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The assay of xylosyltransferase in cartilage extracts. A modified procedure for preparation of Smith-degraded proteoglycan.

机译:软骨提取物中木糖基转移酶的测定。一种改良的制备史密斯降解蛋白聚糖的方法。

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摘要

A modification of the published method [Baker, Rodén & Stoolmiller (1972) J. Biol. Chem. 247, 3838--3847] for preparation of Smith-degraded proteoglycan is described. The new method is based on the finding that most of the chondroitin sulphate is cleaved from proteoglycan core protein by periodate oxidation. The borohydride reduction procedure was modified because the periodate-oxidized core protein is extensively degraded under the highly alkaline conditions previously used. The new method involves the separation of periodate-oxidized core protein from chondroitin sulphate by gel filtration on Sepharose 6B, and the reduction of the former in H3BO3/NaBH4 at pH 8.5 to produce the reduced species. Smith-degraded proteoglycan prepared by this method exhibited high acceptor activity for xylosyltransferase from embryonic-chick cartilage and had an apparent Km of 160 microgram/ml or 45 micrometer on a serine basis. In this assay system an apparent Km of 19 micrometer was obtained for UDP-xylose. The intermediate products periodate-oxidized core protein and reduced proteoglycen were inactive as xylosyltransferase acceptor substrates.
机译:公开方法的修改[Baker,Rodén&Stoolmiller(1972)J. Biol。化学[247,3838--3847]描述了用于制备史密斯降解的蛋白聚糖的方法。该新方法基于以下发现:大部分硫酸软骨素通过高碘酸氧化从蛋白聚糖核心蛋白上裂解下来。修改了硼氢化物的还原程序,因为高碘酸盐氧化的核心蛋白在先前使用的高度碱性条件下会大量降解。新方法涉及通过琼脂糖凝胶6B上的凝胶过滤从硫酸软骨素中分离出高碘酸盐氧化的核心蛋白,以及在pH 8.5的H3BO3 / NaBH4中还原前者以产生还原的物种。通过这种方法制备的史密斯降解蛋白聚糖对来自胚胎小鸡软骨的木糖基转移酶表现出高的受体活性,并且基于丝氨酸的表观Km为160微克/毫升或45微米。在该测定系统中,对于UDP-木糖,获得了19微米的表观Km。中间产物高碘酸盐氧化的核心蛋白和还原的蛋白聚糖作为木糖基转移酶受体底物没有活性。

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