Navigating the translational roadblock: Towards highly specific and effective all-optical interrogations of neural circuits

AbstractTwo-photon (2-P) all-optical approaches combine in vivo 2-P calcium imaging and 2-P optogenetic modulations and have the potential to build a framework for network-based therapies, e.g. for rebalancing maladaptive activity patterns in preclinical models of neurological disorders. Here, our goal was to tailor these approaches for this purpose: Firstly, we combined in vivo juxtacellular recordings and GCaMP6f-based 2-P calcium imaging in layer II/III of mouse visual cortex to tune our detection algorithm towards a 100 % specific identification of AP-related calcium transients. False-positive-free detection was achieved at a sensitivity of approximately 73 %. To further increase specificity, secondly, we minimized photostimulation artifacts as a potential source for false-positives by using extended-wavelength-spectrum laser sources for optogenetic stimulation of the excitatory opsin C1V1. We achieved artifact-free all-optical experiments performing photostimulations at 1100 nm or higher and simultaneous calcium imaging at 920 nm in mouse visual cortex in vivo. Thirdly, we determined the spectral range for maximizing efficacy of optogenetic control by performing 2-P photostimulations of individual neurons with wavelengths up to 1300 nm. The rate of evoked transients in GCaMP6f/C1V1-co-expressing cortical neurons peaked already at 1100 nm. By refining spike detection and defining 1100 nm as the optimal wavelength for artifact-free and effective stimulations of C1V1 in GCaMP-based all-optical interrogations, we increased the translational value of these approaches, e.g. for the use in preclinical applications of network-based therapies.One Sentence SummaryWe maximize translational relevance of 2-P all-optical physiology by increasing specificity, minimizing artifacts and optimizing stimulation efficacy.

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Parallel holographic illumination enables sub-millisecond two-photon optogenetic activation in mouse visual cortex in vivo

10.1101/250795 ◽

2018 ◽

Cited By ~ 5

Author(s):

I-Wen Chen ◽

Emiliano Ronzitti ◽

Brian R. Lee ◽

Tanya L. Daigle ◽

Hongkui Zeng ◽

...

Keyword(s):

Visual Cortex ◽

Temporal Resolution ◽

Optical Control ◽

Target Cells ◽

High Temporal Resolution ◽

Two Photon ◽

Brain Functions ◽

All Optical ◽

Mouse Visual Cortex

AbstractSelective control of action potential generation in individual cells from a neuronal ensemble is desirable for dissecting circuit mechanisms underlying perception and behavior. Here, by using two-photon (2P) temporally focused computer-generated holography (TF-CGH), we demonstrate optical manipulation of neuronal excitability at the supragranular layers of anesthetized mouse visual cortex. Utilizing amplified laser-pulses delivered via a localized holographic spot, our optical system achieves suprathreshold activation by exciting either of the three optogenetic actuators, ReaChR, CoChR or ChrimsonR, with brief illumination (≤ 10 ms) at moderate excitation power ((in average ≤ 0.2 mW/µm2 corresponding to ≤ 25 mW/cell). Using 2P-guided whole-cell or cell-attached recordings in positive neurons expressing respective opsin in vivo, we find that parallel illumination induces spikes of millisecond temporal resolution and sub-millisecond precision, which are preserved upon repetitive illuminations up to tens of Hz. Holographic stimulation thus enables temporally precise optogenetic activation independently of opsin’s channel kinetics. Furthermore, we demonstrate that parallel optogenetic activation can be combined with functional imaging for all-optical control of a neuronal sub-population that co-expresses the photosensitive opsin ReaChR and the calcium indicator GCaMP6s. Parallel optical control of neuronal activity with cellular resolution and millisecond temporal precision should be advantageous for investigating neuronal connections and further yielding causal links between connectivity, microcircuit dynamics, and brain functions.Significance statementRecent development of optogenetics allows probing the neuronal microcircuit with light by optically actuating genetically-encoded light-sensitive opsins expressed in the target cells. Here, we apply holographic light shaping and temporal focusing to simultaneously deliver axially-confined holographic patterns to opsin-positive cells situated in the living mouse cortex. Parallel illumination efficiently induces action potentials with high temporal resolution and precision for three opsins of different kinetics. We demonstrated all-optical experiments by extending the parallel optogenetic activation at low intensity to multiple neurons and concurrently monitoring their calcium dynamics. These results demonstrate fast and temporally precise in vivo control of a neuronal sub-population, opening new opportunities to reveal circuit mechanisms underlying brain functions.

