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光对蝾螈视杆细胞外段钙的影响。

The effect of light on outer segment calcium in salamander rods.

作者信息

Matthews Hugh R, Fain Gordon L

机构信息

Physiological Laboratory, University of Cambridge, Downing Street, Cambridge CB2 3EG, UK.

出版信息

J Physiol. 2003 Nov 1;552(Pt 3):763-76. doi: 10.1113/jphysiol.2003.050724. Epub 2003 Aug 29.

Abstract

Calcium acts as a second messenger in vertebrate rods, regulating the recovery phase of the light response and modulating sensitivity during light-adaptation. Since light not only decreases the outer segment calcium concentration ([Ca2+]i) by closing cyclic nucleotide-gated channels but can also increase [Ca2+]i by releasing Ca2+ from buffer sites or intracellular stores, we examined in detail the effect of light and circulating current on [Ca2+]i by making simultaneous measurements of suction pipette current and [Ca2+]i from isolated rods of the salamander Ambystoma tigrinum after incorporation of the fluorescent dye fluo-5F. When the release of Ca2+ is measured in 0 Ca2+-0 Na+ solution, minimising fluxes of Ca2+ across the plasma membrane, it is substantial only for light bright enough to bleach a significant fraction of the photopigment and is restricted to the part of the outer segment in which the bleach occurred. It is unlikely, therefore, to make a large contribution to [Ca2+]i for most of the physiological operating range of the rod. Nevertheless, since release is half-maximal for a bleach of less than 10 %, it cannot be produced by a simple mechanism such as a change in the affinity of a binding site on rhodopsin itself but must instead require some more complex interaction. In Ringer solution, the Ca2+ in the light-releasable pool can be discharged merely by the decrease in [Ca2+]i that occurs as the outer segment channels close. In steady background light or after exposure to saturating illumination, the fraction of Ca2+ in the pool decreases essentially in proportion to [Ca2+]i as if Ca2+ were being removed from a buffer site within the cytoplasm. Furthermore, [Ca2+]i itself changes in proportion to the circulating current, with little evidence for a contribution from Ca2+ release or other mechanisms of Ca2+ homeostasis. This indicates that flux of Ca2+ across the plasma membrane is the major determinant of outer segment Ca2+ concentration within the rod's normal operating light intensity range. Once Ca2+ has been discharged from the releasable pool, it is restored following dim illumination apparently as the simple result of the subsequent restoration of dark [Ca2+]i and the rebinding of Ca2+ to its release site, but after brighter light perhaps also as a consequence of regeneration of the photopigment.

摘要

钙在脊椎动物视杆细胞中作为第二信使,调节光反应的恢复阶段,并在光适应过程中调节敏感度。由于光不仅通过关闭环核苷酸门控通道降低外段钙浓度([Ca2+]i),还能通过从缓冲位点或细胞内储存库释放Ca2+来增加[Ca2+]i,我们通过在掺入荧光染料fluo-5F后同时测量蝾螈(Ambystoma tigrinum)分离视杆细胞的吸管电流和[Ca2+]i,详细研究了光和循环电流对[Ca2+]i的影响。当在0 Ca2+-0 Na+溶液中测量Ca2+释放时,将跨质膜的Ca2+通量降至最低,只有足够亮的光才能使相当一部分光色素漂白时,Ca2+释放才显著,并且仅限于发生漂白的外段部分。因此,在视杆细胞的大多数生理工作范围内,它不太可能对[Ca2+]i有很大贡献。然而,由于小于10%的漂白就能使释放达到半数最大,它不可能由诸如视紫红质自身结合位点亲和力变化这样的简单机制产生,而必定需要一些更复杂的相互作用。在林格氏溶液中,光可释放池中的Ca2+仅可通过外段通道关闭时发生的[Ca2+]i降低而被排出。在稳定的背景光下或暴露于饱和光照后,池中Ca2+的比例基本上与[Ca2+]i成比例降低,就好像Ca2+是从细胞质内的一个缓冲位点被移除一样。此外,[Ca2+]i本身与循环电流成比例变化,几乎没有证据表明Ca2+释放或其他Ca2+稳态机制有贡献。这表明在视杆细胞正常工作光强度范围内,跨质膜的Ca2+通量是外段Ca2+浓度的主要决定因素。一旦Ca2+从可释放池中排出,在弱光照后它显然会恢复,这显然是随后暗[Ca2+]i恢复以及Ca2+重新结合到其释放位点的简单结果,但在较强光照后,可能也是光色素再生的结果。

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