Putative Quorum-Sensing Regulator BlxR of Brucella melitensis Regulates Virulence Factors Including the Type IV Secretion System and Flagella

Brucella melitensis is an intracellular pathogen that establishesa replicative niche within macrophages. While the intracellularlifestyle of Brucella is poorly understood and few virulencefactors have been identified, components of a quorum-sensingpathway in Brucella have recently been identified. The LuxR-typeregulatory protein, VjbR, and an N-acylhomoserine lactone signalingmolecule are both involved in regulating expression of the virB-encodedtype IV secretion system. We have identified a second LuxR-typeregulatory protein (BlxR) in Brucella. Microarray analysis ofa blxR mutant suggests that BlxR regulates the expression ofa number of genes, including those encoding the type IV secretionsystem and flagella. Confirming these results, deletion of blxRin B. melitensis reduced the transcriptional activities of promotersfor the virB operon, flagellar genes, and another putative virulencefactor gene, bopA. Furthermore, our data suggested that bothBlxR and VjbR are positively autoregulated and cross-regulatethe expression of each other. The blxR deletion strain exhibitedreduced growth in macrophages, similar to that observed fora vjbR deletion strain. However, unlike the vjbR deletion, theblxR deletion did not fully attenuate virulence in mice. Morestrikingly, bioluminescent imaging revealed that disseminationof the blxR mutant was similar to that of wild-type B. melitensis,while the vjbR mutant was defective for systemic spread in IRF-1^–/–mice, suggesting that these regulators are not functionallyredundant but that they converge in a common pathway regulatingbacterial processes.

INTRODUCTION

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INTRODUCTION

Brucella species are intracellular pathogens that establisha replicative niche within macrophages (7, 22). Internalizationof Brucella occurs through lipid raft-mediated macropinocytosis(28, 58). After uptake into the phagosome, Brucella-containingvesicles move by altered intracellular trafficking through membrane-boundcompartments to fuse with endoplasmic reticulum (ER) membranes,where Brucella replicates in vesicles associated with the ER(7, 8, 20, 43). The type IV secretion system, encoded by thevirB operon, is critical to intracellular survival (18, 26,33, 41). Brucella VirB mutants are unable to persist withinmacrophages or HeLa cells, have lost the ability to manipulatethe endosomal pathway to dock with the ER, and are avirulentin mice (1, 4, 5, 10, 41, 52).

Little is known about the mechanisms employed by Brucella forinfection, maintenance of the intracellular lifestyle, and eventualexit from the host cell. One strategy employed by many bacteriafor the coordinated expression of factors influencing interactionwith their environment is gene regulation via quorum sensing,a cell density-dependent system for intracellular communicationallowing coordinated gene regulation within a bacterial population.Quorum-sensing systems in both symbiotic and pathogenic bacteriaregulate factors affecting interaction with the host, such asmotility and chemotaxis (19, 27), biofilm formation (11, 12,23, 27), and the production and secretion of virulence factors(25, 59).

Two proteins form the fundamental components of a typical quorum-sensingsystem: the autoinducer synthase, which synthesizes a smallsignal molecule, and a regulatory protein, which dimerizes andbinds to DNA upon interaction with the signal molecule. Theprototype of this system is the Vibrio fischeri LuxI/LuxR system.LuxI, the autoinducer synthase, produces the autoinducer moleculeN-(3-oxohexanoyl)-homoserine lactone (14). This molecule diffusesthrough the cell wall, allowing the bacterial population toregulate genes coordinately in response to population density.The regulatory protein, LuxR, contains an N-terminal acyl-homoserinelactone autoinducer binding domain (24) and a C-terminal helix-turn-helixDNA binding and dimerization domain (9).

There is evidence that the type IV secretion system and theflagellum in Brucella melitensis are regulated by a quorum-sensingpathway. Although there are no luxI homologs in the B. melitensisgenome, an autoinducer molecule has been identified. The autoinducerN-dodecanoyl-homoserine-lactone (C12-HSL) was purified fromsolvent-extracted supernatant of Brucella grown in RPMI (54).Addition of synthetic C12-HSL suppressed expression of the virBoperon (54), suggesting that the quorum-sensing system of Brucellamay act to repress, rather than to induce, target virulencegenes in response to autoinducer accumulation. A homolog ofthe LuxR transcriptional regulator, VjbR, encoded at locus BMEII1116,was found to be required for expression of the virB and flagellargenes (13, 32). The vjbR deletion strain was also defectivefor growth in macrophages and displayed attenuated virulencein mice (13). Complementation of this strain with an autoinducerbinding domain mutant vjbR allele resulted in expression ofvirB that was not suppressed by addition of exogenous C12-HSL(56), suggesting that this autoinducer interacts with VjbR tomediate suppression of virB.

