Am. J. Respir. Cell Mol. Biol., Vol 17, No. 1, Jul 1997, 97-105.
Isolation and characterization of a peroxidase from the airway
M Salathe, M Holderby, R Forteza, WM Abraham, A Wanner and GE Conner
Division of Pulmonary and Critical Care Medicine, University of Miami School of Medicine, Florida 33136, USA.
Sheep airway mucus can potently scavenge hydrogen peroxide, an important
mediator of airway inflammation. Here, the scavenging activity was
identified as a peroxidase produced by goblet cells of the airway
epithelium and secreted into the airway lumen. Ovine airway peroxidase
activity was purified approximately 100-fold from airway lavage fluid in
two steps, using cation exchange and lectin affinity chromatography,
yielding an apparently homogeneous 82-kD glycoprotein. Ovine airway
peroxidase represented about 1% of the total protein in airway mucus and
thus was an abundant enzyme in airway secretions. The absorbance spectrum
of the purified peroxidase showed a major peak at 412 nm indicative of a
hemoprotein. The ratio of A412/A280 of the purified enzyme was 0.86. The
absorption spectrum of ovine airway peroxidase, its ability to oxidize
halides, its sensitivity to inhibitors and its apparent molecular mass on
sodium dodecyl sulfate gels showed that airway peroxidase was similar to
lactoperoxidase but distinguished from myeloperoxidase, eosinophil
peroxidase as well as from glutathione peroxidases. Based on these
observations, ovine airway peroxidase is a newly isolated and abundant
enzyme of airway mucus which may function to control reactive oxygen
species in the airway and to prevent infection by catalyzing the formation
of biocidal compounds.
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Copyright © 1997 American Thoracic Society.
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