通过凝血酶受体对血小板糖蛋白IIb/IIIa(整合素αIIBβ3)功能的调节
Regulation of platelet glycoprotein IIb/IIIa (integrin alpha IIB beta 3) function via the thrombin receptor.
作者信息
Giesberts A N, van Willigen G, Lapetina E G, Akkerman J W
机构信息
Department of Haematology, University Hospital Utrecht, The Netherlands.
出版信息
Biochem J. 1995 Jul 15;309 ( Pt 2)(Pt 2):613-20. doi: 10.1042/bj3090613.
Binding sites on glycoprotein (GP) IIb/IIIa exposed by 0.5 unit/ml alpha-thrombin are insensitive to prostaglandin I2 (PGI2), in contrast with sites exposed by ADP or platelet-activating factor. Here we show that the thrombin receptor agonist peptide (TRAP) (SFLLRN; 15 microM) opens almost the same number of GPIIb/IIIa molecules as 0.5 unit/ml alpha-thrombin (64840 +/- 8920 compared with 81050 +/- 6030 molecules of fibronectin bound/platelet), but these sites rapidly close on addition of PGI2. To investigate whether alpha-thrombin and TRAP initiate different signalling pathways, we measured phospholipase C (PLC)-mediated control of GPIIb/IIIa and its sensitivity to cyclic AMP. Optimal concentrations of alpha-thrombin and TRAP activated PLC maximally, but TRAP induced only about 50% protein kinase C PKC) activation after 10 min stimulation compared with alpha-thrombin. These concentrations also suppressed PGI2-induced cyclic AMP accumulation, with alpha-thrombin inducing complete inhibition and TRAP about 10% less. Direct activation of PKC by phorbol 12-myristate 13-acetate confirmed earlier observations that PGI2-induced cyclic AMP accumulation is partly inhibited via PKC. Applying different concentration of alpha-thrombin, TRAP or a combination of alpha-thrombin and the thrombin receptor inhibitory peptide (TRIP) (Mpr-F-Cha-Cha-RKPNDK-NH2; 800 microM) (Mpr, 3-mercaptopropionic acid; Cha, cyclohexylalanine), we show that the different means of stimulating the thrombin receptor all suppressed PGI2-induced cyclic AMP accumulation via (i) activation of PKC and (ii) activation of the heterotrimeric G-protein, Gi. We conclude that complete inhibition of cyclic AMP accumulation requires activation of both PKC and Gi, as observed with 0.5 unit/ml alpha-thrombin. Although TRAP almost fully exposes GPIIb/IIIa, its activation of PKC is incomplete, enabling PGI2 to raise cyclic AMP concentration from 1.4 +/- 0.7 to 4.1 +/- 1.3 nmol/10(11) platelets (P < 0.005) which is sufficient to close exposed GPIIb/IIIa molecules.
与由二磷酸腺苷(ADP)或血小板激活因子所暴露的位点不同,0.5单位/毫升的α-凝血酶所暴露的糖蛋白(GP)IIb/IIIa上的结合位点对前列腺素I2(PGI2)不敏感。在此我们表明,凝血酶受体激动肽(TRAP)(SFLLRN;15微摩尔)打开的GPIIb/IIIa分子数量几乎与0.5单位/毫升的α-凝血酶相同(与81050±6030个结合纤连蛋白的分子/血小板相比,为64840±8920个),但在添加PGI2后这些位点会迅速关闭。为了研究α-凝血酶和TRAP是否启动不同的信号通路,我们测量了磷脂酶C(PLC)介导的对GPIIb/IIIa的调控及其对环磷酸腺苷(cAMP)的敏感性。α-凝血酶和TRAP的最佳浓度能最大程度地激活PLC,但与α-凝血酶相比,TRAP在刺激10分钟后仅诱导约50%的蛋白激酶C(PKC)激活。这些浓度也抑制了PGI2诱导的cAMP积累,α-凝血酶诱导完全抑制,而TRAP的抑制作用约少10%。佛波醇12-肉豆蔻酸酯13-乙酸酯对PKC的直接激活证实了早期的观察结果,即PGI2诱导的cAMP积累部分是通过PKC被抑制的。应用不同浓度的α-凝血酶、TRAP或α-凝血酶与凝血酶受体抑制肽(TRIP)(Mpr-F-Cha-Cha-RKPNDK-NH2;800微摩尔)(Mpr,3-巯基丙酸;Cha,环己基丙氨酸)的组合,我们表明刺激凝血酶受体的不同方式均通过(i)PKC的激活和(ii)异源三聚体G蛋白Gi的激活来抑制PGI2诱导的cAMP积累。我们得出结论,如用0.5单位/毫升的α-凝血酶所观察到的,cAMP积累的完全抑制需要PKC和Gi两者的激活。尽管TRAP几乎能完全暴露GPIIb/IIIa,但其对PKC的激活并不完全,使得PGI2能够将cAMP浓度从1.4±0.7提高到4.1±1.3纳摩尔/10^11个血小板(P<0.005),这足以关闭暴露的GPIIb/IIIa分子。
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