Variation in the measurement of DNA damage by comet assay measured by the ECVAG inter-laboratory validation trial
Author(s) -
Lykke Forchhammer,
Catharina Johansson,
Steffen Loft,
L. Moller,
Roger Godschalk,
Sabine A. S. Langie,
George D.D. Jones,
R. W. L. Kwok,
Andrew Collins,
Amaya Azqueta,
David H. Phillips,
Osman Sözeri,
Maciej Stępnik,
Jadwiga Palus,
Ulla Vogel,
Håkan Wallin,
Michael N. Routledge,
Catherine Handforth,
Alessandra Allione,
Giuseppe Matullo,
João Paulo Teixeira,
Solange Costa,
Patrizia Riso,
Marisa Porrini,
Peter Möller
Publication year - 2009
Publication title -
mutagenesis
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.723
H-Index - 91
eISSN - 1464-3804
pISSN - 0267-8357
DOI - 10.1093/mutage/gep048
Subject(s) - comet assay , dna damage , coefficient of variation , ionizing radiation , comet , dna , microbiology and biotechnology , biology , chemistry , physics , irradiation , genetics , chromatography , astrobiology , nuclear physics
The comet assay has become a popular method for the assessment of DNA damage in biomonitoring studies and genetic toxicology. However, few studies have addressed the issue of the noted inter-laboratory variability of DNA damage measured by the comet assay. In this study, 12 laboratories analysed the level of DNA damage in monocyte-derived THP-1 cells by either visual classification or computer-aided image analysis of pre-made slides, coded cryopreserved samples of cells and reference standard cells (calibration curve samples). The reference standard samples were irradiated with ionizing radiation (0-10 Gy) and used to construct a calibration curve to calculate the number of lesions per 10(6) base pair. All laboratories detected dose-response relationships in the coded samples irradiated with ionizing radiation (1.5-7 Gy), but there were overt differences in the level of DNA damage reported by the different laboratories as evidenced by an inter-laboratory coefficient of variation (CV) of 47%. Adjustment of the primary comet assay end points by a calibration curve prepared in each laboratory reduced the CV to 28%, a statistically significant reduction (P < 0.05, Levene's test). A large fraction of the inter-laboratory variation originated from differences in image analysis, whereas the intra-laboratory variation was considerably smaller than the variation between laboratories. In summary, adjustment of primary comet assay results by reference standards reduces inter-laboratory variation in the level of DNA damage measured by the alkaline version of the comet assay.
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