We have identified a second LuxR homolog, termed BlxR (BrucellaluxR-like regulator). Like VjbR, BlxR was required for transcriptionof the type IV secretion system and flagellar genes. Transcriptionalactivity of the vjbR and blxR promoters was reduced in boththe vjbR and blxR deletion strains, indicating that expressionof VjbR and BlxR are autoregulated, as well as cross-regulated.The blxR deletion mutant exhibited reduced growth in macrophagessimilar to that of the vjbR deletion mutant. However, deletionof blxR did not fully attenuate virulence in an IRF-1^–/–mouse model of infection, unlike the vjbR deletion. Lastly,bioluminescent imaging revealed that the spread of the blxRmutant was similar to that of wild-type B. melitensis, whilethe vjbR mutant was defective for in vivo dissemination.

MATERIALS AND METHODS

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MATERIALS AND METHODS

Bacterial strains, plasmids, and culture conditions. All strains and plasmids used in this study are listed in TableS1 in the supplemental material. Brucella strains were maintainedon brucella agar (Becton Dickinson, Sparks, MD) and grown inbrucella broth (BB), tryptic soy broth (TSB), or minimal yeastextract medium (44) at 37°C. E. coli strains were grownin Luria-Bertani broth at 37°C. The following antibioticswere used as appropriate: kanamycin (50 µg/ml for Brucella;20 µg/ml for E. coli), ampicillin (200 µg/ml), chloramphenicol(40 µg/ml), and zeocin (250 µg/ml for Brucella;50 µg/ml for E. coli).

Generation of vjbR and blxR deletion mutants. The vectors used for allelic replacement were generated in twosteps as previously described (46). First, the gene of interestplus $~$ 1 kb of flanking DNA was amplified by PCR. All primer sequencesare listed in Table S2 in the supplemental material. XbaI andKpnI sites added to the primers were used to clone each fragmentinto the KpnI-XbaI sites of pZErO-1. The resulting plasmidswere amplified by inverse PCR to remove a fragment internalto the gene to be mutated ( $~$ 300 bp for blxR; $~$ 500 bp for vjbR)and to introduce BamHI sites. The kanamycin resistance (Km^r)cassette excised from pUC4K using BamHI was inserted to createthe suicide vectors pAGM18 and pAGM19.

Electrocompetent B. melitensis 16M aliquots were electroporatedwith pAGM18 and pAGM19 (400 ${Omega}$ ; 25 µF; 1.8 kV). Transformantswere selected on BB agar supplemented with kanamycin, and resistantcolonies were screened for sensitivity to zeocin. Replacementof target genes was verified by PCR using sets of primers internalto the Km^r cassette and flanking the deleted genes (see TableS2 in the supplemental material). Southern hybridization wasperformed to confirm the replacement of vjbR and blxR usinga DNA fragment internal to vjbR (250 bp) and blxR (273 bp) amplifiedfrom B. melitensis 16M DNA, as well as a 600-bp DNA fragmentinternal to the Km^r cassette, by North2South Detection (Pierce)as described previously (47).

Bioluminescent vjbR and blxR deletion mutants were generatedby allelic replacement of the vjbR and blxR genes in the constitutivelybioluminescent B. melitensis strain GR023 (47) as describedabove.

RNA extraction and labeling. Bacteria were grown in TSB until mid- to late log phase. BeforeRNA isolation, phenol-ethanol (1:19) was added, and the cellswere pelleted by centrifugation and stored at –80°C.Total RNA was extracted from cell pellets using the MasterPureRNA purification kit (Epicenter), and DNA was removed usingTurbo DNA-free (Ambion). cDNA was synthesized from 7 µgof total RNA in the presence of CyDye-3-dCTP (Amersham Biosciences).The labeled cDNA was purified using the ChipShot cDNA System(Promega). For each sample, RNA was extracted from two independentlygrown cultures, and cDNA was generated three times for eachRNA sample.

