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Deep brain optical measurements of cell type–specific neural activity in behaving mice

机译:行为小鼠的大脑特定细胞类型神经活动的深层光学测量

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摘要

Recent advances in genetically encoded fluorescent sensors enable the monitoring of cellular events from genetically defined groups of neurons in vivo. In this protocol, we describe how to use a time-correlated single-photon counting (tcspc)–based fiber optics system to measure the intensity, emission spectra and lifetime of fluorescent biosensors expressed in deep brain structures in freely moving mice. When combined with cre-dependent selective expression of genetically encoded ca2+ indicators (GecIs), this system can be used to measure the average neural activity from a specific population of cells in mice performing complex behavioral tasks. as an example, we used viral expression of GcaMps in striatal projection neurons (spns) and recorded the fluorescence changes associated with calcium spikes from mice performing a lever-pressing operant task. the whole procedure, consisting of virus injection, behavior training and optical recording, takes 3–4 weeks to complete. With minor adaptations, this protocol can also be applied to recording cellular events from other cell types in deep brain regions, such as dopaminergic neurons in the ventral tegmental area. the simultaneously recorded fluorescence signals and behavior events can be used to explore the relationship between the neural activity of specific brain circuits and behavior.
机译:基因编码荧光传感器的最新进展使得能够监测体内神经元的遗传定义组的细胞事件。在此协议中,我们描述如何使用基于时间相关的单光子计数(tcspc)的光纤系统来测量自由移动小鼠深层大脑结构中表达的荧光生物传感器的强度,发射光谱和寿命。当与遗传编码的ca 2 + 指标(GecIs)的cre依赖性选择性表达结合时,该系统可用于测量执行复杂行为任务的小鼠特定细胞群体的平均神经活动。例如,我们使用GcaMps在纹状体投射神经元(spns)中的病毒表达,并记录了与执行杠杆按压操作任务的小鼠中钙峰值相关的荧光变化。整个过程(包括病毒注入,行为训练和光学记录)需要3-4周才能完成。稍作改动,该协议也可以应用于记录深部大脑区域其他细胞类型的细胞事件,例如腹侧被盖区的多巴胺能神经元。同时记录的荧光信号和行为事件可用于探索特定大脑回路的神经活动与行为之间的关系。

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