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光诱导的cGMP代谢通量增加与光感受器的电反应相对应。

Light-induced increases in cGMP metabolic flux correspond with electrical responses of photoreceptors.

作者信息

Ames A, Walseth T F, Heyman R A, Barad M, Graeff R M, Goldberg N D

出版信息

J Biol Chem. 1986 Oct 5;261(28):13034-42.

PMID:2875993
Abstract

The metabolism of photoreceptor cGMP and the relationship of its light-sensitive regulation to rhodopsin photoisomerization and to the photoreceptor electrical response was examined in isolated, intact rabbit retinas. The dynamics of cGMP metabolism were assessed by measuring the rate of 18O incorporation from 18O-water into the alpha-phosphoryls of the guanine nucleotides. The photoreceptor electrical response was determined by measuring the aspartate-isolated mass receptor potential. Basal cGMP flux in dark-adapted retinas was 33 pmol cGMP X mg protein-1 X s-1 which translates into a metabolic rate in the rod outer segment (ROS) of 1.7 mM/min in ATP equivalents. Photic stimulation increased this flux as much as 4.5-fold. With continuous illumination, increasing intensity caused increments in cGMP metabolic flux to a maximum of 4.5-fold, with corresponding increases in the electrical response over the same 3-log unit intensity range. Tight coupling between activation of guanylate cyclase and phosphodiesterase was indicated by either no changes in cGMP steady state concentrations or relatively small fluctuations represented by increases of 50% at lower light intensities and a 12% decrease at one of the highest intensities. A stoichiometry of about 10,000 molecules of cGMP generated and hydrolyzed per photon absorbed was calculated for the lowest light intensity when the increment in cGMP metabolic flux per photon was maximal. Flashing light caused an increase in flux in proportion to frequency up to 1 Hz and a nearly proportional increase in the voltage time integral of the electrical response up to 0.5 Hz. This indicates that the temporal resolution, or "on"/"off" rate, of the cGMP metabolic response was as fast or faster than the temporal resolution of the electrical response. The concentration of cGMP remained relatively stable in spite of the marked acceleration of cGMP flux that occurred over the 32-fold range of frequencies tested. Taken together these results show that the light-accelerated rate of cGMP synthesis tightly coupled to hydrolysis becomes a primary energy-utilizing system in the photoreceptor and represents a response that fulfills certain of the fundamental criteria required of a metabolic event playing an essential role in phototransduction.

摘要

在分离的完整兔视网膜中,研究了光感受器环鸟苷酸(cGMP)的代谢及其光敏感调节与视紫红质光异构化以及光感受器电反应之间的关系。通过测量18O从18O-水掺入鸟嘌呤核苷酸α-磷酸基团的速率,评估cGMP代谢的动力学。通过测量天冬氨酸分离的质量感受器电位来确定光感受器电反应。暗适应视网膜中的基础cGMP通量为33 pmol cGMP×mg蛋白-1×s-1,这相当于视杆外段(ROS)中以ATP当量计的代谢速率为1.7 mM/分钟。光刺激使该通量增加多达4.5倍。在持续光照下,强度增加导致cGMP代谢通量增加至最大4.5倍,在相同的3个对数单位强度范围内,电反应相应增加。鸟苷酸环化酶和磷酸二酯酶激活之间的紧密偶联表现为cGMP稳态浓度无变化,或在较低光强度下增加50%、在最高强度之一时降低12%所代表的相对较小波动。当每个光子的cGMP代谢通量增加最大时,计算出在最低光强度下,每吸收一个光子产生和水解的cGMP分子数约为10,000个。闪光导致通量与频率成正比增加,直至1 Hz,电反应的电压时间积分在高达0.5 Hz时几乎成比例增加。这表明cGMP代谢反应的时间分辨率,即“开”/“关”速率,与电反应的时间分辨率一样快或更快。尽管在测试的32倍频率范围内cGMP通量显著加速,但cGMP浓度仍保持相对稳定。这些结果综合表明,与水解紧密偶联的光加速cGMP合成速率成为光感受器中的主要能量利用系统,并且代表了一种满足在光转导中起重要作用的代谢事件所需某些基本标准的反应。

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