10.1128/iai.71.5.2394-2403.2003
Crossref journal-article
American Society for Microbiology
Infection and Immunity (235)
Abstract

ABSTRACTSeveral novelLegionella pneumophilavirulence genes were previously discovered by use of signature-tagged mutagenesis (P. H. Edelstein, M. A. Edelstein, F. Higa, and S. Falkow, Proc. Natl. Acad. Sci. 96:8190-8195, 1999). One of these mutants appeared to be defective in multiplication in guinea pig lungs and spleens, yet it multiplies normally in guinea pig alveolar macrophages. Here we report further characterization of the mutated gene and its protein and the virulence role of the gene. The complete sequence of the gene, now calledlvgA, is 627 bp long, and its protein product is approximately 27 kDa in size.lvgAwas present in all 50 strains ofL. pneumophilatested. No significant nucleic acid or protein homology was found in the GenBank database for the gene, nor were any distinctive motifs discovered in a search of other databases. The expression of both DotA and IcmX in thelvgAmutant was normal. Subcellular fractionation studies localized LvgA to the outer membrane fraction, and protease digestion studies suggested that at least some of the protein is surface expressed. No change in bacterial lipopolysaccharide composition or reactivity to serogroup-specific antisera was detected in the mutant. Growth competition studies with alveolar macrophages showed that the mutant was outcompeted by its parent 3-fold in 24 h and 24-fold in 48 h, in contrast to what was observed with the null phenotype in parallel testing with alveolar macrophages or with the A549 alveolar epithelial cell line. This macrophage defect of the mutant bacterium was due to slower growth, as the mutant invaded alveolar macrophages normally. Electron microscopy showed that the mutant bacterium resided in a ribosome-studded phagosome in alveolar macrophages, with no distinction from its parent. ThelvgAmutant was outcompeted by its parent about sixfold in guinea pig lungs and spleens; prolonged observation of infected animals showed no late-onset virulence of the mutant. Transcomplementation of the mutant restored the parental phenotype in guinea pigs. ThelvgAmutant was twofold more susceptible to killing by human β-defensin 2 but not to killing by other cationic peptides, serum complement, or polymorphonuclear neutrophils.lvgAis a novel virulence gene that is responsible for pleiotropic functions involving both extracellular and intracellular bacterial resistance mechanisms.

Bibliography

Edelstein, P. H., Hu, B., Higa, F., & Edelstein, M. A. C. (2003). lvgA, a NovelLegionella pneumophilaVirulence Factor. Infection and Immunity, 71(5), 2394–2403.

Authors 4 University of Pennsylvania
  1. Paul H. Edelstein (first) University of Pennsylvania
  2. Baofeng Hu (additional) University of Pennsylvania
  3. Futoshi Higa (additional) University of Pennsylvania
  4. Martha A. C. Edelstein (additional) University of Pennsylvania
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Dates
Type When
Created 22 years, 4 months ago (April 18, 2003, 4:54 p.m.)
Deposited 2 years, 3 months ago (April 26, 2023, 1:27 a.m.)
Indexed 1 year, 2 months ago (June 15, 2024, 3:56 a.m.)
Issued 22 years, 3 months ago (May 1, 2003)
Published 22 years, 3 months ago (May 1, 2003)
Published Print 22 years, 3 months ago (May 1, 2003)
Funders 0

None

@article{Edelstein_2003, title={lvgA, a NovelLegionella pneumophilaVirulence Factor}, volume={71}, ISSN={1098-5522}, url={http://dx.doi.org/10.1128/iai.71.5.2394-2403.2003}, DOI={10.1128/iai.71.5.2394-2403.2003}, number={5}, journal={Infection and Immunity}, publisher={American Society for Microbiology}, author={Edelstein, Paul H. and Hu, Baofeng and Higa, Futoshi and Edelstein, Martha A. C.}, year={2003}, month=may, pages={2394–2403} }