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Bioactive Nanofibers Instruct Cells to Proliferate and Differentiate During Enamel Regeneration
Author(s) -
Huang Zhan,
Sargeant Timothy D,
Hulvat James F,
Mata Alvaro,
Bringas Pablo,
Koh ChungYan,
Stupp Samuel I,
Snead Malcolm L
Publication year - 2008
Publication title -
journal of bone and mineral research
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.882
H-Index - 241
eISSN - 1523-4681
pISSN - 0884-0431
DOI - 10.1359/jbmr.080705
Subject(s) - regeneration (biology) , nanofiber , enamel paint , microbiology and biotechnology , dentistry , biology , medicine , materials science , nanotechnology
During tooth development, ectoderm‐derived ameloblast cells create enamel by synthesizing a complex protein mixture serving to control cell to matrix interactions and the habit of hydroxyapatite crystallites. Using an in vitro cell and organ culture system, we studied the effect of artificial bioactive nanostructures on ameloblasts with the long‐term goal of developing cell‐based strategies for tooth regeneration. We used branched peptide amphiphile molecules containing the peptide motif Arg‐Gly‐Asp, or “RGD” (abbreviated BRGD‐PA), known to self‐assemble in physiologic environments into nanofibers that display on their surfaces high densities of this biological signal. Ameloblast‐like cells (line LS8) and primary enamel organ epithelial (EOE) cells were cultured within PA hydrogels, and the PA was injected into the enamel organ epithelia of mouse embryonic incisors. The expression of amelogenin, ameloblastin, integrin α5, and integrin α6 was detected by quantitative real‐time PCR and immunodetection techniques. We performed cell proliferation assay using BrdU labeling and a biomineralization assay using Alizarin red S staining with quantitative Ca 2+ measurements. In the cell culture model, ameloblast‐like cells (LS8) and primary EOE cells responded to the BRGD‐PA nanostructures with enhanced proliferation and greater amelogenin, ameloblastin, and integrin expression levels. At the site of injection of the BRGD‐PA in the organ culture model, we observed EOE cell proliferation with differentiation into ameloblasts as evidenced by their expression of enamel specific proteins. Ultrastructural analysis showed the nanofibers within the forming extracellular matrix, in contact with the EOE cells engaged in enamel formation and regeneration. This study shows that BRGD‐PA nanofibers present with enamel proteins participate in integrin‐mediated cell binding to the matrix with delivery of instructive signals for enamel formation.

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