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链球菌对透明质酸的生物合成。

Biosynthesis of hyaluronic acid by Streptococcus.

作者信息

Sugahara K, Schwartz N B, Dorfman A

出版信息

J Biol Chem. 1979 Jul 25;254(14):6252-61.

PMID:376529
Abstract

Synthesis of hyaluronic acid was investigated in a cell-free system derived from a strain of Group A streptococci. Preparative procedures were improved so that an enzyme system 70 times more active than that previously reported was obtained. The hyaluronic acid synthesized could be separated into trichloroacetic acid-soluble and -insoluble fractions. On the basis of pulse-chase experiments, it was shown that the trichloroacetic acid-insoluble fraction is a precursor of the soluble fraction. The release of the trichloroacetic acid-insoluble hyaluronic acid is specifically blocked with p-chloromercuribenzoate, without inhibition of chain elongation. The addition of butanol to trichloroacetic acid resulted in solubilization of all of the hyaluronic acid. No detectable difference in molecular size was observed between the two hyaluronic acid fractions, both of which were estimated to be more than one million daltons in size. Testicular hyaluronidase digestion of either one of the two types of hyaluronic acid yielded no high molecular weight fragments, indicating that hyaluronic acid is not bound covalently to protein. However, following incubation of enzyme assay mixtures with UDP-[14C]GlcUA, even in the absence of UDP-GlcNAc, radioactive high molecular weight hyaluronic acid was obtained which suggests that the enzyme system elongates rather than initiates hyaluronic acid chains. Tunicamycin did not inhibit hyaluronic acid synthesis, indicating lack of participation of an intermediate of pyrophosphorylpolyisoprenol type. The results obtained are consistent with the hypothesis that chain elongation of hyaluronic acid proceeds by alternate addition of monosaccharides from UDP-sugars by a membrane-bound synthesizing system followed by release of completed hyaluronic acid chains.

摘要

在源自A组链球菌菌株的无细胞系统中研究了透明质酸的合成。改进了制备程序,从而获得了比先前报道的活性高70倍的酶系统。合成的透明质酸可分为三氯乙酸可溶部分和不溶部分。基于脉冲追踪实验表明,三氯乙酸不溶部分是可溶部分的前体。对氯汞苯甲酸可特异性阻断三氯乙酸不溶透明质酸的释放,而不抑制链的延长。向三氯乙酸中加入丁醇会使所有透明质酸溶解。在两种透明质酸部分之间未观察到可检测到的分子大小差异,两者估计大小均超过一百万个道尔顿。两种类型的透明质酸中的任何一种经睾丸透明质酸酶消化均未产生高分子量片段,这表明透明质酸不是共价结合到蛋白质上。但是,即使在没有UDP-GlcNAc的情况下,将酶分析混合物与UDP-[14C]GlcUA一起孵育后,仍可获得放射性高分子量透明质酸,这表明该酶系统延长而不是起始透明质酸链。衣霉素不抑制透明质酸的合成,表明焦磷酸化聚异戊二烯类型的中间体未参与。获得的结果与以下假设一致:透明质酸的链延长是通过膜结合合成系统从UDP-糖交替添加单糖,然后释放完整的透明质酸链来进行的。

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