages":""},"PeriodicalIF":0.0000,"publicationDate":"2019-01-01","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"1","resultStr":"{\"title\":\"The Effect of Aging and Culture Senescence on Fibroblast Proliferation and Osteogenic Differentiation\",\"authors\":\"Vera Grotheer, D. Eckhardt, J. Schulz, Olga Messel, J. Windolf, C. Suschek\",\"doi\":\"10.37421/jtse.2019.10.222\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"Objective: The use of autologous cortical and cancellous bone remains the gold standard of bone-grafting. However, donor side morbidity, limited availability, and the risk of infections lead surgeons and researchers to seek suitable alternatives. Human fibroblasts are potent immunoregulatory cells with multipotent differentiation potential, which are easy to harvest and proliferate in vitro, which makes them attractive tools for bone tissue engineering. But for an autologous application in cell-based therapies, attention should be paid to the effect of donor age on differentiation potential. Culture senescence must also be considered, as some proliferation steps are necessary to obtain a sufficient cell number for therapeutic use. Methods: The results of this study reveal that an additional supplementation of insulin-like growth factor 1 is more suitable for osteogenic differentiation of foreskin fibroblasts, evaluated with an alkaline phosphatase assay, and quantification of calcium deposition in the extracellular matrix. Results: Our findings demonstrate that increasing donor age and culture senescence negatively affect the proliferation and osteogenic differentiation capacity of foreskin fibroblasts. These results suggest that the best approach to increase cell numbers is to optimize the seeding density, while additional growth factor application has no beneficial effect on the proliferation in early passages, analysed with a cell viability assay. Furthermore, commonly used osteogenic differentiation strategies consist of an application of ascorbate2-phosphate, dexamethasone, and β-glycerophosphate. However, phenotypic and differentiation potential discrepancies exist between multipotent mesenchymal stromal cells from different tissue origins as well as among fibroblasts from different dermal origins. Conclusion: This work illustrates, that human fibroblasts, provided by young donors and in early cell culture passages, are a viable cell source for bone tissue engineering. Differentiation. J Tissue Sci Eng 10: 222. doi: 10.37421/jtse.2019.10.222 DOI: 10.37421/jtse.2019.10.222 Citation: Grotheer V, Eckhardt D, Schulz J, Messel O, Windolf J, et al. 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The Effect of Aging and Culture Senescence on Fibroblast Proliferation and Osteogenic Differentiation
Objective: The use of autologous cortical and cancellous bone remains the gold standard of bone-grafting. However, donor side morbidity, limited availability, and the risk of infections lead surgeons and researchers to seek suitable alternatives. Human fibroblasts are potent immunoregulatory cells with multipotent differentiation potential, which are easy to harvest and proliferate in vitro, which makes them attractive tools for bone tissue engineering. But for an autologous application in cell-based therapies, attention should be paid to the effect of donor age on differentiation potential. Culture senescence must also be considered, as some proliferation steps are necessary to obtain a sufficient cell number for therapeutic use. Methods: The results of this study reveal that an additional supplementation of insulin-like growth factor 1 is more suitable for osteogenic differentiation of foreskin fibroblasts, evaluated with an alkaline phosphatase assay, and quantification of calcium deposition in the extracellular matrix. Results: Our findings demonstrate that increasing donor age and culture senescence negatively affect the proliferation and osteogenic differentiation capacity of foreskin fibroblasts. These results suggest that the best approach to increase cell numbers is to optimize the seeding density, while additional growth factor application has no beneficial effect on the proliferation in early passages, analysed with a cell viability assay. Furthermore, commonly used osteogenic differentiation strategies consist of an application of ascorbate2-phosphate, dexamethasone, and β-glycerophosphate. However, phenotypic and differentiation potential discrepancies exist between multipotent mesenchymal stromal cells from different tissue origins as well as among fibroblasts from different dermal origins. Conclusion: This work illustrates, that human fibroblasts, provided by young donors and in early cell culture passages, are a viable cell source for bone tissue engineering. Differentiation. J Tissue Sci Eng 10: 222. doi: 10.37421/jtse.2019.10.222 DOI: 10.37421/jtse.2019.10.222 Citation: Grotheer V, Eckhardt D, Schulz J, Messel O, Windolf J, et al. (2019) The Effect of Aging and Culture Senescence on Fibroblast Proliferation
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