Multiple Roles for Bordetella Lipopolysaccharide Molecules during Respiratory Tract Infection

doi:10.1128/IAI.68.12.6720-6728.2000

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Infection and Immunity, December 2000, p. 6720-6728, Vol. 68, No. 12
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Multiple Roles for Bordetella Lipopolysaccharide Molecules during Respiratory Tract Infection

Eric T. Harvill,¹^,^* Andrew Preston,² Peggy A. Cotter,¹ Andrew G. Allen,² Duncan J. Maskell,² and Jeff F. Miller¹

Department of Microbiology and Immunology, University of California Los Angeles School of Medicine, Los Angeles, California 90095-1747,¹ and Centre for Veterinary Science, Department of Clinical Veterinary Medicine, University of Cambridge, Cambridge CB3 OES, United Kingdom²

Received 20 April 2000/Returned for modification 6 June 2000/Accepted 4 August 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Bordetella pertussis, Bordetella parapertussis, and Bordetella bronchiseptica are closely related subspecies that cause respiratorytract infections in humans and other mammals and express manysimilar virulence factors. Their lipopolysaccharide (LPS) moleculesdiffer, containing either a complex trisaccharide (B. pertussis),a trisaccharide plus an O-antigen-like repeat (B. bronchiseptica),or an altered trisaccharide plus an O-antigen-like repeat (B.parapertussis). Deletion of the wlb locus results in the lossof membrane-distal polysaccharide domains in the three subspeciesof bordetellae, leaving LPS molecules consisting of lipid A andcore oligosaccharide. We have used wlb deletion ( $Delta$ wlb) mutantsto investigate the roles of distal LPS structures in respiratorytract infection by bordetellae. Each mutant was defective comparedto its parent strain in colonization of the respiratory tractsof BALB/c mice, but the location in the respiratory tract andthe time point at which defects were observed differed significantly.Although the $Delta$ wlb mutants were much more sensitive to complement-mediatedkilling in vitro, they displayed similar defects in respiratorytract colonization in C5^/ mice compared with wild-type (wt) mice, indicating that increasedsensitivity to complement-mediated lysis is not sufficient toexplain the in vivo defects. B. pertussis and B. parapertussis $Delta$ wlb mutants were also defective compared to wt strains in colonizationof SCID-beige mice, indicating that the defects were not limitedto interactions with adaptive immunity. Interestingly, the B.bronchiseptica $Delta$ wlb strain was defective, compared to the wt strain,in colonization of the respiratory tracts of BALB/c mice beginning1 week postinoculation but did not differ from the wt strain inits ability to colonize the respiratory tracts of B-cell- andT-cell-deficient mice, suggesting that wlb-dependent LPS modificationsin B. bronchiseptica modulate interactions with adaptive immunity.These data show that biosynthesis of a full-length LPS moleculeby these three bordetellae is essential for the expression offull virulence for mice. In addition, the data indicate that thedifferent distal structures modifying the LPS molecules on thesethree closely related subspecies serve different purposes in respiratorytract infection, highlighting the diversity of functions attributableto LPS of gram-negativebacteria.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Bordetellae are gram-negative bacteria that cause respiratory tract infections in mammals. Bordetella pertussis infects onlyhumans, causing whooping cough (pertussis) in unvaccinated childrenand a milder coughing illness in adults. B. parapertussis alsoinfects humans and causes a similar, albeit less severe, disease.B. bronchiseptica infects a variety of four-legged mammals, causingatrophic rhinitis in pigs, kennel cough in dogs, and snufflesin rabbits. Most B. bronchiseptica infections, however, are asymptomatic(8). Very small numbers of B. bronchiseptica organisms aresufficient to establish persistent infection in laboratory animalsincluding rabbits, rats, and mice, allowing this subspecies tobe used as a model for studies of naturally occurring host-pathogeninteractions (1, 9, 14, 15). These three Bordetellasubspecies are very closely related and express a similar setof virulence factors under the regulatory control of the BvgAStwo-component system (24, 25). Virulence factors conservedbetween them, such as the putative adhesins filamentous hemagglutinin(FHA), pertactin, and fimbriae and the adenylate cyclase toxin,are likely to perform functions required by all three subspeciesfor successful respiratory tract colonization (8).

Thus far, major phenotypic differences between bordetellae have not been shown to result from the presence or absence of pathogenicityislands, bacteriophage genomes, transposable elements, or plasmids.Instead, several Bvg-regulated loci found in the genomes of thesethree subspecies are differentially expressed. Examples includethe genes and operons that encode a motility apparatus (2,3), the pertussis toxin (7), and possibly a type III secretionsystem (28, 29). These differentially expressed factors arelikely to contribute to subspecies-specific characteristics suchas host specificity and the ability to cause pathology and topersist.

