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血清和胰岛素样生长因子-I对培养的牛关节软骨蛋白聚糖生物合成的刺激作用。

Stimulation of proteoglycan biosynthesis by serum and insulin-like growth factor-I in cultured bovine articular cartilage.

作者信息

McQuillan D J, Handley C J, Campbell M A, Bolis S, Milway V E, Herington A C

出版信息

Biochem J. 1986 Dec 1;240(2):423-30. doi: 10.1042/bj2400423.

Abstract

The addition of foetal calf serum to explant cultures of adult bovine articular cartilage is known to stimulate proteoglycan synthesis in a dose-dependent manner. We have now shown the activity in serum responsible for this effect to be heat- and acid-stable, to be associated with a high-Mr complex in normal serum but converted to a low-Mr form under acid conditions. The activity has an apparent Mr approximately 10,000 and isoelectric points similar to those reported for insulin-like growth factors (IGFs). Addition of a monoclonal antibody against insulin-like growth factor-I (IGF-I) prevented foetal calf serum from stimulating proteoglycan synthesis. Physiological concentrations of recombinant IGF-I or pharmacological levels of insulin when added to cartilage cultures mimicked the proteoglycan-stimulatory activity of serum. IGF-I appeared to act by increasing the rate of proteoglycan synthesis and did not change the nature of the proteoglycan synthesized nor the rate of proteoglycan catabolism by the tissue, suggesting that IGF-I may be important in the regulation of proteoglycan metabolism in adult articular cartilage. Furthermore, IGF-I can replace foetal calf serum in the culture medium, thereby allowing the use of a fully-defined medium which will maintain the synthesis and tissue levels of proteoglycan in adult articular cartilage explants for up to 5 days.

摘要

已知向成年牛关节软骨外植体培养物中添加胎牛血清会以剂量依赖的方式刺激蛋白聚糖合成。我们现已表明,血清中负责此效应的活性物质对热和酸稳定,在正常血清中与一种高分子量复合物相关,但在酸性条件下会转化为低分子量形式。该活性物质的表观分子量约为10,000,等电点与报道的胰岛素样生长因子(IGFs)相似。添加抗胰岛素样生长因子-I(IGF-I)的单克隆抗体可阻止胎牛血清刺激蛋白聚糖合成。向软骨培养物中添加生理浓度的重组IGF-I或药理水平的胰岛素可模拟血清的蛋白聚糖刺激活性。IGF-I似乎通过增加蛋白聚糖合成速率起作用,并且不会改变合成的蛋白聚糖的性质,也不会改变组织中蛋白聚糖分解代谢的速率,这表明IGF-I在成年关节软骨蛋白聚糖代谢的调节中可能很重要。此外,IGF-I可以替代培养基中的胎牛血清,从而允许使用完全确定的培养基,该培养基可使成年关节软骨外植体中的蛋白聚糖合成和组织水平维持长达5天。

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