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A light-dependent increase in free Ca2+ concentration in the salamander rod outer segment

机译:the杆外节中游离Ca2 +浓度的光依赖性增加

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class="enumerated" style="list-style-type:decimal">The Ca2+ indicator dye fluo-5F was excited by an argon ion laser to measure changes in free Ca2+ concentration ([Ca2+]i) in the outer segments of isolated salamander rods rapidly exposed to a 0 Ca2+, 0 Na+ solution designed to minimise surface membrane Ca2+ fluxes. Over 30-60 s of laser illumination, the fluorescence first increased rapidly and then declined at a rate that was much slower than in Ringer solution and consistent with previous physiological evidence that 0 Ca2+, 0 Na+ solution greatly retards light-induced changes in [Ca2+]i.The initial increase in fluorescence was investigated with a sequence of 100 ms laser flashes presented at 5 s intervals. The fluorescence evoked by the second laser flash was on average 30 % larger than the first, and subsequent responses exhibited a slow decline like that measured with continuous laser exposures. The initial increase in fluorescence did not depend upon the timing of exposure to 0 Ca2+, 0 Na+ solution but appeared to be evoked by exposure to the laser light.Both the increase and subsequent decline in fluorescence measured with brief laser flashes could be reduced by incorporation of the Ca2+ chelator BAPTA. This and other results indicate that the fluorescence increase was unlikely to have been caused by a change in the affinity of fluo-5F for Ca2+ or an increase in the quantity of incorporated dye available to bind Ca2+ but reflects an actual release of intracellular Ca2+ within the outer segment.The pool of Ca2+ available to be released could be decreased if, before the first laser flash, the rod was exposed to light bright enough to bleach a substantial fraction of the photopigment. The releasable pool could also be depleted by exposure to saturating light of much lower intensity if delivered in Ringer solution but not if delivered in 0 Ca2+, 0 Na+ solution. We conclude that Ca2+ can be released within the outer segment both by the bleaching of rhodopsin and by the reduction in [Ca2+]i which normally accompanies illumination in Ringer solution.The activation of rhodopsin appears somehow to induce the release of Ca2+ from a binding site or store within the outer segment. Substantial release, however, required stimulating light of an intensity sufficient to bleach a considerable fraction of the visual pigment. It therefore seems unlikely that such release contributes to the normal Ca2+-mediated modulation of transduction during light adaptation. The mechanism and physiological function of light-induced Ca2+ release are unknown.
机译:class =“ enumerated” style =“ list-style-type:decimal”> <!-list-behavior =枚举前缀-word = mark-type = decimal max-label-size = 0-> Ca 2 + 指示剂fluo-5F被氩离子激光激发,测量游离Ca 2 + 浓度([Ca 2 + ] i)在孤立的sal棒的外部迅速暴露于0 Ca 2 + ,0 Na + 溶液中,该溶液旨在最大程度地减少表面膜Ca 2+ 通量。在30-60 s的激光照射下,荧光首先迅速增加,然后以比林格溶液慢得多的速率下降,并且与以前的生理证据一致,即0 Ca 2 + ,0 Na < sup> + 溶液极大地延迟了光诱导的[Ca 2 + ] i的变化。 使用100 ms激光序列研究了荧光的初始增加以5 s的间隔闪烁一次。第二次激光闪光诱发的荧光平均比第一个激光激发荧光大30%,随后的响应显示出缓慢的下降,就像连续激光照射所测得的那样。荧光的初始增加不取决于暴露于0 Ca 2 + ,0 Na + 溶液的时间,但似乎是由于暴露于激光而引起的。 / li> 通过掺入Ca 2 + 螯合剂BAPTA可以减少短暂的激光闪光测量的荧光的增加和减少。该结果和其他结果表明,荧光的增加不太可能是由fluo-5F对Ca 2 + 的亲和力改变或可用于结合Ca < sup> 2 + ,但反映了外部片段中细胞内Ca 2 + 的实际释放。 Ca 2 + 池如果在第一次激光闪光之前,将棒暴露在足够明亮的地方以漂白大部分的光致色素,则可以减少可释放的可用色素。如果在林格溶液中递送,则可释放池也可通过暴露于强度低得多的饱和光中而耗尽,但如果在0 Ca 2 + ,0 Na + 溶液中递送则不能。我们得出结论,视紫红质的漂白和通常伴随林格照明的[Ca 2 + ] i的减少,Ca 2 + 均可在外段释放。溶液。 视紫红质的活化似乎以某种方式诱导了Ca 2 + 从结合位点释放或在外部片段中存储。然而,大量释放需要足够强度的光来漂白相当一部分可视颜料。因此,这种释放似乎不太可能有助于光适应过程中正常的Ca 2 + 介导的转导调节。光诱导Ca 2 + 释放的机理和生理功能尚不清楚。

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