ZIB

11

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Identification of phosphopeptides andγ-carboxyglutamic acid-containing peptides in epiphyseal growth plate cartilage (1979)

Glimcher, Melvin J. ; Kossiva, Dora ; Roufosse, Albert

Springer

Calcified tissue international 27 (1979), S. 187-191

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ISSN: 1432-0827

Keywords: Phosphopeptides ; γ-Carboxyglutamic Acid ; Calcified Cartilage ; Phosphoserine

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine , Physics

Notes: Summary Uncalcified cartilage from the epiphyseal portion of bovine scapulae, both distant and adjacent to the epiphyseal growth plate, and the calcified cartilage of the epiphyseal growth plate itself were analyzed for the presence of O-phosphoserine [Ser(P)], O-phosphothreonine [Thr(P)] and γ-carboxyglutamic acid (Gla). Only trace amounts of these Ca2+-binding amino acids or the peptides containing them were found in the unmineralized tissues. In contrast, whole calcified cartilage, and especially the most mineralized fraction obtained by density centrifugation, contained considerable amounts of all three amino acids. Essentially all of the Gla and the majority of the Ser(P) and Thr(P) were present in non-collagenous, non-diffusible proteins extractable in EDTA at near-neutral pH.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF02441183

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12

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Serine phosphate, threonine phosphate and γ-carboxyglutamic acid in normal and experimentally induced, pathologically calcified rat skin (topical cutaneous calciphylaxis) (1981)

Glimcher, Melvin J. ; Reit, Barry ; Kossiva, Dora

Springer

Calcified tissue international 33 (1981), S. 185-188

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ISSN: 1432-0827

Keywords: Calcification ; Calciphylaxis ; Skin ; Serine Phosphate ; Threonine Phosphate ; γ-Carboxyglutamic Acid

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine , Physics

Notes: Summary The amount of non-collagenous proteins is increased greatly during the pathological calcification of rat skin experimentally induced by dihydrotachysterol (DHT) and Ovalbumin (topical cutaneous calciphylaxis). This is accompanied by an increase in the total amount and concentrations of protein-bound serine phosphate [Ser(P)], threonine phosphate [Thr(P)] and γ-carboxyglutamic acid (Gla), almost all of which can be extracted from the tissue and can be dissociated from collagen in 0.5M EDTA. The EDTA-soluble, non-collagenous proteins are rich in aspartic and glutamic acids, similar to the non-collagenous, EDTA-soluble proteins of bone, cementum and calcified cartilage, and quite distinct from those of dentin and enamel.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF02409434

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13

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Mouse bone collagenase (1973)

Sakamoto, Seizaburo ; Goldhaber, Paul ; Glimcher, Melvin J.

Springer

Calcified tissue international 12 (1973), S. 247-258

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ISSN: 1432-0827

Keywords: Bone ; Collagenase ; Heparin ; Collagen

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine , Physics

Description / Table of Contents: Résumé La quantité de collagénase d'os de souris, obtenue dans un milieu de culture d'os, cultivéin vitro, est augmentée pas l'addition d'héparine à une concentration optimale d'environ 50 unités/ml de milieu de culture. Le sulfate de dextrane et le Treburon (un ester polysaccharide-sulfurique synthétique), qui sont voisins au point de vue chimique et structural à l'héparine, sont aussi efficaces que l'héparine pour augmenter la quantité de collagénase de l'os de souris, récupérée dans le milieu de culture. L'héparine, outre son action de stimulation de synthèse et/ou de libération de callogénase d'os de souris, augmente aussi l'activeté spicifique des préparations globales et purifiées de l'enzyme, dont l'activité est testée sur du collagène à l'état solide comme substrat. Aucune augmentation d'activité enzymatique n'est notée lorsque du collagène en solution est utilisé comme substrat. Le sulfate de dextrane est aussi effectif que l'héparine pour obtenir une augmentation de l'activité enzymatique, en utilisant le collagène solide comme substrat. Ni l'héparine ou le sulfate de dextrane augmente l'activité de la collagénase deClostridium histolyticum. Pour la première fois, une collagénase tissulaire purifiée dégrade et solubilise du collagène tissulaire non dénaturé et insoluble à 37° C. De plus, étant donné que cette action est nettement augmentée par l'addition d'héparine, il semble que cette dernière et des substances similaires peuvent jouer un rôle important dans la régulation de la dégradation collagénique pendant le remaniement des tissus collagéniquesin vivo.

