Oxidative stress and dermal toxicity of iron oxide nanoparticles in vitro

Ashley R Murray; Elena Kisin; Alfred Inman; Shih-Houng Young; Mamoun Muhammed; Terrance Burks; Abdusalam Uheida; Alexey Tkach; Micah Waltz; Vincent Castranova; Bengt Fadeel; Valerian E Kagan; Jim E Riviere; Nancy Monteiro-Riviere; Anna A Shvedova

doi:10.1007/s12013-012-9367-9

Oxidative stress and dermal toxicity of iron oxide nanoparticles in vitro

Cell Biochem Biophys. 2013 Nov;67(2):461-76. doi: 10.1007/s12013-012-9367-9.

Authors

Ashley R Murray¹, Elena Kisin, Alfred Inman, Shih-Houng Young, Mamoun Muhammed, Terrance Burks, Abdusalam Uheida, Alexey Tkach, Micah Waltz, Vincent Castranova, Bengt Fadeel, Valerian E Kagan, Jim E Riviere, Nancy Monteiro-Riviere, Anna A Shvedova

Affiliation

¹ Pathology and Physiology Research Branch, Health Effects Laboratory Division, National Institute for Occupational Safety and Health (NIOSH), M/L 2015, 1095 Willowdale Road, Morgantown, WV, 26505, USA.

PMID: 22669739
DOI: 10.1007/s12013-012-9367-9

Abstract

A number of commercially available metal/metal oxide nanoparticles (NPs) such as superparamagnetic iron oxide (SPION) are utilized by the medical field for a wide variety of applications. These NPs may able to induce dermal toxicity via their physical nature and reactive surface properties. We hypothesize that SPION may be toxic to skin via the ability of particles to be internalized and thereby initiate oxidative stress, inducing redox-sensitive transcription factors affecting/leading to inflammation. Due to the skin's susceptibility to UV radiation, it is also of importance to address the combined effect of UVB and NPs co-exposure. To test this hypothesis, the effects of dextran-coated SPION of different sizes (15-50 nm) and manufacturers (MicroMod, Rostock-Warnemunde, Germany and KTH-Royal Institute of Technology, Stockholm, Sweden) were evaluated in two cell lines: normal human epidermal keratinocytes (HEK) and murine epidermal cells (JB6 P(+)). HEK cells exposed to 20 nm (KTH and MicroMod) had a decrease in viability, while the 15 and 50 nm particles were not cytotoxic. HEK cells were also capable of internalizing the KTH particles (15 and 20 nm) but not the MicroMod SPION (20 and 50 nm). IL-8 and IL-6 were also elevated in HEK cells following exposure to SPION. Exposure of JB6 P(+) cells to all SPIONs evaluated resulted in activation of AP-1. Exposure to SPION alone was not sufficient to induce NF-κB activation; however, co-exposure with UVB resulted in significant NF-κB induction in cells exposed to 15 and 20 nm KTH SPION and 50 nm MicroMod particles. Pre-exposure of JB6 P(+) cells to UVB followed by NPs induced a significant depletion of glutathione, release of cytokines, and cell damage as assessed by release of lactate dehydrogenase. Altogether, these data indicate that co-exposure to UVB and SPIONs was associated with induction of oxidative stress and release of inflammatory mediators. These results verify the need to thoroughly evaluate the adverse effects of UVB when evaluating dermal toxicity of engineered NPs on skin.

Publication types

Research Support, Non-U.S. Gov't
Research Support, U.S. Gov't, P.H.S.

MeSH terms

Biological Transport
Cell Survival / drug effects
Cytokines / metabolism
Glutathione / metabolism
Humans
Keratinocytes / cytology
Keratinocytes / drug effects
Keratinocytes / metabolism
L-Lactate Dehydrogenase / metabolism
Magnetite Nanoparticles / chemistry
Magnetite Nanoparticles / toxicity*
NF-kappa B / metabolism
Oxidative Stress / drug effects*
Particle Size
Skin / cytology
Skin / drug effects*
Transcription Factor AP-1 / metabolism

Substances

Cytokines
Magnetite Nanoparticles
NF-kappa B
Transcription Factor AP-1
L-Lactate Dehydrogenase
Glutathione

Grants and funding

OH008282/OH/NIOSH CDC HHS/United States