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Maintenance of amelogenin gene expression by transformed epithelial cells of mouse enamel organ.
Authors:L S Chen  R I Couwenhoven  D Hsu  W Luo  M L Snead
Affiliation:Center for Craniofacial Molecular Biology, University of Southern California, School of Dentistry, Los Angeles 90033.
Abstract:
Electroporation was used to introduce foreign genes into cells derived from the mouse enamel organ epithelia (EOE). Optimal conditions for this electroporation were established. The introduction of a plasmid construct bearing the coding region for the large T-antigen from polyoma virus into EOE cells permitted the establishment of a derivative cell line that has the following characteristics: (1) the cells could be passaged many times; (2) they expressed a keratin-containing cytoskeleton; and (3) approx. 60% of the cells expressed amelogenin, a tissue-specific gene product unique to ameloblasts. Potential uses for such a cell line include analysis of: (1) the upstream regulatory regions required for temporally and spatially restricted expression of amelogenin; (2) the post-translational modification of amelogenin in synchronized cells and (3) the organization and biomineralization of enamel extracellular matrix in monolayer culture.
Keywords:
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