Abstract: Zusammenfassung Die Menge von Mäuseknochen-Kollagenase, die sich im Gewebezucht-Medium vonin vitro gezüchteten Knochen wiederfindet, konnte durch Zusatz von Heparinat in einer optimalen Konzentration von ungefähr 50 E/ml Medium erhöht werden. Dextransulfat und Treburon (ein synthetischer Polysaccharid-Sulfatester), welche strukturmäßig und chemisch dem Heparin nahestehen, wirkten sich auf die Erhöhung der im Gewebezucht-Medium zurückgewonnenen Mäuseknochen-Kollagenase im gleichen Maße aus wie Heparin. Nebst der stimulierenden Wirkung auf die Synthese und/oder die Freisetzung von Mäuseknochen-Kollagenase vermochte Heparin auch die spezifische Aktivität von ungereinigten und von gereinigten Enzympräparaten zu erhöhen, wenn für den Versuch Kollagen in fester Form als Substrat verwendet wurde. Mit gelöstem Kollagen als Substrat trat diese Wirkung dagegen nicht ein. Dextransulfat zeigte die gleiche Wirksamkeit wie Heparin, indem es die Enzymaktivität zu erhöhen vermochte, wenn Kollagen in fester Form als Substrat vorlag. Weder Heparin noch Dextransulfat erhöhten die Aktivität der Kollagenase ausClostridium histolyticum. Erstmals konnte gezeigt werden, daß eine gereinigte Gewebe-Kollagenase in der Lage ist, nicht-denaturiertes, unlösliches Gewebekollagen bei 37° sowohl abzubauen als auch aufzulösen. Da diese Wirkung durch Zusatz von Heparin noch deutlich erhöht werden konnte, läßt sich überdies vermuten, daß Heparin und heparinähnlichen Substanzen bei der Regulierung des Kollagen-Abbaues während der Umgestaltung von Kollagengewebein vivo eine wichtige Rolle zufällt.

Notes: Abstract The amount of mouse bone collagenase recovered in the tissue culture medium of bone culturedin vitro was increased by the addition of heparin at an optimal concentration of approximately 50 units/ml of tissue culture medium. Dextran sulfate and Treburon (a synthetic polysaccharide-sulfuric ester) which are structurally and chemically related to heparin were as effective as heparin in increasing the amount of mouse bone collagenase recovered in the tissue culture medium. In addition to stimulating the synthesis and/or release of mouse bone collagenase, heparin was also found to increase the specific activity of both crude and purified preparations of the enzyme when assayed using collagen in the solid state as the substrate, but showed no enhancement of enzyme activity when assayed using collagen in solution as the substrate. Dextran sulfate was as effective as heparin in increasing the activity of the enzyme using collagen in the solid state as a substrate. Neither heparin or dextran sulfate enhanced the activity ofClostridium histolyticum collagenase. For the first time, a purified tissue collagenase has been shown to both degrade and solubilize undenatured, insoluble tissue collagen at 37°. Moreover, since this action was markedly enhanced by the addition of heparin, it suggests that heparin and similar substances may play an important role in the regulation of collagen degradation during the remodeling of collagenous tissuesin vivo.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF02013739

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14

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The inhibition of mouse bone collagenase by lysozyme (1974)

Sakamoto, Seizaburo ; Sakamoto, Masako ; Goldhaber, Paul ; [et al.]

