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High-throughput Titration of Luciferase-expressing Recombinant Viruses
Author(s) -
Vanessa da Silva Garcia,
Ramya Krishnan,
Colin Davis,
Cory Batenchuk,
Fabrice Le Bœuf,
Hesham Abdelbary,
JeanSimon Diallo
Publication year - 2014
Publication title -
journal of visualized experiments
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.596
H-Index - 91
ISSN - 1940-087X
DOI - 10.3791/51890
Subject(s) - luciferase , virus quantification , titer , luciferin , microtiter plate , titration , plate reader , bioluminescence , context (archaeology) , recombinant dna , virology , virus , chemistry , biology , cell culture , microbiology and biotechnology , biochemistry , transfection , inorganic chemistry , paleontology , genetics , physics , quantum mechanics , gene , fluorescence
Standard plaque assays to determine infectious viral titers can be time consuming, are not amenable to a high volume of samples, and cannot be done with viruses that do not form plaques. As an alternative to plaque assays, we have developed a high-throughput titration method that allows for the simultaneous titration of a high volume of samples in a single day. This approach involves infection of the samples with a Firefly luciferase tagged virus, transfer of the infected samples onto an appropriate permissive cell line, subsequent addition of luciferin, reading of plates in order to obtain luminescence readings, and finally the conversion from luminescence to viral titers. The assessment of cytotoxicity using a metabolic viability dye can be easily incorporated in the workflow in parallel and provide valuable information in the context of a drug screen. This technique provides a reliable, high-throughput method to determine viral titers as an alternative to a standard plaque assay.

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