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器官培养中兔半月板新合成蛋白聚糖的特性研究

Characterization of newly synthesized proteoglycans from rabbit menisci in organ culture.

作者信息

Webber R J, Norby D P, Malemud C J, Goldberg V M, Moskowitz R W

出版信息

Biochem J. 1984 Aug 1;221(3):875-84. doi: 10.1042/bj2210875.

Abstract

Rabbit menisci were incubated with Na2 35SO4 in short-term organ culture to label newly synthesized proteoglycans. The radioactive products present in both tissue and culture medium were characterized separately with respect to distribution after ultracentrifugation in CsCl isopycnic density gradients, hydrodynamic size, interaction with hyaluronic acid, and glycosaminoglycan composition (types, size and content). Analysis of proteoglycan size by gel-filtration chromatography of the most-dense CsCl fractions (A1) on Sephacryl S-500 (associative conditions) resolved three species. A peak with Kav. approx. 0.7 was present in each chromatogram, and constituted the principal component in tissue extracts. Two other peaks with Kav. values of approx. 0.2 and 0.45 were also found. When the A1 fraction from tissue was subjected to CsCl-density-gradient ultracentrifugation under dissociative conditions, 71% of the recovered radioactivity was present in the most dense (A1D1) fraction. Incubation with hyaluronic acid of either A1 or A1D1 fraction from associative extract did not alter the apparent size of the labelled product, indicating a lack of aggregate formation. Meniscal proteoglycans showed an unusual and marked tendency to adsorb irreversibly to agarose and agarose-containing gel-filtration-chromatography media. High-pressure liquid-chromatographic analyses indicated that the sulphated glycosaminoglycans consisted of chondroitin 6-sulphate (72%), chondroitin 4-sulphate (19%) and dermatan sulphate (5%). Endo-beta-galactosidase (keratanase) digestion of the material failed to detect the presence of keratan sulphate. Of the labelled glycosaminoglycans, 95% was eluted from Sephacryl S-400 as a single symmetrical peak with a Kav. of 0.5. The results of studies with tissue extracts and culture medium were similar.

摘要

将兔半月板在短期器官培养中与Na2 35SO4一起孵育,以标记新合成的蛋白聚糖。分别通过在CsCl等密度密度梯度中进行超速离心后的分布、流体动力学大小、与透明质酸的相互作用以及糖胺聚糖组成(类型、大小和含量)来表征组织和培养基中存在的放射性产物。通过在Sephacryl S - 500(缔合条件)上对最致密的CsCl级分(A1)进行凝胶过滤色谱分析蛋白聚糖大小,解析出三种组分。每个色谱图中都出现了一个Kav约为0.7的峰,并且是组织提取物中的主要成分。还发现了另外两个Kav值约为0.2和0.45的峰。当来自组织的A1级分在解离条件下进行CsCl密度梯度超速离心时,71%的回收放射性存在于最致密的(A1D1)级分中。将缔合提取物中的A1或A1D1级分与透明质酸一起孵育不会改变标记产物的表观大小,表明没有聚集体形成。半月板蛋白聚糖表现出异常且明显的不可逆吸附到琼脂糖和含琼脂糖的凝胶过滤色谱介质上的倾向。高压液相色谱分析表明,硫酸化糖胺聚糖由6 - 硫酸软骨素(72%)、4 - 硫酸软骨素(19%)和硫酸皮肤素(5%)组成。用内切β - 半乳糖苷酶(角蛋白酶)消化该物质未检测到硫酸角质素的存在。在标记的糖胺聚糖中,95%从Sephacryl S - 400上以Kav为0.5的单个对称峰洗脱。组织提取物和培养基的研究结果相似。

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