RIM1/2-Mediated Facilitation of Cav1.4 Channel Opening Is Required for Ca2+-Stimulated Release in Mouse Rod Photoreceptors

被引:41
作者
Grabner, Chad P. [1 ]
Gandini, Maria A. [2 ,3 ]
Rehak, Renata [2 ,3 ]
Le, Yun [4 ]
Zamponi, Gerald W. [2 ,3 ]
Schmitz, Frank [1 ]
机构
[1] Univ Saarland, Inst Anat & Cell Biol, D-66421 Homburg, Germany
[2] Univ Calgary, Hotchkiss Brain Inst, Dept Physiol & Pharmacol, Calgary, AB T2N IN4, Canada
[3] Univ Calgary, Alberta Childrens Hosp, Res Inst, Calgary, AB T2N IN4, Canada
[4] Univ Oklahoma, Dept Med, Hlth Sci Ctr, Oklahoma City, OK 73104 USA
关键词
CaV1.4; evoked release; mouse rod photoreceptor; night blindness; ribbon synapse; RIM; STATIONARY NIGHT BLINDNESS; CALCIUM-CHANNEL; NEUROTRANSMITTER RELEASE; GLUTAMATE-TRANSPORTER; CONE PHOTORECEPTORS; SYNAPTIC RIBBONS; CA2+ CHANNELS; ACTIVE ZONES; RIM PROTEINS; RIM1-ALPHA;
D O I
10.1523/JNEUROSCI.0658-15.2015
中图分类号
Q189 [神经科学];
学科分类号
071006 ;
摘要
Night blindness can result from impaired photoreceptor function and a subset of cases have been linked to dysfunction of Cav1.4 calcium channels and in turn compromised synaptic transmission. Here, we show that active zone proteins RIM1/2 are important regulators of Cav1.4 channel function in mouse rod photoreceptors and thus synaptic activity. The conditional double knock-out (cdko) of RIM1 and RIM2 from rods starting a few weeks after birth did not change Cav1.4 protein expression at rod ribbon synapses nor was the morphology of the ribbon altered. Heterologous overexpression of RIM2 with Cav1.4 had no significant influence on current density when examined with BaCl2 as the charge carrier. Nonetheless, whole-cell voltage-clamp recordings from cdko rods revealed a profound reduction in Ca2+ currents. Concomitantly, we observed a 4-fold reduction in spontaneous miniature release events from the cdko rod terminals and an almost complete absence of evoked responses when monitoring changes in membrane incorporation after strong step depolarizations. Under control conditions, 49 and 83 vesicles were released with 0.2 and 1 s depolarizations, respectively, which is close to the maximal number of vesicles estimated to be docked at the base of the ribbon active zone, but without RIM1/2, only a few vesicles were stimulated for release after a 1 s stimulation. In conclusion, our study shows that RIM1/2 potently enhance the influx of Ca2+ into rod terminals through Cav1.4 channels, which is vitally important for the release of vesicles from the rod ribbon.
引用
收藏
页码:13133 / 13147
页数:15
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