The lipopolysaccharide (LPS) molecules expressed on the surface of B. pertussis, B. parapertussis, and B. bronchiseptica alsodiffer substantially (4, 5, 17, 23). The observationthat LPS structures are regulated by the BvgAS virulence controlsystem suggests that these molecules play a role in respiratorytract infection (16, 17). B. pertussis LPS resolves as twobands when separated by sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE); these bands are designated bandsA and B. Band B (Fig. 1) is composed of lipid A and a branched-chaincore oligosaccharide. Addition of a trisaccharide to the bandB form creates a larger LPS molecule (actually a lipooligosaccharide),referred to as band A (composed of band B plus trisaccharide).B. bronchiseptica expresses LPS molecules that are very similarantigenically and electrophoretically to B. pertussis bands Aand B, as well as a form containing an O-antigen-like homopolymerof 2,3-dideoxy-2,3-di-N-acetylgalactosaminuronic acid (2,3-di-NAcGalA),primarily in the Bvg phase (12). B. parapertussis expresses a faster-migrating minimalmolecule (band B'), as well as a large molecule containing thesame O-antigen-like structure as B. bronchiseptica, and does notexpress the trisaccharide.

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FIG. 1. (A) Diagram depicting the genetic organization of the wlb locus. The locus consists of 12 genes, wlbA to wlbL, that are required for expression of band A LPS (B). The locus is flanked on one side by Bvg accessory factor (baf) and waaA and waaC, which encode the LPS biosynthesis functions 2-keto-3-deoxyoctulosonic acid transferase and heptosyltransferase, respectively. In B. bronchiseptica and B. parapertussis, the other side is flanked by the LPS O-antigen biosynthetic locus (23). In B. pertussis, this locus has been replaced by an insertion sequence. In the $Delta$ wlb mutants, the wlb locus has been deleted (as indicated in the diagram) and replaced by an antibiotic resistance cassette. (B) Schematic diagram of Bordetella LPS, as elucidated for B. pertussis strain 1414 (17). Band B, as viewed by SDS-PAGE (C), is composed of lipid A and a core containing several charged sugars including galactosaminuronic acid, glucuronic acid, and glucosamine. The wlb locus is required for the band B structure to be further substituted by a trisaccharide comprising N-acetylglucosamine (GlcNAc), 2,3-dideoxy-2,3-di-N-acetylmannosaminuronic acid (2,3-diNAcManA), and N-acetyl-N-methylfucosamine (FucNAcMe) to form band A, the predominant LPS form expressed by B. pertussis. B. parapertussis expresses a smaller core, as suggested by the faster-migrating band B, and contains a mutated wlbH, which decreases the efficiency of GlcNAc transfer to the LPS, resulting in a truncated band A (14, 19). On wt B. parapertussis, virtually all band A LPS is further substituted by O antigen and thus a distinct band A is not seen. Both B. bronchiseptica and B. parapertussis synthesize a polymeric O antigen reported to consist of 2,3-dideoxy-2,3-di-N-acetylgalactosaminuronic acid (18). The attachment site for the O antigen is in the core but has not been precisely determined. 2,3-di-NAcGalA, 2,3-dideoxy-2,3-di-N-acetylgalactosaminuronic acid; GlcNAc, N-acetylglucosamine; ManA2,3-diNAc, 2,3-dideoxy-2,3-di-N-acetylmannosaminuronic acid; FucNAcMe, N-acetyl-N-methylfucosamine; GlcN, glucosamine; GalNA, galactosaminuronic acid; Glc, glucose; Hep, L-glycero-D-mannoheptose; GlcA, glucuronic acid; KDO, 2-keto-3-deoxyoctulosonic acid. (C) SDS-PAGE followed by silver staining of LPS prepared from wt B. pertussis (lanes 1 and 7), B. pertussis $Delta$ wlb (lanes 2 and 8), wt B. bronchiseptica (lanes 3 and 9), B. bronchiseptica $Delta$ wlb (lanes 4 and 10), wt B. parapertussis (lanes 5 and 11), and B. parapertussis $Delta$ wlb (lanes 6 and 12). Bacteria were grown in the presence or absence of MgSO₄, as indicated, to produce Bvg or Bvg⁺ bacteria, respectively.

The wlb gene cluster, composed of 12 genes, is required for biosynthesis and addition of the trisaccharide in band A of B.pertussis and B. bronchiseptica and the O-antigen-like repeatin B. bronchiseptica and B. parapertussis (4, 6). Strainscontaining a wlb deletion mutation ( $Delta$ wlb) express only the smallestform of LPS that naturally occurs on these cells, band B on B.pertussis and B. bronchiseptica and band B' on B. parapertussis.The presence of these structurally diverse LPS molecules in otherwiseclosely related bacteria provides an opportunity to investigatethe roles of these structures in infection. Here we have comparedthe wild-type (wt) and $Delta$ wlb strains of each subspecies in mouserespiratory tract infection models. All three mutants were defectivein colonization of the respiratory tracts of BALB/c mice, buteach was defective in different respiratory organs and/or at differentperiods during infection. Immunocompromised mice were used toinvestigate potential interactions between LPS structures andspecific aspects of host immunity. Together, these results suggestthat the distal structures of the LPS molecules of these threesubspecies play different roles in infection. In B. pertussisthey are required for efficient nasal colonization. In B. parapertussisthey are required for initial colonization of the lungs. In B.bronchiseptica they are required for extended survival in thelower respiratory tracts of normal mice but not mice lacking adaptiveimmunity, suggesting that these structures are involved in resistingadaptive immuneresponses.

