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Kv3 channel assembly trafficking and activity are regulated by zinc through different binding sites

机译:锌通过不同的结合位点调节Kv3通道的组装运输和活性

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摘要

Zinc, a divalent heavy metal ion and an essential mineral for life, regulates synaptic transmission and neuronal excitability via ion channels. However, its binding sites and regulatory mechanisms are poorly understood. Here, we report that Kv3 channel assembly, localization and activity are regulated by zinc through different binding sites. Local perfusion of zinc reversibly reduced spiking frequency of cultured neurons most likely by suppressing Kv3 channels. Indeed, zinc inhibited Kv3.1 channel activity and slowed activation kinetics, independent of its site in the N-terminal T1 domain. Biochemical assays surprisingly identified a novel zinc-binding site in the Kv3.1 C-terminus, critical for channel activity and axonal targeting, but not for the zinc inhibition. Finally, mutagenesis revealed an important role of the junction between the first transmembrane (TM) segment and the first extracellular loop in sensing zinc. Its mutant enabled fast spiking with relative resistance to the zinc inhibition. Therefore, our studies provide novel mechanistic insights into the multifaceted regulation of Kv3 channel activity and localization by divalent heavy metal ions.
机译:锌是一种二价重金属离子,是生命必不可少的矿物质,它通过离子通道调节突触传递和神经元兴奋性。但是,对其结合位点和调节机制了解甚少。在这里,我们报告Kv3通道的组装,本地化和活动是由锌通过不同的结合位点来调节的。锌的局部灌注可逆地降低了培养的神经元的峰值频率,这很可能是通过抑制Kv3通道来实现的。确实,锌抑制了Kv3.1通道的活性并减慢了活化动力学,而与N端T1域中的位点无关。生化分析令人惊讶地在Kv3.1 C端发现了一个新的锌结合位点,这对通道活性和轴突靶向作用至关重要,但对锌抑制作用却不重要。最后,诱变揭示了第一个跨膜(TM)区段和第一个细胞外环之间的连接在感应锌中的重要作用。它的突变体使快速尖峰具有对锌抑制的相对抗性。因此,我们的研究为二价重金属离子对Kv3通道活性和定位的多方面调节提供了新颖的力学见解。

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