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G蛋白门控内向整流钾通道通过Src家族激酶调节血小板中ADP诱导的cPLA2活性。

G-protein-gated inwardly rectifying potassium channels regulate ADP-induced cPLA2 activity in platelets through Src family kinases.

作者信息

Shankar Haripriya, Kahner Bryan N, Prabhakar Janani, Lakhani Parth, Kim Soochong, Kunapuli Satya P

机构信息

Department of Physiology, Sol Sherry Thrombosis Research Center, Temple University, Rm 224OMS, 3420 N Broad St, Philadelphia, PA 19140, USA.

出版信息

Blood. 2006 Nov 1;108(9):3027-34. doi: 10.1182/blood-2006-03-010330. Epub 2006 Jul 20.

Abstract

ADP-induced TXA2 generation requires the costimulation of P2Y1, P2Y12, and the GPIIb/IIIa receptors. Signaling events downstream of the P2Y receptors that contribute to ADP-induced TXA2 generation have not been clearly delineated. In this study, we have investigated the role of G-protein-gated inwardly rectifying potassium channels (GIRKs), a recently identified functional effector for the P2Y12 receptor, in the regulation of ADP-induced TXA2 generation. At 10-microM concentrations, the 2 structurally distinct GIRK channel blockers, SCH23390 and U50488H, caused complete inhibition of ADP-induced cPLA2 phosphorylation and TXA2 generation, without affecting the conversion of AA to TXA2 or ADP-induced primary platelet aggregation in aspirin-treated platelets. In addition, Src family kinase selective inhibitors abolished 2MeSADP-mediated cPLA2 phosphorylation and TXA2 generation. Furthermore, these GIRK channel blockers completely blocked Gi-mediated Src kinase activation, suggesting that GIRK channels are upstream of Src family tyrosine kinase activation. In weaver mouse platelets, which have dysfunctional GIRK2 subunits, ADP-induced TXA2 generation was impaired. However, we did not observe any defect in 2MeSADP-induced platelet functional responses in GIRK2-null mouse platelets, suggesting that functional channels composed of other GIRK subunits contribute to ADP-induced TXA2 generation, via the regulation of the Src and cPLA2 activity.

摘要

ADP诱导的血栓素A2(TXA2)生成需要P2Y1、P2Y12和糖蛋白IIb/IIIa受体的共刺激。P2Y受体下游有助于ADP诱导TXA2生成的信号事件尚未明确界定。在本研究中,我们研究了G蛋白门控内向整流钾通道(GIRKs),一种最近确定的P2Y12受体功能效应器,在调节ADP诱导的TXA2生成中的作用。在10微摩尔浓度下,两种结构不同的GIRK通道阻滞剂SCH23390和U50488H完全抑制了ADP诱导的胞质型磷脂酶A2(cPLA2)磷酸化和TXA2生成,而不影响阿司匹林处理的血小板中花生四烯酸(AA)向TXA2的转化或ADP诱导的初级血小板聚集。此外,Src家族激酶选择性抑制剂消除了2-甲基硫代腺苷二磷酸(2MeSADP)介导的cPLA2磷酸化和TXA2生成。此外,这些GIRK通道阻滞剂完全阻断了Gi介导的Src激酶激活,表明GIRK通道在Src家族酪氨酸激酶激活的上游。在具有功能失调的GIRK2亚基的韦弗小鼠血小板中,ADP诱导的TXA2生成受损。然而,我们在GIRK2基因敲除小鼠血小板中未观察到2MeSADP诱导的血小板功能反应有任何缺陷,这表明由其他GIRK亚基组成的功能性通道通过调节Src和cPLA2活性,有助于ADP诱导的TXA2生成。

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