Microarray hybridization. For the minimicroarray, 289 potential open reading frames (ORFs)of the B. melitensis 16M genome were selected based on theirhypothesized involvement in virulence. They included genes forproteins involved in type IV secretion, flagella, outer membranebiogenesis, transcriptional regulation, denitrification, ironuptake, and peptide and small-molecule transport. Oligonucleotides(70-mers) representing these 289 genes were purchased from Qiagen,resuspended in 3x SSC (1x SSC is 0.15 M NaCl plus 0.015 M sodiumcitrate), and spotted onto Ultra Gaps-coated slides (Corning)using the MicroGrid Microarrayer (Apogent Discoveries). Theslides were desiccated in a vacuum oven with Drierite for 48h and UV cross-linked using a Stratalinker at 600 mJ. The printingof each ORF spot was verified by hybridizing it with Cy3-labeled9-mer (Qiagen). The slides were stored under vacuum at roomtemperature with Drierite pellets until further use.

16M genomic DNA (gDNA) was labeled by incorporation of CyDye-5-dCTP(Amersham Biosciences) using High Prime DNA Labeling (Roche)according to the manufacturer's instructions. Unincorporatednucleotides were removed using Micron YM-30 columns (Millipore).

Cy3-labeled cDNA was mixed with 0.75 µg Cy5-labeled gDNA,and hybridization buffer (Pronto Plus Kit; Promega) was addedto a final volume of 35 µl. The entire sample was loadedonto the printed array and covered with a HybriSlip coverslip(Molecular Probes). The arrays were placed in specialized hybridizationchambers (Telechem Inc., Sunnyvale, CA) and incubated at 42°Covernight. The slides were washed using the Pronto Plus HybridizationSystem (Promega) and dried by centrifugation at 1,000 rpm for5 min.

Microarray scanning and data analysis. Slides were scanned using the GenePix4000B scanner (Axon Instruments)with independent excitation of the fluorophores Cy3 and Cy5.Background intensities for each spot were calculated using GenPixPro3.0 software (Axon Instruments) via the segmentation method.The signal intensity for each spot was calculated as the differencebetween the average signal intensity and the average local backgroundintensity. Data were normalized to gDNA levels by calculatingthe ratios of cDNA to gDNA for each spot. The data were thenlog₂ transformed, and the signal ratio for each spot was dividedby the mean signal ratio of the entire array to validate comparisonsbetween different arrays. Data normalization and statisticalanalysis were performed using The Institute for Genomic Research(TIGR) MeV (51).

Generation of a promoterless luxCDABE plasmid. A PCR fragment containing the promoter of the B. melitensisery (erythritol) operon (upstream of BMEII0430) was generatedfrom B. melitensis gDNA using the eryP primer pair. PlasmidpBBR1-MCS4 (31) and the PCR fragment were digested with NsiIand BamHI and ligated together, deleting the lacZ promoter frompBBR1-MCS4 to generate plasmid pBBR-P_ery. To delete the erypromoter, pBBR-P_ery was digested with NsiI and PstI, resultingin identical overhangs, and religated to produce pBBR- ${Delta}$ P_ery.The luxCDABE operon was digested from pXen-13 (Xenogen) usingBamHI and SacI and cloned into pBBR- ${Delta}$ P_ery to generate pEP3, consistingof a promoterless lux operon downstream of KpnI, ApaI, XhoI,and BamHI restriction sites.

Construction of lux transcriptional fusion plasmids. Regions consisting of approximately 300 bp of sequence upstreamof the selected ORFs were amplified by PCR using primers (TableS2) that added a KpnI site to the 5' end and an XhoI site tothe 3' end. The PCR products were cloned into pCR2.1 (Invitrogen).After being sequenced, the promoter regions were subcloned intopEP3 using KpnI and XhoI.

Bioluminescent transcriptional assays. Transcriptional lux fusion reporter plasmids were electroporatedinto B. melitensis strains 16M, 16M ${Delta}$ vjbR, and 16M ${Delta}$ blxR. Singlecolonies from transformants were inoculated into BB and grownfor 72 h. Strains were resuspended to an optical density (OD)or A₆₀₀ of 0.1 in BB and incubated at 37°C. At selectedtime points, 100 µl of each culture was transferred toa black 96-well plate for quantification of bioluminescenceusing a biophotonic imaging system (Xenogen). The values foreach well, in photons/s/sr/cm², were normalized for backgroundluminescence by subtracting the value for a control well. TheOD of the culture was determined, and the bioluminescence valuewas divided by the OD to normalize for the culture cell density.

