Characterization and genetic complementation of a Brucella abortus high-temperature-requirement A (htrA) deletion mutant.

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Infection and Immunity, October 1994, p. 4135-4139, Vol. 62, No. 10
0019-9567/1994/$04.00+0 DOI:

research-article

Characterization and genetic complementation of a Brucella abortus high-temperature-requirement A (htrA) deletion mutant.

P H Elzer, R W Phillips, M E Kovach, K M Peterson, and R M Roop 2nd

Department of Microbiology and Immunology, Louisiana State University Medical Center, Shreveport 71130-3932.

ABSTRACT

In order to evaluate the biological function of the Brucellaabortus high-temperature-requirement A (HtrA) stress responseprotein homolog, the majority of the htrA gene was deleted fromthe chromosome of B. abortus 2308 via gene replacement. In contrastto the parental strain, the resulting htrA deletion mutant,designated PHE1, failed to grow on solid medium at 40 degreesC and demonstrated increased sensitivity to killing by H2O2and O2- in disk sensitivity assays. BALB/c mice were infectedwith strains 2308 and PHE1 to assess the effect of the htrAmutation on virulence, and significantly fewer brucellae wererecovered from the spleens of mice infected with PHE1 than fromthose of mice infected with 2308 at 1 week postinfection. Geneticcomplementation studies were performed to confirm the relationshipbetween the htrA mutation and the phenotype observed for PHE1.Plasmid pRIE1 was constructed by inserting a 1.9-kb EcoRI fragmentencoding the B. abortus htrA gene into the broad-host-rangeplasmid pBBR1MCS. Introduction of pRIE1 into PHE1 relieved thetemperature- and H2O2-sensitive phenotypes of this mutant invitro, and PHE1(pRIE1) colonized the spleens of BALB/c miceat levels equivalent to those of the parental 2308 strain at1 week postinfection. These results support our previous proposalthat the B. abortus htrA gene product functions as a stressresponse protein and further suggest that this protein contributesto virulence. These studies also demonstrate the utility ofthe broad-host-range plasmid pBBR1MCS for genetic complementationstudies in Brucella spp., establishing a key reagent for moredetailed genetic analysis of this important zoonotic pathogen.

Infection and Immunity, October 1994, p. 4135-4139, Vol. 62, No. 10
0019-9567/1994/$04.00+0 DOI:

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