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The toxicity of silver and silica nanoparticles in comparable human and mouse cell lines

Research output: Contribution to conferencePosterResearchpeer-review

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The toxicity of silver and silica nanoparticles in comparable human and mouse cell lines. / Foldbjerg, Rasmus; Beer, Christiane; Sutherland, Duncan S et al.
2011. Poster session presented at Society of Toxicology Annual Meeting, Washington DC, United States.

Research output: Contribution to conferencePosterResearchpeer-review

Harvard

Foldbjerg, R, Beer, C, Sutherland, DS & Autrup, H 2011, 'The toxicity of silver and silica nanoparticles in comparable human and mouse cell lines', Society of Toxicology Annual Meeting, Washington DC, United States, 06/03/2011.

APA

Foldbjerg, R., Beer, C., Sutherland, D. S., & Autrup, H. (2011). The toxicity of silver and silica nanoparticles in comparable human and mouse cell lines. Poster session presented at Society of Toxicology Annual Meeting, Washington DC, United States.

CBE

Foldbjerg R, Beer C, Sutherland DS, Autrup H. 2011. The toxicity of silver and silica nanoparticles in comparable human and mouse cell lines. Poster session presented at Society of Toxicology Annual Meeting, Washington DC, United States.

MLA

Foldbjerg, Rasmus et al. The toxicity of silver and silica nanoparticles in comparable human and mouse cell lines. Society of Toxicology Annual Meeting, 06 Mar 2011, Washington DC, United States, Poster, 2011.

Vancouver

Foldbjerg R, Beer C, Sutherland DS, Autrup H. The toxicity of silver and silica nanoparticles in comparable human and mouse cell lines. 2011. Poster session presented at Society of Toxicology Annual Meeting, Washington DC, United States.

Author

Foldbjerg, Rasmus ; Beer, Christiane ; Sutherland, Duncan S et al. / The toxicity of silver and silica nanoparticles in comparable human and mouse cell lines. Poster session presented at Society of Toxicology Annual Meeting, Washington DC, United States.

Bibtex

@conference{e43bdc8d1fab4ec69cbf45821119456f,
title = "The toxicity of silver and silica nanoparticles in comparable human and mouse cell lines",
abstract = "The toxicity of silica (SiO2) and PVP-coated silver (Ag) nanoparticles (NPs) was investigated in two pairs of human or mouse cell lines originating from lung epithelium (A549 and ASB-XIV) and macrophages (THP-1 and J744A.1). Both NPs were characterized in H2O and cell media and demonstrated to be well dispersed. The primary sizes were 69 nm (Ag) and 27 nm (SiO2) as determined by TEM. Cytotoxicity was tested after 24 h in terms of viability by dehydrogenase activity (WST-8), apoptosis (Annexin V/PI) and the formation of ROS (DCF). Murine cells are more sensitive to NPs than human cells of similar origin, and the toxic response depends on both the NP type and the cell type. Approximately 10- times higher doses were needed for SiO2 NPs to cause a 50 % decrease in cell viability compared to Ag NPs. Significant increases in ROS generally occured at doses close to EC50 or higher leaving the question whether increased ROS were caused by the NPs or as a consequence of cell death. Induction of ROS was also assessed by the comet assay and modifications of DNA. In both human and murine epithelial lung cells, the EC50 NP concentrations from the WST-8 assay correlated well with results from the annexin V/PI assay. Death at EC50 in the lung cells was equally due to apoptosis and necrosis after exposure to either NP. However, large discrepancies were found when comparing EC50 values from the WST-8 assay in macrophages to results from the Annexin V/PI assay. The WST-8 assay appeared to overestimate cell death caused by Ag NPs in J774A.1 cells and by SiO2 NPs in THP-1 cells, whereas the assay underestimated the EC50 values of SiO2 NPs in J774A.1 cells and Ag NPs in THP-1 cells. These discrepancies suggest that dose-responses based on tetrazolium dyes such as WST-8 should be confirmed by additional assays e.g. annexin V/PI. Our preliminary data suggest that NP mediated toxicity can be higher in murine cell lines compared to their human counterparts. This information could be of importance if risk assessment will be based upon animal experimentation. This association will be the subject of investigation in our future work.",
author = "Rasmus Foldbjerg and Christiane Beer and Sutherland, {Duncan S} and Herman Autrup",
note = "Abstract was published in The Toxicologist, Volume 120, Supplement 2, March 2011, ISSN 1096-6080, Oxford University Press. ; Society of Toxicology Annual Meeting ; Conference date: 06-03-2011",
year = "2011",
language = "English",

}

RIS

TY - CONF

T1 - The toxicity of silver and silica nanoparticles in comparable human and mouse cell lines

AU - Foldbjerg, Rasmus

AU - Beer, Christiane

AU - Sutherland, Duncan S

AU - Autrup, Herman

N1 - Abstract was published in The Toxicologist, Volume 120, Supplement 2, March 2011, ISSN 1096-6080, Oxford University Press.

