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多聚磷酸盐与凝血酶的外位 II 以高亲和力结合。

Polyphosphate binds with high affinity to exosite II of thrombin.

机构信息

Department of Biochemistry, College of Medicine, University of Illinois at Urbana-Champaign, Urbana, IL 61801, USA.

出版信息

J Thromb Haemost. 2010 Mar;8(3):548-55. doi: 10.1111/j.1538-7836.2009.03723.x. Epub 2009 Dec 11.

Abstract

BACKGROUND

Polyphosphate (a linear polymer of inorganic phosphate) is secreted from platelet dense granules, and we recently showed that it accelerates factor V activation by thrombin.

OBJECTIVE

To examine the interaction of polyphosphate with thrombin.

METHODS AND RESULTS

Thrombin, but not prothrombin, altered the electrophoretic migration of polyphosphate in gel mobility assays. Thrombin binding to polyphosphate was influenced by ionic strength, and was evident even in plasma. Two positively charged exosites on thrombin mediate its interactions with other proteins and accessory molecules: exosite I (mainly with thrombin substrates), and exosite II (mainly with certain anionic polymers). Free thrombin, thrombin in complex with hirudin's C-terminal dodecapeptide and gamma-thrombin all bound polyphosphate similarly, excluding exosite I involvement. Mutations within exosite II, but not within exosite I, the Na(+)-binding site or hydrophobic pocket, weakened thrombin binding to polyphosphate as revealed by NaCl dependence. Surface plasmon resonance demonstrated tight interaction of polyphosphate with thrombin (K(d) approximately 5 nm) but reduced interaction with a thrombin exosite II mutant. Certain glycosaminoglycans, including heparin, only partially competed with polyphosphate for binding to thrombin, and polyphosphate did not reduce heparin-catalyzed inactivation of thrombin by antithrombin.

CONCLUSION

Polyphosphate interacts with thrombin's exosite II at a site that partially overlaps with, but is not identical to, the heparin-binding site. Polyphosphate interactions with thrombin may be physiologically relevant, as the polyphosphate concentrations achievable following platelet activation are far above the approximately 5 nM K(d) for the polyphosphate-thrombin interaction.

摘要

背景

多聚磷酸盐(无机磷酸盐的线性聚合物)由血小板致密颗粒分泌,我们最近发现它能加速凝血酶对因子 V 的激活。

目的

研究多聚磷酸盐与凝血酶的相互作用。

方法和结果

只有凝血酶而非凝血酶原在凝胶迁移分析中改变了多聚磷酸盐的电泳迁移。凝血酶与多聚磷酸盐的结合受离子强度的影响,即使在血浆中也很明显。凝血酶上的两个带正电荷的外显子与其他蛋白质和辅助分子相互作用:外显子 I(主要与凝血酶底物)和外显子 II(主要与某些阴离子聚合物)。游离凝血酶、与水蛭素 C 末端十二肽结合的凝血酶以及γ-凝血酶都与多聚磷酸盐类似地结合,排除了外显子 I 的参与。外显子 II 内的突变,但不是外显子 I 内、Na(+)结合位点或疏水性口袋内的突变,削弱了凝血酶与多聚磷酸盐的结合,这一点通过 NaCl 依赖性得到了证实。表面等离子体共振显示多聚磷酸盐与凝血酶的紧密相互作用(K(d)约为 5nm),但与凝血酶外显子 II 突变体的相互作用减弱。某些糖胺聚糖,包括肝素,仅部分竞争与凝血酶结合的多聚磷酸盐,并且多聚磷酸盐不会减少肝素催化抗凝血酶失活凝血酶的作用。

结论

多聚磷酸盐与凝血酶的外显子 II 相互作用,该作用与肝素结合位点部分重叠但不完全相同。多聚磷酸盐与凝血酶的相互作用可能具有生理相关性,因为血小板激活后可达到的多聚磷酸盐浓度远远高于多聚磷酸盐-凝血酶相互作用的约 5nm K(d)。

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