Imaging Light Responses of Targeted Neuron Populations in the Rodent Retina

被引:69
作者
Borghuis, Bart G. [1 ]
Tian, Lin [1 ]
Xu, Ying [2 ]
Nikonov, Sergei S. [2 ]
Vardi, Noga [2 ]
Zemelman, Boris V. [1 ]
Looger, Loren L. [1 ]
机构
[1] Howard Hughes Med Inst, Ashburn, VA 20147 USA
[2] Univ Penn, Sch Med, Philadelphia, PA 19104 USA
基金
美国国家卫生研究院;
关键词
ENCODED CALCIUM INDICATOR; AII AMACRINE CELLS; GANGLION-CELLS; IN-VIVO; MAMMALIAN RETINA; DIRECTION SELECTIVITY; RABBIT RETINA; MOUSE RETINA; EXPRESSION; VITRO;
D O I
10.1523/JNEUROSCI.6064-10.2011
中图分类号
Q189 [神经科学];
学科分类号
071006 ;
摘要
Decoding the wiring diagram of the retina requires simultaneous observation of activity in identified neuron populations. Available recording methods are limited in their scope: electrodes can access only a small fraction of neurons at once, whereas synthetic fluorescent indicator dyes label tissue indiscriminately. Here, we describe a method for studying retinal circuitry at cellular and subcellular levels combining two-photon microscopy and a genetically encoded calcium indicator. Using specific viral and promoter constructs to drive expression of GCaMP3, we labeled all five major neuron classes in the adult mouse retina. Stimulus-evoked GCaMP3 responses as imaged by two-photon microscopy permitted functional cell type annotation. Fluorescence responses were similar to those measured with the small molecule dye OGB-1. Fluorescence intensity correlated linearly with spike rates > 10 spikes/s, and a significant change in fluorescence always reflected a significant change in spike firing rate. GCaMP3 expression had no apparent effect on neuronal function. Imaging at subcellular resolution showed compartment-specific calcium dynamics in multiple identified cell types.
引用
收藏
页码:2855 / 2867
页数:13
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