4.4 Article

Osteopontin deficiency increases mineral content and mineral crystallinity in mouse bone

Journal

CALCIFIED TISSUE INTERNATIONAL
Volume 71, Issue 2, Pages 145-154

Publisher

SPRINGER-VERLAG
DOI: 10.1007/s00223-001-1121-z

Keywords

osteopontin; infrared microspectroscopy; infrared imaging; bone mineral; apatite; biomineralization

Funding

  1. NIDCR NIH HHS [DE04141] Funding Source: Medline

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Fourier transform infrared microspectroscopy (FTIRM) and infrared imaging (FTIRI) were used to characterize the mineral in bones of two different lines of Opn-deficient (Opn-/-) mice and their background-matched wild-type controls (Opn+/+). Sections of tibia and femur from 12-week-old and 16-week-old mice were evaluated with a spatial resolution between 10 mum (FTIRM) and 7 mum (FTIRI). FTIRI was used to examine 400 mum x 400 mum areas in cortical bone and trabecular bone and FTIRM examined selected 20 mum x 20 mum areas at sites within these anatomically defined areas. Despite the absence of an obvious phenotype in Opn-deficient mice, being undetectable by radiographic and histological methods, FTIRM analyses revealed that the relative amount of mineral in the more mature areas of the bone (central cortical bone) of Opn-knockout mice was significantly increased. Moreover, mineral maturity (mineral crystal size and perfection) throughout all anatomic regions of the Opn-deficient bone was significantly increased. The 2-dimensional, color-coded data (images) produced by FTIRI showed similar increases in mineral maturity in the Opn-/- bone, however, the crystallinity parameters were less sensitive, and significance was not achieved in all areas analyzed. Nonetheless, the findings of increased mineral content and increased crystal size/perfection in both lines of Opn-deficient mice at both ages are consistent with in vitro data indicating that Opn is a potent inhibitor of mineral formation and mineral crystal growth and proliferation, and also support a role for Opn in osteoclast recruitment and function.

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