To obtain a baseline for the transcriptional activities of thepromoters, the bioluminescence of strain 16M harboring the differentreporter plasmids was measured every 4 h for 28 h during growthin BB, with an additional sample taken at 48 h. The optimaltime for measurement of promoter activity was found to be 20h.

Growth in liquid culture. Cultures were started from isolated colonies and grown for 2days in BB at 37°C and then subcultured to an OD (A₆₀₀)of 0.1 in BB and grown at 37°C. The OD (A₆₀₀) was takenat 8, 16, 24, 32, and 48 h.

Macrophage infection. The murine macrophage-like cell line RAW264.7 was maintainedin RPMI 1640 supplemented with 10% fetal bovine serum at 37°Cwith 5% CO₂. Prior to infection, macrophages were seeded at5 x 10⁵ cells/well in fresh RPMI 1640 supplemented with 10%fetal bovine serum in six-well plates and incubated for 16 hat 37°C with 5% CO₂. Infection assays were performed ata multiplicity of infection of 100, as previously described(6). The cells were incubated for 90 min at 37°C with 5%CO₂, and extracellular bacteria were removed by washing thecells three times with phosphate-buffered saline (PBS), followedby 30 min of incubation in RPMI containing 30 µg/ml gentamicin.Infected cells were maintained in medium containing 2 µg/mlof gentamicin. At specified times, the wells were washed threetimes with PBS, the macrophages were lysed using 0.1% TritonX-100, and viable intracellular bacterial counts were determinedby dilution plating. All dilutions were plated in duplicate.For complementation, the vjbR and blxR ORFs plus 300 bp of upstreamsequence were amplified using primers that added a KpnI siteto the 5' end and an XhoI site to the 3' end. PCR products werecloned into pCR2.1 (Invitrogen). After being sequenced, vjbRwas subcloned into pBBR1-MCS4 (31) and blxR was subcloned intopBBR1-MCS1 (31) using KpnI and XhoI. For the macrophage infectionassay, B. melitensis strains harboring plasmids were dilutionplated with and without antibiotic selective for plasmid maintenanceto confirm that the CFU were representative of bacteria containingthe complementing plasmid.

Mouse virulence assay. The virulence of B. melitensis 16M, 16M ${Delta}$ vjbR, and 16M ${Delta}$ blxR wasevaluated using a murine model of infection (29). Groups of6- to 9-week old female and male IRF-1^–/– mice wereinfected intraperitoneally with 1 x 10⁷ bacteria in 0.2 ml PBS(n = 7 for 16M; n = 8 for 16M ${Delta}$ vjbR and 16M ${Delta}$ blxR). The mice weremonitored for mortality for 2 weeks.

In vivo bioluminescent imaging. Mice were infected intraperitoneally with 1 x 10⁷ bacteria asdescribed above using the bioluminescent strains GR023, ARL01,and ARL02. The mice were anesthetized with isoflurane and imagedusing a charge-coupled device camera every 2 days. The imageswere recorded and analyzed using LivingImage software (Xenogen).

Microarray data accession number. The microarray data have been deposited in the NCBI Gene ExpressionOmnibus (GEO) database (http://www.ncbi.nlm.nih.gov/geo/) underGEO series accession number GSE10735.

RESULTS

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RESULTS

BlxR (BMEI1758) is a LuxR homolog. A gene with homology to members of the luxR family of transcriptionalregulators was identified at locus BMEI1758 by BLAST search(http://www.ncbi.nlm.nih.gov/BLAST) and designated blxR forBrucella LuxR-like regulator (Fig. 1). The predicted amino acidsequence of BlxR was 31% identical and 45% similar to that ofLuxR from V. fischeri and had the highest homology to CepR ofBurkholderia cepacia (43% identity; 58% similarity). BlxR alsoshares 25% identity and 45% similarity with VjbR. BlxR containsthe two domains present in all LuxR family members: an autoinducerbinding domain and a DNA binding domain (Fig. 1) (9). Severalresidues shown to be important for autoinducer or DNA bindingin V. fischeri LuxR are also conserved (15, 30, 55).

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FIG. 1. Amino acid sequence homology of BlxR to quorum-sensing regulators. Shown is a comparison of the BlxR sequence to those of V. fischeri LuxR and B. melitensis VjbR. The autoinducer binding domain is shown in boldface, and the DNA binding domain is underlined. The asterisks indicate residues that are highly conserved in LuxR homologs. Residues shown to be important for autoinducer binding or DNA binding in V. fischeri LuxR (15, 30, 55) are overscored. The conserved aspartic acid shown to be important for autoinducer binding in B. melitensis VjbR (56) is indicated with a box.

