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Ca2+ efflux mechanisms following depolarization evoked calcium transients in cultured rat sensory neurones.

机译:去极化后的Ca2 +外流机制在培养的大鼠感觉神经元中引起钙瞬变。

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摘要

1. We have used a combination of microfluorimetry and patch-clamp techniques to investigate cytoplasmic Ca2+ ([Ca2+]i) buffering in response to physiological Ca2+ loads in neurones cultured from the dorsal root ganglia of the rat. 2. In cells loaded with Indo-1 AM and using high resistance microelectrodes to initiate and record action potentials, single action potentials were associated with a measurable rise in [Ca2+]i. Short trains of action potentials evoked [Ca2+]i transients with monoexponential recovery rates with time constants of around 5 s. 3. Similar Ca2+ buffering properties were seen in cells perfused with patch-clamp pipettes in the whole-cell recording mode suggesting that the slow (seconds) Ca2+ buffering properties were not seriously perturbed by the recording technique. 4. In cells held under voltage clamp, reversal of the Na(+)-Ca2+ exchanger driving force had a small but significant effect on the rate of Ca2+ removal. 5. Increasing extracellular pH or adding vanadate (200 microM) to the internal solution dramatically slowed the rate of recovery. Addition of calmidazolium to the pipette solution also produced a significant but much less dramatic slowing of Ca2+ efflux. 6. The results demonstrate that the activity of a plasmalemmal Ca(2+)-ATPase is important for the removal of somatic Ca2+ loads of a similar amplitude to those generated by the firing of a few action potentials.
机译:1.我们已经使用微荧光法和膜片钳技术的组合来研究细胞质Ca2 +([Ca2 +] i)的缓冲,以响应从大鼠背根神经节培养的神经元中的生理Ca2 +负荷。 2.在装有Indo-1 AM的细胞中,并使用高电阻微电极引发和记录动作电位,单个动作电位与[Ca2 +] i的可测量升高相关。短时间的动作电位序列诱发了[Ca2 +] i瞬态,具有单指数恢复率,时间常数约为5 s。 3.在全细胞记录模式下,在用膜片钳移液器灌注的细胞中观察到了相似的Ca2 +缓冲特性,这表明慢速(秒)的Ca2 +缓冲特性并未受到记录技术的严重干扰。 4.在保持电压钳位的电池中,Na(+)-Ca2 +交换器驱动力的反转对Ca2 +的去除速率影响很小,但影响很大。 5.增加细胞外pH或向内部溶液中添加钒酸盐(200 microM)会大大减慢回收率。在移液器溶液中加入Calidazolium也会显着降低Ca2 +的外流,但幅度要小得多。 6.结果表明,质膜Ca(2 +)-ATPase的活性对于去除体态Ca2 +负荷非常重要,该负荷的幅度与通过发射一些动作电位产生的幅度相似。

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