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首页> 外文期刊>Neuroscience: An International Journal under the Editorial Direction of IBRO >The dynamic range and domain-specific signals of intracellular calcium in photoreceptors.
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The dynamic range and domain-specific signals of intracellular calcium in photoreceptors.

机译:感光细胞内钙的动态范围和结构域特异性信号。

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摘要

Vertebrate photoreceptors consist of strictly delimited subcellular domains: the outer segment, ellipsoid, cell body and synaptic terminal, each hosting crucial cellular functions, including phototransduction, oxidative metabolism, gene expression and transmitter release. We used optical imaging to explore the spatiotemporal dynamics of Ca(2+) signaling in non-outer segment regions of rods and cones. Sustained depolarization, designed to emulate photoreceptor activation in the darkness, evoked a standing Ca(2+) gradient in tiger salamander photoreceptors with spatially-averaged intracellular Ca(2+) concentration within synaptic terminals of approximately 2 muM and lower ( approximately 750 nM) intracellular calcium concentration in the ellipsoid. Measurements from axotomized cell bodies and isolated ellipsoids showed that Ca(2+) enters the two compartments via both local L-type Ca(2+) channels and diffusion. The results from optical imaging studies were supported by immunostaining analysis. L-type voltage-operated Ca(2+) channels and plasma membrane Ca(2+) ATPases were highly expressed in synaptic terminals with progressively lower expression levels in the cell body and ellipsoid. These results show photoreceptor Ca(2+) homeostasis is controlled in a region-specific manner by direct Ca(2+) entry and diffusion as well as Ca(2+) extrusion. Moreover, quantitative measurement of intracellular calcium concentration levels in different photoreceptor compartments indicates that the dynamic range of Ca(2+) signaling in photoreceptors is approximately 40-fold, from approximately 50 nM in the light to approximately 2 muM in darkness.
机译:脊椎动物的感光细胞由严格限定的亚细胞域组成:外部,椭圆形,细胞体和突触末端,每个都具有关键的细胞功能,包括光转导,氧化代谢,基因表达和递质释放。我们使用光学成像来探索时空动力学的Ca(2+)信号杆和视锥细胞的非外段区域中。持续去极化,旨在模拟黑暗中的光感受器激活,在虎sal光感受器中引起站立的Ca(2+)梯度,在突触末端内的空间平均细胞内Ca(2+)浓度约为2μM和更低(约750 nM)椭圆体内的细胞内钙浓度。从轴切细胞体和孤立的椭球体的测量表明,Ca(2+)通过本地L型Ca(2+)通道和扩散进入两个隔室。光学成像研究的结果得到了免疫染色分析的支持。 L型电压操作Ca(2+)通道和质膜Ca(2+)ATPases在突触末端高度表达,并在细胞体和椭球体中逐渐降低表达水平。这些结果表明光感受器Ca(2+)稳态通过直接Ca(2+)进入和扩散以及Ca(2+)挤出以区域特定的方式进行控制。此外,定量测量不同感光器区室中细胞内钙的浓度水平表明,感光器中Ca(2+)信号的动态范围约为40倍,从光照下的约50 nM到黑暗处的约2μM。

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