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Clara cell cultures from the mouse and their reaction to bronchiolar toxins.

The major aim of this study was to determine if small numbers of freshly isolated mouse Clara cells could be used to rapidly screen the toxic effects of a number of diverse pulmonary toxins. A short-term (20 hr) culture of functionally competent (nitotetrazolium reductase positive) Clara cells was d...

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Detalles Bibliográficos
Autores principales: Richards, R J, Oreffo, V I, Lewis, R W
Formato: Texto
Lenguaje:English
Publicado: 1990
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC1568339/
https://www.ncbi.nlm.nih.gov/pubmed/2384058
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author Richards, R J
Oreffo, V I
Lewis, R W
author_facet Richards, R J
Oreffo, V I
Lewis, R W
author_sort Richards, R J
collection PubMed
description The major aim of this study was to determine if small numbers of freshly isolated mouse Clara cells could be used to rapidly screen the toxic effects of a number of diverse pulmonary toxins. A short-term (20 hr) culture of functionally competent (nitotetrazolium reductase positive) Clara cells was developed. In this culture the Clara cells were allowed to attach to an extracellular matrix in 96-well multiwell plates containing a culture medium of DCCM 1 and Ultroser G (0.4%). Pulmonary toxins (a total of 26 agents with concentrations ranging from 10(-7) M to 10(-3) M) were examined for their ability to reduce the attachment efficiency of functionally competent Clara cells and TD50 values (the amount of toxin required to reduce normal attachment efficiency by 50%) were calculated. With the possible exception of some halogenated hydrocarbons, the simple toxicity test in vitro correlated well with the known effects of the bronchiolar necrotic agents in vivo. For 13 compounds studied there was a direct correlation between TD50 values in vitro and LD50 values (mostly oral) in rodents in vivo, the correlation coefficient of the regression line being 0.783.
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spelling pubmed-15683392006-09-18 Clara cell cultures from the mouse and their reaction to bronchiolar toxins. Richards, R J Oreffo, V I Lewis, R W Environ Health Perspect Research Article The major aim of this study was to determine if small numbers of freshly isolated mouse Clara cells could be used to rapidly screen the toxic effects of a number of diverse pulmonary toxins. A short-term (20 hr) culture of functionally competent (nitotetrazolium reductase positive) Clara cells was developed. In this culture the Clara cells were allowed to attach to an extracellular matrix in 96-well multiwell plates containing a culture medium of DCCM 1 and Ultroser G (0.4%). Pulmonary toxins (a total of 26 agents with concentrations ranging from 10(-7) M to 10(-3) M) were examined for their ability to reduce the attachment efficiency of functionally competent Clara cells and TD50 values (the amount of toxin required to reduce normal attachment efficiency by 50%) were calculated. With the possible exception of some halogenated hydrocarbons, the simple toxicity test in vitro correlated well with the known effects of the bronchiolar necrotic agents in vivo. For 13 compounds studied there was a direct correlation between TD50 values in vitro and LD50 values (mostly oral) in rodents in vivo, the correlation coefficient of the regression line being 0.783. 1990-04 /pmc/articles/PMC1568339/ /pubmed/2384058 Text en
spellingShingle Research Article
Richards, R J
Oreffo, V I
Lewis, R W
Clara cell cultures from the mouse and their reaction to bronchiolar toxins.
title Clara cell cultures from the mouse and their reaction to bronchiolar toxins.
title_full Clara cell cultures from the mouse and their reaction to bronchiolar toxins.
title_fullStr Clara cell cultures from the mouse and their reaction to bronchiolar toxins.
title_full_unstemmed Clara cell cultures from the mouse and their reaction to bronchiolar toxins.
title_short Clara cell cultures from the mouse and their reaction to bronchiolar toxins.
title_sort clara cell cultures from the mouse and their reaction to bronchiolar toxins.
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC1568339/
https://www.ncbi.nlm.nih.gov/pubmed/2384058
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