钠钙交换对于有效触发小鼠心脏钙释放是必需的。
Sodium-calcium exchange is essential for effective triggering of calcium release in mouse heart.
机构信息
Departments of Medicine (Cardiology) and Physiology and the Cardiovascular Research Laboratories, David Geffen School of Medicine at UCLA, Los Angeles, California, USA.
出版信息
Biophys J. 2010 Aug 4;99(3):755-64. doi: 10.1016/j.bpj.2010.04.071.
In cardiac myocytes, excitation-contraction coupling depends upon sarcoplasmic reticular Ca2+ release triggered by Ca2+ influx through L-type Ca2+ channels. Although Na+-Ca2+ exchange (NCX) is essential for Ca2+ extrusion, its participation in the trigger process of excitation-contraction coupling is controversial. To investigate the role of NCX in triggering, we examined Ca2+ sparks in ventricular cardiomyocytes isolated from wild-type (WT) and cardiac-specific NCX knockout (KO) mice. Myocytes from young NCX KO mice are known to exhibit normal resting cytosolic Ca2+ and normal Ca2+ transients despite reduced L-type Ca2+ current. We loaded myocytes with fluo-3 to image Ca2+ sparks using confocal microscopy in line-scan mode. The frequency of spontaneous Ca2+ sparks was reduced in KO myocytes compared with WT. However, spark amplitude and width were increased in KO mice. Permeabilizing the myocytes with saponin eliminated differences between spontaneous sparks in WT and KO mice. These results suggest that sarcolemmal processes are responsible for the reduced spark frequency and increased spark width and amplitude in KO mice. When myocytes were loaded with 1 mM fluo-3 and 3 mM EGTA via the patch pipette to buffer diadic cleft Ca2+, the number of sparks triggered by action potentials was reduced by 60% in KO cells compared to WT cells, despite similar SR Ca2+ content in both cell types. When EGTA was omitted from the pipette solution, the number of sparks triggered in KO and WT myocytes was similar. Although the number of sparks was restored in KO cells, Ca2+ release was asynchronous. These results suggest that high subsarcolemmal Ca2+ is required to ensure synchronous triggering with short spark latency in the absence of NCX. In WT mice, high subsarcolemmal Ca2+ is not required for synchronous triggering, because NCX is capable of priming the diadic cleft with sufficient Ca2+ for normal triggering, even when subsarcolemmal Ca(2+) is lowered by EGTA. Thus, reducing subsarcolemmal Ca2+ with EGTA in NCX KO mice reveals the dependence of Ca2+ release on NCX.
在心肌细胞中,兴奋-收缩偶联依赖于肌浆网 Ca2+释放,该释放由通过 L 型 Ca2+通道的 Ca2+内流触发。尽管钠-钙交换(NCX)对于 Ca2+外排是必需的,但它在兴奋-收缩偶联触发过程中的参与仍存在争议。为了研究 NCX 在触发中的作用,我们检查了来自野生型(WT)和心脏特异性 NCX 敲除(KO)小鼠的心室心肌细胞中的 Ca2+火花。尽管 L 型 Ca2+电流减少,但年轻的 NCX KO 小鼠的心肌细胞表现出正常的静息胞质 Ca2+和正常的 Ca2+瞬变。我们用 fluo-3 负载心肌细胞,并用共聚焦显微镜以线扫描模式成像 Ca2+火花。与 WT 相比,KO 心肌细胞中的自发 Ca2+火花频率降低。然而,在 KO 小鼠中,火花幅度和宽度增加。用皂素通透心肌细胞消除了 WT 和 KO 小鼠之间自发火花的差异。这些结果表明,肌膜过程是导致 KO 小鼠中火花频率降低以及火花幅度和宽度增加的原因。当用 1 mM fluo-3 和 3 mM EGTA 通过膜片钳加载肌浆网以缓冲二联体腔 Ca2+时,与 WT 细胞相比,KO 细胞中由动作电位触发的火花数量减少了 60%,尽管两种细胞类型的 SR Ca2+含量相似。当从管腔溶液中省略 EGTA 时,KO 和 WT 心肌细胞中触发的火花数量相似。尽管在 KO 细胞中恢复了火花数量,但 Ca2+释放是异步的。这些结果表明,高细胞下的 Ca2+对于在没有 NCX 的情况下确保具有短火花潜伏期的同步触发是必需的。在 WT 小鼠中,由于 NCX 能够为正常触发用足够的 Ca2+启动二联体腔,因此不需要高细胞下的 Ca2+来实现同步触发,即使通过 EGTA 降低细胞下的 Ca2+。因此,用 EGTA 在 NCX KO 小鼠中降低细胞下的 Ca2+揭示了 Ca2+释放对 NCX 的依赖性。
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