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用短杆菌肽穿孔膜片钳记录法研究大鼠中枢神经系统神经元中的甘氨酸反应。

Glycine responses in rat CNS neurons studied with gramicidin perforated patch recording.

作者信息

Akaike N

机构信息

Department of Physiology, Kyushu University Faculty of Medicine, Fukuoka, Japan.

出版信息

Jpn J Physiol. 1994;44 Suppl 2:S113-8.

PMID:7538604
Abstract

The conventional whole-cell recording of the patch-clamp technique has a great advantage over other electrical recording methods in that it could perfectly control the extra- and intracellular concentrations of ions (such as Na+, K+, Ca2+, and Cl-). However, this advantage is a two-edged sword: it disrupts the physiological ionic environment inside cells. Thus, various Cl(-)-mediated responses in neurons, such as those elicited by inhibitory amino acids, gamma-amino butyric acid (GABA) and glycine (Gly), have been recorded only under an artificial condition. Subsequently, measurement of the normal concentration of intracellular Cl- ([Cl-]i) has been much hampered. [Cl-]i is suggested to play a role in membrane excitability (Deisz and Lux: J Physiol 326: 123-138, 1982) and intracellular signal transduction (Higashijima, Ferguson, and Sternweis: J Biol Chem 262: 3597-3602, 1987), yet the detailed analysis of these fundamental roles has been left undone due to technical difficulties. We have recently developed a "gramicidin perforated patch recording", a novel method of patch-clamp technique that enables analysis of membrane currents with intact [Cl-]i. We here report that by applying this method to acutely dissociated CNS neurons of the rat, we could analyze the Gly-induced membrane currents in the normal ionic environment. And using the reversal potentials, we could deduce the actual [Cl-]i of central neurons.

摘要

膜片钳技术的传统全细胞记录法相较于其他电记录方法具有很大优势,因为它能够完美地控制细胞外和细胞内的离子浓度(如Na +、K +、Ca2 +和Cl -)。然而,这一优势也是一把双刃剑:它会破坏细胞内的生理离子环境。因此,神经元中各种由Cl -介导的反应,如由抑制性氨基酸、γ -氨基丁酸(GABA)和甘氨酸(Gly)引发的反应,仅在人工条件下被记录到。随后,细胞内Cl -正常浓度([Cl -]i)的测量受到了很大阻碍。有研究表明[Cl -]i在膜兴奋性(Deisz和Lux:《生理学杂志》326:123 - 138,1982)和细胞内信号转导(Higashijima、Ferguson和Sternweis:《生物化学杂志》262:3597 - 3602,1987)中发挥作用,然而由于技术困难,对这些基本作用的详细分析尚未完成。我们最近开发了一种“短杆菌肽穿孔膜片记录法”,这是一种新型的膜片钳技术方法,能够在[Cl -]i完整的情况下分析膜电流。在此我们报告,通过将该方法应用于大鼠急性分离的中枢神经系统神经元,我们能够在正常离子环境中分析甘氨酸诱导的膜电流。并且利用反转电位,我们可以推断中枢神经元的实际[Cl -]i。

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Jpn J Physiol. 1994;44 Suppl 2:S113-8.
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