To study the effect of BlxR on gene expression, bacterial growth,and pathogenicity, deletion mutants were constructed in whicheither the blxR or vjbR gene in B. melitensis 16M was replacedwith a kanamycin resistance cassette. The deletion was confirmedby PCR and Southern hybridization (data not shown).

BlxR affects multiple genes, as detected by microarray. Since LuxR homologs in other bacteria are involved in regulatinggenes involved in a number of bacterial processes, includingvirulence, the effect of blxR deletion on the expression ofB. melitensis potential virulence genes was determined usinga microarray. A minimicroarray containing spotted oligonucleotidescorresponding to 289 B. melitensis genes was used to identifycandidate genes whose transcription is influenced by BlxR. Thismicroarray contains genes encoding the type IV secretion system,flagella, transcriptional regulators, transporters, and proteinsinvolved in outer membrane biogenesis, iron acquisition, anddenitrification. RNA was prepared from both B. melitensis 16Mand the blxR deletion strain, 16M ${Delta}$ blxR, grown to late log phasein TSB. Microarray analysis identified 36 genes with alteredtranscript levels in 16M ${Delta}$ blxR compared to 16M, using Welch'sapproximation with a critical P value of 0.01 (Table 1). TheORFs included in the microarray are listed in Tables S3 (chromosomeI) and S4 (chromosome II) in the supplemental material, alongwith the corresponding P values. Interestingly, five flagellargenes and eight genes from the virB type IV secretion systemoperon were identified in this screen. Transcription from boththe fliF and the virB promoters was downregulated in a vjbRmutant (13).

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TABLE 1. Genes identified with significant changes in transcript levels between 16M and the BlxR mutant

BlxR is involved in transcription of virB and flagellar genes. To further investigate the effect of the blxR deletion on regulationof the type IV secretion system and flagella, lux transcriptionalfusions to the virB and flagellar promoters flhB and flgJ wereconstructed by cloning the promoter regions of selected genesupstream of a promoterless lux operon in the Brucella shuttlevector pBBR1-MCS4 (31). A lux transcriptional fusion to theinitiation factor 1 (infA) promoter region (BMEI1671) was constructedas a control, since this gene was not predicted to be underquorum-sensing control and a green fluorescent protein fusionto the IF-1 promoter was constitutively fluorescent (16). Atranscriptional fusion was also constructed to the upstreamregion of Brucella outer protein (bopA) at locus BMEII0188,which was not included in the microarray. BopA is a hypotheticalprotein with homology to secreted R-factor proteins involvedin host specificity in plant pathogens. BMEI0188 is locatedwithin genomic island 5 (45), a region that is not present inBrucella ovis, a species that is nonpathogenic to humans.

Plasmids harboring the transcriptional fusions were electroporatedinto wild-type B. melitensis 16M, 16M ${Delta}$ vjbR, and 16M ${Delta}$ blxR. Culturesgrown for 72 h were used to inoculate fresh BB, and after 20h of incubation at 37°C, samples were removed for measurementof bioluminescence and OD. Bioluminescence values were dividedby the OD to normalize for slight differences in culture growth.As expected, transcription from the infA promoter was not reducedin the regulatory-gene mutant strains compared to wild-typeB. melitensis 16M (Fig. 2A). Transcription from the virB promoterwas significantly reduced in 16M ${Delta}$ blxR (Fig. 2B) and was alsoreduced in the vjbR mutant, consistent with previously publishedresults (13). Transcription of the flagellar genes flhB andflgJ was also significantly reduced in 16M ${Delta}$ blxR (Fig. 2C and D),confirming the microarray result, and in 16M ${Delta}$ vjbR, consistentwith the effect of a vjbR deletion on other flagellar genes(13). Additionally, transcription of bopA was reduced in both16M ${Delta}$ vjbR and 16M ${Delta}$ blxR relative to expression in the wild type(Fig. 2E), suggesting that transcription of bopA is regulatedthrough the quorum-sensing pathway.

