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纤维蛋白原延长γ链抑制凝血酶诱导的血小板反应,阻碍其与不同受体的相互作用。

Fibrinogen-elongated gamma chain inhibits thrombin-induced platelet response, hindering the interaction with different receptors.

作者信息

Lancellotti Stefano, Rutella Sergio, De Filippis Vincenzo, Pozzi Nicola, Rocca Bianca, De Cristofaro Raimondo

机构信息

Institute of Internal Medicine and Geriatrics, and Haemostasis Research Centre, Catholic University School of Medicine, 00168 Rome, Italy.

出版信息

J Biol Chem. 2008 Oct 31;283(44):30193-204. doi: 10.1074/jbc.M803659200. Epub 2008 Sep 8.

Abstract

The expression of the elongated fibrinogen gamma chain, termed gamma', derives from alternative splicing of mRNA and causes an insertion sequence of 20 amino acids. This insertion domain interacts with the anion-binding exosite (ABE)-II of thrombin. This study investigated whether and how gamma' chain binding to ABE-II affects thrombin interaction with its platelet receptors, i.e. glycoprotein Ibalpha (GpIbalpha), protease-activated receptor (PAR) 1, and PAR4. Both synthetic gamma' peptide and fibrinogen fragment D*, containing the elongated gamma' chain, inhibited thrombin-induced platelet aggregation up to 70%, with IC(50) values of 42+/-3.5 and 0.47+/-0.03 microm, respectively. Solid-phase binding and spectrofluorimetric assays showed that both fragment D* and the synthetic gamma' peptide specifically bind to thrombin ABE-II and competitively inhibit the thrombin binding to GpIbalpha with a mean K(i) approximately 0.5 and approximately 35 microm, respectively. Both these gamma' chain-containing ligands allosterically inhibited thrombin cleavage of a synthetic PAR1 peptide, of native PAR1 molecules on intact platelets, and of the synthetic chromogenic peptide D-Phe-pipecolyl-Arg-p-nitroanilide. PAR4 cleavage was unaffected. In summary, fibrinogen gamma' chain binds with high affinity to thrombin and inhibits with combined mechanisms the platelet response to thrombin. Thus, its variations in vivo may affect the hemostatic balance in arterial circulation.

摘要

被称为γ'的延长型纤维蛋白原γ链的表达源自mRNA的可变剪接,并导致一个20个氨基酸的插入序列。该插入结构域与凝血酶的阴离子结合外位点(ABE)-II相互作用。本研究调查了γ'链与ABE-II的结合是否以及如何影响凝血酶与其血小板受体,即糖蛋白Ibalpha(GpIbalpha)、蛋白酶激活受体(PAR)1和PAR4的相互作用。合成的γ'肽和含有延长型γ'链的纤维蛋白原片段D均能抑制凝血酶诱导的血小板聚集达70%,IC(50)值分别为42±3.5和0.47±0.03 microm。固相结合和荧光光谱分析表明,片段D和合成的γ'肽均能特异性结合凝血酶ABE-II,并分别以平均K(i)约为0.5和约35 microm竞争性抑制凝血酶与GpIbalpha的结合。这两种含γ'链的配体均变构抑制合成PAR1肽、完整血小板上天然PAR1分子以及合成生色肽D-Phe-哌啶基-Arg-对硝基苯胺的凝血酶切割。PAR4的切割不受影响。总之,纤维蛋白原γ'链与凝血酶高亲和力结合,并通过联合机制抑制血小板对凝血酶的反应。因此,其在体内的变化可能会影响动脉循环中的止血平衡。

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