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钙离子跨盘膜的通量。对完整视杆光感受器和纯化盘膜的研究。

Calcium flux across disk membranes. Studies with intact rod photoreceptors and purified disks.

作者信息

Szuts E Z

出版信息

J Gen Physiol. 1980 Sep;76(3):253-86. doi: 10.1085/jgp.76.3.253.

Abstract

Calcium accumulation by rod disks was studied in excised bullfrog retinas with 45Ca tracer-exchange methods. Ca uptake by disks is a necessary requirement if light-induced Ca releases from disks mediate photoreceptor excitation. In an hour-long incubation, disks exchanged less than or equal to 0.01 mole of Ca per mole of rhodopsin, or less than or equal to 10% of their total Ca. This corresponds to a unidirectional flux of less than or equal to 0.01 fmol/cm2 S, or less than or equal to 5 ions/disk-second across the disk membrane. Neither incubation in 10 mM Ca (which increases cytoplasmic activity 10--100-fold) nor photostimulation (which photoactivated up to 50% rhodopsin/h) had measurable effect on exchange rate, though an increase of several orders of magnitude would have been expected according to the hypothesis. The observed exchange could not be explained by: (a) 45Ca losses from disks before measurement (neither the net efflux nor the Ca-Ca exchange property of disks adequately explains such losses), (b) a limited pool of exchangeables Ca from strongly binding intradiskal sites, or (c) rate-limiting flux across the plasma membrane during incubation. For the study of the Ca efflux properties of disks, separate experiments were performed with 45Ca-loaded disks. Intradiskal activity could be estimated from the disks' hyperosmotically sensitive 45Ca pool and from their intradiskal volume (indirectly assayed by density). Ca-Ca exchange was undetectable (less than or equal to 0.1 fmol/cm2 S) in disks whose intradiskal activity was at least 0.3 mM. Net efflux was 0.2 fmol/cm2 S for an intradiskal activity of approximately 1 mM and is comparable to published fluxes for phospholipid vesicles. These results seem to exclude the internal space of disks as the source of Ca for photoreceptor excitation.

摘要

采用⁴⁵Ca示踪交换法,对摘除的牛蛙视网膜中视杆圆盘的钙积累进行了研究。如果光诱导的视杆圆盘钙释放介导光感受器兴奋,那么圆盘摄取钙是一个必要条件。在长达一小时的孵育过程中,每摩尔视紫红质圆盘交换的钙小于或等于0.01摩尔,即小于或等于其总钙含量的10%。这相当于单向通量小于或等于0.01飞摩尔/平方厘米·秒,或小于或等于每秒每个圆盘5个离子穿过圆盘膜。无论是在10毫摩尔/升钙中孵育(这会使细胞质活性增加10 - 100倍)还是光刺激(光激活视紫红质的比例高达50%/小时),对交换率都没有可测量的影响,尽管根据该假设预计会有几个数量级的增加。观察到的交换不能用以下情况解释:(a) 测量前视杆圆盘中⁴⁵Ca的损失(视杆圆盘的净流出量或钙 - 钙交换特性都不能充分解释这种损失),(b) 来自圆盘内强结合位点的有限可交换钙池,或(c) 孵育期间穿过质膜的限速通量。为了研究视杆圆盘的钙流出特性,用负载⁴⁵Ca的视杆圆盘进行了单独实验。圆盘内活性可以从圆盘的高渗敏感⁴⁵Ca池及其圆盘内体积(通过密度间接测定)来估计。在圆盘内活性至少为0.3毫摩尔的视杆圆盘中,未检测到钙 - 钙交换(小于或等于0.1飞摩尔/平方厘米·秒)。对于圆盘内活性约为1毫摩尔的情况,净流出量为0.2飞摩尔/平方厘米·秒,这与已发表的磷脂囊泡通量相当。这些结果似乎排除了视杆圆盘内部空间是光感受器兴奋钙源的可能性。

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