首页> 美国卫生研究院文献>The Journal of Physiology >Properties and functions of Na(+)-activated K+ channels in the soma of rat motoneurones.
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Properties and functions of Na(+)-activated K+ channels in the soma of rat motoneurones.

机译:大鼠运动神经元的体中Na(+)激活的K +通道的性质和功能。

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摘要

1.Properties and functions of Na(+)-activated K+ (KNa) channels in the soma of motoneurones were studied in spinal cord slices of newborn rat. KNa channels had a conductance of 44.8 pS in 5.6 mM external K+ (Ko+)/106 mM internal K+ (Ki+) solutions and 139.2 pS in 155 mM Ko+/85 mM Ki+ solutions. KNa channels were voltage independent and needed a relatively high [Na+]i to become active (EC50 = 39.9 mM). Li+ could not substitute for Na+ in activation of KNa channels. The channels were predominantly found in the vicinity of cell processes, in the regions of most probable accumulation of cytoplasmic Na+. 2. In current-clamp experiments, the shape of the single action potential (AP) recorded in Ca(2+)-free Ringer solution was not changed after substitution of external Na+ with Li+. However, 0.4-0.8 s trains of APs were followed by a slow (1-2s) after-hyperpolarization (sAHP), which reversibly disappeared when external Na+ was replaced by Li+. Na(+)-activated sAHP persisted after addition of ouabain and its amplitude was even increased in K(+)-free Ringer solution. sAHP disappeared when the membrane potential was equal to the K+ equilibrium potential. This indicated that sAHP resulted from activation of a Na(+)-dependent K+ conductance, rather than from activation of the electrogenic Na(+)-K+ pump. 3. In conclusion, KNa channels can play an important role in excitability of motoneurones. KNa channels do not make a contribution to the single AP, but they can be activated by a local accumulation of internal Na+ during trains of APs. A Na(+)-activated K+ conductance can reduce membrane excitability and contribute to regulation of AP firing in motoneurones.
机译:1,在新生大鼠的脊髓切片中研究了运动神经元体中Na(+)激活的K +(KNa)通道的性质和功能。 KNa通道在5.6 mM外部K +(Ko +)/ 106 mM内部K +(Ki +)溶液中的电导率为44.8 pS,在155 mM Ko + / 85 mM Ki +溶液中的电导率为139.2 pS。 KNa通道不受电压影响,需要相对较高的[Na +] i才能激活(EC50 = 39.9 mM)。在激活KNa通道中,Li +不能替代Na +。该通道主要在细胞过程附近,最可能的细胞质Na +积累区域中发现。 2.在电流钳实验中,用Li +取代外部Na +后,无Ca(2+)的林格溶液中记录的单作用电位(AP)的形状没有改变。但是,在0.4-0.8 s的AP序列之后是缓慢的(1-2s)超极化后(sAHP),当外部Na +被Li +替代时,可逆极化消失。加入哇巴因后,Na(+)活化的sAHP持续存在,并且在无K(+)的林格溶液中其幅度甚至增加。当膜电位等于K +平衡电位时,sAHP消失。这表明sAHP是由Na(+)依赖性K +电导的激活引起的,而不是由电致Na(+)-K +泵的激活引起的。 3.总之,KNa通道在运动神经元的兴奋性中起重要作用。 KNa通道对单个AP不起任何作用,但是可以在AP训练期间由内部Na +的局部积累来激活。 Na(+)激活的K +电导可以降低膜的兴奋性,并有助于调节运动神经元中AP的发射。

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