Comparing synthetic refocusing to deconvolution for the extraction of neuronal calcium transients from light-fields

Author:

Howe Carmel L.ORCID,Quicke PeterORCID,Song PingfanORCID,Jadan Herman VerinazORCID,Dragotti Pier LuigiORCID,Foust Amanda J.ORCID

Abstract

AbstractSignificanceLight-field microscopy (LFM) enables fast, light-efficient, volumetric imaging of neuronal activity with calcium indicators. Calcium transients differ in temporal signal-to-noise ratio (tSNR) and spatial confinement when extracted from volumes reconstructed by different algorithms.AimWe evaluated the capabilities and limitations of two light-field reconstruction algorithms for calcium fluorescence imaging.ApproachWe acquired light-field image series from neurons either bulk-labeled or filled intracellularly with the red-emitting calcium dye CaSiR-1 in acute mouse brain slices. We compared the tSNR and spatial confinement of calcium signals extracted from volumes reconstructed with synthetic refocusing and Richardson-Lucy 3D deconvolution with and without total variation regularization.ResultsBoth synthetic refocusing and Richardson-Lucy deconvolution resolved calcium signals from single cells and neuronal dendrites in three dimensions. Increasing deconvolution iteration number improved spatial confinement but reduced tSNR compared to synthetic refocusing. Volumetric light-field imaging did not decrease calcium signal tSNR compared to interleaved, widefield image series acquired in matched planes.ConclusionsLFM enables high-volume rate, volumetric imaging of calcium transients in single cells (bulk-labeled), somata and dendrites (intracellular loaded). The trade-offs identified for tSNR, spatial confinement, and computational cost indicate which of synthetic refocusing or deconvolution can better realize the scientific requirements of future LFM calcium imaging applications.

Publisher

Cold Spring Harbor Laboratory

Reference45 articles.

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