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Issue title: Cell and Tissue Bioengineering and Therapy, Nancy 2005, 10–11 May
Article type: Research Article
Authors: Builles, Nicolas; | Bechetoille, Nicolas | Justin, Virginie | Ducerf, Amélie | Auxenfans, Céline | Burillon, Carole | Sergent, Michèle | Damour, Odile
Affiliations: Banque de Cornées des Hospices Civils de Lyon, 69437 Lyon, France | Engelhard-Coletica, 69007 Lyon, France | Service d'Ophtalmologie, Pavillon C, Hôpital Ed. Herriot, 69437 Lyon, France | Laboratoire de Mathématiques expérimentales, Marseille, France
Note: [] Corresponding authors: Nicolas Builles, Odile Damour, Hôpital Edouard Herriot, Place d'Arsonval, Pavillon i, 1er étage, Banque de Cornées des Hospices Civils de Lyon, 69437 Lyon, France. Tel.: +33 4 72 11 06 18 / +33 4 72 11 04 70; Fax: +33 4 72 11 62 14; E-mail: [email protected].
Abstract: Our objective was to formulate a medium for monolayer culture optimising both keratocyte growth and preservation of the keratocyte phenotype. Methods: An experimental matrix selected 14 media to test, using 7 components. Selection criteria were growth rates over 5 passages and expression of the CD34 marker. Results: Acetylcholine, insulin and vitamin C had no effect on growth and differentiation. The DMEM + Ham F12 1 : 1 based medium was selected for its initial effect on growth. At concentrations of 5 ng/ml, b-FGF improved the percentage of CD34+ cells without reducing growth rates. New-born calf serum (NCS) had a greater effect on growth than foetal calf serum (FCS). We showed three major interactions: between b-FGF and IGF-1, FCS and IGF-1 and NCS and b-FGF. Conclusion: We selected the following medium, which provides optimal growth and preservation of the CD34+ phenotype: DMEM/HAM-F12 + 10% NCS + 5 ng/ml b-FGF + antibiotics.
Keywords: Keratocytes, culture, medium
Journal: Bio-Medical Materials and Engineering, vol. 16, no. 4, pp. S95-S104, 2006
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