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Single-channel properties of the reconstituted voltage-regulated Na channel isolated from the electroplax of Electrophorus electricus.

机译:重组电压调节的Na通道的单通道性质,该通道与Electrophorus electrous的电浆分离。

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摘要

The tetrodotoxin-binding protein purified from electroplax of Electrophorus electricus has been reincorporated into multilamellar vesicles that were used for patch recording. When excised patches of these reconstituted membranes were voltage clamped in the absence of neurotoxins, voltage-dependent single-channel currents were recorded. These displayed properties qualitatively and quantitatively similar to those reported for Na channels from nerve and muscle cells, including uniform single-channel conductances of the appropriate magnitude (approximately equal to 11 pS in 95 mM Na+), mean open times of approximately equal to 1.9 msec, and 7-fold selectively for Na+ over K+. Currents averaged from many depolarizations showed initial voltage-dependent activation and subsequent inactivation. In the presence of batrachotoxin, channels were observed with markedly different properties, including conductances of 20-25 pS (95 mM Na+), mean open times of approximately equal to 28 msec, and no indication of inactivation. Collectively, these findings indicate that the tetrodotoxin-binding protein of electroplax is a voltage-regulated sodium channel.
机译:从电泳的电质粒纯化的河豚毒素结合蛋白已被重新掺入用于膜片记录的多层囊泡中。当在没有神经毒素的情况下将这些重组膜的切下的片进行电压钳制时,记录了电压依赖性单通道电流。这些显示的性质在质量和数量上与神经和肌肉细胞的Na通道报道的相似,包括适当大小的均匀单通道电导(在95 mM Na +中约等于11 pS),平均打开时间约1.9毫秒,对Na +的选择性是对K +的7倍。来自许多去极化的平均电流显示出初始的电压依赖性激活和随后的失活。在存在巴曲毒素的情况下,观察到具有明显不同特性的通道,包括电导为20-25 pS(95 mM Na +),平均打开时间约为28毫秒,并且没有灭活的迹象。总的来说,这些发现表明电pla的河豚毒素结合蛋白是一个电压调节的钠通道。

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