首页> 美国卫生研究院文献>The Journal of Physiology >A non-inactivating K+ current sensitive to muscarinic receptor activation in rat cultured cerebellar granule neurons.
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A non-inactivating K+ current sensitive to muscarinic receptor activation in rat cultured cerebellar granule neurons.

机译:对大鼠培养的小脑颗粒神经元中毒蕈碱受体激活敏感的非灭活K +电流。

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摘要

1. Whole-cell recordings were made from cultured cerebellar granule neurons using perforated patch clamp techniques. The primary cultures were prepared using 6- to 9-day-old Sprague-Dawley rats. 2. Neurons in culture for less than 48 h possessed resting membrane potentials of -29 mV. However, neurons in culture for 7 days had much more hyperpolarized resting membrane potentials (-89 mV). Over the same period, these neurons developed an additional component of outward current. 3. This non-inactivating current was activated by depolarization, exhibited outward rectification and reversed close to the potassium equilibrium potential. The kinetics of activation and deactivation were very rapid. 4. Muscarine ((+)-muscarine chloride) reversibly inhibited the current with an EC50 of 0.17 microM. The inhibition by muscarine was unaffected by pre-incubation for 17-20 h with 120 micrograms ml-1 pertussis toxin. 5. The current and its inhibition by muscarine were unaffected by 100 microM Cd2+. In Ca(2+)-free conditions, the current was significantly larger than in 0.5 mM Ca2+, but inhibition by 10 microM muscarine was significantly reduced. 6. The standing outward current was not obviously affected by 50 microM 5-HT, 50 microM noradrenaline, 50 microM 2-chloroadenosine or 5 mM tetraethylammonium. It was reduced by 10 microM La3+, 10 microM Zn2+ and 1 mM Ba2+. 7. Muscarinic agonists increased the input resistance of neurons and shifted the zero current level in the depolarized direction when voltage clamped. This enhanced excitability was evident under current clamp, where 10 microM muscarine depolarized granule neurons such that action potentials became evident.
机译:1.使用穿孔膜片钳技术从培养的小脑颗粒神经元进行全细胞记录。使用6至9天大的Sprague-Dawley大鼠制备原代培养物。 2.培养少于48小时的神经元具有-29 mV的静息膜电位。但是,培养7天的神经元具有更多的超极化静息膜电位(-89 mV)。在同一时期,这些神经元发展了外向电流的额外组成部分。 3.该非灭活电流通过去极化激活,表现出向外的整流作用,并在接近钾平衡电位时反转。活化和失活的动力学非常快。 4.毒蕈碱((+)-毒蕈碱氯化物)可逆地抑制电流,EC50为0.17 microM。与120微克ml-1百日咳毒素的预孵育17-20小时不会影响毒蕈碱的抑制作用。 5.电流及其对毒蕈碱的抑制作用不受100 microM Cd2 +的影响。在无Ca(2+)的条件下,电流明显大于0.5 mM Ca2 +,但10 microM毒蕈碱的抑制作用明显降低。 6. 50 microM 5-HT,50 microM去甲肾上腺素,50 microM 2-氯腺苷或5 mM四乙铵对站立的向外电流没有明显影响。减少了10 microM La3 +,10 microM Zn2 +和1 mM Ba2 +。 7.毒蕈碱激动剂在钳位电压时会增加神经元的输入电阻,并使零电流水平沿去极化方向移动。这种增强的兴奋性在电流钳下很明显,其中有10 microM毒蕈碱使细胞神经元去极化,从而使动作电位变得明显。

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