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FIG. 2. Transcriptional activities of potential target genes. Shown are transcriptional activities of the following promoters in wild-type B. melitensis 16M and the regulatory-gene deletion strains 16M ${Delta}$ vjbR and 16M ${Delta}$ blxR: P_infA (BMEI1671) (A), P_virB (BMEI0025) (B), P_flhB (BMEII1114) (C), P_flgJ (BMEI1692) (D), and P_bopA (BMEII0188) (E). Units of intensity (I) are photons·s^–1·sr^–1·cm^–2. The asterisks indicate transcription levels that are significantly lower than transcription in strain 16M, as determined by paired t tests (P < 0.05). The error bars represent standard deviations for three independent experiments.

BlxR and VjbR are autoregulatory and cross-regulatory. Several LuxR homologs regulate their own transcription (36,39, 49), and in bacteria that contain more than one LuxR homolog,LuxR proteins can regulate the transcription of each other (35,37, 42, 57). To determine whether autoregulation and cross talkalso occur with VjbR and BlxR, we constructed lux transcriptionalfusions to regions upstream of the vjbR and blxR genes. Thetranscriptional activity of the regulatory gene promoters wasmonitored in B. melitensis 16M, 16M ${Delta}$ vjbR, and 16M ${Delta}$ blxR (Fig. 3).Transcription of blxR was down-regulated in 16M ${Delta}$ blxR, indicatingthat BlxR is an activator of its own transcription, and transcriptionof vjbR was down-regulated in 16M ${Delta}$ vjbR, suggesting that VjbRis also a positive regulator of its own transcription. Likewise,blxR was downregulated in 16M ${Delta}$ vjbR and vjbR was downregulatedin 16M ${Delta}$ blxR, suggesting that both transcriptional regulatorscross-activate transcription of each other, although the reductionin expression was less than twofold for the vjbR promoter andabout twofold for the blxR promoter. This result confirms theconnection between the regulatory networks of the two quorum-sensingregulators. However, analysis of the genes directly regulatedby each protein may be complicated by the fact that deletionof either the vjbR or blxR gene reduces transcription of theother gene by about half.

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FIG. 3. Autoregulation and cross talk between VjbR and BlxR. Shown are transcriptional activities of the regulatory-gene promoter-lux fusions in wild-type 16M and the regulatory-gene deletion strains. (A) vjbR activity. (B) blxR activity. The asterisks indicate transcription levels significantly lower than transcription in strain 16M, as determined by paired t tests (P < 0.05). The error bars represent standard deviations of four independent experiments for P_blxR and six independent experiments for P_vjbR.

Deletion of blxR reduced intracellular growth in macrophages. During growth in BB, the overall growth of the mutants was similarto that of wild-type B. melitensis 16M (Fig. 4A), although 16M ${Delta}$ vjbRappeared to transition into stationary phase earlier and reachedstationary phase at a slightly lower OD (A₆₀₀) than wild-typeB. melitensis. The OD of 16M ${Delta}$ vjbR at 16 and 24 h was significantlydifferent from that of 16M (P < 0.05), while the OD of 16M ${Delta}$ blxRwas not significantly different from that of 16M at either time,suggesting that VjbR expression affects growth in late-log phasewhile BlxR expression does not.

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FIG. 4. Growth of B. melitensis 16M vjbR and blxR mutants. (A) Growth in BB. The error bars represent the standard deviations for three independent trials. (B) Growth in RAW264.7 cells. (C) Complementation of blxR and vjbR mutants. Bacterial counts were determined after 48 h of infection of RAW264.7 cells. The error bars represent the standard deviations for four independent trials.

The abilities of 16M ${Delta}$ vjbR and 16M ${Delta}$ blxR to infect and persist withinhost cells in vitro were evaluated using the murine macrophagecell line RAW 264.7 (Fig. 4B). Both 16M ${Delta}$ vjbR and 16M ${Delta}$ blxR enteredmacrophages at levels similar to that of the wild type, indicatingno defect in adherence or entry. In all three strains, an initialdrop in intracellular bacteria occurred, followed by a steadyincrease in intracellular bacteria from 6 to 48 h postinfection.Intracellular counts of strains 16M ${Delta}$ vjbR and 16M ${Delta}$ blxR increasedat a slightly lower rate than that of the wild type. By 48 h,the number of intracellular bacteria was 1.34 log units lowerfor the vjbR mutant than for the wild type (P < 0.01), adifference consistent with previously published data for thistime point (13, 56), and 0.96 log units lower for the blxR mutant(P < 0.02). The difference in intracellular growth betweenthe two deletion strains was not statistically significant,suggesting that loss of either LuxR homolog has a similar effecton intracellular survival.

