首页> 美国卫生研究院文献>The Journal of General Physiology >Voltage-dependence of Ion Permeation in Cyclic GMP–gated Ion Channels Is Optimized for Cell Function in Rod and Cone Photoreceptors
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Voltage-dependence of Ion Permeation in Cyclic GMP–gated Ion Channels Is Optimized for Cell Function in Rod and Cone Photoreceptors

机译:循环GMP门控离子通道中离子渗透的电压依赖性针对杆和锥体感光器的细胞功能进行了优化。

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摘要

The kinetics of the photocurrent in both rod and cone retinal photoreceptors are independent of membrane voltage over the physiological range (−30 to −65 mV). This is surprising since the photocurrent time course is regulated by the influx of Ca2+ through cGMP-gated ion channels (CNG) and the force driving this flux changes with membrane voltage. To understand this paradigm, we measured Pf, the fraction of the cyclic nucleotide–gated current specifically carried by Ca2+ in intact, isolated photoreceptors. To measure Pf we activated CNG channels by suddenly increasing free 8-Br-cGMP in the cytoplasm of rods or cones loaded with a caged ester of the cyclic nucleotide. Simultaneous with the uncaging flash, we measured the cyclic nucleotide–dependent changes in membrane current and fluorescence of the Ca2+ binding dye, Fura-2, also loaded into the cells. We determined Pf under physiological solutions at various holding membrane voltages between −65 and −25 mV. Pf is larger in cones than in rods, but in both photoreceptor types its value is independent of membrane voltage over the range tested. This biophysical feature of the CNG channels offers a functional advantage since it insures that the kinetics of the phototransduction current are controlled by light, and not by membrane voltage. To explain our observation, we developed a rate theory model of ion permeation through CNG channels that assumes the existence of two ion binding sites within the permeation pore. To assign values to the kinetic rates in the model, we measured experimental I-V curves in membrane patches of rods and cones over the voltage range −90 to 90 mV in the presence of simple biionic solutions at different concentrations. We optimized the fit between simulated and experimental data. Model simulations describe well experimental photocurrents measured under physiological solutions in intact cones and are consistent with the voltage-independence of Pf, a feature that is optimized for the function of the channel in photoreceptors.
机译:视杆和视锥视网膜感光器中的光电流动力学与生理范围(-30至-65 mV)的膜电压无关。这是令人惊讶的,因为光电流的时程受Ca 2 + 通过cGMP门控离子通道(CNG)的流入调节,并且驱动该通量的力随膜电压而变化。为了理解这一范例,我们测量了Pf,即Ca 2 + 在完整的分离的感光细胞中特异性携带的环状核苷酸门控电流的一部分。为了测量Pf,我们通过突然增加装有环状核苷酸笼状酯的视杆或视锥细胞质中的游离8-Br-cGMP来激活CNG通道。与开卷闪光同时,我们测量了也加载到细胞中的Ca 2 + 结合染料Fura-2的膜电流和荧光的环状核苷酸依赖性变化。我们在生理溶液下在-65至-25 mV的各种保持膜电压下确定Pf。圆锥体中的Pf比棒中的Pf大,但是在两种感光体类型中,Pf的值均与测试范围内的膜电压无关。 CNG通道的这种生物物理特征提供了功能上的优势,因为它确保了光转导电流的动力学是由光而不是由膜电压控制的。为了解释我们的观察,我们开发了一个通过CNG通道进行离子渗透的速率理论模型,该模型假设渗透孔内存在两个离子结合位点。为了给模型中的动力学速率赋值,我们在存在简单浓度的简单的双离子溶液的情况下,在电压范围为-90至90 mV的情况下,测量了杆和锥的膜片中的实验I-V曲线。我们优化了模拟数据与实验数据之间的拟合度。模型仿真描述了在完好的视锥细胞中生理溶液下测得的良好实验光电流,并且与Pf的电压无关性一致,Pf是针对感光器通道功能进行优化的功能。

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