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硬骨鱼类心室肌细胞中通过L型钙通道的肌膜钙内流。

Sarcolemmal Ca influx through L-type Ca channels in ventricular myocytes of a teleost fish.

作者信息

Vornanen M

机构信息

Department of Biology, University of Joensuu, Finland.

出版信息

Am J Physiol. 1997 May;272(5 Pt 2):R1432-40. doi: 10.1152/ajpregu.1997.272.5.R1432.

Abstract

The whole cell patch clamp method was used to measure Ca current through L-type Ca channels in enzymatically isolated ventricular myocytes of crucian carp (Carassius carassius L.) heart. Fish were acclimated to 22 degrees C for more than 4 wk, and properties of Ca current were measured at room temperature (21 +/- 1 degrees C). Depolarizing voltage steps from -50 mV evoked rapidly activating Ca currents, which exhibited a bell-shaped voltage dependence with peak amplitude at 0 mV. The currents were suppressed by nifedipine (5 microM), verapamil (2.5 microM), and Cd2+ (175 microM). The current amplitude was increased by 67.5 +/- 17.2% (n = 5) in the presence of 1 microM isoproterenol. Steady-state inactivation and activation curves showed half-maximal inactivation at -31.3 +/- 0.95 mV, with a slope factor of 5.88 +/- 0.51, and half-maximal activation at -10.6 +/- 1.65 mV, with a slope factor of 7.84 +/- 0.54 (n = 9). The overlap of inactivation and activation curves suggests the presence of a small window current, which is maximally 4% of the peak current at -27 mV. The density of L-type Ca current was 6.95 +/- 0.79 pA/pF at 0 mV (n = 35). A total increment in cellular Ca contributed by L-type Ca current during a 500-ms voltage clamp pulse was calculated from the integral of Ca current and cell volume. The charge transfer through L-type Ca current was 0.325 +/- 0.023 pC/pF, and the mean cell volume was 1,377 +/- 44 microns3. The increment in total cellular Ca by Ca influx through L-type Ca channels was calculated to be 39.3 +/- 2.8 microM. These findings imply that Ca influx through L-type Ca channels can contribute significantly to the activation of contraction in the ventricular myocytes of fish heart.

摘要

采用全细胞膜片钳技术,测量酶解分离的鲫鱼(Carassius carassius L.)心脏心室肌细胞中通过L型钙通道的钙电流。将鱼在22℃下驯化4周以上,在室温(21±1℃)下测量钙电流特性。从 -50 mV开始的去极化电压阶跃诱发快速激活的钙电流,该电流呈现钟形电压依赖性,在0 mV时达到峰值幅度。该电流被硝苯地平(5 μM)、维拉帕米(2.5 μM)和Cd2+(175 μM)抑制。在1 μM异丙肾上腺素存在下,电流幅度增加了67.5±17.2%(n = 5)。稳态失活和激活曲线显示,半最大失活电压为 -31.3±0.95 mV,斜率因子为5.88±0.51;半最大激活电压为 -10.6±1.65 mV,斜率因子为7.84±0.54(n = 9)。失活和激活曲线的重叠表明存在一个小的窗电流,在 -27 mV时最大为峰值电流的4%。在0 mV时,L型钙电流密度为6.95±0.79 pA/pF(n = 35)。通过钙电流积分和细胞体积计算出在500 ms电压钳脉冲期间,L型钙电流对细胞内钙的总增量。通过L型钙电流的电荷转移为0.325±0.023 pC/pF,平均细胞体积为1377±44立方微米。通过L型钙通道钙内流导致的细胞内总钙增量计算为39.3±2.8微摩尔。这些发现表明,通过L型钙通道的钙内流可显著促进鱼心脏心室肌细胞收缩的激活。

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