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完整细胞中电压对环鸟苷酸门控电导的影响揭示视网膜视杆和视锥光感受器之间钙稳态的差异。

Differences in calcium homeostasis between retinal rod and cone photoreceptors revealed by the effects of voltage on the cGMP-gated conductance in intact cells.

作者信息

Miller J L, Korenbrot J I

机构信息

Department of Physiology, School of Medicine, University of California at San Francisco 94143.

出版信息

J Gen Physiol. 1994 Nov;104(5):909-40. doi: 10.1085/jgp.104.5.909.

Abstract

We measured currents under voltage clamp in intact retinal rod photoreceptors with tight seal electrodes in the perforated patch mode. In the dark, membrane depolarization to voltages > or = +20 mV activates a time- and voltage-dependent outward current in the outer segment. This dark voltage-activated current (DVAC) increases in amplitude with a sigmoidal time course that is voltage dependent. DVAC reaches its maximum enhancement of approximately 30% in 4-6 s at +60 mV. DVAC is entirely suppressed by light and its current-voltage curve and reversal potential are the same as those of the photocurrent. Therefore, DVAC arises from the opening in darkness of the cGMP-gated channels of the outer segment. DVAC is blocked by BAPTA loaded into the cell's cytoplasm and is enhanced by lowering extracellular Ca2+ concentration. Because the cGMP-gated channels are not directly gated by voltage and because BAPTA blocks DVAC, we suggest this signal arises from a voltage-dependent decrease in cytoplasmic Ca2+ concentration that, in turn, activates guanylyl cyclase and causes cGMP synthesis. In rods loaded with high cytoplasmic Na+, membrane depolarization in darkness to voltages > or = +20 mV inactivates the outward current in the outer segment with an exponential time course. We call this DVIC (dark, voltage-inactivated current). DVIC reflects voltage-dependent closing of the cGMP-gated channel in the dark. DVIC, too, is blocked by cytoplasmic BAPTA, and it arises from a voltage-dependent rise in cytoplasmic Ca2+ in darkness, which occurs only if cytoplasmic Na is high. We develop a quantitative model to calculate the rate and extent of the voltage-dependent change in cytoplasmic Ca2+ concentration in a normal rod. We assume that this concentration is controlled by the balance between Ca2+ influx through the cGMP-gated channels and its efflux through a Na+/Ca2+, K+ exchanger. Lowered cytoplasmic Ca2+ is linked to guanylyl cyclase activation with characteristics determined from biochemical studies. The model considers the cytoplasmic buffering of both Ca2+ and cGMP. Simulated data generated by the model fit well DVAC measured in rods and also DVAC previously measured in cones. DVAC in cones is larger in magnitude and faster in time course than that in rods. The successful fit of DVAC by the model leads us to suggest that the activity and Ca2+ dependence of the enzymes of transduction are not different in rods and cones, but the quantitative features of Ca2+ homeostasis in the outer segment of the two receptor types differ profoundly.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

我们在穿孔膜片钳模式下,使用高阻封接电极在完整的视网膜视杆光感受器中进行电压钳电流测量。在黑暗中,当膜去极化至电压≥ +20 mV时,外段会激活一种时间和电压依赖性外向电流。这种暗电压激活电流(DVAC)的幅度以电压依赖性的S形时间进程增加。在 +60 mV时,DVAC在4 - 6秒内达到约30%的最大增强。DVAC完全被光抑制,其电流 - 电压曲线和反转电位与光电流相同。因此,DVAC源于外段cGMP门控通道在黑暗中的开放。DVAC被注入细胞胞质的BAPTA阻断,并通过降低细胞外Ca2+浓度而增强。由于cGMP门控通道不直接受电压门控,且BAPTA阻断DVAC,我们认为该信号源于胞质Ca2+浓度的电压依赖性降低,进而激活鸟苷酸环化酶并导致cGMP合成。在胞质Na+浓度高的视杆细胞中,黑暗中膜去极化至电压≥ +20 mV会使外段外向电流以指数时间进程失活。我们将此称为DVIC(暗,电压失活电流)。DVIC反映了黑暗中cGMP门控通道的电压依赖性关闭。DVIC同样被胞质BAPTA阻断,它源于黑暗中胞质Ca2+的电压依赖性升高,这种情况仅在胞质Na+高时发生。我们开发了一个定量模型来计算正常视杆细胞中胞质Ca2+浓度电压依赖性变化的速率和程度。我们假设该浓度由通过cGMP门控通道的Ca2+内流与其通过Na+/Ca2+、K+交换器的外流之间的平衡控制。降低的胞质Ca2+与鸟苷酸环化酶激活相关,其特性由生化研究确定。该模型考虑了Ca2+和cGMP的胞质缓冲作用。该模型生成的模拟数据与视杆细胞中测量的DVAC以及先前在视锥细胞中测量的DVAC拟合良好。视锥细胞中的DVAC在幅度上更大,时间进程更快。该模型对DVAC的成功拟合使我们认为,转导酶的活性和Ca2+依赖性在视杆和视锥细胞中并无差异,但两种受体类型外段中Ca2+稳态的定量特征却有很大不同。(摘要截短至400字)

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