PY - 2011

Y1 - 2011

N2 - The toxicity of silica (SiO2) and PVP-coated silver (Ag) nanoparticles (NPs) was investigated in two pairs of human or mouse cell lines originating from lung epithelium (A549 and ASB-XIV) and macrophages (THP-1 and J744A.1). Both NPs were characterized in H2O and cell media and demonstrated to be well dispersed. The primary sizes were 69 nm (Ag) and 27 nm (SiO2) as determined by TEM. Cytotoxicity was tested after 24 h in terms of viability by dehydrogenase activity (WST-8), apoptosis (Annexin V/PI) and the formation of ROS (DCF). Murine cells are more sensitive to NPs than human cells of similar origin, and the toxic response depends on both the NP type and the cell type. Approximately 10- times higher doses were needed for SiO2 NPs to cause a 50 % decrease in cell viability compared to Ag NPs. Significant increases in ROS generally occured at doses close to EC50 or higher leaving the question whether increased ROS were caused by the NPs or as a consequence of cell death. Induction of ROS was also assessed by the comet assay and modifications of DNA. In both human and murine epithelial lung cells, the EC50 NP concentrations from the WST-8 assay correlated well with results from the annexin V/PI assay. Death at EC50 in the lung cells was equally due to apoptosis and necrosis after exposure to either NP. However, large discrepancies were found when comparing EC50 values from the WST-8 assay in macrophages to results from the Annexin V/PI assay. The WST-8 assay appeared to overestimate cell death caused by Ag NPs in J774A.1 cells and by SiO2 NPs in THP-1 cells, whereas the assay underestimated the EC50 values of SiO2 NPs in J774A.1 cells and Ag NPs in THP-1 cells. These discrepancies suggest that dose-responses based on tetrazolium dyes such as WST-8 should be confirmed by additional assays e.g. annexin V/PI. Our preliminary data suggest that NP mediated toxicity can be higher in murine cell lines compared to their human counterparts. This information could be of importance if risk assessment will be based upon animal experimentation. This association will be the subject of investigation in our future work.

AB - The toxicity of silica (SiO2) and PVP-coated silver (Ag) nanoparticles (NPs) was investigated in two pairs of human or mouse cell lines originating from lung epithelium (A549 and ASB-XIV) and macrophages (THP-1 and J744A.1). Both NPs were characterized in H2O and cell media and demonstrated to be well dispersed. The primary sizes were 69 nm (Ag) and 27 nm (SiO2) as determined by TEM. Cytotoxicity was tested after 24 h in terms of viability by dehydrogenase activity (WST-8), apoptosis (Annexin V/PI) and the formation of ROS (DCF). Murine cells are more sensitive to NPs than human cells of similar origin, and the toxic response depends on both the NP type and the cell type. Approximately 10- times higher doses were needed for SiO2 NPs to cause a 50 % decrease in cell viability compared to Ag NPs. Significant increases in ROS generally occured at doses close to EC50 or higher leaving the question whether increased ROS were caused by the NPs or as a consequence of cell death. Induction of ROS was also assessed by the comet assay and modifications of DNA. In both human and murine epithelial lung cells, the EC50 NP concentrations from the WST-8 assay correlated well with results from the annexin V/PI assay. Death at EC50 in the lung cells was equally due to apoptosis and necrosis after exposure to either NP. However, large discrepancies were found when comparing EC50 values from the WST-8 assay in macrophages to results from the Annexin V/PI assay. The WST-8 assay appeared to overestimate cell death caused by Ag NPs in J774A.1 cells and by SiO2 NPs in THP-1 cells, whereas the assay underestimated the EC50 values of SiO2 NPs in J774A.1 cells and Ag NPs in THP-1 cells. These discrepancies suggest that dose-responses based on tetrazolium dyes such as WST-8 should be confirmed by additional assays e.g. annexin V/PI. Our preliminary data suggest that NP mediated toxicity can be higher in murine cell lines compared to their human counterparts. This information could be of importance if risk assessment will be based upon animal experimentation. This association will be the subject of investigation in our future work.

M3 - Poster

T2 - Society of Toxicology Annual Meeting

Y2 - 6 March 2011

ER -