A Workingperson’s Guide to Deconvolution in Light Microscopy

Wes Wallace; Lutz H. Schaefer; Jason R. Swedlow

doi:10.2144/01315bi01

BioTechniques (Nov 2001)

A Workingperson’s Guide to Deconvolution in Light Microscopy

Wes Wallace,
Lutz H. Schaefer,
Jason R. Swedlow

Affiliations

Wes Wallace: 1University of Dundee, Dundee, Scotland
Lutz H. Schaefer: 1University of Dundee, Dundee, Scotland
Jason R. Swedlow: 1University of Dundee, Dundee, Scotland

DOI: https://doi.org/10.2144/01315bi01
Journal volume & issue: Vol. 31, no. 5
pp. 1076 – 1097

Abstract

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The fluorescence microscope is routinely used to study cellular structure in many biomedical research laboratories and is increasingly used as a quantitative assay system for cellular dynamics. One of the major causes of image degradation in the fluorescence microscope is blurring. Deconvolution algorithms use a model of the microscope imaging process to either subtract or reassign out-of-focus blur. A variety of algorithms are now commercially available, each with its own characteristic advantages and disadvantages. In this article, we review the imaging process in the fluorescence microscope and then discuss how the various deconvolution methods work. Finally, we provide a summary of practical tips for using deconvolution and discuss imaging artifacts and how to minimize them.

Published in BioTechniques

ISSN: 0736-6205 (Print); 1940-9818 (Online)
Publisher: Taylor & Francis Group
Country of publisher: United Kingdom
LCC subjects: Science: Biology (General)
Website: https://www.tandfonline.com/journals/ibtn20

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