Opsonized Virulent Edwardsiella tarda Strains Are Able To Adhere to and Survive and Replicate within Fish Phagocytes but Fail To Stimulate Reactive Oxygen Intermediates

doi:10.1128/IAI.69.9.5689-5697.2001

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Infection and Immunity, September 2001, p. 5689-5697, Vol. 69, No. 9
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.9.5689-5697.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Opsonized Virulent Edwardsiella tarda Strains Are Able To Adhere to and Survive and Replicate within Fish Phagocytes but Fail To Stimulate Reactive Oxygen Intermediates

Putanae S. Srinivasa Rao,¹ Tit Meng Lim,¹ and Ka Yin Leung¹^,²^,^*

Department of Biological Sciences, Faculty of Science,¹ and Tropical Marine Science Institute,² National University of Singapore, Singapore 119260

Received 2 January 2001/Returned for modification 12 March 2001/Accepted 7 June 2001

Edwardsiella tarda is responsible for hemorrhagic septicemia (edwardsiellosis) in fish and also causes diseases in highervertebrates such as birds, reptiles, and mammals, including humans.Interactions of E. tarda with blue gourami phagocytes were studiedby light microscopy as well as by adherence, intracellular replication,and superoxide anion assays. Both nonopsonized virulent (PPD130/91and AL9379) and avirulent (PPD125/87 and PPD76/87) bacteria couldadhere to and survive and replicate within phagocytes, while onlyopsonized virulent strains replicated within the phagocytes. Furthermore,only avirulent E. tarda elicited a higher rate of production ofreactive oxygen intermediates (ROIs) by phagocytes, indicatingthat they were unable to avoid and/or resist reactive oxygen radical-basedkilling by the fish phagocytes. TnphoA transposon mutagenesiswas used to construct a library of 200 alkaline phosphatase (PhoA⁺) fusion mutants from a total of 182,000 transconjugants derivedfrom E. tarda PPD130/91. Five of these mutants induced more ROIproduction in phagocytes than the wild-type strain. Two mutantshad lower replication ability inside phagocytes and moderatelyhigher 50% lethal dose values than the wild-type strain. Sequenceanalysis revealed that three of these mutants had insertions atsequences having homology to PhoS, dipeptidase, and a surfacepolymer ligase of lipid A core proteins of other pathogens. Thesethree independent mutations might have changed the cell surfacecharacteristics of the bacteria, which in turn induced phagocytesto produce increased ROIs. Sequences from two other mutants hadno homology to known genes, indicating that they may be novelgenes for antiphagocytic killing. The present study showed thatthere are differences in the interactions of virulent and avirulentE. tarda organisms with fish phagocytes and PhoA⁺ fusion mutants that could be used successfully to identify virulencegenes. The information elucidated here would help in the developmentof suitable strategies to combat the disease caused by E. tarda.

^* Corresponding author. Mailing address: Department of Biological Sciences, Faculty of Science, The National University of Singapore,Science Drive 4, Singapore 117543, Singapore. Phone: (65) 8747835. Fax: (65) 779 2486. E-mail: dbslky{at}nus.edu.sg.

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