In vitro genotoxicity of airborne Ni‐NP in air–liquid interface

In vitro genotoxicity of airborne Ni‐NP in air–liquid interface

Studies using advanced toxicological methods enabling in vitro conditions that are more realistic are currently needed for understanding the risks of pulmonary exposure to airborne nanoparticles. Owing to the carcinogenicity of certain nickel compounds, the increased production of nickel nanoparticl...

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Veröffentlicht in:Journal of applied toxicology 2017-12, Vol.37 (12), p.1420-1427
Hauptverfasser: Latvala, Siiri, Vare, Daniel, Karlsson, Hanna L., Elihn, Karine
Format: Artikel
Sprache:eng
Schlagworte:
Air Pollutants - toxicity
air-liquid interface
alkaline DNA unwinding
Animals
Base excision repair
Carcinogenicity
Carcinogens
Cell Culture Techniques
Cell Line
Cell Survival - drug effects
Cricetulus
Cytotoxicity
Damage
Deoxyribonucleic acid
DNA
DNA Damage
DNA repair
Exposure
Fibroblasts
Genotoxicity
HPRT
Hypoxanthine Phosphoribosyltransferase - genetics
In vitro methods and tests
Inhibitors
Lesions
Lungs
Medicin och hälsovetenskap
Metal Nanoparticles - toxicity
Mutagenicity
Mutagenicity Tests
Mutagens - toxicity
Mutation
Nanoparticles
nanotoxicology
Nickel
Nickel - toxicity
Nickel compounds
Occupational safety
Particle Size
Particulate Matter - toxicity
Poly(ADP-ribose) polymerase
Poly(ADP-ribose) Polymerase 1
Repair
Toxicity
Unwinding
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Zusammenfassung:Studies using advanced toxicological methods enabling in vitro conditions that are more realistic are currently needed for understanding the risks of pulmonary exposure to airborne nanoparticles. Owing to the carcinogenicity of certain nickel compounds, the increased production of nickel nanoparticles (Ni‐NPs) raises occupational safety concerns. The aim of this study was to investigate the genotoxicity of airborne Ni‐NPs using a recently developed air–liquid interface exposure system. The wild‐type Chinese hamster lung fibroblast cell line (V79) was used and cytotoxicity, DNA damage and mutagenicity were studied by testing colony forming efficiency, alkaline DNA unwinding and HPRT mutation assays, respectively. Additionally, co‐exposure to a PARP‐1 inhibitor was performed to test possible involvement of base excision repair (BER) in repair of Ni‐induced DNA damage. The results showed that cell viability was reduced significantly (to 45% and 46%) after 48 hours Ni‐NP exposure at concentrations of 0.15 and 0.32 μg cm−2. DNA damage was significantly increased after Ni‐NP exposure in the presence of the BER inhibitor indicating that Ni‐NP‐induced DNA damages are subsequently repaired by BER. Furthermore, there was no increased HPRT mutation frequency following Ni‐NP exposure. In conclusion, this study shows that Ni‐NP treatment of lung fibroblasts in an air–liquid interface system that mimics real‐life exposure, results in increased DNA strand breaks and reduced cellular viability. These DNA lesions were repaired with BER in an error‐free manner without resulting in mutations. This study also underlines the importance of appropriate quantification of the actual exposure concentrations during air–liquid interface exposure studies. The aim of this study was to investigate the genotoxicity of airborne Ni nanoparticles using a recently developed air‐liquid interface exposure system that mimics real‐life exposure. Cytotoxicity, DNA damage and mutagenicity were in the V79 cell line. Ni nanoparticle exposure of the cells in the air‐liquid interface resulted in increased DNA strand breaks and reduced cellular viability at concentrations of 0.15 and 0.32 μg cm −2. These DNA lesions were repaired with BER in an error‐free manner without resulting in mutations
ISSN:0260-437X
1099-1263
1099-1263
DOI:10.1002/jat.3510