首页> 外文期刊>Pfluegers Archiv: European Journal of Physiology >The Fura-2 transient can show two types of voltage dependence at 36 degrees C in ventricular myocytes isolated from the rat heart.
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The Fura-2 transient can show two types of voltage dependence at 36 degrees C in ventricular myocytes isolated from the rat heart.

机译:从大鼠心脏分离的心室肌细胞中,Fura-2瞬变在36摄氏度时可能显示两种电压依赖性。

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We used the whole-cell patch-clamp method to investigate the voltage dependence of the L-type Ca current (ICa,L) and intracellular Ca (Cai) transient in ventricular myocytes isolated from the rat heart. Intracellular Ca was monitored using Fura-2 and the experiments were carried out at 36 degrees C. We measured ICa,L by using a caesium-based internal dialysis solution to eliminate interfering K currents. The voltage dependence of peak ICa,L amplitude was bell-shaped: ICa,L was maximal at +10 mV and declined at more positive potentials. When ICa,L was integrated over the first 25 ms to estimate the magnitude of Ca entry, this had a very similar voltage dependence to peak ICa,L. In all cells, phasic Fura-2 transients were abolished by 5 microM ryanodine (a blocker of the sarcoplasmic reticulum, SR) showing that the Fura-2 transient provided an index of the magnitude of SR Ca release. For experiments measuring the Cai transient, we used a K-based internal dialysis solution to preserve normal excitation-contraction coupling. In 30-40% of cells, we found that the Fura-2 transient had a bell-shaped voltage dependence. This suggests that, in these cells, the primary trigger mechanism for Ca-induced Ca-release might have been Ca entry via ICa,L. In the remaining 60-70% of cells, the voltage dependence of the Fura-2 transient was not bell-shaped. The Fura-2 transient reached a maximum with a pulse to +10 mV, and the amplitude of the transient did not decline significantly at more positive potentials to this. In cells with a non-bell-shaped voltage dependence of the Fura-2 transient, pulses to potentials as far positive as +140 mV elicited phasic Fura-2 transients. Since this potential exceeded the Nernst potential for Ca, it was unlikely there was any trigger Ca entry via ICa,L at this potential. This would suggest that, in these cells, another trigger for SR Ca release (in addition to ICa,L) might be present. We conclude that rat ventricular myocytes, produced using a standard isolation technique and under standard recording conditions, can show either a bell-shaped or a sigmoidal voltage dependence of the Fura-2 transient.
机译:我们使用全细胞膜片钳方法来研究从大鼠心脏分离的心室肌细胞中L型Ca电流(ICa,L)和细胞内Ca(Cai)瞬态的电压依赖性。使用Fura-2监测细胞内Ca,并在36摄氏度下进行实验。我们使用基于铯的内部透析溶液以消除干扰的K电流来测量ICa,L。峰值ICa,L振幅的电压依赖性呈钟形:ICa,L在+10 mV时最大,而在更多正电位时下降。当在最初的25 ms内对ICa,L进行积分以估计Ca进入的幅度时,这与峰值ICa,L具有非常相似的电压依赖性。在所有细胞中,阶段性Fura-2瞬变被5 microM ryanodine(肌浆网SR的阻滞剂)消除,表明Fura-2瞬变提供了SR Ca释放量的指标。对于测量Cai瞬态的实验,我们使用了基于K的内部渗析溶液来保持正常的激发-收缩耦合。在30-40%的电池中,我们发现Fura-2瞬态具有钟形电压依赖性。这表明在这些细胞中,Ca诱导的Ca释放的​​主要触发机制可能是通过ICa,L进入Ca。在其余60-70%的电池中,Fura-2瞬态的电压依赖性不是钟形的。 Fura-2瞬变达到最大,脉冲达到+10 mV,并且在此产生更多正电势时,瞬变幅度没有明显下降。在对Fura-2瞬态电压无钟形依赖性的电池中,脉冲至高达+140 mV的正电势会引起相性Fura-2瞬态电压。由于该电势超过了Ca的能斯特电势,因此在该电势下不太可能通过ICa,L触发任何Ca进入。这表明,在这些细胞中,可能存在SR Ca释放的​​另一个触发因素(除了ICa,L)。我们得出的结论是,使用标准分离技术并在标准记录条件下产生的大鼠心室肌细胞可以显示出Fura-2瞬态的钟形或S型电压依赖性。

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