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肝素在小鼠肥大细胞瘤组织中的降解

Degradation of heparin in mouse mastocytoma tissue.

作者信息

Ogren S, Lindahl U

出版信息

Biochem J. 1971 Dec;125(4):1119-29. doi: 10.1042/bj1251119.

Abstract
  1. Heparin was prepared from mouse mastocytoma tissue by mild procedures, including extraction of mast-cell granules with 2m-potassium chloride, precipitation of the extracted polysaccharide with cetylpyridinium chloride from 0.8m-potassium chloride and finally digestion of the isolated material with testicular hyaluronidase. The resulting product (fraction GE(H)) represented approx. 40% of the total heparin content of the tissue. 2. Fraction GE(H) was fractionated by gel chromatography on Sepharose 4B into three subfractions, with average molecular weights ( M(w)) of approx. 60000-70000 (highly polydisperse material), 26000 and 9000 respectively. Treatment of each of the subfractions with alkali or with papain did not affect their behaviour on gel chromatography. Amino acid and neutral sugar analyses indicated that the two low-molecular-weight fractions consisted largely of single polysaccharide chains lacking the carbohydrate-protein linkage region. It was suggested that these heparin molecules had been degraded by an endopolysaccharidase. 3. Pulse labelling in vivo of mastocytoma heparin with [(35)S]sulphate showed initial labelling of large molecules followed by a progressive shift of radioactivity toward fractions of lower molecular weight. Further, heparin-depolymerizing activity was demonstrated by incubating (35)S-labelled heparin in vitro with a mastocytoma 10000g-supernatant fraction. Appreciable degradation of the polysaccharide occurred, as demonstrated by gel chromatography. In contrast, no depolymerization was observed on subjecting (14)C-labelled chondroitin sulphate to the same procedure.
摘要
  1. 肝素是通过温和的程序从小鼠肥大细胞瘤组织中制备的,包括用2M氯化钾提取肥大细胞颗粒,从0.8M氯化钾中用十六烷基吡啶氯化物沉淀提取的多糖,最后用睾丸透明质酸酶消化分离出的物质。所得产物(组分GE(H))约占组织中肝素总含量的40%。2. 组分GE(H)通过在琼脂糖4B上进行凝胶色谱分离为三个亚组分,平均分子量(M(w))分别约为60000 - 70000(高度多分散物质)、26000和9000。用碱或木瓜蛋白酶处理每个亚组分均不影响它们在凝胶色谱上的行为。氨基酸和中性糖分析表明,两个低分子量组分主要由缺乏碳水化合物 - 蛋白质连接区的单多糖链组成。有人提出这些肝素分子已被一种内切多糖酶降解。3. 用[³⁵S]硫酸盐对肥大细胞瘤肝素进行体内脉冲标记显示,大分子最初被标记,随后放射性逐渐向较低分子量组分转移。此外,通过将³⁵S标记的肝素与肥大细胞瘤10000g上清液组分在体外孵育,证明了肝素解聚活性。如凝胶色谱所示,多糖发生了明显降解。相比之下,对¹⁴C标记的硫酸软骨素进行相同操作未观察到解聚现象。

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Biochem Pharmacol. 1963 Jun;12:588-90. doi: 10.1016/0006-2952(63)90137-0.
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Arch Biochem Biophys. 1961 Feb;92:224-31. doi: 10.1016/0003-9861(61)90341-1.
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