Juxtacellular opto-tagging of hippocampal CA1 neurons in freely moving mice

Author:

Ding Lingjun123ORCID,Balsamo Giuseppe123,Chen Hongbiao123ORCID,Blanco-Hernandez Eduardo12,Zouridis Ioannis S123ORCID,Naumann Robert45,Preston-Ferrer Patricia12,Burgalossi Andrea12ORCID

Affiliation:

1. Institute of Neurobiology, Eberhard Karls University of Tübingen

2. Werner-Reichardt Centre for Integrative Neuroscience

3. Graduate Training Centre of Neuroscience – International Max-Planck Research School (IMPRS)

4. Chinese Academy of Sciences, Key Laboratory of Brain Connectome and Manipulation, The Brain Cognition and Brain Disease Institute, Shenzhen Institute of Advanced Technology, Chinese Academy of Sciences

5. Shenzhen-Hong Kong Institute of Brain Science-Shenzhen Fundamental Research Institutions

Abstract

Neural circuits are made of a vast diversity of neuronal cell types. While immense progress has been made in classifying neurons based on morphological, molecular, and functional properties, understanding how this heterogeneity contributes to brain function during natural behavior has remained largely unresolved. In the present study, we combined the juxtacellular recording and labeling technique with optogenetics in freely moving mice. This allowed us to selectively target molecularly defined cell classes for in vivo single-cell recordings and morphological analysis. We validated this strategy in the CA1 region of the mouse hippocampus by restricting Channelrhodopsin expression to Calbindin-positive neurons. Directly versus indirectly light-activated neurons could be readily distinguished based on the latencies of light-evoked spikes, with juxtacellular labeling and post hoc histological analysis providing ‘ground-truth’ validation. Using these opto-juxtacellular procedures in freely moving mice, we found that Calbindin-positive CA1 pyramidal cells were weakly spatially modulated and conveyed less spatial information than Calbindin-negative neurons – pointing to pyramidal cell identity as a key determinant for neuronal recruitment into the hippocampal spatial map. Thus, our method complements current in vivo techniques by enabling optogenetic-assisted structure–function analysis of single neurons recorded during natural, unrestrained behavior.

Funder

Deutsche Forschungsgemeinschaft

Shenzhen city grant

University of Tübingen

Publisher

eLife Sciences Publications, Ltd

Subject

General Immunology and Microbiology,General Biochemistry, Genetics and Molecular Biology,General Medicine,General Neuroscience

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