Kv2.1钾通道中钾离子依赖性增强的两种机制。
Two mechanisms of K(+)-dependent potentiation in Kv2.1 potassium channels.
作者信息
Wood M J, Korn S J
机构信息
Department of Physiology and Neurobiology, University of Connecticut, Storrs, Connecticut 06269, USA.
出版信息
Biophys J. 2000 Nov;79(5):2535-46. doi: 10.1016/S0006-3495(00)76494-0.
Elevation of external [K(+)] potentiates outward K(+) current through several voltage-gated K(+) channels. This increase in current magnitude is paradoxical in that it occurs despite a significant decrease in driving force. We have investigated the mechanisms involved in K(+)-dependent current potentiation in the Kv2.1 K(+) channel. With holding potentials of -120 to -150 mV, which completely removed channels from the voltage-sensitive inactivated state, elevation of external [K(+)] up to 10 mM produced a concentration-dependent increase in outward current magnitude. In the absence of inactivation, currents were maximally potentiated by 38%. At more positive holding potentials, which produced steady-state inactivation, K(+)-dependent potentiation was enhanced. The additional K(+)-dependent potentiation (above 38%) at more positive holding potentials was precisely equal to a K(+)-dependent reduction in steady-state inactivation. Mutation of two lysine residues in the outer vestibule of Kv2.1 (K356 and K382), to smaller, uncharged residues (glycine and valine, respectively), completely abolished K(+)-dependent potentiation that was not associated with inactivation. These mutations did not influence steady-state inactivation or the K(+)-dependent potentiation due to reduction in steady-state inactivation. These results demonstrate that K(+)-dependent potentiation can be completely accounted for by two independent mechanisms: one that involved the outer vestibule lysines and one that involved K(+)-dependent removal of channels from the inactivated state. Previous studies demonstrated that the outer vestibule of Kv2.1 can be in at least two conformations, depending on the occupancy of the selectivity filter by K(+) (Immke, D., M. Wood, L. Kiss, and S. J. Korn. 1999. J. Gen. Physiol. 113:819-836; Immke, D., and S. J. Korn. 2000. J. Gen. Physiol. 115:509-518). This change in conformation was functionally defined by a change in TEA sensitivity. Similar to the K(+)-dependent change in TEA sensitivity, the lysine-dependent potentiation depended primarily (>90%) on Lys-356 and was enhanced by lowering initial K(+) occupancy of the pore. Furthermore, the K(+)-dependent changes in current magnitude and TEA sensitivity were highly correlated. These results suggest that the previously described K(+)-dependent change in outer vestibule conformation underlies the lysine-sensitive, K(+)-dependent potentiation mechanism.
细胞外[K⁺]升高可通过多种电压门控K⁺通道增强外向K⁺电流。电流幅度的这种增加是自相矛盾的,因为尽管驱动力显著降低,但这种增加仍会发生。我们研究了Kv2.1 K⁺通道中与K⁺相关的电流增强所涉及的机制。在 -120至 -150 mV的钳制电位下,该电位可使通道完全脱离电压敏感的失活状态,将细胞外[K⁺]升高至10 mM会使外向电流幅度产生浓度依赖性增加。在无失活的情况下,电流最大增强38%。在更正向的钳制电位下,会产生稳态失活,与K⁺相关的增强作用会增强。在更正向钳制电位下额外的与K⁺相关的增强作用(超过38%)恰好等于与K⁺相关的稳态失活的降低。将Kv2.1外前庭的两个赖氨酸残基(K356和K382)突变为较小的不带电荷的残基(分别为甘氨酸和缬氨酸),完全消除了与失活无关的与K⁺相关的增强作用。这些突变不影响稳态失活或由于稳态失活降低导致的与K⁺相关的增强作用。这些结果表明,与K⁺相关的增强作用可完全由两种独立机制解释:一种涉及外前庭赖氨酸,另一种涉及与K⁺相关的使通道从失活状态恢复。先前的研究表明,Kv2.1的外前庭至少可以处于两种构象,这取决于K⁺对选择性过滤器的占据情况(Immke, D., M. Wood, L. Kiss, and S. J. Korn. 1999. J. Gen. Physiol. 113:819 - 836; Immke, D., and S. J. Korn. 2000. J. Gen. Physiol. 115:509 - 518)。这种构象变化在功能上由TEA敏感性的变化定义。与TEA敏感性的K⁺依赖性变化类似,赖氨酸依赖性增强主要(>90%)取决于Lys - 356,并且通过降低孔的初始K⁺占据情况而增强。此外,电流幅度和TEA敏感性的K⁺依赖性变化高度相关。这些结果表明,先前描述的外前庭构象的K⁺依赖性变化是赖氨酸敏感的、与K⁺相关的增强机制的基础。
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