Please use this identifier to cite or link to this item: http://hdl.handle.net/1942/29985
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dc.contributor.authorMuruzabal, Damian-
dc.contributor.authorLANGIE, Sabine-
dc.contributor.authorPourrut, Bertrand-
dc.contributor.authorAzqueta, Amaya-
dc.date.accessioned2019-11-14T15:02:40Z-
dc.date.available2019-11-14T15:02:40Z-
dc.date.issued2019-
dc.identifier.citationMUTATION RESEARCH-GENETIC TOXICOLOGY AND ENVIRONMENTAL MUTAGENESIS, 845(SI) (Art N° UNSP 402981)-
dc.identifier.issn1383-5718-
dc.identifier.urihttp://hdl.handle.net/1942/29985-
dc.description.abstractThe enzyme-modified comet assay is a commonly used method to detect specific DNA lesions. However, still a lot of errors are made by many users, leading to dubious results and even misinterpretations. This technical note describes some critical points in the use of the enzyme-modified comet assay, such as the enzyme concentration, the time of incubation, the format used and the equipment. To illustrate the importance of these conditions/ parameters, titration experiments of formamidopyrimidine DNA glycosylase (Fpg) were performed using the 2 gels/slide and the 12 minigels/slide formats (plus the 12-Gel Comet Assay Unit (TM)). Incubation times of 15 and 30 min, and 1 h were used. Results showed that the 12 minigels/slide system requires a lower volume and concentration of Fpg. A longer time of incubation has a bigger impact when using such format. Moreover, the paper describes how to perform and interpret a titration experiment when using the enzyme. modified comet assay.-
dc.description.sponsorshipThis work was supported by the BIOGENSA project (AGL2015-70640-R) of the Ministry of Economy, Industry and Competitiveness of the Spanish Government and the European Regional Development Fund (ERDF).-
dc.language.isoen-
dc.publisherELSEVIER-
dc.rights2018 Elsevier B.V. All rights reserved.T-
dc.subject.otherComet assay; Formamidopyrimidine DNA glycosylase; Titration; 12 minigels; 2 gels; Enzyme incubation-
dc.subject.otherComet assay; Formamidopyrimidine DNA glycosylase; Titration; 12 minigels; 2 gels; Enzyme incubation-
dc.titleThe enzyme-modified comet assay: Enzyme incubation step in 2 vs 12-gels/slide systems-
dc.typeJournal Contribution-
dc.identifier.issueSI-
dc.identifier.volume845-
local.format.pages6-
local.bibliographicCitation.jcatA1-
dc.description.notes[Muruzabal, Damian; Azqueta, Amaya] Univ Navarra, Dept Pharmacol & Toxicol, C Irunlarrea 1,CIFA Bldg, Pamplona 31009, Spain. [Langie, Sabine A. S.] VITO Sustainable Hlth, Boeretang 200, B-2400 Mol, Belgium. [Langie, Sabine A. S.] Hasselt Univ, Ctr Environm Sci, Diepenbeek, Belgium. [Pourrut, Bertrand] Univ Lille Nord France, ISA Lille LGCgE, 48 Blvd Vauban, F-59046 Lille, France. [Azqueta, Amaya] Navarra Inst Hlth Res, IdiSNA, Navarra, Spain.-
local.publisher.placeAMSTERDAM-
local.type.refereedRefereed-
local.type.specifiedArticle-
local.bibliographicCitation.artnrUNSP 402981-
dc.identifier.doi10.1016/j.mrgentox.2018.11.005-
dc.identifier.isi000489193400004-
item.fulltextWith Fulltext-
item.fullcitationMuruzabal, Damian; LANGIE, Sabine; Pourrut, Bertrand & Azqueta, Amaya (2019) The enzyme-modified comet assay: Enzyme incubation step in 2 vs 12-gels/slide systems. In: MUTATION RESEARCH-GENETIC TOXICOLOGY AND ENVIRONMENTAL MUTAGENESIS, 845(SI) (Art N° UNSP 402981).-
item.accessRightsRestricted Access-
item.validationecoom 2020-
item.contributorMuruzabal, Damian-
item.contributorLANGIE, Sabine-
item.contributorPourrut, Bertrand-
item.contributorAzqueta, Amaya-
crisitem.journal.issn1383-5718-
crisitem.journal.eissn1879-3592-
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