Vitamin D metabolites regulate matrix vesicle metalloproteinase content in a cell maturation-dependent manner

Vitamin D metabolites regulate matrix vesicle metalloproteinase content in a cell maturation-dependent manner

Matrix vesicles are extracellular organelles produced by cells that mineralize their matrix. They contain enzymes that are associated with calcification and are regulated by vitamin D metabolites in a cell maturation-dependent manner. Matrix vesicles also contain metalloproteinases that degrade prot...

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Veröffentlicht in:Calcified tissue international 1996-08, Vol.59 (2), p.109-116
Hauptverfasser: Dean, D D, Boyan, B D, Muniz, O E, Howell, D S, Schwartz, Z
Format: Artikel
Sprache:eng
Schlagworte:
24,25-Dihydroxyvitamin D 3 - pharmacology
Alkaline Phosphatase - blood
Alkaline Phosphatase - metabolism
Animals
Calcitriol - metabolism
Calcitriol - pharmacology
Cartilage - cytology
Cartilage - drug effects
Cartilage - ultrastructure
Cell Membrane - drug effects
Cell Membrane - enzymology
Cell Survival - drug effects
Cells, Cultured
Extracellular Matrix - drug effects
Extracellular Matrix - enzymology
Metalloendopeptidases - blood
Metalloendopeptidases - metabolism
Organelles - drug effects
Organelles - enzymology
Plasminogen Activators - metabolism
Rats
Rats, Sprague-Dawley
Synaptic Vesicles - drug effects
Synaptic Vesicles - enzymology
Synaptic Vesicles - metabolism
Transforming Growth Factor beta - biosynthesis
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Zusammenfassung:Matrix vesicles are extracellular organelles produced by cells that mineralize their matrix. They contain enzymes that are associated with calcification and are regulated by vitamin D metabolites in a cell maturation-dependent manner. Matrix vesicles also contain metalloproteinases that degrade proteoglycans, macromolecules known to inhibit calcification in vitro, as well as plasminogen activator, a proteinase postulated to play a role in activation of latent TGF-beta. In the present study, we examined whether matrix vesicle metalloproteinase and plasminogen activator are regulated by 1, 25(OH)2D3 and 24,25(OH)2D3. Matrix vesicles and plasma membranes were isolated from fourth passage cultures of resting zone chondrocytes that had been incubated with 10(-10)-10(-7) M24, 25(OH)2D3 or growth zone chondrocytes incubated with 10(-11)-10(-8) M 1,25(OH)2D3, and their alkaline phosphatase, active and total neutral metalloproteinase, and plasminogen activator activities determined. 24,25(OH)2D3 increased alkaline phosphatase by 35-60%, decreased active and total metalloproteinase by 75%, and increased plasminogen activator by fivefold in matrix vesicles from resting zone chondrocyte cultures. No effect of vitamin D treatment was observed in plasma membranes isolated from these cultures. In contrast, 1,25(OH)2D3 increased alkaline phosphatase by 35-60%, but increased active and total metalloproteinase three- to fivefold and decreased plasminogen activator by as much as 75% in matrix vesicles isolated from growth zone chondrocyte cultures. Vitamin D treatment had no effect on plasma membrane alkaline phosphatase or metalloproteinase, but decreased plasminogen activator activity. The results demonstrate that neutral metalloproteinase and plasminogen activator activity in matrix vesicles are regulated by vitamin D metabolites in a cell maturation-specific manner. In addition, they support the hypothesis that 1,25(OH)2D3 regulation of matrix vesicle function facilitates calcification by increasing alkaline phosphatase and phospholipase A2 specific activities as well as metalloproteinases which degrade proteoglycans.
ISSN:0171-967X
1432-0827
DOI:10.1007/s002239900096