	MATERIALS AND METHODS

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Bacteria. Bacteria were maintained on Bordet-Gengou (BG) agar (Difco), inoculated into Stainer-Scholte broth at optical densities of0.1 or lower, and grown to mid-log phase at 37°C on a roller drumfor assays and inoculations. For Bvg phase cultures, MgSO₄ was added to a final concentration of 40mM. Wild-type (wt) strains (BP536, RB50, and CN2591) and the $Delta$ wlbderivatives of these three Bordetella subspecies have been describedpreviously (4).

LPS preparation and SDS-PAGE. LPS was purified, using a modification of the method of Hitchcock and Brown (6, 16), from bacteria grown on BG agar plateswith 15% defibrinated blood and supplemented with 200 µg of streptomycinper ml. LPS was analyzed using the PAGE-Tricine buffer systemby method of Lesse et al. (18). Silver staining was performedby the method of Tsai and Frasch (22).

Animal experiments. Female BALB/c mice, 4 to 6 weeks old, were obtained from Charles River Laboratories. SCID-beige mice were obtained from Universityof California Los Angeles facilities. C5^/ mice (B10.D2-H2^dH2-T18^cHc⁰/nSnJ) and congenic controls (B10.D2-H2^dH2-T18^cHc¹/nSnJ) were obtained from Jackson Laboratory. Mice lightly sedatedwith halothane were inoculated with the indicated dose of bacteriaby pipetting either 5 or 50 µl of the inoculum onto the tip ofthe external nares. For time course experiments, groups of fouranimals were sacrificed on day 0, 3, 5, 7, 14, 21, 28, or 50 postinoculation.Colonization of various organs was quantified by homogenizingeach tissue in phosphate-buffered saline (PBS), plating aliquotsonto BG-blood agar, and counting colonies after 2 (B. bronchiseptica),3 (B. parapertussis) or 4 (B. pertussis) days of incubation at37°C. For the production of survival curves, after the progressionof disease became clear, moribund animals were euthanized to preventunnecessary suffering. Animals were handled in accordance withinstitutional guidelines. Statistical significance was determinedusing an unpaired ttest.

Serum-killing assays. Bordetella-free rabbits were obtained from Charles River Laboratories, and their serum was confirmed to be free of Bordetella-specificantibodies by enzyme-linked immunosorbent assay and a Westernimmunoblot assay (data not shown). Immune serum was obtained fromrabbits inoculated with B. bronchiseptica and colonized for 6months (14). The serum was maintained complement active andwas frozen in single-use aliquots at $-$ 80°C. Bacteria were grownin Stainer-Scholte broth to mid-log phase and diluted in PBS to100 CFU/µl. Serum was thawed on ice, and 90 µl of serum, heat-killedserum, or PBS was mixed with 10 µl of PBS containing 1,000 CFUof bacteria. The mixture was incubated at 37°C for 1 h. Sampleswere spread on BG agar plates and incubated for 2 to 4 days todetermine bacterialnumbers.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Deletion of the wlb locus results in truncated LPS structures. To examine the effect of deleting the wlb locus on LPS biosynthesis under Bvg⁺ and Bvg conditions, we compared, by silver-stained Tricine-SDS-PAGE,LPS structures of wt and $Delta$ wlb strains grown at 37°C on BG agar(Bvg⁺ conditions) or BG agar with 40 mM MgSO₄ (Bvg conditions). In agreement with previous reports, deletion ofthe wlb locus in B. pertussis resulted in the loss of the slower-migratingband A and the accumulation of the faster-migrating band B, representingthe loss of the terminal trisaccharide (Fig. 1C, lanes 1, 2, 7,and 8) (6). wt B. bronchiseptica expressed molecules that comigratewith bands A and B, as well as slower-migrating molecules thatcontain O-antigen-like repeats (20), which are observed primarilyin the Bvg phase (lanes 3 and 9). Deletion of the wlb locus in B. bronchisepticaresulted in the loss of the slower-migrating forms of LPS andthe accumulation of band B (lanes 4 and 10). B. parapertussislacks band A but expresses a molecule that migrates somewhat fasterthan band B (band B'), as well as a larger form containing O-antigen-likerepeats (lanes 5 and 11) (20). We have previously shown thatdeletion of genes required for O-antigen assembly in B. parapertussisresults in accumulation of a species intermediate in size betweenbands A and B, probably representing the addition of a disaccharideby the wlb genes (20). This molecule is presumably efficientlysubstituted by O-antigen-like repeats in wt bacteria. Deletionof the entire wlb locus in B. parapertussis resulted in slightaccumulation of the faster-migrating band B' and loss of the high-molecular-weightO-antigen-containing species (lanes 6 and 12). Under Bvg⁺ growth conditions, additional bands appeared above bands B andB' in B. bronchiseptica and B. parapertussis wt and $Delta$ wlb strains,indicating that BvgAS-dependent modifications of these moleculesoccur that are not dependent on the presence of the terminal trisaccharideor the O-antigen-like repeat. Together, these data show that inall three subspecies, deletion of the wlb locus resulted in theloss of larger forms of LPS and an apparent accumulation of thesmaller forms, bands B and B'. Because it is possible that changingthe LPS structure could affect other molecules that associatewith or pass through the outer membrane, we extensively characterizedthe $Delta$ wlb mutants in vitro. Deletion of the wlb locus did not affectgrowth rate, colony morphology, hemolysis, or expression of antigenicsurface or secreted proteins as assessed by immunoblotting usingsera from infected animals and serum raised against specific factorsincluding pertactin, FHA, and adenylate cyclase toxin (data notshown). The $Delta$ wlb mutation did not affect FHA-dependent bindingto L2 cells in vitro, indicating that FHA is present and functionalon the surface of these cells (10).