Springer

Calcified tissue international 14 (1974), S. 291-299

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ISSN: 1432-0827

Keywords: Bone ; Collagenase ; Lysozyme

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine , Physics

Description / Table of Contents: Résumé Du lysozyme de blanc d'œuf, ainsi que des protéines basiques, telles que de l'histone et une base dépourvue de protamine, semblent inhiber la collagénase osseuse de souris. L'inhibition de collagénase osseuse de souris par le lysozyme est mise en évidence lorsque l'activité de la collagénase est étudiée en utilisant du collagène comme substrat à l'état solide, mais non lorsque le collagène est utilisé en solution. D'autre part, l'inhibition de l'activité en collagénase par l'histone et une base dépourvue de protamine est observée dans les deux systèmes. L'inhibition de collagénase ossuese de souris par des molécules polyanioniques est intéressante, étant donné que des travaux antérieurs ont montré que plusieurs molécules polyanioniques telles que l'héparine, le sulfate de dextrane et l'acide polyethylenesulfonique augmentent l'activité de collagénase osseuse de souris dans les mêmes conditions expérimentales. Comme le lysozyme est largement présent dans les tissus conjonctifs et que sa concentration carie avec l'ampleur du remaniement tissulaire, l'inhibition de la collagénase osseuse de souris suggère un role éventuel dans la régulation de la dégradation du collagène, pendant le remaniement des tissus collagéniquesin vivo au cours d'états normaux et pathologiques.

Abstract: Zusammenfassung Lysozyme aus Hühnereiweiß sowie Basis-Proteine, wie z. B. Histon und Protamin-freie Basen, erwiesen sich als Hemmer der Mäuseknochen-Kollagenase. Diese Hemmung durch Lysozym wurde festgestellt, wenn für die Messung der Kollagenase-Aktivität Kollagen in Substanz als Substrat verwendet wurde, nicht aber, wenn das Substrat aus gelöstem Kollagen bestand. Andererseits wurde die Hemmung der Kollagenase-Aktivität durch Histon und Protamin-freie Basen in beiden Versuchssystemen festgestellt. Die Hemmung von Mäuseknochen-Kollagenase durch polykationische Moleküle ist interessant, vor allem im Hinblick auf frühere Feststellungen, daß mehrere polyanionische Moleküle, wie Heparin, Dextransulfat und Polyaethylensulfonsäure, die Aktivität der Mäuseknochen-Kollagenase unter denselben experimentellen Bedingungen erhöhen. Da Lysozym in Bindegeweben überall verteilt ist und da dessen Konzentration mit der Neubildungsrate des Gewebes variiert, läßt die Hemmung der Mäuseknochen-Kollagenase durch Lysozym dessen mögliche Rolle in der Regulierung des Kollagenabbaues vermuten, und zwar während der Neubildung von Kollagengeweben in vivo in normalen und pathologischen Zuständen.

Notes: Abstract Egg white lysozyme, as well as basic proteins such as histone and protamine-free base, were found to inhibit mouse bone collagenase. The inhibition of mouse bone collagenase by lysozyme was detected when the activity of the collagenase was assayed using collagen as the substrate in the solid state, but not when the collagenase activity was assayed using collagen in solution as the substrate. On the other hand, the inhibition of collagenase activity by histone and protamine-free base was observed in both assay systems. The inhibition of mouse bone collagenase by polycationic molecules is interesting in light of previous findings that several polyanionic molecules, such as heparin, dextran sulfate and polyethylenesulphonic acid, enhance the activity of mouse bone collagenase under the same experimental conditions. Since lysozyme is widely distributed in connective tissues and its concentration varies with the rate of tissue remodeling, the inhibition of mouse bone collagenase by lysozyme suggests its possible role in the regulation of collagen degradation during the remodeling of collagenous tissuesin vivo during normal and pathological states.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF02060303

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15

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Phosphopeptides and γ-carboxyglutamic acid-containing peptides in calcified turkey tendon: Their absence in uncalcified tendon (1979)

