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心脏停搏和心肌缺血期间钙离子(Ca2+)与烟酰胺腺嘌呤二核苷酸(NADH)荧光信号的分离

Separation of fluorescence signals from Ca2+ and NADH during cardioplegic arrest and cardiac ischemia.

作者信息

Brachmanski Monika, Gebhard Martha Maria, Nobiling Rainer

机构信息

Department of Experimental Surgery, University of Heidelberg, Im Neuenheimer Feld 365, D-69120 Heidelberg, Germany.

出版信息

Cell Calcium. 2004 Apr;35(4):381-91. doi: 10.1016/j.ceca.2003.10.001.

Abstract

Determinations of intracellular Ca(2+) during ischemia using fluorescent indicators are hampered by overlapping cellular autofluorescence (AF), which largely depends on NADH. If Ca(2+) is to be determined under different kinds of ischemia, signal separation merits special attention. We used triple wavelength excitation fluorescence to separate autofluorescence from [Ca(2+)]-dependent fura-2 fluorescence. Excitation at 360 nm served as third, Ca(2+)-insensitive wavelength. Using an appropriate evaluation procedure, we separated Ca(2+)-dependent signals from autofluorescence which is semiquantitatively associated with NADH, an indicator of the cellular redox state. We compared changes of Ca(2+) in isolated hearts during ischemia following cardioplegic arrest with those after transient stop of nutritive perfusion. We observed [Ca(2+)] transients in spontaneously beating hearts, persisting during ischemic episodes, and an increase of mean Ca(2+). In contrast, cardioplegic arrest stopped periodical Ca(2+) transients and heart beats simultaneously. Ca(2+) remained at diastolic values, tended to decrease during the first minutes of cardioplegic arrest and then increased slowly. Autofluorescence increased under both conditions. During ischemia, this increase was faster than in cardioplegia experiments. It started after the last heart beat despite persisting perfusion. Our measurements demonstrate that rhythmical heart beat is essential for sufficient perfusion. Reduced Ca(2+) under cardioplegic arrest may influence metabolism.

摘要

使用荧光指示剂测定缺血期间的细胞内[Ca(2+)]i受到细胞自发荧光(AF)重叠的阻碍,细胞自发荧光在很大程度上取决于NADH。如果要在不同类型的缺血条件下测定Ca(2+),信号分离值得特别关注。我们使用三波长激发荧光将自发荧光与[Ca(2+)]依赖性fura-2荧光分离。360nm的激发光作为第三个对Ca(2+)不敏感的波长。通过适当的评估程序,我们将Ca(2+)依赖性信号与自发荧光分离,自发荧光与细胞氧化还原状态的指标NADH半定量相关。我们比较了心脏停搏后缺血期间离体心脏中[Ca(2+)]i的变化与短暂停止营养灌注后的变化。我们观察到自发搏动心脏中的[Ca(2+)]瞬变,在缺血期间持续存在,并且平均[Ca(2+)]i增加。相比之下,心脏停搏同时停止了周期性的[Ca(2+)]i瞬变和心跳。[Ca(2+)]i保持在舒张期值,在心脏停搏的最初几分钟内趋于下降,然后缓慢上升。在两种情况下自发荧光均增加。在缺血期间,这种增加比心脏停搏实验中更快。尽管持续灌注,但在最后一次心跳后开始增加。我们的测量表明,有节律的心跳对于充分灌注至关重要。心脏停搏时[Ca(2+)]i降低可能会影响代谢。

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