B. bronchiseptica requires wlb-dependent LPS modification for efficient colonization of the trachea and lungs of BALB/c mice. To determine the role of the trisaccharide and O-antigen-like structures of LPS in B. bronchiseptica respiratory tract colonization,BALB/c mice were inoculated intranasally with 5 × 10⁵ CFU of wt or $Delta$ wlb B. bronchiseptica in 50 µl of PBS (Fig. 2).This inoculation regimen consistently delivers approximately 10⁵ CFU to the nasal cavity, 10⁵ CFU to the lungs, and 10³ CFU to the trachea (Fig. 2 to 4, day 0). On subsequent days,B. bronchiseptica was recovered from all three sites at numberslarger than the initial inoculum, indicating that it was ableto colonize and multiply throughout the respiratory tract as wehave previously shown (14). After 1 week the numbers of wt bacteriacolonizing the respiratory tract decreased but bacteria were stillrecovered from both the trachea and the lungs 28 days after inoculation.In contrast, the $Delta$ wlb mutant did not increase in numbers in thetrachea and lungs during the first week and could no longer berecovered from the lower respiratory tract by day 14 postinoculation.At multiple consecutive time points beginning on day 3, the numbersof $Delta$ wlb bacteria were significantly smaller (P < 0.01) than thoseof the wt strain in both the trachea and the lungs. Although defectivein tracheal and lung infection, the $Delta$ wlb strain was indistinguishablefrom the wt strain in colonization of the nasal cavity.

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FIG. 2. The B. bronchiseptica $Delta$ wlb mutant is defective in tracheal and lung colonization in BALB/c mice. Groups of 4-week-old female mice were inoculated with 5 × 10⁵ CFU of either wt B. bronchiseptica or its $Delta$ wlb derivative delivered in a 50-µl volume of PBS into the nares. Data points are presented as mean log₁₀ CFU and standard error. P values are shown where P < 0.02.

B. parapertussis requires wlb-dependent LPS modification for efficient colonization of the trachea and lungs of BALB/c mice. Clinical isolates of B. parapertussis from humans are essentially clonal and appear to have diverged from B. bronchisepticarelatively recently (27). wt B. parapertussis behaved similarlyin most respects to wt B. bronchiseptica in BALB/c mice inoculatedintranasally as above (compare Fig. 2 and 3). By day 3 postinoculation,wt B. parapertussis was recovered from the nasal cavity, trachea,and lungs at numbers larger than the initial inoculum, indicatingthat it was able to colonize and multiply throughout the respiratorytract. After about 5 days, the numbers of wt bacteria began todecrease in all three organs and were below detectable levelsin the trachea and lungs by day 21 and in the nasal cavity byday 50 postinoculation. The B. parapertussis $Delta$ wlb strain was similarto the B. bronchiseptica $Delta$ wlb strain in that it was recoveredat relatively constant numbers in the trachea for the first weekand was absent by the second week. However, the B. parapertussis $Delta$ wlb mutant differed from the B. bronchiseptica mutant in themagnitude of its defect in the lungs observed by day 3 postinoculation.On postinoculation days 3, 5, and 7, the numbers of B. parapertussis $Delta$ wlb bacteria were 1/100 those of the wt strain in the tracheaand 1/10,000 those of the wt strain in the lungs. The B. parapertussis $Delta$ wlb mutant was similar to the B. bronchiseptica $Delta$ wlb mutant inthat it was indistinguishable from the wt strain in colonizationof the nasal cavity.

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FIG. 3. The B. parapertussis $Delta$ wlb mutant is defective in tracheal and lung colonization in BALB/c mice. Groups of 4-week-old female mice were inoculated with 5 × 10⁵ CFU of either wt B. parapertussis or its $Delta$ wlb derivative delivered in a 50-µl volume of PBS into the nares. Data points are presented as mean log₁₀ CFU and standard error. P values are shown where P < 0.02.

B. pertussis requires wlb-dependent LPS modification for efficient colonization of the nose, trachea, and lungs of BALB/c mice. In the mouse model, B. pertussis efficiently colonizes the lungs but is defective, compared to B. bronchiseptica, in persistencein the nasal cavity (14). Although the wt B. pertussis strainwas recovered from the nasal cavity, trachea, and lungs at numberslarger than the initial inoculum (Fig. 4, compare days 0 and 3),after a week the numbers of wt bacteria decreased and were belowdetectable levels in the trachea and nose by day 28 postinoculation.On day 28 postinoculation a small number of wt bacteria were recoveredfrom the lungs, but by day 50 none were detected in any of thesites surveyed. The B. pertussis $Delta$ wlb mutant was similar to theB. bronchiseptica and B. parapertussis $Delta$ wlb mutants in that itwas recovered at relatively constant numbers in the trachea forthe first week. In contrast to the B. parapertussis mutant, theB. pertussis $Delta$ wlb mutant multiplied roughly 10-fold in numbersin the lungs during the first few days postinoculation and stayedat that approximate level for 2 weeks before declining and disappearingby day 28. Although neither the B. bronchiseptica nor the B. parapertussis $Delta$ wlb mutants were defective in the nasal cavity of BALB/c mice,the B. pertussis $Delta$ wlb mutant was defective, with bacterial numbersapproximately 1/1,000 those of the wt strain on days 3, 5, and7 and below detectable levels by day 14 postinoculation. The numbersof B. pertussis $Delta$ wlb mutant bacteria were decreased, comparedto the wt strain, in all three organs (P < 0.01 at multiple timepoints) but were most severely defective in colonization of thenasal cavity, a phenotype not observed with $Delta$ wlb mutants of theother two subspecies.

