Irradiated Human Dermal Fibroblasts Are as Efficient as Mouse Fibroblasts as a Feeder Layer to Improve Human Epidermal Cell Culture Lifespan

Bisson, Francis; Rochefort, Éloise; Lavoie, Amélie; Larouche, Danielle; Zaniolo, Karine; Simard-Bisson, Carolyne; Damour, O.; Auger, François A.; Guérin, Sylvain L.; Germain, Lucie

doi:10.3390/ijms14034684

Cited by 64 publications

(60 citation statements)

References 54 publications

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“…23 Irradiated human dermal fibroblasts provide a suitable human feeder layer that has similar efficiency as mouse fibroblasts for effective expansion of keratinocytes in vitro, but keratinocytes grown without a feeder layer may stop growth after a few passages. 19 Researchers showed that coculture of follicular keratinocytes with dermal fibroblasts treated with mitomycin C supported the proliferation of keratinocytes. They noted that it is easier to handle human fibroblasts than 3T3 cells, and homologous fibroblasts better mimic the physiologic state.…”

Section: Discussionmentioning

confidence: 99%

“…Keratinocytes usually are cultured for 3 to 4 passages for clinical applications. 19 We could culture these cells up to 3 passages. When the keratinocytes could be cultivated after cryopreservation, it was evident that growth of cells with normal morphology was possible on feeder cells in serum-free medium.…”

Section: Discussionmentioning

confidence: 99%

“…19,20 The key to obtaining suitable keratinocytes is optimization of the culture system to support keratinocyte growth. We compared various conditions such as the presence of a feeder layer and type of medium on the growth of these cells.…”

Section: Discussionmentioning

confidence: 99%

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2015

Exp Clin Transplant

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Objectives: Large-scale expansion of epidermal keratinocytes is essential in the application of these cells for severe burn treatment in patients. Therefore, this study was designed to evaluate various conditions in the expansion of human epidermal keratinocytes. Materials and Methods:The epidermis was separated from the dermis of skin samples using dispase. The epidermis was trypsinized for keratinocyte isolation. Keratinocytes were cultured in various conditions, with or without a human dermal fibroblast feeder layer, mitomycin C treatment, and different culture media. Results: Our results suggest that keratinocytes cultured on a human dermal fibroblast feeder layer were grown for several passages. Extensive deformation and rapid deterioration were observed in the cultured cells without a feeder layer and in serum-free medium. Conclusions: Human dermal fibroblasts treated with mitomycin C can provide optimal conditions for proliferation of keratinocytes.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

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2015

Exp Clin Transplant

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“…16,17 However, application of 3T3 cells for keratinocyte expansion is associated with the risk of contamination with infections and animal antigens. 18 At present, the focus of research is to discover an optimal protocol for keratinocyte culture.…”

Section: Discussionmentioning

confidence: 99%

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2015

Exp Clin Transplant

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“…HDF feeder could be used for iPSCs culture and provides suitable base to support the stem cells. HDF feeder in low passages (P 1-3) could decrease the immune response, easy handling, removing the contamination with animal pathogens, and maintains for long-term periods in the culture (Richards et al 2002;Tecirlioglu et al 2010;Bisson et al 2013;Ghasemi-Dehkordi et al 2014). In recent years, feeder-free culture such as BD Matrigel™ using MEF conditioned medium has been reported to be efficient for culture of stem cells.…”

Section: Introductionmentioning

confidence: 99%

Comparison between the cultures of human induced pluripotent stem cells (hiPSCs) on feeder-and serum-free system (Matrigel matrix), MEF and HDF feeder cell lines

Ghasemi-Dehkordi

Farsani

Abdian

et al. 2015

J. Cell Commun. Signal.

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Human induced pluripotent stem cells (hiPSCs) are a type of pluripotent stem cells artificially derived from an adult somatic cell (typically human fibroblast) by forced expression of specific genes. In recent years, different feeders like inactivated mouse embryonic fibroblasts (MEFs), human dermal fibroblasts (HDFs), and feeder free system have commonly been used for supporting the culture of stem cells in undifferentiated state. In the present work, the culture of hiPSCs and their characterizations on BD Matrigel (feederand serum-free system), MEF and HDF feeders using cell culture methods and molecular techniques were evaluated and compared. The isolated HDFs from foreskin samples were reprogrammed to hiPSCs using gene delivery system. Then, the pluripotency ability of hiPSCs cultured on each layer was determined by teratoma formation and immunohistochemical staining. After EBs generation the expression level of three germ layers genes were evaluated by Q-real-time PCR. Also, the cytogenetic stability of hiPSCs cultured on each condition was analyzed by karyotyping and comet assay. Then, the presence of pluripotency antigens were confirmed by Immunocytochemistry (ICC) test and alkaline phosphatase staining. This study were showed culturing of hiPSCs on BD Matrigel, MEF and HDF feeders had normal morphology and could maintain in undifferentiated state for prolonged expansion. The hiPSCs cultured in each system had normal karyotype without any chromosomal abnormalities and the DNA lesions were not observed by comet assay. Moreover, upregulation in three germ layers genes in cultured hiPSCs on each layer (same to ESCs) compare to normal HDFs were observed (p<0.05). The findings of the present work were showed in stem cells culturing especially hiPSCs both MEF and HDF feeders as well as feeder free system like Matrigel are proper despite benefits and disadvantages. Although, MEFs is suitable for supporting of stem cell culturing but it can animal pathogens transferring and inducing immune response. Furthermore, HDFs have homologous source with hiPSCs and can be used as feeder instead of MEF but in therapeutic approaches the cells contamination is a problem. So, this study were suggested feeder free culturing of hiPSCs on Matrigel in supplemented media (without using MEF conditioned medium) resolves these problems and could prepare easy applications of hiPSCs in therapeutic approaches of regenerative medicine such as stem-cell therapy and somatic cell nuclear in further researches.

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Irradiated Human Dermal Fibroblasts Are as Efficient as Mouse Fibroblasts as a Feeder Layer to Improve Human Epidermal Cell Culture Lifespan

Cited by 64 publications

References 54 publications

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Comparison between the cultures of human induced pluripotent stem cells (hiPSCs) on feeder-and serum-free system (Matrigel matrix), MEF and HDF feeder cell lines

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