Hilber Karlheinz, Sandtner Walter, Kudlacek Oliver, Schreiner Blanca, Glaaser Ian, Schütz Wolfgang, Fozzard Harry A, Dudley Samuel C, Todt Hannes
Institute of Pharmacology, University of Vienna, A-1090 Vienna, Austria.
J Biol Chem. 2002 Oct 4;277(40):37105-15. doi: 10.1074/jbc.M205661200. Epub 2002 Jul 23.
Recently, we reported that mutation A1529D in the domain (D) IV P-loop of the rat skeletal muscle Na(+) channel mu(1) (DIV-A1529D) enhanced entry to an inactivated state from which the channels recovered with an abnormally slow time constant on the order of approximately 100 s. Transition to this "ultra-slow" inactivated state (USI) was substantially reduced by binding to the outer pore of a mutant mu-conotoxin GIIIA. This indicated that USI reflected a structural rearrangement of the outer channel vestibule and that binding to the pore of a peptide could stabilize the pore structure (Hilber, K., Sandtner, W., Kudlacek, O., Glaaser, I. W., Weisz, E., Kyle, J. W., French, R. J., Fozzard, H. A., Dudley, S. C., and Todt, H. (2001) J. Biol. Chem. 276, 27831-27839). Here, we tested the hypothesis that occlusion of the inner vestibule of the Na(+) channel by the fast inactivation gate inhibits ultra-slow inactivation. Stabilization of the fast inactivated state (FI) by coexpression of the rat brain beta(1) subunit in Xenopus oocytes significantly prolonged the time course of entry to the USI. A reduction in USI was also observed when the FI was stabilized in the absence of the beta(1) subunit, suggesting a causal relation between the occurrence of the FI and inhibition of USI. This finding was further confirmed in experiments where the FI was destabilized by introducing the mutations I1303Q/F1304Q/M1305Q. In DIV-A1529D + I1303Q/F1304Q/M1305Q channels, occurrence of USI was enhanced at strongly depolarized potentials and could not be prevented by coexpression of the beta(1) subunit. These results strongly suggest that FI inhibits USI in DIV-A1529D channels. Binding to the inner pore of the fast inactivation gate may stabilize the channel structure and thereby prevent USI. Some of the data have been published previously in abstract form (Hilber, K., Sandtner, W., Kudlacek, O., Singer, E., and Todt, H. (2002) Soc. Neurosci. Abstr. 27, program number 46.12).
最近,我们报道大鼠骨骼肌钠通道μ1的结构域(D)IV P环中的A1529D突变(DIV - A1529D)增强了通道进入失活状态的能力,通道从该失活状态恢复的时间常数异常缓慢,约为100秒。与突变型μ - 芋螺毒素GIIIA的外孔结合可显著减少向这种“超慢”失活状态(USI)的转变。这表明USI反映了通道外前庭的结构重排,并且与肽孔的结合可以稳定孔结构(希尔伯,K.,桑特纳,W.,库德拉克,O.,格拉泽,I. W.,魏斯,E.,凯尔,J. W.,弗伦奇,R. J.,福扎德,H. A.,达德利,S. C.,和托特,H.(2001年)《生物化学杂志》276,27831 - 27839)。在此,我们测试了以下假设:快速失活门对钠通道内前庭的阻塞会抑制超慢失活。在非洲爪蟾卵母细胞中共表达大鼠脑β1亚基来稳定快速失活状态(FI),显著延长了进入USI的时间进程。在没有β1亚基的情况下稳定FI时,也观察到USI减少,这表明FI的出现与USI的抑制之间存在因果关系。在通过引入I1303Q/F1304Q/M1305Q突变使FI不稳定的实验中,这一发现得到了进一步证实。在DIV - A1529D + I1303Q/F1304Q/M1305Q通道中,在强去极化电位下USI的出现增加,并且β1亚基的共表达无法阻止这种情况。这些结果强烈表明FI抑制DIV - A1529D通道中的USI。与快速失活门的内孔结合可能稳定通道结构,从而防止USI。部分数据先前已以摘要形式发表(希尔伯,K.,桑特纳,W.,库德拉克,O.,辛格,E.,和托特,H.(2002年)《神经科学学会摘要》27,编号46.12)。
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