Glimcher, Melvin J. ; Brickley-Parsons, Diane ; Kossiva, Dora

Springer

Calcified tissue international 27 (1979), S. 281-284

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ISSN: 1432-0827

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine , Physics

Notes: Summary Uncalcified samples of turkey tendon obtained prior to calcification, and other samples from areas of tendon that never calcify, contain little or no 0-phosphoserine [Ser(P)], 0-phosphothreonine [Thr(P)] and γ-carboxyglutamic acid (Gla). Significant amounts of all three of these Ca2+-binding amino acids, which are found in EDTA-extractable, non-collagenous proteins, are detected coincident with the onset of mineralization of a tendon and increase in concentration as mineralization proceeds.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF02441198

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16

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Identification of O-phosphoserine, O-phosphothreonine and γ-carboxyglutamic acid in the non-collagenous proteins of bovine cementum; comparison with dentin, enamel and bone (1979)

Glimcher, Melvin J. ; Lefteriou, Beatrice ; Kossiva, Dora

Springer

Calcified tissue international 28 (1979), S. 83-86

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ISSN: 1432-0827

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine , Physics

Notes: Summary O-phosphoserine [Ser(P)], O-phosphothreonine [Thr(P)], and γ-carboxyglutamic acid (Gla) have been identified in native, calcified cementum and in non-collagenous proteins which can be extracted from the tissue in EDTA at neutral pH. The concentrations of Ser(P) and Thr(P) and the amino acid composition of the EDTA extractable proteins are more similar to those found in bone than in dentin or enamel. The concentration of Gla in cementum is lower than it is in bone and higher than it is in enamel, which contains essentially no Gla. Based on the contents of Gla in these mineralized tissues and the distribution of alkaline and acid phosphatases in these tissues, it is speculated that Gla may be part of these or other proenzymes rather than being involved directly and structurally with the deposition of the mineral phase.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF02441222

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17

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X-ray diffraction radial distribution function studies on bone mineral and synthetic calcium phosphates (1984)

Grynpas, M. D. ; Bonar, L. C. ; Glimcher, Melvin J.

Springer

Journal of materials science 19 (1984), S. 723-736

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ISSN: 1573-4803

Source: Springer Online Journal Archives 1860-2000

Topics: Mechanical Engineering, Materials Science, Production Engineering, Mining and Metallurgy, Traffic Engineering, Precision Mechanics

Notes: Abstract An investigation of the molecular structure of bone mineral and synthetic calcium phosphates was carried out using radial distribution function (RDF) techniques. The X-ray data were collected using CuKα and MoKα radiation to insure the validity of the RDFs. Synthetic preparations of hydroxyapatite (HA) varying in their crystal size and crystallinity, and amorphous calcium phosphate (ACP), were studied, as well as bone samples from a 1-year-old chicken and 16-day embryonic chicks. Mixtures of embryonic bone and synthetic ACP were also investigated. The RDFs of bone and crystalline HA samples are similar in peak position, and show evidence of an atomic order extending to 2.5 nm and beyond. The RDF of ACP differs from that of HA, showing only short range order up to 0.9 nm, as well as small differences in peak shape. The decrease in intensity of the RDF function with increasing distance (r), observed with both HA and bone samples can be related to a decrease in crystallinity and crystal size. The RDF data indicate there is no significant amount of ACP in either very young or mature bone. The RDFs of the embryonic bone + synthetic ACP mixtures showed that a small amount of ACP can be readily detected in a sample of bone with a poorly crystalline mineral phase; from this we estimate the threshold for detection of ACP in bone to be 12% or less.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00540442

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Mechanism of calcification: Role of collagen fibrils and collagen-phosphoprotein complexes in vitro and in vivo (1989)

Glimcher, Melvin J.