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In Vivo Calcium Imaging of Neural Network Function

Physiology ◽

10.1152/physiol.00032.2007 ◽

2007 ◽

Vol 22 (6) ◽

pp. 358-365 ◽

Cited By ~ 105

Author(s):

Werner Göbel ◽

Fritjof Helmchen

Keyword(s):

Calcium Imaging ◽

Activity Patterns ◽

Network Activity ◽

Network Function ◽

Two Photon ◽

Calcium Indicators ◽

Recent Developments ◽

In Vivo Calcium Imaging ◽

Function Network

Spatiotemporal activity patterns in local neural networks are fundamental to brain function. Network activity can now be measured in vivo using two-photon imaging of cell populations that are labeled with fluorescent calcium indicators. In this review, we discuss basic aspects of in vivo calcium imaging and highlight recent developments that will help to uncover operating principles of neural circuits.

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Experience-dependent reorganization drives development of a binocularly unified cortical representation of orientation

10.1101/761395 ◽

2019 ◽

Cited By ~ 2

Author(s):

David Whitney ◽

Jeremy T. Chang ◽

David Fitzpatrick

Keyword(s):

Visual Cortex ◽

Calcium Imaging ◽

Developmental Process ◽

Activity Patterns ◽

External World ◽

Neural Representations ◽

Binocular Stimulation ◽

Early Developmental ◽

Dependent Processes

SummaryAcross sensory areas, neural microcircuits consolidate diverse streams of information into unified, representations of the external world. In the carnivore visual cortex, where eye-specific inputs converge, it has been posited that a single, shared columnar representation of orientation develops independent of sensory experience. In this study, in vivo calcium imaging with columnar and cellular resolution reveals a strikingly different developmental process in ferret visual cortex, starting with an early developmental period in which contralateral, ipsilateral or binocular stimulation each yield distinct well-organized representations of orientation that are misaligned at the columnar and cellular scale. Experience-dependent processes drive the reorganization of these three representations towards a single binocularly-aligned representation resembling the early binocular representation through concerted shifts in the preferred orientation of individual neurons. Thus, contrary to previous findings, a unified binocular representation of orientation results from an experience-dependent process that aligns the activity patterns of three distinct neural representations.

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In Vivo Two-Photon Ca2+ Imaging Reveals Selective Reward Effects on Stimulus-Specific Assemblies in Mouse Visual Cortex

Journal of Neuroscience ◽

10.1523/jneurosci.1341-12.2013 ◽

2013 ◽

Vol 33 (28) ◽

pp. 11540-11555 ◽

Cited By ~ 32

Author(s):

P. M. Goltstein ◽

E. B. J. Coffey ◽

P. R. Roelfsema ◽

C. M. A. Pennartz

Keyword(s):

Visual Cortex ◽

Two Photon ◽

Mouse Visual Cortex ◽

Reward Effects

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In vivo two-photon imaging analysis of development of direction and orientation selectivity in the mouse visual cortex

Neuroscience Research ◽

10.1016/j.neures.2011.07.1122 ◽

2011 ◽

Vol 71 ◽

pp. e257

Author(s):

Madoka Narushima ◽

Nathalie L. Rochefort ◽

Christine Grienberger ◽

Nima Marandi ◽

Arthur Konnerth

Keyword(s):

Visual Cortex ◽

Orientation Selectivity ◽

Imaging Analysis ◽

Two Photon ◽

Photon Imaging ◽

Two Photon Imaging ◽

Mouse Visual Cortex

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Dendritic nonlinearities are tuned for efficient spike-based computations in cortical circuits

eLife ◽

10.7554/elife.10056 ◽

2015 ◽

Vol 4 ◽

Cited By ~ 20

Author(s):

Balázs B Ujfalussy ◽

Judit K Makara ◽

Tiago Branco ◽

Máté Lengyel

Keyword(s):

Cortical Neurons ◽

Activity Patterns ◽

Pyramidal Cells ◽

Cortical Circuits ◽

Functional Link ◽

Synaptic Inputs ◽

Two Photon ◽

Highly Nonlinear ◽

Efficient Integration

Cortical neurons integrate thousands of synaptic inputs in their dendrites in highly nonlinear ways. It is unknown how these dendritic nonlinearities in individual cells contribute to computations at the level of neural circuits. Here, we show that dendritic nonlinearities are critical for the efficient integration of synaptic inputs in circuits performing analog computations with spiking neurons. We developed a theory that formalizes how a neuron's dendritic nonlinearity that is optimal for integrating synaptic inputs depends on the statistics of its presynaptic activity patterns. Based on their in vivo preynaptic population statistics (firing rates, membrane potential fluctuations, and correlations due to ensemble dynamics), our theory accurately predicted the responses of two different types of cortical pyramidal cells to patterned stimulation by two-photon glutamate uncaging. These results reveal a new computational principle underlying dendritic integration in cortical neurons by suggesting a functional link between cellular and systems--level properties of cortical circuits.

