蛙单个去表皮心肌细胞中Ca2+对力的调节
Force regulation by Ca2+ in skinned single cardiac myocytes of frog.
作者信息
Brandt P W, Colomo F, Piroddi N, Poggesi C, Tesi C
机构信息
Department of Anatomy and Cell Biology, Columbia University, New York, New York 10032, USA.
出版信息
Biophys J. 1998 Apr;74(4):1994-2004. doi: 10.1016/S0006-3495(98)77906-8.
Atrial and ventricular myocytes 200 to 300 microm long containing one to five myofibrils are isolated from frog hearts. After a cell is caught and held between two suction micropipettes the surface membrane is destroyed by briefly jetting relaxing solution containing 0.05% Triton X-100 on it from a third micropipette. Jetting buffered Ca2+ from other pipettes produces sustained contractions that relax completely on cessation. The pCa/force relationship is determined at 20 degrees C by perfusing a closely spaced sequence of pCa concentrations (pCa = -log[Ca2+]) past the skinned myocyte. At each step in the pCa series quick release of the myocyte length defines the tension baseline and quick restretch allows the kinetics of the return to steady tension to be observed. The pCa/force data fit to the Hill equation for atrial and ventricular myocytes yield, respectively, a pK (curve midpoint) of 5.86 +/- 0.03 (mean +/- SE.; n = 7) and 5.87 +/- 0.02 (n = 18) and an nH (slope) of 4.3 +/- 0.34 and 5.1 +/- 0.35. These slopes are about double those reported previously, suggesting that the cooperativity of Ca2+ activation in frog cardiac myofibrils is as strong as in fast skeletal muscle. The shape of the pCa/force relationship differs from that usually reported for skeletal muscle in that it closely follows the ideal fitted Hill plot with a single slope while that of skeletal muscle appears steeper in the lower than in the upper half. The rate of tension redevelopment following release restretch protocol increases with Ca2+ >10-fold and continues to rise after Ca2+ activated tension saturates. This finding provides support for a strong kinetic mechanism of force regulation by Ca2+ in frog cardiac muscle, at variance with previous reports on mammalian heart muscle. The maximum rate of tension redevelopment following restretch is approximately twofold faster for atrial than for ventricular myocytes, in accord with the idea that the intrinsic speed of the contractile proteins is faster in atrial than in ventricular myocardium.
从蛙心分离出长度为200至300微米、含有一至五条肌原纤维的心房和心室肌细胞。在用两个吸引微吸管捕获并固定一个细胞后,通过从第三个微吸管向其短暂喷射含有0.05% Triton X - 100的松弛溶液来破坏表面膜。从其他吸管喷射缓冲的Ca2 +会产生持续收缩,停止喷射后收缩会完全松弛。通过向去表皮肌细胞灌注一系列紧密排列的pCa浓度(pCa = -log[Ca2 +])来确定20℃时的pCa / 力关系。在pCa系列的每一步,快速释放肌细胞长度定义张力基线,快速再拉伸可观察到恢复到稳定张力的动力学过程。拟合心房和心室肌细胞的Hill方程的pCa / 力数据分别得出pK(曲线中点)为5.86±0.03(平均值±标准误差;n = 7)和5.87±0.02(n = 18),nH(斜率)为4.3±0.34和5.1±0.35。这些斜率约为先前报道值的两倍,表明蛙心肌原纤维中Ca2 +激活的协同性与快速骨骼肌中的一样强。pCa / 力关系的形状与通常报道的骨骼肌不同,它紧密遵循具有单一斜率的理想拟合Hill图,而骨骼肌的在较低部分比在上半部分显得更陡峭。释放 - 再拉伸方案后张力重新发展的速率随着Ca2 +增加超过10倍,并且在Ca2 +激活的张力饱和后继续上升。这一发现支持了Ca2 +在蛙心肌中强力调节力的动力学机制,这与先前关于哺乳动物心肌的报道不同。再拉伸后张力重新发展的最大速率,心房肌细胞比心室肌细胞快约两倍,这与收缩蛋白在心房肌中的内在速度比心室肌更快的观点一致。
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