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人软骨溶菌酶

Human cartilage lysozyme.

作者信息

Greenwald R A, Josephson A S, Diamond H S, Tsang A

出版信息

J Clin Invest. 1972 Sep;51(9):2264-70. doi: 10.1172/JCI107035.

Abstract

The lysozyme content of human cartilage was measured by incubation of lyophilized, powdered cartilage in a variety of buffers and salt solutions, and the factors controlling the binding of lysozyme within cartilage were studied. Lysozyme was extracted from hyaline cartilage by buffers of pH greater than 9.0 by solutions 1 M in monovalent cations, and by solutions 0.12-0.40 M in divalent cations. The ability of cations to extract lysozyme from cartilage agreed with their known affinities for binding to chondroitin sulfate. The total extractable lysozyme content of five samples of human costal cartilage ranged from 1.45 to 3.36 mug lysozyme per mg of cartilage; for five samples of hyaline cartilage from peripheral joints the range was 0.80-3.03 mug lysozyme per mg of cartilage. Cartilage incubated in excess exogenous lysozyme could bind 0.053 equivalents of lysozyme per equivalent of chondroitin sulfate. Fibrocartilage and synovium from knee joints yielded no detectable lysozyme, despite the fact that synovium, a tissue rich in lysosomes, contained measurable quantities of beta-glucuronidase. Lysozyme extraction from cartilage was not augmented by incubation with streptolysin S. When incubation was carried out with mild extraction techniques, lysozyme extraction from cartilage tended to parallel uronic acid release, both as a function of time and from one specimen to another. The active material as lysozyme. Lysozyme occurs in human hyaline cartilage as a counterion to polyanionic glycosaminoglycans. Carextracted from cartilage met five criteria for identification tilage lysozyme appears to be extracellular and nonlysosomal. Degradation of cartilage may contribute to the increased serum and synovial fluid lysozyme levels often present in patients with rheumatoid arthritis.

摘要

通过将冻干的粉末状软骨在多种缓冲液和盐溶液中孵育来测量人软骨中的溶菌酶含量,并研究控制溶菌酶在软骨内结合的因素。pH大于9.0的缓冲液、1M单价阳离子溶液以及0.12 - 0.40M二价阳离子溶液可从透明软骨中提取溶菌酶。阳离子从软骨中提取溶菌酶的能力与其已知的与硫酸软骨素结合的亲和力一致。五个样本的人肋软骨中可提取的溶菌酶总量为每毫克软骨1.45至3.36微克溶菌酶;五个外周关节透明软骨样本的范围是每毫克软骨0.80 - 3.03微克溶菌酶。在过量外源性溶菌酶中孵育的软骨每当量硫酸软骨素可结合0.053当量的溶菌酶。膝关节的纤维软骨和滑膜未检测到溶菌酶,尽管滑膜是富含溶酶体的组织,含有可测量量的β - 葡萄糖醛酸酶。用链球菌溶血素S孵育并不会增加从软骨中提取的溶菌酶量。当采用温和提取技术进行孵育时,从软骨中提取溶菌酶的量在时间上以及从一个样本到另一个样本上都倾向于与糖醛酸释放平行。活性物质为溶菌酶。溶菌酶在人透明软骨中作为多阴离子糖胺聚糖的抗衡离子存在。从软骨中提取的溶菌酶符合鉴定的五个标准。软骨溶菌酶似乎是细胞外的且非溶酶体的。软骨降解可能导致类风湿性关节炎患者血清和滑液中溶菌酶水平经常升高。

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