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锌作为富含组氨酸糖蛋白中和肝素的辅助因子。

Zinc as a cofactor for heparin neutralization by histidine-rich glycoprotein.

作者信息

Kluszynski B A, Kim C, Faulk W P

机构信息

Division of Experimental Pathology, Center for Reproduction and Transplantation Immunology, Methodist Hospital, Indianapolis, Indiana 46202, USA.

出版信息

J Biol Chem. 1997 May 23;272(21):13541-7. doi: 10.1074/jbc.272.21.13541.

Abstract

We have studied the ability of histidine-rich glycoprotein (HRG) to neutralize the anticoagulant activity of heparin in plasma and in a purified component clotting assay. Addition of HRG to plasma or to the purified component assay did not neutralize the anticoagulant activity of heparin unless micromolar concentrations of zinc were present. Higher zinc concentrations were required for citrated than for heparinized plasmas due to competition of citrate with HRG for zinc binding. Zinc concentrations as low as 1.25 microM revealed HRG to be a powerful competitor of antithrombin for heparin in the purified component assays. HRG binding of heparin also was shown by affinity chromatography of HRG from immobilized heparin in the presence and absence of zinc. In the absence of zinc, HRG was eluted by 0.1 M NaCl, but, in the presence of zinc, elution of HRG required 1.0 M NaCl. Investigation of other divalent cations (copper and magnesium) indicated that augmentation of heparin binding by HRG in the presence of antithrombin was restricted to zinc. The HRG.Zn complex effectively competes with antithrombin for heparin, which restricts the availability of heparin to bind antithrombin and allows thrombin-mediated fibrinogenesis to proceed unimpeded. This could be initiated by zinc released from activated platelets.

摘要

我们研究了富含组氨酸糖蛋白(HRG)在血浆和纯化成分凝血试验中中和肝素抗凝活性的能力。向血浆或纯化成分试验中添加HRG不会中和肝素的抗凝活性,除非存在微摩尔浓度的锌。由于柠檬酸盐与HRG竞争锌结合,柠檬酸盐血浆所需的锌浓度高于肝素化血浆。在纯化成分试验中,低至1.25微摩尔的锌浓度显示HRG是抗凝血酶与肝素竞争的有力对手。在有无锌的情况下,通过固定化肝素对HRG进行亲和层析,也显示了HRG与肝素的结合。在没有锌的情况下,HRG用0.1M氯化钠洗脱,但在有锌的情况下,HRG的洗脱需要1.0M氯化钠。对其他二价阳离子(铜和镁)的研究表明,在抗凝血酶存在的情况下,HRG增强与肝素的结合仅限于锌。HRG-Zn复合物有效地与抗凝血酶竞争肝素,这限制了肝素与抗凝血酶结合的可用性,并使凝血酶介导的纤维蛋白生成不受阻碍地进行。这可能由活化血小板释放的锌引发。

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