The influence of type I collagen on the development and maintenance of the osteoblast phenotype in primary and passaged rat calvarial osteoblasts: modification of expression of genes supporting cell growth, adhesion, and extracellular matrix mineralization
UMass Chan Affiliations
Department of Cell BiologyDocument Type
Journal ArticlePublication Date
1995-01-01Keywords
Alkaline PhosphataseAnimals
Biological Markers
Calcification, Physiologic
Calcium-Binding Proteins
Cell Adhesion
Cell Differentiation
Cell Division
Cells, Cultured
Cholecalciferol
Collagen
Embryonic and Fetal Development
Extracellular Matrix Proteins
*Gene Expression Regulation, Developmental
Osteoblasts
Osteopontin
Phenotype
Plastics
RNA, Messenger
Rats
Sialoglycoproteins
Skull
Up-Regulation
Cell Biology
Metadata
Show full item recordAbstract
Osteoblasts derived from Day 21 fetal rat calvaria grown on films of collagen type I exhibit an earlier and enhanced expression of the differentiated phenotype, compared to cells cultured on plastic. The temporal expression of genes characterizing three distinct periods of growth and differentiation are dramatically modified. During the initial proliferation period, expression of genes normally expressed at high levels on plastic (fibronectin, beta 1 integrin, and actin) was decreased from 50 to 70% in cells grown on collagen. Genes normally expressed at maximal levels in the postproliferative period (osteonectin, osteocalcin, and osteopontin) were up-regulated severalfold very early. Alkaline phosphatase enzyme activity was elevated 2- to 3-fold during the proliferation period, while mRNA levels remained low, suggesting post-transcriptional modifications. The most dramatic consequence of culture of cells on collagen is the accelerated and uniform mineralization of the matrix in contrast to the focal mineralization confined to bone nodules in cultures on plastic. Type I collagen supports maintenance of osteoblast phenotypic properties of passaged cells in the absence of glucocorticoid supplementation required for differentiation of osteoblasts subcultivated on plastic. Treatment of proliferating rat osteoblasts on plastic with 1,25(OH)2D3 blocks osteoblast differentiation and matrix mineralization. Although differentiation-related genes (alkaline phosphatase and osteocalcin) were up-regulated by vitamin D, culture on the collagen matrix could not overcome the inhibition of mineralization. Taken together, these studies define the critical role of type I collagen in mediating the signaling cascade for expression of a mature osteoblast phenotype and mineralization of the extracellular matrix in a physiological manner.Source
Exp Cell Res. 1995 Jan;216(1):35-45. Link to article on publisher's siteDOI
10.1006/excr.1995.1005Permanent Link to this Item
http://hdl.handle.net/20.500.14038/49654PubMed ID
7813631Related Resources
Link to Article in PubMedae974a485f413a2113503eed53cd6c53
10.1006/excr.1995.1005