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Culture medium modulates the behaviour of human dental pulp-derived cells: Technical Note
Author(s) -
Séréna Lopez-Cazaux,
Gilles Bluteau,
David Magne,
Blandine Lieubeau,
Jérôme Guicheux,
Brigitte AlliotLicht
Publication year - 2006
Publication title -
european cells and materials
Language(s) - English
Resource type - Journals
ISSN - 1473-2262
DOI - 10.22203/ecm.v011a05
Subject(s) - dentin sialophosphoprotein , osteonectin , odontoblast , pulp (tooth) , dentinogenesis , chemistry , parathyroid hormone , microbiology and biotechnology , dentin , alkaline phosphatase , dental pulp stem cells , progenitor cell , osteocalcin , in vitro , calcium , dentistry , stem cell , biology , biochemistry , medicine , organic chemistry , enzyme
In vitro approaches have extensively been developed to study reparative dentinogenesis. While dental pulp is a source of unidentified progenitors able to differentiate into odontoblast-like cells, we investigated the effect of two media; MEM (1.8 mM Ca and 1 mM Pi) and RPMI 1640 (0.8 mM Ca and 5 mM Pi) on the behaviour of human dental pulp cells. Our data indicate that MEM significantly increased cell proliferation and markedly enhanced the proportion of alpha-smooth muscle actin positive cells, which represent a putative source of progenitors able to give rise to odontoblast-like cells. In addition, MEM strongly stimulated alkaline phosphatase activity and was found to induce expression of transcripts encoding dentin sialophosphoprotein, an odontoblastic marker, without affecting that of parathyroid hormone/parathyroid hormone related protein-receptor and osteonectin. In conclusion, these observations demonstrate that not only proliferation but also differentiation into odontoblast-like cells was induced by rich calcium and poor phosphate medium (MEM) as compared to RPMI 1640. This study provides important data for the determination of the optimal culture conditions allowing odontoblast-like differentiation in human pulp cell culture.

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