Literature DB >> 2993364

Localization of collagenase in the growth plate of rachitic rats.

D D Dean, O E Muniz, I Berman, J C Pita, M R Carreno, J F Woessner, D S Howell.   

Abstract

In the transition from proliferation to hypertrophic cell zones in the growth plate, there is an increase in chondrocyte volume and a corresponding decrease in collagen content to accommodate the enlarging cells. It is postulated that collagenase accounts for this collagen loss. To test this hypothesis, tibial growth plates were obtained from normal rats, rachitic rats deficient in vitamin D and phosphate, and rats after 48 and 72 h of healing from rickets. Collagenase was quantitated by a pellet assay based on the release of solubilized collagen from the endogenous insoluble collagen in the tissue homogenates. A fourfold greater collagen release and a concomitant sixfold greater hypertrophic cell volume were measured in rachitic growth plates compared with normal age-matched controls. During healing of rickets, collagenase activity and hypertrophic cell volume returned almost to control levels. Rachitic growth plates were dissected into the juxtaepiphyseal 1/3 and the juxtametaphyseal 2/3. The latter portion contained greater than 95% of the hypertrophic cells and 86% of the collagenase. The collagen-degrading activity was extracted from this region and was shown to be a true collagenase by its production of typical A fragments of tropocollagen produced by collagenase action. The enzyme was activated by aminophenylmercuric acetate and trypsin and was inhibited by EDTA, 1,10-phenanthroline, and a tissue inhibitor of metalloproteinases from human articular cartilage. Inhibitors of aspartic, cysteine, and serine proteases had no effect. Micropuncture fluids aspirated from rachitic cartilage contained latent collagenase activity, indicating an extracellular localization. Negative tests for hemoglobin in the rachitic cartilage samples indicated that there was no contamination by capillaries and that this was not a source of collagenase. It is concluded that extracellular collagenase accounts for the loss of cartilage matrix in the hypertrophic zone, and that this process may be distinct from that of capillary invasion.

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Year:  1985        PMID: 2993364      PMCID: PMC423885          DOI: 10.1172/JCI112026

Source DB:  PubMed          Journal:  J Clin Invest        ISSN: 0021-9738            Impact factor:   14.808


  31 in total

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4.  The collagen substrate specificity of human skin fibroblast collagenase.

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5.  Persistence of Cartilage proteoglycan and link protein during matrix-induced endochondral bone development: an immunofluorescent study.

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6.  The extraction of a neutral metalloproteinase from the involuting rat uterus, and its action on cartilage proteoglycan.

Authors:  A Sellers; J F Woessner
Journal:  Biochem J       Date:  1980-09-01       Impact factor: 3.857

7.  Ultramicro spectrophotometric determination of calcium in biologic fluids.

Authors:  D S Howell; J C Pita; J F Marquez
Journal:  Anal Chem       Date:  1966-03       Impact factor: 6.986

8.  Demonstration of macromolecular inhibitors of calcification and nucleational factors in fluid from calcifying sites in cartilage.

Authors:  D S Howell; J C Pita; J F Marquez; R A Gatter
Journal:  J Clin Invest       Date:  1969-04       Impact factor: 14.808

9.  Identification of two further collagenous fractions from articular cartilage.

Authors:  M Shimokomaki; V C Duance; A J Bailey
Journal:  Biosci Rep       Date:  1981-07       Impact factor: 3.840

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Authors:  D S Howell; J C Pita; J F Marquez; J E Madruga
Journal:  J Clin Invest       Date:  1968-05       Impact factor: 14.808

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  15 in total

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Journal:  Endocrine       Date:  2001-04       Impact factor: 3.633

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Review 5.  Extracellular matrix roles during cardiac repair.

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Journal:  Life Sci       Date:  2010-07-27       Impact factor: 5.037

Review 6.  Neovascularisation and its role in the osteoarthritic process.

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7.  Matrix metalloproteinase-9 in a unique proteoglycan form in avian embryonic growth plate cartilage.

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8.  PTHrP overexpression partially inhibits a mechanical strain-induced arthritic phenotype in chondrocytes.

Authors:  D Wang; J M Taboas; R S Tuan
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9.  Phospholipases of mineralization competent cells and matrix vesicles: roles in physiological and pathological mineralizations.

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10.  Regional and temporal changes in the synthesis of matrix metalloproteinases and TIMP-1 during development of the rabbit mandibular condyle.

Authors:  J J Breckon; R M Hembry; J J Reynolds; M C Meikle
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