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Potential in vitro model for testing the effect of exposure to nanoparticles on the lung alveolar epithelial barrier()

Pulmonary barrier function plays a pivotal role in protection from inhaled particles. However, some nano-scaled particles, such as carbon nanotubes (CNT), have demonstrated the ability to penetrate this barrier in animal models, resulting in an unusual, rapid interstitial fibrosis. To delineate the...

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Autores principales: Derk, Raymond, Davidson, Donna C., Manke, Amruta, Stueckle, Todd A., Rojanasakul, Yon, Wang, Liying
Formato: Online Artículo Texto
Lenguaje:English
Publicado: 2015
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5425160/
https://www.ncbi.nlm.nih.gov/pubmed/28503407
http://dx.doi.org/10.1016/j.sbsr.2014.12.002
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author Derk, Raymond
Davidson, Donna C.
Manke, Amruta
Stueckle, Todd A.
Rojanasakul, Yon
Wang, Liying
author_facet Derk, Raymond
Davidson, Donna C.
Manke, Amruta
Stueckle, Todd A.
Rojanasakul, Yon
Wang, Liying
author_sort Derk, Raymond
collection PubMed
description Pulmonary barrier function plays a pivotal role in protection from inhaled particles. However, some nano-scaled particles, such as carbon nanotubes (CNT), have demonstrated the ability to penetrate this barrier in animal models, resulting in an unusual, rapid interstitial fibrosis. To delineate the underlying mechanism and specific bio-effect of inhaled nanoparticles in respiratory toxicity, models of lung epithelial barriers are required that allow accurate representation of in vivo systems; however, there is currently a lack of consistent methods to do so. Thus, this work demonstrates a well-characterized in vitro model of pulmonary barrier function using Calu-3 cells, and provides the experimental conditions required for achieving tight junction complexes in cell culture, with trans-epithelial electrical resistance measurement used as a biosensor for proper barrier formation and integrity. The effects of cell number and serum constituents have been examined and we found that changes in each of these parameters can greatly affect barrier formation. Our data demonstrate that use of 5.0 × 10(4) Calu-3 cells/well in the Transwell cell culture system, with 10% serum concentrations in culture media is optimal for assessing epithelial barrier function. In addition, we have utilized CNT exposure to analyze the dose-, time-, and nanoparticle property-dependent alterations of epithelial barrier permeability as a means to validate this model. Such high throughput in vitro cell models of the epithelium could be used to predict the interaction of other nanoparticles with lung epithelial barriers to mimic respiratory behavior in vivo, thus providing essential tools and bio-sensing techniques that can be uniformly employed.
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spelling pubmed-54251602017-05-10 Potential in vitro model for testing the effect of exposure to nanoparticles on the lung alveolar epithelial barrier() Derk, Raymond Davidson, Donna C. Manke, Amruta Stueckle, Todd A. Rojanasakul, Yon Wang, Liying Sens Biosensing Res Article Pulmonary barrier function plays a pivotal role in protection from inhaled particles. However, some nano-scaled particles, such as carbon nanotubes (CNT), have demonstrated the ability to penetrate this barrier in animal models, resulting in an unusual, rapid interstitial fibrosis. To delineate the underlying mechanism and specific bio-effect of inhaled nanoparticles in respiratory toxicity, models of lung epithelial barriers are required that allow accurate representation of in vivo systems; however, there is currently a lack of consistent methods to do so. Thus, this work demonstrates a well-characterized in vitro model of pulmonary barrier function using Calu-3 cells, and provides the experimental conditions required for achieving tight junction complexes in cell culture, with trans-epithelial electrical resistance measurement used as a biosensor for proper barrier formation and integrity. The effects of cell number and serum constituents have been examined and we found that changes in each of these parameters can greatly affect barrier formation. Our data demonstrate that use of 5.0 × 10(4) Calu-3 cells/well in the Transwell cell culture system, with 10% serum concentrations in culture media is optimal for assessing epithelial barrier function. In addition, we have utilized CNT exposure to analyze the dose-, time-, and nanoparticle property-dependent alterations of epithelial barrier permeability as a means to validate this model. Such high throughput in vitro cell models of the epithelium could be used to predict the interaction of other nanoparticles with lung epithelial barriers to mimic respiratory behavior in vivo, thus providing essential tools and bio-sensing techniques that can be uniformly employed. 2015-03 /pmc/articles/PMC5425160/ /pubmed/28503407 http://dx.doi.org/10.1016/j.sbsr.2014.12.002 Text en This is an open access article under the CC BY-NC-ND license (http://creativecommons.org/licenses/by-nc-nd/4.0/).
spellingShingle Article
Derk, Raymond
Davidson, Donna C.
Manke, Amruta
Stueckle, Todd A.
Rojanasakul, Yon
Wang, Liying
Potential in vitro model for testing the effect of exposure to nanoparticles on the lung alveolar epithelial barrier()
title Potential in vitro model for testing the effect of exposure to nanoparticles on the lung alveolar epithelial barrier()
title_full Potential in vitro model for testing the effect of exposure to nanoparticles on the lung alveolar epithelial barrier()
title_fullStr Potential in vitro model for testing the effect of exposure to nanoparticles on the lung alveolar epithelial barrier()
title_full_unstemmed Potential in vitro model for testing the effect of exposure to nanoparticles on the lung alveolar epithelial barrier()
title_short Potential in vitro model for testing the effect of exposure to nanoparticles on the lung alveolar epithelial barrier()
title_sort potential in vitro model for testing the effect of exposure to nanoparticles on the lung alveolar epithelial barrier()
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5425160/
https://www.ncbi.nlm.nih.gov/pubmed/28503407
http://dx.doi.org/10.1016/j.sbsr.2014.12.002
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