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通过添加透明质酸钠抑制白细胞介素1介导的牛关节软骨外植体中蛋白聚糖的降解。

Inhibition of interleukin 1-mediated proteoglycan degradation in bovine articular cartilage explants by addition of sodium hyaluronate.

作者信息

Morris E A, Wilcon S, Treadwell B V

机构信息

Department of Medicine, Tufts University School of Veterinary Medicine, North Grafton, MA 01536.

出版信息

Am J Vet Res. 1992 Nov;53(11):1977-82.

PMID:1466488
Abstract

The effect of exogenous hyaluronate on normal cartilage metabolism and interleukin-1 (IL-1)-induced cartilage matrix degradation was investigated in a bovine cartilage explant culture system. Addition of hyaluronate at a concentration of 1.5 mg/ml to cartilage culture explants consistently decreased normal proteoglycan release from the matrix to a value less than that found in control cultures. Addition of 1.5 mg of hyaluronate/ml to IL-1 stimulated cartilage culture systems reduced proteoglycan release from the matrix by 83 to 113%. The reduction in control and IL-1-stimulated proteoglycan degradation by hyaluronate had a concentration-dependent trend. Evaluation of alterations in protein (enzyme) release by IL-1-stimulated chondrocytes after introduction of hyaluronate was evaluated by use of sodium dodecyl sulfate agar gel electrophoresis of cartilage-conditioned media. The quantity or the molecular weight profile of IL-1-induced proteins did not differ after introduction of hyaluronate into the culture system. Results indicate that introduction of high molecular weight hyaluronate into cartilage culture systems results in a decrease in proteoglycan release from the matrix in control systems, as well as in cultures incubated with IL-1. Because IL-1-stimulated protein synthesis by chondrocytes remains unchanged after addition of exogenous hyaluronate, the mechanism of inhibition of matrix degradation does not appear to be interference with binding of IL-1 to chondrocytes or to be inhibition of the production of neutral metalloproteases, including stromelysin.

摘要

在牛软骨外植体培养系统中研究了外源性透明质酸盐对正常软骨代谢及白细胞介素-1(IL-1)诱导的软骨基质降解的影响。向软骨培养外植体中添加浓度为1.5mg/ml的透明质酸盐,始终能使基质中正常蛋白聚糖的释放量降低至低于对照培养物中的水平。向IL-1刺激的软骨培养系统中添加1.5mg/ml透明质酸盐,可使基质中蛋白聚糖的释放减少83%至113%。透明质酸盐对对照及IL-1刺激的蛋白聚糖降解的降低具有浓度依赖性趋势。通过对软骨条件培养基进行十二烷基硫酸钠琼脂凝胶电泳,评估了添加透明质酸盐后IL-1刺激的软骨细胞释放蛋白质(酶)的变化。将透明质酸盐引入培养系统后,IL-1诱导的蛋白质的量或分子量分布没有差异。结果表明,将高分子量透明质酸盐引入软骨培养系统会导致对照系统以及与IL-1一起孵育的培养物中基质蛋白聚糖释放减少。由于添加外源性透明质酸盐后,IL-1刺激的软骨细胞蛋白质合成保持不变,因此抑制基质降解的机制似乎不是干扰IL-1与软骨细胞的结合,也不是抑制包括基质溶解素在内的中性金属蛋白酶的产生。

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