Zeitz Oliver, Maass A Eveline, Van Nguyen Phuc, Hensmann Geerd, Kögler Harald, Möller Karsten, Hasenfuss Gerd, Janssen Paul M L
Georg-August-Universität Göttingen Universitätsklinik, Abteilung Kardiologie und Pneumologie, Göttingen, Germany.
Circ Res. 2002 May 17;90(9):988-95. doi: 10.1161/01.res.0000018625.25212.1e.
Hydroxyl radicals (OH) are involved in the development of reperfusion injury and myocardial failure. In the acute phase of the OH-mediated diastolic dysfunction, increased intracellular Ca(2+) levels and alterations of myofilaments may play a role, but the relative contribution of these systems to myocardial dysfunction is unknown. Intact contracting cardiac trabeculae from rabbits were exposed to OH, resulting in an increase in diastolic force (F(dia)) by 540%. Skinned fiber experiments revealed that OH-exposed preparations were sensitized for Ca(2+) (EC(50): 3.27+/-0.24 x 10(-6) versus 2.69+/-0.15 x 10(-6) mol/L; P<0.05), whereas maximal force development was unaltered. Western blots showed a proteolytic degradation of troponin T (TnT) with intact troponin I (TnI). Blocking of calpain I by MDL-28.170 inhibited both TnT-proteolysis and Ca(2+) sensitization, but failed to prevent the acute diastolic dysfunction in the intact preparation. The OH-induced diastolic dysfunction was similar in preparations with intact (540+/-93%) and pharmacologically blocked sarcoplasmic reticulum (539+/-77%), and was also similar in presence of the L-type Ca(2+)-channel antagonist verapamil. In sharp contrast, inhibition of the reverse-mode sodium-calcium exchange by KB-R7943 preserved diastolic function completely. Additional experiments were performed in rat myocardium; the rise in diastolic force was comparable to rabbit myocardium, but Ca(2+) sensitivity was unchanged and maximal force development was reduced. This was associated with a degradation of TnI, but not TnT. Electron microscopic analysis revealed that OH did not cause irreversible membrane damage. We conclude that OH-induced acute diastolic dysfunction is caused by Ca(2+) influx via reverse mode of the sodium-calcium exchanger. Degradation of troponins appears to be species-dependent but does not contribute to the acute diastolic dysfunction.
羟自由基(OH)参与再灌注损伤和心肌衰竭的发展过程。在OH介导的舒张功能障碍急性期,细胞内Ca(2+)水平升高和肌丝改变可能起作用,但这些系统对心肌功能障碍的相对贡献尚不清楚。将兔完整的收缩性心脏小梁暴露于OH中,导致舒张期张力(F(dia))增加540%。脱细胞纤维实验表明,暴露于OH的制剂对Ca(2+)敏感(半数有效浓度:3.27±0.24×10(-6)对2.69±0.15×10(-6)mol/L;P<0.05),而最大张力发展未改变。蛋白质印迹显示肌钙蛋白T(TnT)发生蛋白水解降解,而肌钙蛋白I(TnI)完整。用MDL-28.170阻断钙蛋白酶I可抑制TnT蛋白水解和Ca(2+)致敏,但未能预防完整制剂中的急性舒张功能障碍。在完整(540±93%)和经药理学阻断肌浆网(539±77%)的制剂中,OH诱导的舒张功能障碍相似,在L型Ca(2+)通道拮抗剂维拉帕米存在的情况下也相似。形成鲜明对比的是,用KB-R7943抑制逆向钠钙交换可完全保留舒张功能。在大鼠心肌中进行了额外实验;舒张期张力的升高与兔心肌相当,但Ca(2+)敏感性未改变,最大张力发展降低。这与TnI降解有关,但与TnT无关。电子显微镜分析显示OH未引起不可逆的膜损伤。我们得出结论,OH诱导的急性舒张功能障碍是由钠钙交换体逆向模式的Ca(2+)内流引起的。肌钙蛋白的降解似乎具有物种依赖性,但对急性舒张功能障碍没有影响。
