Journal
INFECTION AND IMMUNITY
Volume 71, Issue 9, Pages 4977-4984Publisher
AMER SOC MICROBIOLOGY
DOI: 10.1128/IAI.71.9.4977-4984.2003
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Funding
- NIAID NIH HHS [R01 AI051477, AI051477-01 A1] Funding Source: Medline
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Previous studies have demonstrated that the Moraxella catarrhalis surface antigen UspA1 is an adhesin for Chang human conjunctival cells. The present report demonstrates that lack of UspA1 expression does not affect the adherence of strain 035E to A549 human lung cells or primary cultures of human middle ear epithelial (HMEE) cells. These results imply that another molecule mediates the adherence of M. catarrhalis to these two cell lines. To identify this adhesin, strain 035E was mutagenized with a transposon and 1,000 mutants were screened in a microcolony formation assay using A:549 cells. Nine independent isolates exhibited an 8- to 19-fold reduction in adherence and contained a transposon in the same locus. Nucleotide sequence data and PCR analysis indicated that the transposons were inserted in different locations in the gene encoding the surface protein Hag. Quantitative assays using one representative transposon mutant, 035E. TN2, showed considerably decreased binding to A549 as well as HMEE cells. However, this mutant adhered at wild-type levels to Chang conjunctival cells. These findings suggest that the M. catarrhalis Hag protein is an adhesin for cell lines derived from human lung and middle ear tissues.
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