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Relationship between the fluorescence intensity of rhodamine-labeled orexin A and the calcium responses in cortical neurons: An in vivo two-photon calcium imaging study

Journal of Pharmacological Sciences ◽

10.1016/j.jphs.2018.09.005 ◽

2018 ◽

Vol 138 (1) ◽

pp. 76-82

Author(s):

Saori Ohtani ◽

Satoshi Fujita ◽

Koki Hasegawa ◽

Hiromasa Tsuda ◽

Morio Tonogi ◽

...

Keyword(s):

Fluorescence Intensity ◽

Calcium Imaging ◽

Cortical Neurons ◽

Imaging Study ◽

Orexin A ◽

Two Photon

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Astrocytes in the mouse visual cortex reliably respond to visual stimulation

10.1101/429985 ◽

2018 ◽

Author(s):

Keita Sonoda ◽

Teppei Matsui ◽

Haruhiko Bito ◽

Kenichi Ohki

Keyword(s):

Visual Cortex ◽

Primary Visual Cortex ◽

Common Mechanism ◽

List Type ◽

Visual Responses ◽

Two Photon ◽

Dual Color ◽

Cross Correlation Analysis ◽

Mouse Visual Cortex

AbstractAstrocytes are known to contact with a great number of synapses and may integrate sensory inputs. In the ferret primary visual cortex, astrocytes respond to a visual stimulus with a delay of several seconds with respect to the surrounding neurons. However, in the mouse visual cortex, it remains unclear whether astrocytes respond to visual stimulations. In this study, using dual-color simultaneous in vivo two-photon Ca2+ imaging of neurons and astrocytes in the awake mouse visual cortex, we examined the visual responsiveness of astrocytes and their precise response timing relative to the surrounding neurons. Neurons reliably responded to visual stimulations, whereas astrocytes often showed neuromodulator-mediated global activities, which largely masked small periodic activities. Administration of the selective α1-adrenergic receptor antagonist prazosin substantially reduced such global astrocytic activities without affecting the neuronal visual responses. In the presence of prazosin, astrocytes showed weak but consistent visual responses mostly at their somata. Cross-correlation analysis estimated that the astrocytic visual responses were delayed by approximately 5 s relative to the surrounding neuronal responses. In conclusion, our research demonstrated that astrocytes in the primary visual cortex of awake mice responded to visual stimuli with a delay of several seconds relative to the surrounding neurons, which may indicate the existence of a common mechanism of neuron–astrocyte communication across species.HighlightsWe performed dual-color in vivo two-photon Ca2+ imaging of neurons and astrocytes.α1-adrenoblocker prazosin substantially reduced global astrocytic activities.Astrocytes showed weak but reliable visual responses in the awake mouse visual cortex.Astrocytic visual responses were delayed by 5 s relative to the neuronal ones.

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Three-dimensional Two-Photon Optogenetics and Imaging of Neural Circuits in vivo

10.1101/132506 ◽

2017 ◽

Cited By ~ 1

Author(s):

Weijian Yang ◽

Luis Carrillo-Reid ◽

Yuki Bando ◽

Darcy S. Peterka ◽

Rafael Yuste

Keyword(s):

Visual Cortex ◽

Neural Activity ◽

Calcium Imaging ◽

Pyramidal Neurons ◽

Neural Circuits ◽

Three Dimensional ◽

Two Photon ◽

Cellular Resolution ◽

Photon Excitation

We demonstrate a holographic system for simultaneous three-dimensional (3D) two-photon stimulation and imaging of neural activity in the mouse neocortex in vivo with cellular resolution. Dual two-photon excitation paths are implemented with independent 3D targeting for calcium imaging and precision optogenetics. We validate the usefulness of the microscope by photoactivating local pools of interneurons in awake mice visual cortex in 3D, which suppress the nearby pyramidal neurons’ response to visual stimuli.

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