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Simultaneous all-optical manipulation and recording of neural circuit activity with cellular resolution in vivo

机译:同时进行全光学操作并以体内细胞分辨率记录神经回路活动

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摘要

We describe an all-optical strategy for simultaneously manipulating and recording the activity of multiple neurons with cellular resolution in vivo. Concurrent two-photon optogenetic activation and calcium imaging is enabled by coexpression of a red-shifted opsin and a genetically encoded calcium indicator. A spatial light modulator allows tens of user-selected neurons to be targeted for spatiotemporally precise optogenetic activation, while simultaneous fast calcium imaging provides high-resolution network-wide readout of the manipulation with negligible optical crosstalk. Proof-of-principle experiments in mouse barrel cortex demonstrate interrogation of the same neuronal population during different behavioral states, and targeting of neuronal ensembles based on their functional signature. This approach extends the optogenetic toolkit beyond the specificity obtained with genetic or viral approaches, enabling high-throughput, flexible and long-term optical interrogation of functionally defined neural circuits with single-cell and single-spike resolution in the mammalian brain in vivo.
机译:我们描述了一种全光学策略,用于同时操纵和记录具有体内细胞分辨率的多个神经元的活动。通过红移视蛋白和遗传编码的钙指示剂的共表达,可以同时进行两个光子的光遗传激活和钙成像。空间光调制器允许将数十个用户选择的神经元作为时空精确的光遗传学激活的目标,而同时快速的钙成像则提供了可在网络范围内以高分辨率进行光学串扰的高分辨率读出。在小鼠桶状皮质中进行的原理验证实验表明,在不同的行为状态下对相同神经元种群的询问,以及基于其功能特征的神经元集成体的靶向。这种方法将光遗传学工具包扩展到通过遗传或病毒方法获得的特异性之外,从而可以在哺乳动物的体内体内以单细胞和单峰分辨力对功能明确的神经回路进行高通量,灵活和长期的光学询问。

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