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FIG. 4. The B. pertussis $Delta$ wlb mutant is defective in nasal, tracheal, and lung colonization in BALB/c mice. Groups of 4-week-old female mice were inoculated with 5 × 10⁵ CFU of either wt B. pertussis or its $Delta$ wlb derivative delivered in a 50-µl volume of PBS into the nares. Data points are presented as mean log₁₀ CFU and standard error. P values are shown where P < 0.02.

wlb-dependent LPS modification is required for lethal infection of SCID-beige mice by B. bronchiseptica and B. parapertussis. The decrease in colonization levels throughout the respiratory tracts of BALB/c mice after day 7 postinoculation suggeststhat adaptive immunity is effective, albeit to different extents,against all three subspecies. We have previously used mice deficientin B and T cells (SCID, SCID-beige, and RAG-1 knockout mice) toidentify interactions between bacterial virulence factors andinnate versus adaptive immune responses (14, 15, 28). B.bronchiseptica is highly virulent in SCID, SCID-beige, and RAG-1knockout mice, causing lethal systemic infections. B. pertussisis less virulent and does not kill these animals but persistsfor at least 200 days in the nose, trachea, and lungs (14).To identify potential roles for wlb-dependent LPS modificationsin persistence and virulence, we compared the ability of thesethree Bordetella subspecies and their $Delta$ wlb mutants to infect SCID-beigemice (BALB/c genetic background), which are deficient in B andT cells as well as NK-cell activities. The beige mutation alonedoes not affect B. bronchiseptica infection, but in the contextof SCID mice it speeds the progression of disease (15).

A low-dose, low-volume inoculum of 500 CFU in 5 µl of PBS was delivered to the external nares, and survival was monitoredover time. All six groups of mice remained healthy for 30 days,after which the animals infected with wt B. bronchiseptica beganto display signs of illness such as piloerection, weight loss,hunched stature, listlessness, and, eventually, loss of responsivenessfollowed by death of 100% of the animals between days 40 and 70postinoculation (Fig. 5A) (15). Mice inoculated with the B.bronchiseptica $Delta$ wlb mutant, in contrast, remained healthy formore than 200 days, indicating that wlb-dependent LPS modificationis required for B. bronchiseptica to cause lethal infection inSCID-beige mice. Animals infected with either wt B. pertussis,B. parapertussis, or their $Delta$ wlb mutants remained healthy for morethan 200 days.

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FIG. 5. Survival of SCID-beige mice following inoculation with Bordetella subspecies and their $Delta$ wlb mutants. SCID-beige mice were inoculated with either wt (open symbols) or $Delta$ wlb mutant (solid symbols) B. bronchiseptica (circles), B. parapertussis (triangles), or B. pertussis (squares). Percent survival is presented as a function of time following low-dose, low-volume intranasal inoculation with 500 CFU in a 5-µl PBS droplet (A) or high-dose, high-volume intranasal inoculation with 5 × 10⁵ CFU in 50 µl of PBS (B).

SCID-beige mice were also inoculated with a high-dose high-volume regimen (5 × 10⁵ CFU in 50 µl of PBS), which seeds the entire respiratory tractwith bacteria and deposits approximately 10⁵ CFU in the lungs (Fig. 5B). B. bronchiseptica delivered by thisregimen killed SCID-beige mice with slightly faster kinetics thanthe low-dose regimen did. wt B. parapertussis, which did not killSCID-beige mice following low-dose inoculation, killed SCID-beigemice within 30 days following high-dose inoculation. B. pertussisand all three $Delta$ wlb mutants, however, did not cause lethal infectionsin these immunocompromised mice, even using the high-dose, high-volumeregimen. These results highlight major differences in the virulenceof B. pertussis, B. parapertussis, and B. bronchiseptica in thismodel and show that wlb-dependent LPS modification is requiredfor the virulence of both B. bronchiseptica and B. parapertussisin SCID-beigemice.

