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首页> 外文期刊>The Journal of general physiology >Regulation of intracellular cyclic GMP concentration by light and calcium in electropermeabilized rod photoreceptors.
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Regulation of intracellular cyclic GMP concentration by light and calcium in electropermeabilized rod photoreceptors.

机译:光和钙在电透杆感光细胞中对细胞内循环GMP浓度的调节。

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摘要

This study examines the regulation of cGMP by illumination and by calcium during signal transduction in vertebrate retinal photoreceptor cells. We employed an electropermeabilized rod outer segment (EP-ROS) preparation which permits perfusion of low molecular weight compounds into the cytosol while retaining many of the features of physiologically competent, intact rod outer segments (ROS). When nucleotide-depleted EP-ROS were incubated with MgGTP, time- and dose-dependent increases in intracellular cGMP levels were observed. The steady state cGMP concentration in EP-ROS (0.007 mol cGMP per mol rhodopsin) approached the cGMP concentration in intact ROS. Flash illumination of EP-ROS in a 250-nM free calcium medium resulted in a transient decrease in cGMP levels; this occurred in the absence of changes in calcium concentration. The kinetics of the cGMP response to flash illumination of EP-ROS were similar to that of intact ROS. To further examine the effects of calcium on cGMP metabolism, dark-adapted EP-ROS were incubated with MgGTP containing various concentrations of calcium. We observed a twofold increase in cGMP steady state levels as the free calcium was lowered from 1 microM to 20 nM; this increase was comparable to the behavior of intact ROS. Measurements of guanylate cyclase activity in EP-ROS showed a 3.5-fold increase in activity over this range of calcium concentrations, indicating a retention of calcium regulation of guanylate cyclase in EP-ROS preparations. Flash illumination of EP-ROS in either a 50- or 250-nM free calcium medium revealed a slowing of the recovery time course at the lower calcium concentration. This observation conflicts with any hypothesis whereby a reduction in free calcium concentration hastens the recovery of cytoplasmic cGMP levels, either by stimulating guanylate cyclase activity or by inhibiting phosphodiesterase activity. We conclude that changes in the intracellular calcium concentration during visual transduction may have more complex effects on the recovery of the photoresponse than can be accounted for solely by guanylate cyclase activation.
机译:这项研究检查了脊椎动物视网膜感光细胞信号传导过程中光照和钙对cGMP的调节作用。我们采用了电渗透杆外段(EP-ROS)制剂,该制剂允许将低分子量化合物灌注到细胞质中,同时保留了生理上完整的杆外段(ROS)的许多特征。当将核苷酸耗尽的EP-ROS与MgGTP孵育时,观察到细胞内cGMP水平随时间和剂量的增加。 EP-ROS中的稳态cGMP浓度(每摩尔视紫红质0.007 mol cGMP)接近完整ROS中的cGMP浓度。在250nM游离钙培养基中对EP-ROS进行闪光灯照明会导致cGMP水平短暂下降;这发生在钙浓度没有变化的情况下。对EP-ROS闪光灯照明的cGMP响应动力学与完整ROS相似。为了进一步检查钙对cGMP代谢的影响,将暗适应的EP-ROS与含有各种浓度钙的MgGTP孵育。我们观察到,随着游离钙从1 microM降低到20 nM,cGMP稳态水平增加了两倍。这种增加与完整ROS的行为相当。对EP-ROS中鸟苷酸环化酶活性的测量表明,在该钙浓度范围内,活性增加了3.5倍,表明在EP-ROS制剂中保留了鸟苷酸环化酶的钙调节。在50nM或250nM的游离钙介质中对EP-ROS进行的闪光灯照明显示,在较低的钙浓度下,恢复时间的进程变慢。该观察结果与任何假说相抵触,在假说中,游离钙浓度的降低通过刺激鸟苷酸环化酶活性或抑制磷酸二酯酶活性而加快了细胞质cGMP水平的恢复。我们得出的结论是,视觉传导过程中细胞内钙浓度的变化可能对光响应的恢复产生更复杂的影响,而不能单独由鸟苷酸环化酶激活来解释。

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