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Variation of membrane properties in hair cells isolated from the turtle cochlea.

机译:从乌龟耳蜗中分离出的毛细胞中膜特性的变化。

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摘要

1. Hair cells were enzymatically isolated from identified regions of the turtle basilar papilla and studied with the patch-electrode technique. The experimental aim was to relate the resonance properties seen during current injection to the membrane currents measured in the same cell under whole-cell voltage clamp. 2. Solitary hair cells had resting potentials of about -50 mV, and produced a damped oscillation in membrane potential at the onset and termination of a small current step; the resonant frequency varied from 9 to 350 Hz between cells, and was correlated with the region of papilla from which a cell had been isolated. The inferred frequency map was consistent with the tonotopic arrangement described previously in the intact papilla. 3. Depolarizations from the resting potential under voltage clamp activated a large net outward current with a steep voltage dependence, and the steady-state current-voltage relationship was strongly rectified about the resting potential. Input resistances tended to be smaller in cells with higher resonant frequencies, although there was no concurrent variation in membrane area as inferred from the cell capacitance. 4. The kinetics of the outward current evoked by a small depolarizing step depended upon the resonant frequency, fo, of the hair cell, and were slower in low-frequency cells. On repolarization to the resting potential the current decayed exponentially with a time constant that changed from 150 ms in the lowest-frequency cell to less than 1 ms in the highest-frequency one. The time constant was approximately proportional to 1/f0(2). 5. Following repolarization to different membrane potentials, the tail current was found to reverse around -80 mV, indicating that the outward current was due mainly to K+. 6. The outward current was abolished by extracellular application of 25 mM-tetraethylammonium chloride (TEA), or on exchange of Cs+ for K+ in the intracellular medium filling the recording electrode, each experiment supporting the contention that K+ is the major current carrier. Such treatments also removed the oscillations in membrane potential evoked by imposed current steps. 7. Addition of TEA or intracellular perfusion with Cs+ also revealed a fast inward current with an ionic sensitivity consistent with its being carried by Ca2+. Like the K+ current, the Ca2+ current was activated by small depolarization from the resting potential, and over this voltage range it was about five to ten times smaller than the K+ current. Its activation was more rapid than the fastest outward currents in high-frequency cells.(ABSTRACT TRUNCATED AT 400 WORDS)
机译:1.从确定的乌龟基底乳头区域中酶分离毛细胞,并用贴片电极技术进行研究。实验目的是将电流注入期间看到的共振特性与在全细胞电压钳下在同一细胞中测得的膜电流相关联。 2.孤立的毛细胞的静息电位约为-50 mV,并在小电流阶跃开始和终止时在膜电位上产生阻尼振荡;细胞之间的共振频率从9到350 Hz不等,并且与分离细胞的乳头区域相关。推断的频率图与先前在完整乳头中描述的色调排列方式一致。 3.在电压钳制下从静息电位去极化激活了一个大的净输出电流,并具有陡峭的电压依赖性,并且在静息电位上,稳态电流-电压关系得到了强有力的纠正。具有较高谐振频率的电池中的输入电阻往往较小,尽管从电池电容推断出膜面积没有同时发生变化。 4.一个小的去极化步骤引起的向外电流的动力学取决于毛细胞的共振频率fo,而在低频细胞中则较慢。在重新极化到静止电位时,电流以时间常数呈指数衰减,该时间常数从最低频率的单元中的150 ms变为最高频率的单元中的1 ms以下。时间常数大约与1 / f0(2)成正比。 5.在重新极化为不同的膜电位后,发现尾电流在-80 mV附近反转,这表明向外的电流主要归因于K +。 6.通过在细胞外施加25 mM-四乙基氯化铵(TEA)或在填充记录电极的细胞内介质中将Cs +交换为K +来消除向外的电流,每个实验都支持K +是主要电流载体的观点。这样的处理还消除了施加的电流阶跃引起的膜电位的振荡。 7.添加TEA或用Cs +进行细胞内灌注也显示出快速的内向电流,其离子敏感性与Ca2 +携带的离子敏感性一致。像K +电流一样,Ca2 +电流是通过从静止电位进行的较小去极化激活的,并且在此电压范围内,它比K +电流小大约五到十倍。它的激活比高频单元中最快的向外电流更快。(抽象截断为400字)

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