Growth in macrophages was restored to wild-type levels by complementationwith the replicating plasmid pBBR1 containing the deleted geneplus 300 bp of upstream sequence but was not affected by thepresence of the vector plasmid alone (Fig. 4C).

Deletion of blxR increased the mean number of days to mortality but did not affect bacterial spread in mice. To determine whether BlxR is required for virulence in vivo,IRF-1^–/– mice were infected with 1 x 10⁷ bacteriavia intraperitoneal injection. IRF-1^–/– mice arehighly susceptible to Brucella infection and succumb to infectionwith B. melitensis 16M in 7 to 10 days (29). All mice in thecontrol group infected with B. melitensis 16M died between 7and 9 days postinfection, whereas mice infected with 16M ${Delta}$ vjbRdid not show any symptoms of disease and did not succumb toinfection (Fig. 5). Mice infected with 16M ${Delta}$ blxR died between8 and 11 days postinfection. The death of 16M ${Delta}$ blxR-infected micewas slightly delayed compared to 16M-infected mice (7.4 versus10 mean days to death), indicating that BlxR may be requiredfor full virulence, although loss of BlxR did not fully attenuateB. melitensis virulence in IRF-1^–/– mice.

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FIG. 5. Virulence in IRF-1^–/– mice. Mice were infected with B. melitensis strain 16M and isogenic vjbR and blxR mutants (1 x 10⁷ CFU/mouse intraperitoneally; n = 7 for 16M; n = 8 for 16M ${Delta}$ vjbR and 16M ${Delta}$ blxR). The mice were monitored daily.

Real-time in vivo imaging was used to examine the disseminationof the mutants within the host. The vjbR and blxR genes weredeleted from the constitutively bioluminescent B. melitensisstrain GR023 (47) by gene replacement. The resultant B. melitensisstrains ARL01, ARL02, and GR023 were used to infect IRF-1^–/–mice as described above. The mice were imaged every 2 days usingan in vivo imaging system (Xenogen). Dissemination of the wild-typebioluminescent strain was consistent with previously publishedreports for this strain in IRF-1^–/– mice (47, 48),and dissemination of the blxR mutant (ARL02) was similar tothat of the wild type (GR023) (Fig. 6A and B). By day 3, bioluminescencewas visible in the upper abdominal cavity, indicating a bacterialload in the liver, and in the paws and submandibular area. Incontrast, the vjbR mutant (ARL01) did not disseminate from theinjection site during the first week of infection (Fig. 6C).Although bacterial bioluminescence was visible at the injectionsite from day 1 and in the paws and submandibular area fromthe second week of infection, bioluminescence was not detectedin the upper abdominal cavity.

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FIG. 6. Dissemination in IRF-1^–/– mice. Mice were infected with 1 x 10⁷ CFU/mouse bioluminescent B. melitensis strain GR023 or an isogenic deletion mutant, ARL01 (GR023 ${Delta}$ vjbR) or ARL02 (GR023 ${Delta}$ blxR), and imaged every 2 days beginning on day 1 (immediately postinfection). The numbers indicate days postinfection. Mice infected with GR023 and GR023 ${Delta}$ blxR died 7 days postinfection.

Spleens taken from two 16M ${Delta}$ vjbR-infected animals on day 16 contained2,500 and <100 CFU/spleen, confirming that bacterial numberswere low. The difference in pathogenicity of the two mutantstrains suggests that there are differences between the regulatorypathways of the VjbR and BlxR proteins that play an importantrole in vivo.

DISCUSSION

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DISCUSSION

The identification of a second quorum-sensing regulatory proteinsuggests a greater level of complexity to the Brucella quorum-sensingnetwork than has been previously proposed. While BlxR and VjbRare both involved in regulation of the VirB type IV secretionsystem and flagella, microarray analysis identified other systemsthat may be involved in the quorum-sensing network. They includenine transcriptional-regulatory proteins and seven proteinspredicted to be involved in cell envelope biogenesis. Althoughthe targets of the transcriptional-regulatory proteins are currentlyunidentified, the lysR family transcriptional regulator encodedat locus BMEI1573 is known to be involved in virulence in mice(21). BMEI1573 is located near genes for purine catabolism andmay be involved in their regulation. Another gene known to beinvolved in pathogenicity was identified among the cell envelopebiogenesis proteins. BacA (BMEI1553) is involved in very long-chainfatty acid modification of lipid A (17) and has been shown toplay a role in the persistence of infection (34). These microarrayresults, combined with the very different effects of vjbR andblxR deletions on in vivo dissemination and pathogenicity, suggestthat the quorum-sensing network of Brucella regulates numeroussystems associated with host-pathogen interaction. However,much of the network remains to be elucidated.