Colonization levels in SCID-beige mice. The three $Delta$ wlb mutants differed in the time points and anatomical locations at which they were defective in immunocompetentmice. To determine which, if any, of these colonization defectsmay relate to an ability to resist adaptive immune responses,we inoculated SCID-beige mice by the high-dose, high-volume regimenand determined colonization levels in various organs 25 days postinoculation.wt B. bronchiseptica was recovered at large numbers throughoutthe respiratory tract and at systemic sites including the liversof SCID-beige mice (Fig. 6) (14, 15). The B. bronchiseptica $Delta$ wlb strain was recovered at similar numbers to the wt strainthroughout the respiratory tract but was not recovered from systemicsites such as the liver. Even at 100 and 200 days postinoculation,the B. bronchiseptica $Delta$ wlb strain maintained a high level of colonizationin the respiratory tract but was not recovered from the liveror spleen (data not shown). These data indicate that in SCID-beigemice, wlb-dependent LPS modification is not required for B. bronchisepticacolonization of the respiratory tract, suggesting that the defectof the $Delta$ wlb mutant in the lungs and trachea of BALB/c mice after1 week is a result of B-cell, T-cell, and/or NK-cell function.The B. bronchiseptica wlb locus is, however, absolutely requiredfor systemic spread to the liver and for lethal infection in SCID-beigemice.

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FIG. 6. Colonization of various tissues of SCID-beige mice by wt and $Delta$ wlb strains. Groups of four female 4-week-old SCID-beige mice were inoculated with 5 × 10⁵ CFU in 50 µl of PBS. The mice were sacrificed and the colonization levels in various organs were determined on day 25 postinoculation for B. pertussis strains (Bp) and B. bronchiseptica strains (Bb) and day 21 for B. parapertussis strains (Bpp). Data are presented as mean log₁₀ CFU and standard error. The dashed line represents the lower limit of detection.

SCID-beige mice inoculated with wt B. parapertussis contained large numbers of bacteria throughout the respiratory tract aswell as the liver at 25 days postinoculation (Fig. 6). In BALB/cmice inoculated with the same dose of wt B. parapertussis, thetrachea and lungs were cleared and the nasal cavity was nearlycleared by day 21 postinoculation (Fig. 3). These data indicatethat immune mechanisms present in BALB/c mice but absent fromSCID-beige mice are required to clear B. parapertussis infection.The $Delta$ wlb mutant was only slightly defective, compared to wt B.parapertussis, in colonization of the nasal cavities of SCID-beigemice but was severely defective in colonization of the tracheasand lungs of these animals. The striking defects of the B. parapertussis $Delta$ wlb mutant in the tracheas and lungs of SCID-beige mice and thesimilar defect observed within 3 days postinoculation in BALB/cmice indicate that B. parapertussis wlb-dependent LPS modificationis required for colonization of these sites even in the absenceof adaptive immunity. These data suggest that in B. parapertussisthe wlb-dependent LPS modifications are involved in some aspectof infection other than interactions with adaptiveimmunity.

wt B. pertussis was recovered at large numbers throughout the respiratory tracts of SCID-beige mice 25 days postinoculationbut not elsewhere in these animals (Fig. 6). We have previouslyshown that wt B. pertussis remains at relatively constant levelsthroughout the respiratory tracts of SCID-beige mice for at least200 days but causes no overt signs of disease (14). The B. pertussis $Delta$ wlb mutant was defective, compared to the wt strain, in the noses,tracheas, and lungs of both BALB/c and SCID-beige mice, indicatingthat wlb-dependent LPS structures are required for some functionother than evading the host adaptive immuneresponses.

wlb-dependent LPS modification is required by B. bronchiseptica and B. parapertussis for resistance to killing by naive serum. wt B. bronchiseptica and B. parapertussis, but not their $Delta$ wlb mutants, were able to infect the livers of SCID-beige mice,suggesting that they could survive the antimicrobial activitiesof blood and lymph fluids encountered during transit to the liver.We reasoned that these $Delta$ wlb mutants could be defective in causinglethal systemic disease due to an increased susceptibility toantimicrobial factors in serum. We therefore compared wt and $Delta$ wlbstrains of the three Bordetella subspecies for their survivalin complement-active serum from B. bronchiseptica-free rabbits(naive serum). Bacteria (1,000 CFU) from mid-log-phase liquidcultures, grown under Bvg⁺ phase conditions, were incubated in 100 µl of 90% serum to ensurethat serum components were not limiting. wt B. bronchisepticawas not killed by a 1-h incubation at 37°C in 90% naive serum(Fig. 7). In contrast, the B. bronchiseptica $Delta$ wlb mutant was highlysensitive to naive serum (>99% of bacteria were killed), indicatingthat wlb-dependent LPS modification is required for B. bronchisepticaserum resistance. B. parapertussis was similar to B. bronchisepticain that the wt strain was resistant but the $Delta$ wlb strain was killed(>99%) by naive serum. Unlike the other two subspecies, both wtand $Delta$ wlb B. pertussis strains were killed by naive serum in thisassay.

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FIG. 7. Serum resistance of wt and $Delta$ wlb strains. Bacteria were grown to mid-log phase in Stainer-Scholte broth and diluted in PBS. A total of 1,000 bacteria were incubated at 37°C for 1 h in 100 µl of 90% naive serum. Serum resistance is presented as the percent survival relative to a PBS control. Naive and immune sera are described in Materials and Methods.

