Thirunavukkarasu M, Addya S, Juhasz B, Pant R, Zhan L, Surrey S, Maulik G, Menon V P, Maulik N
Department of Surgery, Molecular Cardiology and Angiogenesis Laboratory, University of Connecticut Health Center, Farmington, CT 06030-1110, USA.
J Cell Mol Med. 2008 Aug;12(4):1284-302. doi: 10.1111/j.1582-4934.2008.00269.x. Epub 2008 Feb 8.
This study addresses an important clinical issue by identifying potential candidates of vascular endothelial growth factor (VEGF) signalling through the Flk-1 receptor that trigger cardioprotective signals under ischaemic stress. Isolated working mouse hearts of both wild-type (WT) and Flk-1(+/-) were subjected to global ischaemia (I) for 30 min. followed by 2 hrs of reperfusion (R). Flk-1(+/-) myocardium displayed almost 50% reduction in Flk-1 mRNA as examined by quantitative real-time RT-PCR at the baseline level. Flk-1(+/-) mouse hearts displayed reduction in left ventricular functional recovery throughout reperfusion (dp/dt 605 versus 884), after 2 hrs (P<0.05). Coronary (1.9 versus 2.4 ml) and aortic flow (AF) (0.16 versus 1.2 ml) were reduced in Flk-1(+/-) after 2 hrs of reperfusion. In addition, increased infarct size (38.4%versus 28.41%, P<0.05) and apoptotic cardiomyocytes (495 versus 213) were observed in Flk-1(+/-) knockout (KO) mice. We also examined whether ischaemic preconditioning (PC), a novel method to induce cardioprotection against ischaemia reperfusion injury, through stimulating the VEGF signalling pathway might function in Flk-1(+/-) mice. We found that knocking down Flk-1 resulted in significant reduction in the cardioprotective effect by PC compared to WT. Affymetrix gene chip analysis demonstrated down-regulation of important genes after IR and preconditioning followed by ischaemia reperfusion in Flk-1(+/-) mice compared to WT. To get insight into the underlying molecular pathways involved in ischaemic PC, we determined the distinct and overlapping biological processes using Ingenuity pathway analysis tool. Independent evidence at the mRNA level supporting the Affymetrix results were validated using real-time RT-PCR for selected down-regulated genes, which are thought to play important roles in cardioprotection after ischaemic insult. In summary, our data indicated for the first time that ischaemic PC modifies genomic responses in heterozygous VEGFR-2/Flk-1 KO mice and abolishes its cardioprotective effect on ischaemic myocardium.
本研究通过识别血管内皮生长因子(VEGF)信号通路中通过Flk-1受体触发缺血应激下心脏保护信号的潜在候选者,解决了一个重要的临床问题。对野生型(WT)和Flk-1(+/-)的离体工作小鼠心脏进行30分钟的全心缺血(I),随后进行2小时的再灌注(R)。通过定量实时RT-PCR检测,Flk-1(+/-)心肌在基线水平时Flk-1 mRNA减少了近50%。Flk-1(+/-)小鼠心脏在整个再灌注过程中左心室功能恢复降低(dp/dt 605对884),2小时后差异有统计学意义(P<0.05)。再灌注2小时后,Flk-1(+/-)的冠状动脉流量(1.9对2.4 ml)和主动脉流量(AF)(0.16对1.2 ml)减少。此外,在Flk-1(+/-)基因敲除(KO)小鼠中观察到梗死面积增加(38.4%对28.41%,P<0.05)和凋亡心肌细胞增多(495对213)。我们还研究了缺血预处理(PC),一种通过刺激VEGF信号通路诱导对缺血再灌注损伤的心脏保护的新方法,在Flk-1(+/-)小鼠中是否起作用。我们发现,与WT相比,敲低Flk-1导致PC的心脏保护作用显著降低。与WT相比,Affymetrix基因芯片分析显示,Flk-1(+/-)小鼠在缺血再灌注及预处理后,重要基因下调。为了深入了解缺血预处理涉及的潜在分子途径,我们使用Ingenuity通路分析工具确定了不同的和重叠的生物学过程。使用实时RT-PCR对选定的下调基因进行验证,在mRNA水平上为支持Affymetrix结果提供了独立证据,这些基因被认为在缺血损伤后的心脏保护中起重要作用。总之,我们的数据首次表明,缺血预处理改变了杂合VEGFR-2/Flk-1 KO小鼠的基因组反应,并消除了其对缺血心肌的心脏保护作用。
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