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首页> 外文期刊>Journal of cell biology >The calcification of cartilage matrix in chondrocyte culture: studies of the C-propeptide of type II collagen (chondrocalcin).
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The calcification of cartilage matrix in chondrocyte culture: studies of the C-propeptide of type II collagen (chondrocalcin).

机译:软骨细胞培养中软骨基质的钙化:II型胶原蛋白(Chondrocalcin)的C肽研究。

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We have shown that when chondrocytes are isolated by collagenase digestion of hyaline cartilage from growth plate, nasal, and epiphyseal cartilages of bovine fetuses they rapidly elaborate an extracellular matrix in culture. Only growth plate chondrocytes can calcify this matrix as ascertained by incorporation of 45Ca2+, detection of mineral with von Kossa's stain and electron microscopy. There is an extremely close direct correlation between 45Ca2+ incorporation in the first 24 h of culture and the content of the C-propeptide of type II collagen, measured by radioimmunoassay, at the time of isolation and during culture. Moreover, growth plate cells have an increased intracellular content of the C-propeptide per deoxyribonucleic acid and, during culture, per hydroxyproline (as a measure of helical collagen) compared with nasal and epiphyseal chondrocytes. In growth plate chondrocytes 24,25-dihydroxycholecalciferol (24,25-[OH]2D3), but not 1,25-dihydroxycholecalciferol alone, stimulates the net synthesis of the C-propeptide and calcification; proteoglycan net synthesis is unaffected. Together, these metabolites of vitamin D further stimulate C-propeptide net synthesis but do not further increase calcification stimulated by 24,25-(OH)2D3. These observations further demonstrate the close correlation between the C-propeptide of type II collagen and the calcification of cartilage matrix.
机译:我们已经表明,当通过生长板的生长板,鼻腔和骨骺软骨的酸蛋白酶消化分离软骨蛋白酶,它们在培养中迅速详细阐述细胞外基质。只有通过掺入45ca2 +,刚刚通过掺入von kossa的染色和电子显微镜的矿物检测,才能钙化该基质。在分离和培养期间,在培养的前24小时内,在培养的前24小时和II型胶原肽的含量之间存在极其紧密的直接相关性。此外,生长板细胞每脱氧核糖核酸的C肽的细胞内含量增加,并且在与鼻和骨骺软骨细胞相比的每羟脯氨酸(作为螺旋胶原蛋白)的培养物期间。在生长蛋白质中软骨细胞24,25-二羟基吡啶吡喃(24,25- [OH] 2D3),但单独的不是1,25-二羟基胆嘧啶,刺激C肽和钙化的净合成;蛋白生成的净合成不受影响。这些代谢物在一起,维生素D的这种代谢物进一步刺激C肽净合成,但不再进一步增加钙化刺激24,25-(OH)2D3。这些观察结果进一步证明了II型胶原蛋白的C肽与软骨基质的钙化之间的紧密相关性。

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