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Two-photon imaging of spatially extended neuronal network dynamics with high temporal resolution.


ABSTRACT: We describe a simple two-photon fluorescence imaging strategy, called targeted path scanning (TPS), to monitor the dynamics of spatially extended neuronal networks with high spatiotemporal resolution. Our strategy combines the advantages of mirror-based scanning, minimized dead time, ease of implementation, and compatibility with high-resolution low-magnification objectives. To demonstrate the performance of TPS, we monitor the calcium dynamics distributed across an entire juvenile rat hippocampus (>1.5mm), at scan rates of 100 Hz, with single cell resolution and single action potential sensitivity. Our strategy for fast, efficient two-photon microscopy over spatially extended regions provides a particularly attractive solution for monitoring neuronal population activity in thick tissue, without sacrificing the signal-to-noise ratio or high spatial resolution associated with standard two-photon microscopy. Finally, we provide the code to make our technique generally available.

SUBMITTER: Lillis KP 

PROVIDER: S-EPMC2582024 | biostudies-literature | 2008 Jul

REPOSITORIES: biostudies-literature

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Two-photon imaging of spatially extended neuronal network dynamics with high temporal resolution.

Lillis Kyle P KP   Eng Alfred A   White John A JA   Mertz Jerome J  

Journal of neuroscience methods 20080503 2


We describe a simple two-photon fluorescence imaging strategy, called targeted path scanning (TPS), to monitor the dynamics of spatially extended neuronal networks with high spatiotemporal resolution. Our strategy combines the advantages of mirror-based scanning, minimized dead time, ease of implementation, and compatibility with high-resolution low-magnification objectives. To demonstrate the performance of TPS, we monitor the calcium dynamics distributed across an entire juvenile rat hippocamp  ...[more]

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2021-08-13 | GSE85722 | GEO