Literature DB >> 27798186

Genetically Targeted All-Optical Electrophysiology with a Transgenic Cre-Dependent Optopatch Mouse.

Shan Lou1, Yoav Adam1, Eli N Weinstein1,2, Erika Williams3, Katherine Williams1, Vicente Parot1, Nikita Kavokine1, Stephen Liberles3, Linda Madisen4, Hongkui Zeng4, Adam E Cohen5,2,6.   

Abstract

Recent advances in optogenetics have enabled simultaneous optical perturbation and optical readout of membrane potential in diverse cell types. Here, we develop and characterize a Cre-dependent transgenic Optopatch2 mouse line that we call Floxopatch. The animals expressed a blue-shifted channelrhodopsin, CheRiff, and a near infrared Archaerhodopsin-derived voltage indicator, QuasAr2, via targeted knock-in at the rosa26 locus. In Optopatch-expressing animals, we tested for overall health, genetically targeted expression, and function of the optogenetic components. In offspring of Floxopatch mice crossed with a variety of Cre driver lines, we observed spontaneous and optically evoked activity in vitro in acute brain slices and in vivo in somatosensory ganglia. Cell-type-specific expression allowed classification and characterization of neuronal subtypes based on their firing patterns. The Floxopatch mouse line is a useful tool for fast and sensitive characterization of neural activity in genetically specified cell types in intact tissue. SIGNIFICANCE STATEMENT: Optical recordings of neural activity offer the promise of rapid and spatially resolved mapping of neural function. Calcium imaging has been widely applied in this mode, but is insensitive to the details of action potential waveforms and subthreshold events. Simultaneous optical perturbation and optical readout of single-cell electrical activity ("Optopatch") has been demonstrated in cultured neurons and in organotypic brain slices, but not in acute brain slices or in vivo Here, we describe a transgenic mouse in which expression of Optopatch constructs is controlled by the Cre-recombinase enzyme. This animal enables fast and robust optical measurements of single-cell electrical excitability in acute brain slices and in somatosensory ganglia in vivo, opening the door to rapid optical mapping of neuronal excitability.
Copyright © 2016 the authors 0270-6474/16/3611059-15$15.00/0.

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Keywords:  optogenetics; optopatch; transgenic mice; voltage imaging

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Year:  2016        PMID: 27798186      PMCID: PMC5098841          DOI: 10.1523/JNEUROSCI.1582-16.2016

Source DB:  PubMed          Journal:  J Neurosci        ISSN: 0270-6474            Impact factor:   6.167


  60 in total

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2.  Targeting Cre recombinase to specific neuron populations with bacterial artificial chromosome constructs.

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3.  Unbiased classification of sensory neuron types by large-scale single-cell RNA sequencing.

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Review 4.  Optical properties of biological tissues: a review.

Authors:  Steven L Jacques
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Review 6.  Generation of somatic sensory neuron diversity and implications on sensory coding.

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Authors:  Michael Z Lin; Mark J Schnitzer
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9.  Subcellular Imaging of Voltage and Calcium Signals Reveals Neural Processing In Vivo.

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10.  Anatomical characterization of Cre driver mice for neural circuit mapping and manipulation.

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Review 6.  Voltage and Calcium Imaging of Brain Activity.

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Review 10.  Genetically Encoded Tools for Research of Cell Signaling and Metabolism under Brain Hypoxia.

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