在体内大鼠心脏中,再灌注时PAR-2激活通过ERK1/2途径挽救心肌。
PAR-2 activation at the time of reperfusion salvages myocardium via an ERK1/2 pathway in in vivo rat hearts.
作者信息
Jiang Rong, Zatta Amanda, Kin Hajime, Wang Ningping, Reeves James G, Mykytenko James, Deneve Jeremiah, Zhao Zhi-Qing, Guyton Robert A, Vinten-Johansen Jakob
机构信息
Department of Cardiothoracic Surgery, Cardiothoracic Research Laboratory, Carlyle Fraser Heart Center of Crawford Long Hospital, Emory University School of Medicine, Atlanta, GA, USA.
出版信息
Am J Physiol Heart Circ Physiol. 2007 Nov;293(5):H2845-52. doi: 10.1152/ajpheart.00209.2007. Epub 2007 Aug 24.
Protease-activated receptor-2 (PAR-2) may have proinflammatory effects in some tissues and protective effects in other tissues. The role of PAR-2 in in vivo myocardial ischemia-reperfusion has not yet been determined. This study tested the hypothesis that PAR-2 activation with the PAR-2 agonist peptide SLIGRL (PAR-2 AP) reduces myocardial infarct size when given at reperfusion in vivo, and this cardioprotection involves the ERK1/2 pathway. Anesthetized rats were randomly assigned to the following groups with 30 min of regional ischemia and 3 h reperfusion: 1) control with saline; 2) vehicle (DMSO); 3) PAR-2 AP, 1 mg/kg given intravenously 5 min before reperfusion; 4) scrambled peptide (SP), 1 mg/kg; 5) the ERK1/2 inhibitor PD-98059 (PD), 0.3 mg/kg given 10 min before reperfusion; 6) the phosphatidylinositol 3-kinase inhibitor LY-294002 (LY), 0.3 mg/kg given 10 min before reperfusion; 7) PD + PAR-2 AP, 0.3 mg/kg PD given 5 min before PAR-2 AP; 8) LY + PAR-2 AP, 0.3 mg/kg LY given 5 min before PAR-2 AP; 9) chelerythrine (Chel) alone, 5 mg/kg given 10 min before reperfusion; and 10) Chel + PAR-2 AP, Chel was given 5 min before PAR-2 AP (10 min before reperfusion). Activation of ERK1/2, ERK5, Akt, and the downstream targets of ERK1/2 [P90 RSK and bcl-xl/bcl-2-associated death promoter (BAD)] was determined by Western blot analysis in separate experiments. PAR-2 AP significantly reduced infarct size compared with control (36 +/- 2% vs. 53 +/- 1%, P < 0.05), and SP had no effect on infarct size (53 +/- 3%). PAR-2 AP significantly increased phosphorylation of ERK1/2, p90RSK, and BAD but not Akt or ERK5. Accordingly, the infarct-size sparing effect of PAR-2 AP was abolished by PD (PAR-2 AP, 36 +/- 2% vs. PD + PAR-2 AP, 50 +/- 1%; P < 0.05) and by Chel (Chel + PAR-2 AP, 58 +/- 2%) but not by LY (PAR-2 AP, 36 +/- 2% vs. LY + PAR-2 AP, 38 +/- 3%; P > 0.05). Therefore, PAR-2 activation is cardioprotective in the in vivo rat heart ischemia-reperfusion model, and this protection involves the ERK1/2 pathway and PKC.
蛋白酶激活受体-2(PAR-2)在某些组织中可能具有促炎作用,而在其他组织中则具有保护作用。PAR-2在体内心肌缺血再灌注中的作用尚未确定。本研究检验了以下假设:在体内再灌注时给予PAR-2激动剂肽SLIGRL(PAR-2 AP)激活PAR-2可减小心肌梗死面积,且这种心脏保护作用涉及ERK1/2通路。将麻醉大鼠随机分为以下几组,进行30分钟的局部缺血和3小时再灌注:1)生理盐水对照组;2)溶剂(二甲基亚砜)组;3)PAR-2 AP组,再灌注前5分钟静脉注射1 mg/kg;4)乱序肽(SP)组,1 mg/kg;5)ERK1/2抑制剂PD-98059(PD)组,再灌注前10分钟给予0.3 mg/kg;6)磷脂酰肌醇3-激酶抑制剂LY-294002(LY)组,再灌注前10分钟给予0.3 mg/kg;7)PD + PAR-2 AP组,在给予PAR-2 AP前5分钟给予0.3 mg/kg PD;8)LY + PAR-2 AP组,在给予PAR-2 AP前5分钟给予0.3 mg/kg LY;9)单独使用白屈菜红碱(Chel)组,再灌注前10分钟给予5 mg/kg;10)Chel + PAR-2 AP组,在给予PAR-2 AP前5分钟给予Chel(再灌注前10分钟)。在单独的实验中,通过蛋白质印迹分析确定ERK1/2、ERK5、Akt以及ERK1/2的下游靶点[P90 RSK和bcl-xl/bcl-2相关死亡促进因子(BAD)]的激活情况。与对照组相比,PAR-2 AP显著减小了梗死面积(36±2%对53±1%,P<0.05),而SP对梗死面积无影响(53±3%)。PAR-2 AP显著增加了ERK1/2、p90RSK和BAD的磷酸化,但对Akt或ERK5无影响。因此,PD(PAR-2 AP组为36±2%对PD + PAR-2 AP组为50±1%;P<0.05)和Chel(Chel + PAR-2 AP组为58±2%)消除了PAR-2 AP对梗死面积的减小作用,但LY未消除(PAR-2 AP组为36±2%对LY + PAR-2 AP组为
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