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首页> 外文期刊>Thrombosis Research: An International Journal on Vascular Obstruction, Hemorrhage and Hemostasis >Antithrombin and first complement protein recognize the same active heparin fraction.
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Antithrombin and first complement protein recognize the same active heparin fraction.

机译:抗凝血酶和第一补体蛋白识别相同的活性肝素级分。

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Antithrombin (AT) high affinity of unfractionated heparin (UFH) resides in a specific pentasaccharide sequence. Heparin also regulates complement activity on the classical and the alternative pathways. Most experimental pieces of evidence accumulated show that these important activities reside in different segments of the heparin molecule. We demonstrated in previous papers that a low ionic strength and the presence of calcium ions are essential to detect specific interactions between glycosaminoglycans and proteins. Then these very strict conditions were used, and we demonstrated that the first protein complex of the human complement cascade recognizes in the UFH a fraction with very high anticoagulant activity. After isolation from the precipitate of the interaction, this fraction of heparin also contained the pentasaccharide sequence responsible for the great affinity with AT: in fact, it was strongly bound to a resin of AT agarose, and to detach it, an ionic strength of 0.6 M sodium chloride was required. In this way, the heparin regions responsible for the anticoagulant activity and also for the effects over the complement system were identified on the same short segment of the heparin molecule, which includes the active fraction of the glycosaminoglycan. The differences with early results could be explained by our experimental conditions of low ionic strength and the presence of calcium ions used for the interaction of the protein and the glycosaminoglycan.
机译:普通肝素(UFH)的抗凝血酶(AT)高亲和力存在于特定的五糖序列中。肝素还调节经典途径和替代途径上的补体活性。积累的大多数实验证据表明,这些重要的活性存在于肝素分子的不同部分。我们在以前的论文中证明,低离子强度和钙离子的存在对于检测糖胺聚糖和蛋白质之间的特定相互作用至关重要。然后使用这些非常严格的条件,我们证明了人类补体级联的第一个蛋白质复合物在UFH中识别出具有非常高抗凝活性的部分。从相互作用的沉淀物中分离后,这部分肝素还含有与AT产生巨大亲和力的五糖序列:实际上,它与AT琼脂糖树脂牢固结合并分离,离子强度为0.6需要氯化钠。以此方式,在肝素分子的相同短链段上鉴定了负责抗凝活性以及负责补体系统作用的肝素区域,所述短链段包括糖胺聚糖的活性部分。与早期结果的差异可以通过我们低离子强度的实验条件以及用于蛋白质与糖胺聚糖相互作用的钙离子的存在来解释。

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