4.6 Article

CpxRA Influences Xenorhabdus nematophila Colonization Initiation and Outgrowth in Steinernema carpocapsae Nematodes through Regulation of the nil Locus

Journal

APPLIED AND ENVIRONMENTAL MICROBIOLOGY
Volume 75, Issue 12, Pages 4007-4014

Publisher

AMER SOC MICROBIOLOGY
DOI: 10.1128/AEM.02658-08

Keywords

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Funding

  1. Burroughs-Wellcome Foundation
  2. National Institutes of Health (NIH) [GM59776, T32 AI007414]

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The gammaproteobacterium Xenorhabdus nematophila mutualistically colonizes an intestinal region of a soil-dwelling nematode and is a blood pathogen of insects. The X. nematophila CpxRA two-component regulatory system is necessary for both of these host interactions (E. Herbert et al., Appl. Environ. Microbiol. 73:7826-7836, 2007). Mutualistic association of X. nematophila with its nematode host consists of two stages: initiation, where a small number of bacterial cells establish themselves in the colonization site, and outgrowth, where these cells grow to fill the space. In this study, we show that the Cpx system is necessary for both of these stages. X. nematophila Delta cpxR1 colonized fewer nematodes than its wild-type parent and did not achieve as high a density as did the wild type within a portion of the colonized nematodes. To test whether the Delta cpxR1 host interaction phenotypes are due to its overexpression of mrxA, encoding the type I pilin subunit protein, we assessed the colonization phenotype of a Delta cpxR1 Delta mrxA1 double mutant. This mutant displayed the same colonization defect as Delta cpxR1, indicating that CpxR negative regulation of mrxA does not play a detectable role in X. nematophila-host interactions. CpxR positively regulates expression of nilA, nilB, and nilC genes necessary for nematode colonization. Here we show that the nematode colonization defect of the Delta cpxR1 mutant is rescued by elevating nil gene expression through mutation of nilR, a negative regulator of nilA, nilB, and nilC. These data suggest that the nematode colonization defect previously observed in Delta cpxR1 is caused, at least in part, by altered regulation of nilA, nilB, and nilC.

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