Our data raise questions regarding the regulation of the typeIV secretion system in broth culture versus macrophage infection.It was previously reported that the VirB8 protein was undetectablein a VjbR mutant during growth in broth, and it was suggestedthat the phenotype of the VjbR mutant was due to loss of thetype IV secretion complex (13). Although virB transcriptionwas dependent on both the BlxR and VjbR proteins, deletion ofeither regulatory-protein gene did not produce a phenotype consistentwith complete loss of type IV secretion during macrophage infection.Intracellular bacterial counts of 16M ${Delta}$ blxR and 16M ${Delta}$ vjbR increasedsteadily between 6 and 48 h at a slightly lower rate than thatof wild-type 16M. The numbers of intracellular bacteria werenot significantly different at 24 h postinfection. However,by 48 h, the intracellular bacterial counts of 16M ${Delta}$ blxR were0.96 log units lower than those of 16M, and the intracellularbacterial counts of 16M ${Delta}$ vjbR were 1.34 log units lower than thoseof 16M. These results are consistent with previously publishedreports for a vjbR mutant B. melitensis strain at 48 h postinfection(13, 56). However, previously published results for the growthof virB mutant B. melitensis are considerably different (46).The virB mutant exhibited a continuing drop in intracellularnumbers after the initial decrease, reaching 4 log units lowerthan the wild-type 16M by 48 h postinfection.

A lower level of virB transcription in the mutants may stillallow assembly of sufficient functional type IV secretion complexesfor correct trafficking of the Brucella-containing vacuole inearly infection. However, it is possible that the level of attenuationof virB expression observed in the regulatory-gene mutants grownin broth is not representative of quorum-sensing regulationduring macrophage infection. The VirB proteins are expressedconstitutively in B. melitensis during growth in rich mediabut are upregulated by incubation at pH 4.5 (50). The environmentwithin the phagocytic vacuole is nutritionally poor (38, 40),and survival within the macrophage involves exposure to manystresses, including transient low pH (2, 3). Therefore, generegulation may be much different within macrophages than duringgrowth in rich medium.

Although the effects of the vjbR and blxR deletions on intracellulargrowth of B. melitensis were similar, the in vivo effects ofthese deletions were strikingly different. The vjbR mutant failedto disseminate early in infection and was fully attenuated inIRF-1^–/– mice. In contrast, the blxR deletion onlydelayed the death of infected mice compared to infection withwild-type B. melitensis 16M and did not affect dissemination.Overall, these observations suggest that the two regulatoryproteins are not redundant in function. Although the regulatorynetworks are convergent, their different contributions to pathogenesisdemonstrate that certain elements of the two networks are independent.

An autoinducer binding domain mutation in VjbR rendered B. melitensisunresponsive to the C12-HSL autoinducer (56), demonstratingthat VjbR responds to C12-HSL, but also suggesting that BlxRdoes not. The interaction of heterologous LuxR homologs hasbeen reported in Erwinia carotovora, where ExpR1 and ExpR2 actcooperatively to repress the negative regulator RsmA in thepresence of autoinducer signal (53). ExpR1 and ExpR2 bind preferentiallyto different autoinducer molecules, allowing the quorum-sensingsystem to respond to multiple signals (53). In the quorum-sensingpathway of Brucella, loss of either protein is sufficient forsuppression of the type IV secretion system and flagellar genes,suggesting that the two transcriptional regulators may providea way for genes at the intersection of the regulatory pathwaysto be suppressed in response to different environmental stimuli.

ACKNOWLEDGMENTS

This work was supported in part by the following grants: NIH/NIAIDRCE for Biodefense and Emerging Infectious Diseases DevelopmentalProjects grant 1-U54-AI-057153, BARD US-3829-06, NIH 1-R01-AI-073558-01,and NIH 1-R21-AI-070229.

FOOTNOTES

* Corresponding author. Mailing address: Department of Pathobiological Sciences, University of Wisconsin—Madison, 1656 Linden Dr., Madison, WI 53706. Phone: (608) 262-0661. Fax: (608) 262-5111. E-mail: arl{at}svm.vetmed.wisc.edu

Published ahead of print on 29 February 2008.

Supplemental material for this article may be found at http://jb.asm.org/.

REFERENCES

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