Versatile Surface Electrodes for Combined Electrophysiology and Two-Photon Imaging of the Mouse Central Nervous System

Schweigmann, Michael; Caudal, Laura C.; Stopper, Gebhard; Scheller, Anja; Koch, Klaus Peter; Kirchhoff, Frank

doi:10.3389/fncel.2021.720675

Cited by 6 publications

(2 citation statements)

References 100 publications

(127 reference statements)

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“…Also, glial Ca 2+ signaling is differentially affected by anesthesia used during the in vivo recording. In line with our observations, previous work shows a reduced Ca 2+ activity in astroglia both in brain and spinal cord ( Thrane et al, 2012 ; Poskanzer and Yuste, 2016 ; Sekiguchi et al, 2016 ; Schweigmann et al, 2021 ) and an increased Ca 2+ activity in microglia in the brain under anesthesia ( Umpierre et al, 2020 ). Although microglial ROA density is higher in vivo , the ROA area itself is smaller than for astrocytes both ex vivo and in vivo in the early phase ( d1 and d2 ) after the window implantation ( Figures 3F , 5F ), suggesting that activated microglial Ca 2+ dynamics are reduced compared to physiological conditions.…”

Section: Discussionsupporting

confidence: 93%

Astrocytes and Microglia Exhibit Cell-Specific Ca2+ Signaling Dynamics in the Murine Spinal Cord

Rieder

Gobbo

Stopper

et al. 2022

Front. Mol. Neurosci.

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The spinal cord is the main pathway connecting brain and peripheral nervous system. Its functionality relies on the orchestrated activity of both neurons and glial cells. To date, most advancement in understanding the spinal cord inner mechanisms has been made either by in vivo exposure of its dorsal surface through laminectomy or by acute ex vivo slice preparation, likely affecting spinal cord physiology in virtue of the necessary extensive manipulation of the spinal cord tissue. This is especially true of cells immediately responding to alterations of the surrounding environment, such as microglia and astrocytes, reacting within seconds or minutes and for up to several days after the original insult. Ca2+ signaling is considered one of the most immediate, versatile, and yet elusive cellular responses of glia. Here, we induced the cell-specific expression of the genetically encoded Ca2+ indicator GCaMP3 to evaluate spontaneous intracellular Ca2+ signaling in astrocytes and microglia. Ca2+ signals were then characterized in acute ex vivo (both gray and white matter) as well as in chronic in vivo (white matter) preparations using MSparkles, a MATLAB-based software for automatic detection and analysis of fluorescence events. As a result, we were able to segregate distinct astroglial and microglial Ca2+ signaling patterns along with method-specific Ca2+ signaling alterations, which must be taken into consideration in the reliable evaluation of any result obtained in physiological as well as pathological conditions. Our study revealed a high degree of Ca2+ signaling diversity in glial cells of the murine spinal cord, thus adding to the current knowledge of the astonishing glial heterogeneity and cell-specific Ca2+ dynamics in non-neuronal networks.

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Section: Discussionsupporting

confidence: 93%

Astrocytes and Microglia Exhibit Cell-Specific Ca2+ Signaling Dynamics in the Murine Spinal Cord

Rieder

Gobbo

Stopper

et al. 2022

Front. Mol. Neurosci.

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“…[19] Schweigmann et al used a liquid crystal polymer (LCP)-based array for 28 days to capture GCaMP3 signals of neurons and astrocytes. [38] Even though each of these studies reported on a novel material science approach to create a transparent MEA, none of these studies addressed the longevity of optical signals captured through these devices. Our group was first investigating the optical performance of such a transparent microdevice quantitatively, where a Parylene HT/ITO-based ECoG array was implanted and tested for 51 days.…”

Section: Discussionmentioning

confidence: 99%

Transparent Thiol‐ene/Acrylate‐Based MicroECoG Devices Used for Concurrent Recording of Fluorescent Calcium Signals and Electrophysiology in Awake Animals

Szabó

Madarász

Lantos

et al. 2022

Adv Materials Inter

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voltage-sensitive dye imaging catalyzed the development of transparent neural interfaces that enable the application of both modalities. Electrophysiological methods with high temporal resolution are therefore often used in parallel with a non-invasive optical method with high spatial resolution. [2] Electrocorticogram (ECoG) register neural activity on the cortical surface, circumventing the electrical insulation of the scalp with minimally invasive surgical intervention. [3] By using of ECoG instead of the non-invasive electroencephalography (EEG) the difficulty to achieve efficient electrodeskin impedance [4] can be overcome. Twophoton microscopy is a laser-scanning, multifocal technique that typically collects fluorescent light from a single location. [5] Since two photons combine their energy during measurement, they are less harmful to biological tissues than the single-photon techniques. The two-photon calcium imaging is an efficient way to monitor the calcium-binding kinetics with a highly precise morphological image. [6] This method uses the fact, that in the living cells most of the depolarizing signals are in connection with the Ca 2+ influx, because of the voltagegated Ca 2+ channels. [7] Optogenetics provides molecular tools to selectively manipulate neuronal activity with light. [8] This technique uses genetic engineering to insert photosensitive protein channels into a specific population of neurons. [9] Shape memory polymers (SMPs) are suitable substrate materials for soft neural interfaces due to their tunable elastic characteristics. The stability and biocompatibility of intracortical SMP probes are demonstrated. In this work, a SMP-based cortical implant capable of recording high-density micro-electrocorticography is utilized in a multimodal neuroimaging scheme. The transparent nature of thiol-ene/acrylate substrate is exploited, and the feasibility of measuring intracranial electroencephalogram and fluorescent GCaMP6 signals with two-photon imaging through the device is presented in mice. The potential influence of the optical properties of the microdevice is investigated using fluorescent microbeads, hippocampal brain slices, and awake animals. It is found that neurites and cell soma can be efficiently detected with sufficient resolution to follow changes in the calcium signal. These chronically implanted devices do not suppress the quality of optical signals exceeding 22 weeks after implantation. These results indicate that thiol-ene/acrylate ECoG is an appropriate tool to combine electrophysiology with two-photon imaging while leveraging the inherent tissue-friendly properties of SMPs.

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Analogous cognitive strategies for tactile learning in the rodent and human brain

Banerjee

Wang

Teutsch

et al. 2023

Progress in Neurobiology

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Versatile Surface Electrodes for Combined Electrophysiology and Two-Photon Imaging of the Mouse Central Nervous System

Cited by 6 publications

References 100 publications

Astrocytes and Microglia Exhibit Cell-Specific Ca2+ Signaling Dynamics in the Murine Spinal Cord

Astrocytes and Microglia Exhibit Cell-Specific Ca2+ Signaling Dynamics in the Murine Spinal Cord

Transparent Thiol‐ene/Acrylate‐Based MicroECoG Devices Used for Concurrent Recording of Fluorescent Calcium Signals and Electrophysiology in Awake Animals

Analogous cognitive strategies for tactile learning in the rodent and human brain

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