Sera from B. bronchiseptica-infected rabbits (immune serum) were shown to contain antibodies recognizing all three Bordetellasubspecies by ELISA and Western analysis (reference 14 and datanot shown). wt B. pertussis and all three subspecies of $Delta$ wlb mutants,which were killed by naive serum, were killed by immune serum,as expected (data not shown). Immune serum also killed wt B. bronchiseptica(>98% killing) and B. parapertussis (>95% killing), which werenot killed by naive serum, suggesting that antibody-mediated complementactivation is responsible for the killing. Similar results wereobtained in multiple experiments with naive sera from mice, rats,and rabbits or immune sera from mice, rats, rabbits, and humans.Inhibition of complement with EDTA or by heat treatment preventedkilling in these assays (data not shown). Together, these dataindicate that wlb-dependent LPS modification is required for resistanceof B. bronchiseptica and B. parapertussis to the alternative complementcascade (naive serum) but is not sufficient for resistance tothe classical pathway of complement (immuneserum).

Complement-deficient mice. The sensitivity of the B. bronchiseptica and B. parapertussis $Delta$ wlb mutants to naive serum may be related to their defectsin the BALB/c infection model. Serum components are present atlow concentrations in normal respiratory fluids but increase inconcentration in response to bacterial infection (13), suggestingthat complement could affect colonization in the mouse model.SCID-beige mice contain normal complement levels, and the B. parapertussis $Delta$ wlb mutant was also defective in colonization of these animals,but the B. bronchiseptica $Delta$ wlb mutant colonized the respiratorytracts of SCID-beige animals to levels similar to those of thewt strain (Fig. 6). These data suggest that the colonization defectof the B. bronchiseptica $Delta$ wlb strain does not involve increasedsensitivity to complement but that the defect of the B. parapertussis $Delta$ wlb mutant may do so. To directly determine if complement-mediatedlysis contributes to control of respiratory tract infection bybordetellae, we compared the wt and $Delta$ wlb strains in congenic mousestrains with and without the ability to express the C5 componentof complement (11, 19), which is required for the assemblyof the membrane attack complex involved in complement-mediatedlysis of gram-negative bacteria. In C5^/ mice, complement activation by classical, alternative, or lectinpathways does not proceed past the point where these three pathwaysconverge at the level of C5 activation prior to membrane attackcomplex formation, so that complement-mediated lysis is abrogated.In vitro, serum from C5^+/+ mice killed B. pertussis and the $Delta$ wlb but not wt B. bronchisepticaand B. parapertussis strains but serum from congenic C5^/ mice did not (data not shown). In vivo, the B. bronchiseptica $Delta$ wlb mutant was defective in colonization of the trachea, comparedto the wt strain, in both C5^+/+ and C5^/ mice on day 5 postinoculation (Fig. 8). Apparently the defectin tracheal colonization is not due to the increased sensitivityof the $Delta$ wlb mutant to complement-mediated killing. Likewise, bothB. pertussis and B. parapertussis $Delta$ wlb mutants showed as greata defect in colonization of C5^/ mice as in C5^+/+ mice, indicating that the defects are not due to increased sensitivityto complement-mediated killing. Interestingly, the B. parapertussis $Delta$ wlb strain, which was severely defective (1/10,000 of wt numbers)in the lungs of BALB/c mice on day 5 (Fig. 3) and SCID-beige mice(BALB/c genetic background) on day 21 (Fig. 6), showed littledefect in the lungs of either C5^+/+ or C5^/ mice (B10.D2 genetic background). These data suggest that thesubstantial defect of the B. parapertussis $Delta$ wlb mutant in BALB/clung colonization is not due to its sensitivity to complement-mediatedkilling but, rather, involves some other host factor that differsbetween mice of these two genetic backgrounds. The $Delta$ wlb mutantsof all three subspecies, compared to their wt parent strains,were at least as defective in C5^/ mice as in C5^+/+ mice, indicating that the role of the wlb locus is not merelyto render the bacteria complement resistant. Some other functionof the wlb-dependent LPS modification is therefore involved inthe observed phenotypes. The $Delta$ wlb strains did not show increasedsensitivity to defensins (data not shown).

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FIG. 8. Bordetella $Delta$ wlb mutants are defective in colonization of the respiratory tracts of complement-deficient mice. Groups of four 6-week-old female C5^+/+ and C5^/ mice were inoculated with 5 × 10⁵ CFU in 50 µl of PBS. Colonization levels were determined in the nose, trachea, and lungs on day 5 postinoculation. Open bars represent wt strains, and solid bars represent $Delta$ wlb strains. Data are presented as mean log₁₀ CFU and standard error. The lower limit of detection is approximately 1.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

LPS structures expressed by gram-negative bacteria have been proposed to contribute to infection by a variety of mechanismsincluding the mediation of adherence to host cells, antigenicvariation, molecular mimicry, and induction of blocking antibodies(21). The LPS structures of Bordetella subspecies are less wellstudied and have not been documented to perform any of these functions,although they are modified in a Bvg-dependent manner, suggestingthat they are involved in infection (26). We have compared B.bronchiseptica, B. parapertussis, and B. pertussis wt and $Delta$ wlbstrains in vitro and in vivo, in normal and immunodeficient mice,to investigate the roles of the distal domains of their LPS moleculesininfection.

