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光感受器内段中钙敏感的钙内流。

Calcium-sensitive calcium influx in photoreceptor inner segments.

作者信息

Baldridge W H, Kurennyi D E, Barnes S

机构信息

Neuroscience Research Group, University of Calgary, Faculty of Medicine, Calgary, Alberta T2N 4N1, Canada.

出版信息

J Neurophysiol. 1998 Jun;79(6):3012-8. doi: 10.1152/jn.1998.79.6.3012.

Abstract

The effect of external calcium concentration ([Ca2+]o) on membrane potential-dependent calcium signals in isolated tiger salamander rod and cone photoreceptor inner segments was investigated with patch-clamp and calcium imaging techniques. Mild depolarizations led to increases in intracellular Ca2+ levels ([Ca2+]i) that were smaller when [Ca2+]o was elevated to 10 mM than when it was 3 mM, even though maximum Ca2+ conductance increased 30% with the increase in [Ca2+]o. When external calcium was lowered to 1 mM [Ca2+]o, maximum Ca2+ conductance was reduced, as expected, but the mild depolarization-induced increase in [Ca2+]i was larger than in 3 mM [Ca2+]o. In contrast, when photoreceptors were strongly depolarized, the increase in [Ca2+]i was less when [Ca2+]o was reduced. An explanation for these observations comes from an assessment of Ca2+ channel gating in voltage-clamped photoreceptors under changing conditions of [Ca2+]o. Although Ca2+ conductance increased with increasing [Ca2+]o, surface charge effects dictated large shifts in the voltage dependence of Ca2+ channel gating. Relative to the control condition (3 mM [Ca2+]o), 10 mM [Ca2+]o shifted Ca2+ channel activation 8 mV positive, reducing channel open probability over a broad range of potentials. Reducing [Ca2+]o to 1 mM reduced Ca2+ conductance but shifted Ca2+ channel activation negative by 6 mV. Thus the intracellular calcium signals reflect a balance between competing changes in gating and permeation of Ca2+ channels mediated by [Ca2+]o. In mildly depolarized cells, the [Ca2+]o-induced changes in Ca2+ channel activation proved stronger than the [Ca2+]o-induced changes in conductance. In response to the larger depolarizations caused by 80 mM [K+]o, the opposite is true, with conductance changes dominating the effects on channel activation.

摘要

采用膜片钳和钙成像技术,研究了外部钙浓度([Ca2+]o)对离体虎螈视杆和视锥光感受器内段膜电位依赖性钙信号的影响。轻度去极化导致细胞内Ca2+水平([Ca2+]i)升高,当[Ca2+]o升高到10 mM时,[Ca2+]i的升高幅度小于[Ca2+]o为3 mM时,尽管最大Ca2+电导随[Ca2+]o的增加而增加了30%。当外部钙降至1 mM [Ca2+]o时,最大Ca2+电导如预期那样降低,但轻度去极化诱导的[Ca2+]i升高幅度大于[Ca2+]o为3 mM时。相反,当光感受器强烈去极化时,[Ca2+]o降低时[Ca2+]i的升高幅度较小。对这些观察结果的一种解释来自于在[Ca2+]o变化条件下对电压钳制光感受器中Ca2+通道门控的评估。尽管Ca2+电导随[Ca2+]o的增加而增加,但表面电荷效应导致Ca2+通道门控的电压依赖性发生较大偏移。相对于对照条件(3 mM [Ca2+]o),10 mM [Ca2+]o使Ca2+通道激活向正向偏移8 mV,在很宽的电位范围内降低了通道开放概率。将[Ca2+]o降至1 mM降低了Ca2+电导,但使Ca2+通道激活向负向偏移6 mV。因此,细胞内钙信号反映了由[Ca2+]o介导的Ca2+通道门控和通透的竞争性变化之间的平衡。在轻度去极化的细胞中,[Ca2+]o诱导的Ca2+通道激活变化比[Ca2+]o诱导的电导变化更强。响应于80 mM [K+]o引起的更大去极化,情况则相反,电导变化主导了对通道激活的影响。

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