Smith Robert M, Suleman Naushaad, Lacerda Lydia, Opie Lionel H, Akira Shizuo, Chien Kenneth R, Sack Michael N
Hatter Institute for Cardiology Research, Faculty of Health Sciences, University of Cape Town Observatory, Cape Heart Centre, Chris Barnard Building, Cape Town 7925, South Africa.
Cardiovasc Res. 2004 Sep 1;63(4):611-6. doi: 10.1016/j.cardiores.2004.06.019.
To evaluate the functional requirement of signal transducer and activator of transcription-3 (STAT-3) in cardiac myocyte tolerance to ischemia (I) and in classical preconditioning.
Cardiac myocyte STAT-3 was depleted in mice using Cre-lox p technology. Isolated cardiomyocytes from wild-type (WT) and STAT-3-deficient mice were evaluated for viability following simulated ischemia (SI; 26 h). Cardiomyocytes were then preconditioned by exposure to transient simulated ischemia or via the administration of preconditioning mimetics (100 microM adenosine, 100 microM diazoxide and 0.5 ng ml(-1) TNFalpha, individually and in combination) prior to index ischemia. To evaluate the effect of cardiac myocyte depletion of STAT-3 in the context of the intact heart, these experiments were performed in isolated perfused Langendorff heart preparations which were exposed to an index insult of 30-min global ischemia and 45-min reperfusion. Ischemic preconditioning was achieved by subjecting the hearts to four cycles of 5-min ischemia followed by 5-min reperfusion prior to index ischemia. Infarct size was measured following reperfusion.
Cell viability was diminished equally in wild-type and STAT-3-depleted cardiomyocytes. In contrast, ischemic and pharmacological preconditioning protected wild-type cardiomyocytes but not STAT-3-deficient cardiomyocytes. These results were mirrored in the intact heart.
The depletion of functional STAT-3 does not modulate tolerance to ischemic injury in cardiomyocytes. This signaling molecule, however, is crucial for the ischemic and all the tested pharmacological preconditioning programs.
评估信号转导子与转录激活子3(STAT-3)在心肌细胞对缺血(I)的耐受性及经典预处理中的功能需求。
利用Cre-lox p技术在小鼠体内使心肌细胞STAT-3缺失。对野生型(WT)和STAT-3缺陷型小鼠分离出的心肌细胞进行模拟缺血(SI;26小时)后的活力评估。然后在指数缺血前,通过短暂暴露于模拟缺血或给予预处理模拟物(100微摩尔腺苷、100微摩尔二氮嗪和0.5纳克/毫升肿瘤坏死因子α,单独或联合使用)对心肌细胞进行预处理。为了评估在完整心脏背景下心肌细胞STAT-3缺失的影响,这些实验在离体灌注的Langendorff心脏标本上进行,使其暴露于30分钟全心缺血和45分钟再灌注的指数性损伤。缺血预处理通过在指数缺血前使心脏经历四个5分钟缺血然后5分钟再灌注的周期来实现。再灌注后测量梗死面积。
野生型和STAT-3缺失的心肌细胞的细胞活力均同等程度降低。相比之下,缺血和药物预处理可保护野生型心肌细胞,但不能保护STAT-3缺陷型心肌细胞。这些结果在完整心脏中得到了体现。
功能性STAT-3的缺失并不调节心肌细胞对缺血损伤的耐受性。然而,这种信号分子对于缺血及所有测试的药物预处理程序至关重要。