首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >A neutral amino acid change in segment IIS4 dramatically alters the gating properties of the voltage-dependent sodium channel.
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A neutral amino acid change in segment IIS4 dramatically alters the gating properties of the voltage-dependent sodium channel.

机译:区段IIS4中的中性氨基酸变化显着改变了电压依赖性钠通道的门控特性。

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摘要

Sodium channels encoded by the rat IIA cDNA clone [Auld, V. J., Goldin, A. L., Krafte, D. S., Marshall, J., Dunn, J., Catterall, W. A., Lester, H. A., Davidson, N. & Dunn, R. J. (1988) Neuron 1, 449-461] differ at seven amino acid residues from those encoded by the rat II cDNA [Noda, M., Ikeda, T., Kayano, T., Suzuki, H., Takeshima, H., Kurasaki, M., Takahashi, H. & Numa, S. (1986) Nature (London) 320, 188-192]. When expressed in Xenopus oocytes, rat IIA channels display a current-voltage relationship that is shifted 20-25 mV in the depolarizing direction relative to channels expressed from rat II cDNA or rat brain poly(A)+ mRNA. By modifying each variant residue in rat IIA to the corresponding residue in rat II, we demonstrate that a single Phe----Leu substitution at position 860 in the S4 segment of domain II is sufficient to shift the current-voltage relationship to that observed for channels expressed from rat brain poly(A)+ RNA or rat II cDNA. Rat genomic DNA encodes leucine but not phenylalanine at position 860, indicating that the phenylalanine at this position in rat IIA cDNA likely results from reverse transcriptase error.
机译:大鼠IIA cDNA克隆编码的钠通道[Auld,VJ,Goldin,AL,Krafte,DS,Marshall,J.,Dunn,J.,Catterall,WA,Lester,HA,Davidson,N.&Dunn,RJ(1988) )神经元1,449-461]与大鼠II cDNA编码的氨基酸残基有7个氨基酸残基[Noda,M.,Ikeda,T.,Kayano,T.,Suzuki,H.,Takeshima,H.,Kurasaki, M.,Takahashi,H。&Numa,S。(1986)Nature(London)320,188-192]。当在非洲爪蟾卵母细胞中表达时,大鼠IIA通道显示的电流-电压关系相对于大鼠II cDNA或大鼠脑poly(A)+ mRNA表达的通道在去极化方向上偏移了20-25 mV。通过将大鼠IIA中的每个变异残基修饰为大鼠II中的相应残基,我们证明了结构域II S4区段860位的单个Phe ---- Leu取代足以将电流-电压关系转变为观察到的用于从大鼠大脑poly(A)+ RNA或大鼠II cDNA表达的通道。大鼠基因组DNA在860位编码亮氨酸,但不编码苯丙氨酸,这表明大鼠IIA cDNA此位置的苯丙氨酸可能是由逆转录酶错误引起的。

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