Multifocal fluorescence microscope for fast optical recordings of neuronal action potentials.

Abstract:

:In recent years, optical sensors for tracking neural activity have been developed and offer great utility. However, developing microscopy techniques that have several kHz bandwidth necessary to reliably capture optically reported action potentials (APs) at multiple locations in parallel remains a significant challenge. To our knowledge, we describe a novel microscope optimized to measure spatially distributed optical signals with submillisecond and near diffraction-limit resolution. Our design uses a spatial light modulator to generate patterned illumination to simultaneously excite multiple user-defined targets. A galvanometer driven mirror in the emission path streaks the fluorescence emanating from each excitation point during the camera exposure, using unused camera pixels to capture time varying fluorescence at rates that are ∼1000 times faster than the camera's native frame rate. We demonstrate that this approach is capable of recording Ca(2+) transients resulting from APs in neurons labeled with the Ca(2+) sensor Oregon Green Bapta-1 (OGB-1), and can localize the timing of these events with millisecond resolution. Furthermore, optically reported APs can be detected with the voltage sensitive dye DiO-DPA in multiple locations within a neuron with a signal/noise ratio up to ∼40, resolving delays in arrival time along dendrites. Thus, the microscope provides a powerful tool for photometric measurements of dynamics requiring submillisecond sampling at multiple locations.

journal_name

Biophys J

journal_title

Biophysical journal

authors

Shtrahman M,Aharoni DB,Hardy NF,Buonomano DV,Arisaka K,Otis TS

doi

10.1016/j.bpj.2014.12.005

subject

Has Abstract

pub_date

2015-02-03 00:00:00

pages

520-9

issue

3

eissn

0006-3495

issn

1542-0086

pii

S0006-3495(14)04748-1

journal_volume

108

pub_type

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