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首页> 美国卫生研究院文献>The Journal of Physiology >Block of ATP-regulated and Ca2(+)-activated K+ channels in mouse pancreatic beta-cells by external tetraethylammonium and quinine.
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Block of ATP-regulated and Ca2(+)-activated K+ channels in mouse pancreatic beta-cells by external tetraethylammonium and quinine.

机译:外部四乙铵和奎宁对小鼠胰腺β细胞中ATP调节和Ca2(+)活化的K +通道的阻滞作用。

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1. The whole-cell and outside-out patch configurations of the patch-clamp technique were used to investigate the effects of extracellular tetraethylammonium ions (TEA+) and quinine on both Ca2(+)-activated and ATP-regulated K+ channels in mouse pancreatic beta-cells. 2. The Ca2(+)-activated K+ channel has a single-channel K+ permeability of 4.7 x 10(-13) cm3 s-1 when recorded with physiological ionic gradients. This value decreased to 2.9 x 10(-13) cm3 s-1 after addition of 0.3 mM-TEA+. 3. Two exponentials with time constants of 0.2 and 4.7 ms were required to describe the distribution of the channel openings suggesting that the Ca2(+)-activated K+ channel has at least two open states. The fast and slow components comprised 16 and 84% of the total number of openings respectively. 4. TEA+ caused a concentration-dependent decrease in the single-channel amplitude and open probability of the Ca2(+)-activated K+ channel. A Kd for the reduction in the mean current of 0.14 mM was observed. The stoichiometry was approximately 1:1. 5. Quinine blocked the Ca2(+)-activated K+ channel in a concentration-dependent manner. Half-maximal block was observed at 0.10 mM and binding was 1:1. Inhibition by 20 microM-quinine was not associated with a decrease in channel amplitude but markedly reduced the lifetime of the channel openings. Two exponentials, with time constants of 0.5 and 1.3 ms, were required to describe the channel openings. The rapid component contained 55% of the events. 6. TEA+ reduced the single-channel amplitude of the ATP-regulated K+ channel in a concentration-dependent manner. Kd for the block was 22 mM and the binding approximately 1:1. The block was not associated with changes in the open probability or channel kinetics. Two exponentials were required to describe the distribution of the open times. The time constants for the fast and slow components were approximately 2 and approximately 20 ms respectively. The rapid component accounted for approximately 35% of the events. 7. Quinine (10-20 microM) almost abolished activity of the ATP-regulated K+ channels. Inhibition was characterized by slow onset and reversibility but not associated with a change in the appearance of the single-channel events. Quinine-induced block could not be reversed by diazoxide. 8. We conclude that TEA+ produces rapid block of both Ca2(+)-activated and ATP-regulated K+ channels.(ABSTRACT TRUNCATED AT 400 WORDS)
机译:1.使用膜片钳技术的全细胞和由外而外的膜片配置来研究细胞外四乙基铵离子(TEA +)和奎宁对小鼠胰腺Ca2(+)激活和ATP调节的K +通道的影响β细胞。 2.当用生理离子梯度记录时,Ca2(+)激活的K +通道具有4.7 x 10(-13)cm3 s-1的单通道K +渗透率。加入0.3 mM-TEA +后,该值降至2.9 x 10(-13)cm3 s-1。 3.需要两个时间常数分别为0.2和4.7 ms的指数来描述通道开口的分布,这表明Ca2(+)激活的K +通道具有至少两个打开状态。快速和慢速组件分别占开口总数的16%和84%。 4. TEA +导致Ca2(+)激活的K +通道的单通道幅度和打开概率的浓度依赖性降低。观察到平均电流降低0.14mM的Kd。化学计量比约为1:1。 5.奎宁以浓度依赖性方式阻断Ca2(+)激活的K +通道。在0.10 mM处观察到最大半峰阻滞,结合为1:1。 20 microM-奎宁的抑制作用与通道振幅的降低无关,但显着降低了通道开口的寿命。需要两个指数,其时间常数分别为0.5和1.3 ms,以描述通道的开口。快速部分包含55%的事件。 6. TEA +以浓度依赖的方式降低了ATP调节的K +通道的单通道幅度。该嵌段的Kd为22mM,结合约为1∶1。阻滞与打开概率或通道动力学的变化无关。需要两个指数来描述开放时间的分布。快速和慢速分量的时间常数分别约为2 ms和20 ms。快速事件约占事件总数的35%。 7.奎宁(10-20 microM)几乎消除了ATP调节的K +通道的活性。抑制的特征是起效缓慢和可逆性,但与单通道事件的外观变化无关。奎宁诱导的阻滞不能被二氮嗪逆转。 8.我们得出结论,TEA +可以快速阻断Ca2(+)激活和ATP调节的K +通道。(抽象截断为400字)

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