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Single Channel Properties of Rat Acid–sensitive Ion Channel-1α, -2a, and -3 Expressed in Xenopus Oocytes

机译:在非洲爪蟾卵母细胞中表达的大鼠酸敏感性离子通道-1α,-2a和-3的单通道特性

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摘要

The mammalian nervous system expresses proton-gated ion channels known as acid-sensing ion channels (ASICs). Depending on their location and specialization some neurons express more than one type of ASIC where they may form homo- or heteromeric channels. Macroscopic characteristics of the ASIC currents have been described, but little is known at the single channel level. Here, we have examined the properties of unitary currents of homomeric rat ASIC1α, ASIC2a, and ASIC3 expressed in Xenopus oocytes with the patch clamp technique. We describe and characterize properties unique to each of these channels that can be used to distinguish the various types of ASIC channels expressed in mammalian neurons. The amplitudes of the unitary currents in symmetrical Na+ are similar for the three types of channels (23–18 pS) and are not voltage dependent. However, ASIC1α exhibits three subconductance states, ASIC2a exhibits only one, and ASIC3 none. The kinetics of the three types of channels are different: ASIC1α and ASIC2a shift between modes of activity, each mode has different open probability and kinetics. In contrast, the kinetics of ASIC3 are uniform throughout the burst of activity. ASIC1α, ASIC2a, and ASIC3 are activated by external protons with apparent pH50 of 5.9, 5.0, and 5.4, respectively. Desensitization in the continual presence of protons is fast and complete in ASIC1α and ASIC3 (2.0 and 4.5 s−1, respectively) but slow and only partial in ASIC2a (0.045 s−1). The response to external Ca2+ also differs: μM concentrations of extracellular Ca2+ are necessary for proton gating of ASIC3 (EC50 = 0.28 μM), whereas ASIC1α and ASIC2a do not require Ca2+. In addition, Ca2+ inhibits ASIC1α (KD = 9.2 ± 2 mM) by several mechanisms: decrease in the amplitude of unitary currents, shortening of the burst of activity, and decrease in the number of activated channels. Contrary to previous reports, our results indicate that the Ca2+ permeability of ASIC1α is very small.
机译:哺乳动物的神经系统表达质子门控离子通道,称为酸敏感离子通道(ASICs)。根据它们的位置和专长,某些神经元会表达不止一种类型的ASIC,在那里它们可能形成同型或异型通道。已经描述了ASIC电流的宏观特性,但是在单通道级别了解甚少。在这里,我们用膜片钳技术检查了在爪蟾卵母细胞中表达的同质大鼠ASIC1α,ASIC2a和ASIC3的单位电流的特性。我们描述和表征每个通道独特的属性,可用于区分哺乳动物神经元中表达的各种类型的ASIC通道。对于三种类型的通道(23–18 pS),对称Na +中的单位电流幅度相似,并且与电压无关。但是,ASIC1α呈现三种子导电状态,ASIC2a仅呈现一种状态,而ASIC3无。三种类型的通道的动力学是不同的:ASIC1α和ASIC2a在活动模式之间转换,每种模式具有不同的打开概率和动力学。相反,ASIC3的动力学在整个活动过程中是一致的。 ASIC1α,ASIC2a和ASIC3由外部质子激活,其表观pH50分别为5.9、5.0和5.4。质子连续存在时的脱敏作用在ASIC1α和ASIC3中是快速而完整的(分别为2.0和4.5 s-1),而在ASIC2a中则是缓慢而仅有一部分(0.045 s-1)。对外部Ca2 +的响应也不同:ASIC3的质子门控需要μM浓度的细胞外Ca2 +(EC50 = 0.28μM),而ASIC1α和ASIC2a不需要Ca2 +。另外,Ca2 +通过几种机制抑制ASIC1α(KD = 9.2±2 mM):单位电流幅度的减小,活动爆发的缩短以及激活通道的数量的减少。与以前的报告相反,我们的结果表明ASIC1α的Ca2 +渗透性很小。

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  • 年度 2002
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  • 正文语种 {"code":"en","name":"English","id":9}
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