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体外研究生长板钙化之前及钙化时的细胞和基质变化:X型胶原蛋白合成停滞,钙化开始时胶原蛋白净损失。

Cellular and matrix changes before and at the time of calcification in the growth plate studied in vitro: arrest of type X collagen synthesis and net loss of collagen when calcification is initiated.

作者信息

Alini M, Carey D, Hirata S, Grynpas M D, Pidoux I, Poole A R

机构信息

Joint Diseases Laboratory, Shriners Hospital for Crippled Children, Montreal, Canada.

出版信息

J Bone Miner Res. 1994 Jul;9(7):1077-87. doi: 10.1002/jbmr.5650090716.

Abstract

To understand the growth, maturation, and regulation of growth plate chondrocytes, it is necessary to isolate the different chondrocytes into distinct subpopulations of maturational development. Five subpopulations (A-E) of bovine fetal growth plate chondrocytes were separated by discontinuous gradient centrifugation. Four subpopulations (B, C, D, and E, from low to high density) with good viability were cultured at high density in microwells for up to 30 days. They all established an extensive extracellular matrix composed of proteoglycan and collagen. The largest and last dense cells in subpopulation B were the first to synthesize (at days 5-6) type X collagen and to calcify this matrix. Matrix calcification (formation of hydroxyapatite in the presence of sodium beta-glycerophosphate) always followed the initiation of type X synthesis. All the other subpopulations synthesized type X collagen and calcified their extracellular matrix. Although these events occurred in the same order, they were delayed according to the order of increasing cell size. These observations indicate that these subpopulations represent different stages in cellular maturation that lead to expression of the hypertrophic phenotype. Once mineral formation was well established, there was an increase in the matrix content of the C-propeptide of type II collagen (which is known to bind to hydroxyapatite and accumulate in calcifying extracellular matrix). This was accompanied by a reduction in the total collagen content, which accompanied an abrupt reduction in type X collagen synthesis, whereas type II collagen synthesis was largely maintained. These reductions in collagen content and type II collagen synthesis were not observed in the absence of calcification (beta-glycerophosphate omitted from culture). This new culture system recreates many of the sequential cellular and extracellular changes exhibited in situ during the development of the physis and provides new information about cellular and extracellular matrix changes that occur before and at the time of calcification.

摘要

为了解生长板软骨细胞的生长、成熟及生长调节机制,有必要将不同的软骨细胞分离成成熟发育的不同亚群。通过不连续梯度离心法分离出牛胎儿生长板软骨细胞的五个亚群(A - E)。将四个活力良好的亚群(B、C、D和E,从低密度到高密度)在微孔板中进行高密度培养,长达30天。它们都形成了由蛋白聚糖和胶原蛋白组成的广泛细胞外基质。亚群B中最大且最致密的细胞最先(在第5 - 6天)合成X型胶原蛋白并使该基质钙化。基质钙化(在β - 甘油磷酸钠存在下形成羟基磷灰石)总是在X型胶原蛋白合成开始之后发生。所有其他亚群都合成X型胶原蛋白并使其细胞外基质钙化。尽管这些事件按相同顺序发生,但根据细胞大小增加的顺序而延迟。这些观察结果表明,这些亚群代表细胞成熟的不同阶段,这些阶段导致肥大表型的表达。一旦矿物质形成充分建立,II型胶原蛋白C - 前肽的基质含量就会增加(已知其与羟基磷灰石结合并积聚在钙化的细胞外基质中)。这伴随着总胶原蛋白含量的减少,同时伴随着X型胶原蛋白合成的突然减少,而II型胶原蛋白合成在很大程度上得以维持。在没有钙化的情况下(培养中省略β - 甘油磷酸钠)未观察到胶原蛋白含量和II型胶原蛋白合成的这些减少。这种新的培养系统重现了在生长板发育过程中原位表现出的许多连续的细胞和细胞外变化,并提供了有关钙化之前和钙化时发生的细胞和细胞外基质变化的新信息。

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