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首页> 外文期刊>Analytical Biochemistry: An International Journal of Analytical and Preparative Methods >Profiling glycol-split heparins by high-performance liquid chromatography/mass spectrometry analysis of their heparinase-generated oligosaccharides
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Profiling glycol-split heparins by high-performance liquid chromatography/mass spectrometry analysis of their heparinase-generated oligosaccharides

机译:通过高效液相色谱/质谱分析其肝素酶生成的寡糖来分析乙二醇裂解的肝素

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摘要

Glycol-split (gs) heparins, obtained by periodate oxidation/borohydride reduction of heparin currently used as an anticoagulant and antithrombotic drug, are arousing increasing interest in anticancer and anti-inflammation therapies. These new medical uses are favored by the loss of anticoagulant activity associated with glycol-splitting-induced inactivation of the antithrombin III (AT) binding site. The structure of gs heparins has not been studied yet in detail. In this work, ion pair reversed-phase high-performance liquid chromatography (IPRP-HPLC) coupled with electrospray ionization mass spectrometry (ESI-MS) widely used for unmodified heparin has been adapted to the analysis of oligosaccharides generated by digestion with heparinases of gs heparins usually prepared from porcine mucosal heparin. The method was also found to be very effective in analyzing gs derivatives obtained from heparins of different animal and tissue origins. Besides the major 2-O-sulfated disaccharides, heparinase digests of gs heparins contain mainly tetra- and hexasaccharides incorporating one or two gs residues, with distribution patterns typical for individual gs heparins. A heptasulfated, mono-N-acetylated hexasaccharide with two gs residues was shown to be a marker of the gs-modified AT binding site within heparin chains.
机译:通过高碘酸氧化/硼氢化物还原肝素(目前用作抗凝剂和抗血栓形成药物)获得的乙二醇裂解(gs)肝素引起了人们对抗癌和抗炎治疗的日益增长的兴趣。这些新的医学用途因与乙二醇裂解引起的抗凝血酶III(AT)结合位点失活有关的抗凝活性丧失而受到青睐。 gs肝素的结构尚未被详细研究。在这项工作中,广泛用于未修饰肝素的离子对反相高效液相色谱(IPRP-HPLC)结合电喷雾电离质谱(ESI-MS)已被用于分析gs肝素酶消化产生的寡糖肝素通常由猪粘膜肝素制备。还发现该方法在分析从不同动物和组织来​​源的肝素获得的gs衍生物方面非常有效。除主要的2-O硫酸化二糖外,gs肝素的肝素酶消化液主要含有四糖和六糖,其中掺入一个或两个gs残基,典型的分布模式为单个gs肝素。显示具有两个gs残基的七硫酸盐化,单N-乙酰化的六糖是肝素链中gs修饰的AT结合位点的标志物。

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