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在活体家蝇光感受器中测量钙和膜电位的光依赖性。

Light dependence of calcium and membrane potential measured in blowfly photoreceptors in vivo.

作者信息

Oberwinkler J, Stavenga D G

机构信息

Department of Neurobiophysics, University of Groningen, 9747 AG Groningen, The Netherlands.

出版信息

J Gen Physiol. 1998 Aug;112(2):113-24. doi: 10.1085/jgp.112.2.113.

Abstract

Light adaptation in insect photoreceptors is caused by an increase in the cytosolic Ca2+ concentration. To better understand this process, we measured the cytosolic Ca2+ concentration in vivo as a function of adapting light intensity in the white-eyed blowfly mutant chalky. We developed a technique to measure the cytosolic Ca2+ concentration under conditions as natural as possible. The calcium indicator dyes Oregon Green 1, 2, or 5N (Molecular Probes, Inc., Eugene, OR) were iontophoretically injected via an intracellular electrode into a photoreceptor cell in the intact eye; the same electrode was also used to measure the membrane potential. The blue-induced green fluorescence of these dyes could be monitored by making use of the optics of the facet lens and the rhabdomere waveguide. The use of the different Ca2+-sensitive dyes that possess different affinities for Ca2+ allowed the quantitative determination of the cytosolic Ca2+ concentration in the steady state. Determining the cytosolic Ca2+ concentration as a function of the adapting light intensity shows that the Ca2+ concentration is regulated in a graded fashion over the whole dynamic range where a photoreceptor cell can respond to light. When a photoreceptor is adapted to bright light, the cytosolic Ca2+ concentration reaches stable values higher than 10 microM. The data are consistent with the hypothesis that the logarithm of the increase in cytosolic Ca2+ concentration is linear with the logarithm of the light intensity. From the estimated values of the cytosolic Ca2+ concentration, we conclude that the Ca2+-buffering capacity is limited. The percentage of the Ca2+ influx that is buffered gradually decreases with increasing Ca2+ concentrations; at cytosolic Ca2+ concentration levels above 10 microM, buffering becomes minimal.

摘要

昆虫光感受器中的光适应是由胞质Ca2+浓度升高引起的。为了更好地理解这一过程,我们在白眼果蝇突变体“垩白”中测量了体内胞质Ca2+浓度随适应光强度的变化。我们开发了一种在尽可能自然的条件下测量胞质Ca2+浓度的技术。将钙指示剂染料俄勒冈绿1、2或5N(分子探针公司,俄勒冈州尤金市)通过细胞内电极离子导入完整眼中的光感受器细胞;同一电极也用于测量膜电位。这些染料的蓝光诱导绿色荧光可以利用小眼透镜和视杆微管的光学系统进行监测。使用对Ca2+具有不同亲和力的不同Ca2+敏感染料,可以定量测定稳态下的胞质Ca2+浓度。将胞质Ca2+浓度作为适应光强度的函数进行测定表明,在光感受器细胞能够响应光的整个动态范围内,Ca2+浓度以分级方式调节。当光感受器适应强光时,胞质Ca2+浓度达到高于10 microM的稳定值。这些数据与胞质Ca2+浓度增加的对数与光强度的对数呈线性关系的假设一致。根据估计的胞质Ca2+浓度值,我们得出Ca2+缓冲能力有限的结论。随着Ca2+浓度的增加,被缓冲的Ca2+流入百分比逐渐降低;在胞质Ca2+浓度高于10 microM时,缓冲作用变得最小。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/848d/2525746/3705b12c050f/JGP7710.f1.jpg

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