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Calcium-sensitive and insensitive transient outward current in rabbit ventricular myocytes.

机译:钙敏感和不敏感的瞬时心室肌细胞外向电流。

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摘要

1. A suction pipette whole-cell voltage-clamp technique was used to record membrane currents and potentials of isolated ventricular myocytes from rabbit hearts. 2. Transient outward current (Ito) was activated by voltage steps positive to -20 mV, increasing in amplitude with further depolarization to reach a maximum around +70 mV. The current attained its peak within 10 ms and then it inactivated for 100-200 ms. 3. A large portion of Ito still remained after the calcium current (ICa) was blocked when depolarizing pulses were applied at a frequency of 0.1 Hz or less. Therefore, this current component is referred to as calcium-insensitive Ito or It. 4. It showed voltage- and time-dependent inactivation similar to that observed in Purkinje fibres and other cardiac preparations. 5. The reversal potential of It depended on external K+ concentration, [K+]o, with a slope of 32 mV per 10-fold change in the presence of a normal [Na+]o (143 mM), while the slope was 48 mV per 10-fold change in low [Na+]o (1.0 mM). 6. It was completely inhibited by 2-4 mM-4-aminopyridine. Ito in the presence of ICa was also partially blocked by 4-aminopyridine and the remainder was abolished by 5 mM-caffeine. 7. The calcium-insensitive and caffeine-sensitive Ito differed in their decay rates as well as in their recovery time courses. The former was predominantly available at a slow pulsing rate, while the latter increased its amplitude with high-frequency depolarization. 8. The caffeine-sensitive Ito was inhibited by a blockade of ICa, by replacing Ca2+ with Sr2+, by external application of ryanodine and by internal application of EGTA. This indicates that the current is calcium-sensitive and is dependent on increased myoplasmic Ca2+ through Ca2+ influx via the sarcolemma and Ca2+ release from the sarcoplasmic reticulum. The current is therefore designated as IK, Ca. 9. The physiological functions of IK, Ca and It are indicated by their contribution to ventricular repolarization at fast and slow heart rates, respectively.
机译:1.用吸管全细胞电压钳技术记录来自兔心脏的膜电流和分离的心室心肌细胞的电位。 2.瞬态向外电流(Ito)由正至-20 mV的电压阶跃激活,幅度增加,并进一步去极化,达到+70 mV的最大值。电流在10毫秒内达到峰值,然后在100-200毫秒内失活。 3.当以0.1 Hz或更低的频率施加去极化脉冲时,在阻止钙电流(ICa)之后,大部分Ito仍然保留。因此,该电流分量称为钙不敏感的Ito或It。 4.它显示出与电压和时间有关的失活,类似于在Purkinje纤维和其他心脏制剂中观察到的失活。 5. It的逆转电位取决于外部K +浓度[K +] o,在存在正常[Na +] o(143 mM)的情况下,每10倍变化的斜率是32 mV,而斜率是48 mV低[Na +] o(1.0 mM)时每变化10倍。 6.被2-4mM-4-氨基吡啶完全抑制。存在ICa的Ito也被4-氨基吡啶部分阻断,其余被5 mM-咖啡因消除。 7.对钙不敏感和对咖啡因敏感的伊藤在腐烂率和恢复时间上各不相同。前者主要以较低的脉冲频率提供,而后者通过高频去极化增加了振幅。 8.对咖啡因敏感的Ito被ICa阻滞抑制,通过用Sr2 +取代Ca2 +,外部使用雷诺丹和内部使用EGTA抑制。这表明该电流对钙敏感,并且依赖于通过肌膜通过Ca2 +流入而增加的肌质Ca2 +和从肌浆网释放的Ca2 +。因此,电流指定为IK,Ca。 9. IK,Ca和Ik的生理功能分别通过其在心律快和慢时对心室复极的贡献来表明。

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