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Ιδρυματικό Αποθετήριο Πανεπιστημίου Θεσσαλίας
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The metabolism of imidacloprid by aldehyde oxidase contributes to its clastogenic effect in New Zealand rabbits

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Συγγραφέας
Vardavas A.I., Ozcagli E., Fragkiadaki P., Stivaktakis P.D., Tzatzarakis M.N., Alegakis A.K., Vasilaki F., Kaloudis K., Tsiaoussis J., Kouretas D., Tsitsimpikou C., Carvalho F., Tsatsakis A.M.
Ημερομηνία
2018
Γλώσσα
en
DOI
10.1016/j.mrgentox.2018.03.002
Λέξη-κλειδί
aldehyde oxidase
enzyme inhibitor
imidacloprid
sodium tungstate dihydrate
unclassified drug
aldehyde oxidase
cytochrome P450
DNA
imidacloprid
insecticide
mutagenic agent
neonicotinoid
nitro derivative
sodium tungstate(VI)
tungsten derivative
analytical parameters
animal cell
animal experiment
Article
atmospheric pressure
clinical protocol
comet assay
controlled study
cytokinesis
Cytokinesis Block Proliferation Index
drug metabolism
electrophoresis
environmental exposure
enzyme activity
ion monitoring
ionization
limit of detection
limit of quantitation
male
micronucleus
micronucleus test
nonhuman
oxidation
oxidative stress
priority journal
single cell electrophoresis
animal
antagonists and inhibitors
drug effect
Leporidae
metabolism
single cell analysis
Aldehyde Oxidase
Animals
Cytochrome P-450 Enzyme System
DNA
Insecticides
Male
Metabolic Networks and Pathways
Micronucleus Tests
Mutagens
Neonicotinoids
Nitro Compounds
Oxidative Stress
Rabbits
Single-Cell Analysis
Tungsten Compounds
Elsevier B.V.
Εμφάνιση Μεταδεδομένων
Επιτομή
Imidacloprid (IMI) is a systemic, chloro-nicotinyl insecticide classified in Regulation N° 1272/2008 of the European Commision as “harmful if swallowed and very toxic to aquatic life, with long-lasting effects”. IMI is metabolized in vitro both by aldehyde oxidase (AOX) (reduction) and by cytochrome P450s enzymes (CYPs). In the present study, the AOX inhibitor sodium tungstate dihydrate (ST) was used to elucidate the relative contribution of CYP 450 and AOX metabolic pathways on IMI metabolism, in male rabbits exposed to IMI for two months. To evaluate the inhibition effectiveness, various metabolite concentrations in the IMI and IMI + ST exposed groups were monitored. DNA damage was also evaluated in micronucleus (MN) and single cell electrophoresis (SCGC) assays in both groups, along with oxidative stress (OS) with the inflammatory status of the exposed animals, in order to clarify which metabolic pathway is more detrimental in this experimental setting. A significant increase in the frequency of binucleated cells with MN (BNMN, 105%) and micronuclei (MN, 142%) was observed after exposure to IMI (p < 0.001). The increase in the ST co-exposed animals was less pronounced (BNMN 75%, MN 95%). The Cytokinesis Block Proliferation Index (CBPI) showed no significant difference between controls and exposed animals at any time of exposure (p > 0.05), which indicates no cytotoxic effect. Similarly, comet results show that the IMI group exhibited the highest achieved tail intensity, which reached 70.7% over the control groups, whereas in the IMI + ST groups the increase remained at 48.5%. No differences were observed between all groups for oxidative-stress biomarkers. The results indicate that the AOX metabolic pathway plays a more important role in the systemic toxicity of IMI. © 2018 Elsevier B.V.
URI
http://hdl.handle.net/11615/80401
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