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培养的小鼠脊髓神经元中钙和电压依赖性氯电导的电压钳分析。

Voltage-clamp analysis of a Ca2+- and voltage-dependent chloride conductance in cultured mouse spinal neurons.

作者信息

Owen D G, Segal M, Barker J L

出版信息

J Neurophysiol. 1986 Jun;55(6):1115-35. doi: 10.1152/jn.1986.55.6.1115.

Abstract

Current and voltage-clamp recordings were made at room temperature from cultured mouse spinal neurons using conventional two-electrode voltage-clamp techniques and electrodes filled with either 3 M KCl, 3 M CsCl, or 3 M Cs2SO4. In the presence of tetraethylammonium and tetrodotoxin, "fast" (rapidly rising and falling) action potentials (FAP) of variable duration were recorded in most neurons. "Slow" (slowly rising and falling) depolarizing potentials (SDP) occurred in 23% of the cells, when using KCl-filled electrodes, and in 82% of the cells with CsCl-filled electrodes. The SDP was frequently preceded by an FAP, although in some cells activation of the SDP occurred before the FAP threshold was reached and in a graded fashion. Both the FAP and SDP were abolished by Cd2+ and other Ca2+ antagonists. In cells exhibiting SDPs, voltage-clamp analysis revealed a sustained (noninactivating) inward current (Isin) during depolarizing steps to potentials more positive than -45 mV. Repolarizing steps resulted in slowly decaying inward tail currents (Itail). Both Isin and Itail were abolished in solutions nominally free of Cao2+, or containing Ca2+-channel antagonists. Bao2+ did not support Isin. The data indicated a U-shaped activation curve for Isin, peaking at about -10 mV. Activation of Isin occurred exponentially with a time constant of approximately 140 ms at -23 mV, becoming faster at more depolarized potentials (ca. 50 ms at -2 mV). Deactivation was slow, giving rise to tail currents lasting seconds. In some cases deactivation could be described by a single exponential process, although frequently the kinetics were more complex. Deactivation was faster at hyperpolarized potentials and sensitive to extracellular ([Ca2+]o), duration of activating voltage steps, and the degree of activation of Isin. Using CsCl-filled electrodes, the reversal potential (Erev) for Isin was -1.7 mV (SEM 3.5 mV, n = 20). Erev always corresponded to the reversal potential for gamma-aminobutyric acid-evoked currents in the same cell. In experiments in which Cs2SO4-filled electrodes were used, Erev was estimated to be -44 mV (SEM 2.3 mV, n = 9). Neither complete substitution of Nao+ with choline ions nor elevation of [K+]o 10-fold significantly affected the estimated Erev. However, substitution of Cl0- with isethionate or methanesulphonate increased the amplitude of inward currents (recorded with CsCl-filled electrodes) and shifted Erev to more depolarized potentials. The results indicate that Cl- are the primary charge carriers for this current and that Cai2+ is required for its activation, leading us to identify it as ICl(Ca).(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

在室温下,使用传统的双电极电压钳技术,从培养的小鼠脊髓神经元中进行电流钳和电压钳记录,电极填充有3M KCl、3M CsCl或3M Cs2SO4。在四乙铵和河豚毒素存在的情况下,大多数神经元记录到了持续时间可变的“快”(快速上升和下降)动作电位(FAP)。当使用填充KCl的电极时,23%的细胞出现“慢”(缓慢上升和下降)去极化电位(SDP),而使用填充CsCl的电极时,82%的细胞出现SDP。SDP之前常常有一个FAP,尽管在一些细胞中,SDP的激活在达到FAP阈值之前就已发生,且呈分级方式。FAP和SDP都被Cd2+和其他Ca2+拮抗剂所消除。在表现出SDP的细胞中,电压钳分析显示,在去极化至比-45mV更正的电位时,有一个持续(非失活)的内向电流(Isin)。复极化步骤导致内向尾电流(Itail)缓慢衰减。在名义上无Ca2+或含有Ca2+通道拮抗剂的溶液中,Isin和Itail都被消除。Ba2+不支持Isin。数据表明Isin的激活曲线呈U形,在约-10mV处达到峰值。在-23mV时,Isin的激活呈指数形式,时间常数约为140ms,在更去极化的电位时变得更快(在-2mV时约为50ms)。失活缓慢,导致尾电流持续数秒。在某些情况下,失活可以用单个指数过程来描述,尽管其动力学通常更复杂。在超极化电位时失活更快,且对细胞外([Ca2+]o)、激活电压步骤的持续时间以及Isin的激活程度敏感。使用填充CsCl的电极时,Isin的反转电位(Erev)为-1.7mV(标准误3.5mV,n = 20)。Erev总是与同一细胞中γ-氨基丁酸诱发电流的反转电位相对应。在使用填充Cs2SO4电极的实验中,Erev估计为-44mV(标准误2.3mV,n = 9)。用胆碱离子完全替代Na+或使[K+]o升高10倍,均未显著影响估计的Erev。然而,用羟乙磺酸盐或甲磺酸盐替代Cl-会增加内向电流的幅度(用填充CsCl的电极记录),并使Erev向更去极化的电位移动。结果表明,Cl-是该电流的主要电荷载体,Ca2+是其激活所必需的,这使我们将其鉴定为ICl(Ca)。(摘要截断于400字)

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