Am. J. Respir. Crit. Care Med., Vol 154, No. 6, Dec 1996, 1700-1705.
Antioxidant kinetics in lung lavage fluid following exposure of humans to nitrogen dioxide
FJ Kelly, A Blomberg, A Frew, ST Holgate and T Sandstrom
Rayne Institute, St. Thomas' Hospital, London, United Kingdom.
To determine if nitrogen dioxide (NO2), a gaseous free radical, modifies
the protective antioxidant pool present in respiratory tract lining fluids,
a random, double-blind study utilizing flexible fiberoptic bronchoscopy
with bronchial and bronchoalveolar lavage was performed. Healthy,
nonsmoking, asymptomatic subjects were exposed to filtered air and 2 ppm
NO2 for 4 h on separate occasions. To examine the kinetics of the
NO2-induced antioxidant reactions, 44 subjects were randomly assigned to
one of three groups. Bronchoscopy was performed 1.5 h (group 1), 6 h (group
2) or 24 h (group 3) after each exposure. Reduced glutathione (GSH), uric
acid, and ascorbic acid concentrations were determined in both bronchial
and bronchoalveolar lavage fluid fractions. In addition, bronchoalveolar
lavage fluid was screened for malondialdehyde as a marker of lipid
peroxidation. Exposure to NO2 resulted in a rapid (1.5 h) loss of uric acid
from the bronchial region, however by 6 h after exposure it had increased
significantly above control uric acid concentration in this region. At 24 h
after exposure, uric acid concentration had returned to the control level.
A similar response of uric acid to NO2 was seen in the bronchoalveolar
region. Ascorbic acid was also decreased in bronchial and bronchoalveolar
lavage fluids 1.5 h after exposure to NO2, but returned to control values
by 6 h. In marked contrast, significant increases in GSH concentration were
seen at 1.5 and 6 h in bronchial lavage fluid after exposure to NO2, which
subsequently returned to control levels by 24 h. No change in
bronchoalveolar lavage fluid GSH concentration or malondialdehyde content
was seen after NO2 exposure. These data support the view that antioxidants
present in lung fluids react with, and hence modulate the impact of, NO2 on
the lung.
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Copyright © 1996 American Thoracic Society
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