C. Modricky scite author profile

C. Modricky

5Publications

102Citation Statements Received

35Citation Statements Given

How they've been cited

274

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Affiliations

University of Trieste

Publications

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Biochemical and immunohistochemical evidence that in cartilage an alkaline phosphatase is a Ca2+-binding glycoprotein.

Bernard¹,

Bianco²,

Bonucci³

et al. 1986

148

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A glycoprotein that exhibits alkaline phosphatase activity and binds Ca2+ with high affinity has been extracted and purified from cartilage matrix vesicles by fast protein liquid chromatography. Antibodies against this glycoprotein were used to analyze its distribution in chondrocytes and in the matrix of calcifying cartilage. Under the light microscope, using immunoperoxidase or immunofluorescence techniques, the glycoprotein is localized in chondrocytes of the resting zone. At this level, the extracellular matrix does not show any reaction. In the cartilage plate, between the proliferating and the hypertrophic region, a weak immune reactivity is seen in the cytoplasm, whereas in the intercolumnar matrix the collagen fibers appear clearly stained. Stained granular structures, distributed with a pattern similar to that of matrix vesicles, are also visible. Calcified matrix is the most stained area. These results were confirmed under the electron microscope using both immunoperoxidase and protein A-gold techniques. In parallel studies, enzyme activity was also analyzed by histochemical methods. Whereas resting cartilage, the intercellular matrix of the resting zone, and calcified matrix do not exhibit any enzyme activity, the zones of maturing and hypertrophic chondrocytes are highly reactive. Some weak reactivity is also shown by chondrocytes of the resting zone. The observation that this glycoprotein (which binds Ca2+ and has alkaline phosphatase activity) is synthesized in chondrocytes and is exported to the extracellular matrix at the time when calcification begins, suggests that it plays a specific role in the process of calcification.

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Determination of galactosyl hydroxylysine in urine as a means for the identification of osteoporotic women

Moro¹,

Modricky²,

Rovis³

et al. 1988

Maturitas

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High-performance liquid chromatographic analysis of urinary hydroxylysyl glycosides as indicators of collagen turnover

Moro¹,

Modricky²,

Stagni³

et al. 1984

Analyst

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Urinary β-1-galactosyl-0-hydroxylysine (GH) as a marker of collagen turnover of bone

Moro¹,

Mucelli

Gazzarrini³

et al. 1988

Calcif Tissue Int

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beta-1-galactosyl-0-hydroxylysine (GH) was measured in the urine of 59 women and 48 men, aged 30-79 years, by High Performance Liquid Chromatography (HPLC) of the dansylated derivative. Vertebral mineral density, measured by quantitative computed tomography (QCT), and urinary GH were inversely correlated (r = -0.74; P less than 0.001). High rate of bone mineral loss is associated with a high urinary GH excretion. Measurement of GH in urine provides a simple and noninvasive method for the evaluation of the extent of bone resorption in large groups of subjects and appears to be more specific than urinary hydroxyproline excretion.

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High-performance liquid chromatographic preparation of galactosyl-hydroxylsine, a specific bone collagen marker

Moro

Battista

Modricky

et al. 1989

Journal of Chromatography B: Biomedical Sciences and Applicatio

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C. Modricky

Biochemical and immunohistochemical evidence that in cartilage an alkaline phosphatase is a Ca2+-binding glycoprotein.

Determination of galactosyl hydroxylysine in urine as a means for the identification of osteoporotic women

High-performance liquid chromatographic analysis of urinary hydroxylysyl glycosides as indicators of collagen turnover

Urinary β-1-galactosyl-0-hydroxylysine (GH) as a marker of collagen turnover of bone

High-performance liquid chromatographic preparation of galactosyl-hydroxylsine, a specific bone collagen marker

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