4.5 Article

EntE, EntS and TolC synergistically contributed to the pathogenesis of APEC strain E058

Journal

MICROBIAL PATHOGENESIS
Volume 141, Issue -, Pages -

Publisher

ACADEMIC PRESS LTD- ELSEVIER SCIENCE LTD
DOI: 10.1016/j.micpath.2020.103990

Keywords

EntE; EntS; TolC; Pathogenesis; Avian pathogenic E. coli

Funding

  1. National Natural Science Foundation of China [31672553, 31972711, 31272559, 30972196, 30771604, 30471281]
  2. National Key R&D Program of China [2017YFD0500203, YFD0500705]
  3. Natural Science Foundation of Jiangsu Agri-animal Husbandry Vocational College [NSF201621]
  4. National Program for High Technology Research and Development in China [2003 AA 222141]
  5. Special Fund for Agroscientific Research in the Public Interest [201303044]
  6. Priority Academic Program Development of Jiangsu Higher Education Institutions (PAPD)

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Extraintestinal pathogenic Escherichia coil (ExPEC) shows an enhanced ability to cause infection outside the intestinal tract. Avian pathogenic E. coli (APEC), one type of ExPEC, causes avian colibacillosis, a disease of significant economic importance to poultry producers worldwide that is characterized by systemic infection. Some ExPEC strains as well as other pathogenic enterobacteria produce enterobactin, a catecholate siderophore used to sequester iron during infection. Here, we showed that disruption of enterobactin efflux via outer membrane protein TolC significantly decreased the pathogenicity of APEC strain E058. Furthermore, colonization and persistence assays performed using a chicken infection model showed that the AtoIC mutant was obviously attenuated (p(<)0.001). In contrast, disruption of enterobactin synthesis gene entE and/or the inner membrane transporter gene entS had little effect on pathogenicity. Analysis of growth kinetics revealed a significant reduction in the growth of triple mutant strain E058 Delta entE Delta entS Delta tolC in iron-deficient medium compared with the wild-type strain (p(<)0.001), while no growth impairment was noted for the E058 Delta 6tolC mutant in either Luria-Bertani broth or iron-deficient medium. The E058 Delta entE Delta entS Delta tolC mutant also showed significantly decreased virulence compared with single mutant strain E058 Delta 6tolC. Low-copy complementation of strains E058 Delta 6tolC and E0584entEAentSAto1C with plasmid-borne to/C restored virulence to wild-type levels in the chicken infection model. Macrophage infection assays showed that ingestion of E058 Delta 6tolC by macrophage cell line HD11 cells was reduced compared with ingestion of the E058 Delta entE Delta entS Delta tolC mutant. However, no significant differences were observed between the mutants and the wild-type in a chicken serum resistance assay. Together, these results suggest that EntE, EntS and TolC synergistically contributed to the pathogenesis of APEC strain E058 in an iron-deficient environment.

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