New York, NY [u.a.] : Wiley-Blackwell

The @Anatomical Record 224 (1989), S. 139-153

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ISSN: 0003-276X

Keywords: Life and Medical Sciences ; Cell & Developmental Biology

Source: Wiley InterScience Backfile Collection 1832-2000

Topics: Medicine

Notes: Samples of decalcified chicken bone together with varying concentrations of phosphoproteins from bone or egg yolk (phosvitin) were used in vitro as heterogenous nucleators for the induction of Ca-P apatite crystals. The lag time between exposure of the collagen-phosphoprotein complexes and the time nucleation of crystals occurred decreased as the concentration of Ser(P) and Thr(P) increased. Enzymatic cleavage of the phosphate groups by wheat germ and phosphatase reversed this effort, indicating that the phosphate group per se principally facilitated the nucleation of Ca-P crystals by the phosphoprotein complex and collagen.

Additional Material: 3 Ill.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1002/ar.1092240205

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19

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In situ hybridization studies suggest a role for the basic region-leucine zipper protein hXBP-1 in exocrine gland and skeletal development during mouse embryogenesis (1993)

Clauss, Isabelle M. ; Gravallese, Ellen M. ; Darling, Jama M. ; [et al.]

New York, NY [u.a.] : Wiley-Blackwell

Developmental Dynamics 197 (1993), S. 146-156

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ISSN: 1058-8388

Keywords: Embryonic development ; hXBP-1 ; Basic domain/leucine zipper protein ; Pancreas ; Salivary glands ; TIMP ; Alkaline phosphatase ; Life and Medical Sciences ; Cell & Developmental Biology

Source: Wiley InterScience Backfile Collection 1832-2000

Topics: Medicine

Notes: The spatial and temporal distribution of transcripts for the TRE/CRE-binding basic region-leucine zipper protein hXBP-1 was determined by in situ hybridization. Analysis of embryos from day 10.5 to 18.5 pc revealed high level expression of hXBP-1 RNA in two developing organ systems: (1) in bone and cartilage cells of the developing skeleton and toothbuds, and (2) in exocrine glands including the pancreas and the submandibular and salivary glands. High level expression was also found in whisker follicles and in selected cells in brown adipose tissue. In the developing skeleton, hXBP-1 RNA was expressed starting on day 11.5 pc in osteoblasts of newly formed intramembranous bone. Thereafter, hXBP-1 was expressed in both osteoblasts and preosteoblasts in bone formed directly by intramembranous formation as well as in bone formed during endochondral ossification. The most intese signal was observed in preosteoblasts and osteoblasts of newly forming bone. At day 11.5 pc low level hXBP-1 expression was also observed in matrix secreting chondroblasts of bones which are formed initially of cartilage, at the stage where they consist entirely of cartilage, at the stage where they consist entirely of cartilage. Signal was also present in matrix producing chondroblasts of the mature zone of the growth region during endochondral ossification although at significantly lower level than in osteoblasts. hXBP-1 is thus the first transcription factor described, to our knowledge, whose level of expression is modulated during the osteoblast developmental sequence in vivo. The pattern of expression of hXBP-1 in the developing skeleton was found to be very similar to that of the genes encoding the tissue inhibitor of metalloproteinase and alkaline phosphatase throughout development. These observations suggest that hXBP-1 may play a role in regulating the expression of tissue specific genes (TIMP, osteonectin, osteopontin, osteocalcin) expressed in osteoblasts. It is intriguing that the promoter regions of several such genes contain potential hXBP-1 binding sites. © 1993 Wiley-Liss, Inc.

Additional Material: 5 Ill.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1002/aja.1001970207

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A mixed β-turn and β-sheet structure for bovine tooth enamel amelogenin: Raman spectroscopic evidence (1987)

Zheng, Siding ; Tu, Antony T. ; Renugopalakrishnan, V. ; [et al.]

New York : Wiley-Blackwell

Biopolymers 26 (1987), S. 1809-1813

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ISSN: 0006-3525

Keywords: Chemistry ; Polymer and Materials Science

Source: Wiley InterScience Backfile Collection 1832-2000

Topics: Chemistry and Pharmacology

Additional Material: 2 Ill.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1002/bip.360261012

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