All three $Delta$ wlb strains were similarly defective, compared to their wt parent strains, in colonization of the tracheas of BALB/cmice; they failed to increase in numbers in the trachea over thefirst week postinoculation and declined in numbers rapidly inthe second week. Although deletion of the wlb locus increasedthe sensitivity of B. bronchiseptica and B. parapertussis to complement-mediatedkilling in vitro, the $Delta$ wlb mutants were defective in colonizationof the tracheas of C5^/ mice, in which complement-mediated killing is abrogated. Theseresults indicate that complement-mediated lysis was not the onlymechanism involved in the clearance of the $Delta$ wlb strains from thetrachea, although it is possible that opsonization by C3, an eventthat does not require C5, could result in phagocytosis of the $Delta$ wlb strains. Interestingly, loss of distal LPS structures inthe three Bordetella subspecies resulted in different phenotypesin the lungs and nasal cavities of various mice, supporting theview that these structures perform different functions for thesethreeorganisms.

Colonization of the lungs of BALB/c mice by the B. bronchiseptica $Delta$ wlb mutant was not significantly reduced compared to thewt strain until about 7 days postinoculation. The mutant was clearedfrom the lungs by 14 days postinoculation, whereas the wt strainwas not cleared until day 50. Therefore, wlb-dependent LPS modificationis not required for initial infection of the lungs by B. bronchisepticabut appears to contribute to persistence at a time consistentwith the development of adaptive immune responses. In mice lackingadaptive immunity, the $Delta$ wlb mutant colonized the respiratory tractto similar levels to those of the wt strain, supporting the viewthat wlb gene products are primarily involved in resisting clearanceby adaptive immune functions. Together, these data suggest thatwlb-dependent LPS structures are required for B. bronchisepticato resist clearance by the adaptive immune response. In preliminaryexperiments in µMT(C57BL/6-Igh-6^tm1Cgn) mice, lacking B cells, both wt and $Delta$ wlb strains persist in thetrachea and lungs, consistent with the primary role of wlb-dependentLPS modification being modulation of antibody-mediated bacterialclearance (data not shown). The inability of the $Delta$ wlb mutant tocause systemic infections and kill mice lacking adaptive immunity(SCID-beige mice) may be due to its increased sensitivity to serumcomplement-mediated killing compared to wt B. bronchiseptica.Although B. bronchiseptica is not believed to invade cells ortissues during natural infection, these observation may be relevantto aspects of infection that are not yetunderstood.

The role of distal LPS structures in B. parapertussis and B. pertussis infections appears to be substantially different fromthat in B. bronchiseptica. The B. parapertussis $Delta$ wlb mutant wasrecovered from the lungs of BALB/c mice at 1/10,000 the numbersof the wt strain by day 3 postinoculation. A defect of similarmagnitude was observed for this mutant in the lungs of SCID-beigemice. These data indicate that, in contrast to B. bronchiseptica,wlb-dependent LPS modification is required for B. parapertussisto colonize the lungs of mice even in the absence of adaptiveimmunity. Interestingly, the dramatic defect of the B. parapertussis $Delta$ wlb mutant in the lungs of BALB/c and SCID-beige mice (BALB/cgenetic background) was not observed in C5^+/+ or C5^/ mice (B10.D2 genetic background). It is possible that wlb-dependentLPS modification protects bacteria from an antimicrobial activitypresent in BALB/c mice but absent in B10 mice. Alternatively,wlb-dependent LPS modification could be directly or indirectlyrequired for binding to a receptor in BALB/c mice. B10 mice couldexpress an alternative receptor(s), relieving the need for wlb-dependentLPS modification for lung infection in theseanimals.

Only B. pertussis required the wlb locus for efficient colonization of the nasal cavity. The B. pertussis $Delta$ wlb mutant wasrecovered from that organ at 1/1,000 the numbers of the wt strain.This defect was observed in the nasal cavities of BALB/c, SCID-beige,C5^+/+, and C5^/ mice, indicating that the defect did not involve complement-mediatedkilling, adaptive immunity, or other interstrain differences betweenthese animals. Interestingly, the B. pertussis $Delta$ wlb mutant wasrecovered from the tracheas and lungs of BALB/c mice at smallernumbers than the wt strain was on days 3, 5, and 7 postinoculationbut thereafter the two strains were indistinguishable in thesetissues. In contrast, the B. bronchiseptica $Delta$ wlb mutant was defectiveonly on or after day 7 postinoculation and the B. parapertussis $Delta$ wlb mutant was severely defective at all time points from day3 postinoculationonward.

The three Bordetella subspecies examined here are very closely related and are believed to have diverged from a common ancestorrelatively recently (27). They maintain similar habitats, therespiratory tracts of mammals, and appear to differ primarilyin their host ranges and in their ability to cause either acutedisease with moderate to severe pathology or chronic infectionwith moderate to no pathology. Many of the factors involved ininfection are highly conserved among the three subspecies, aswould be expected for molecules that perform a function requiredfor respiratory tract colonization in general. In contrast, theLPS structures of these three organisms appear to be substantiallydifferent. Although this could indicate that these structureshave diverged because they are not important in infection, thedata presented here show that they are critical to efficient respiratorytract colonization. The more likely explanation for these observationsis therefore that these structures have evolved to meet the specificneeds of these three organisms. For B. bronchiseptica, distalLPS structures are apparently required only when adaptive immunityhas been generated, suggesting that they contribute to the persistenttracheal and lung infections characteristic of this subspecies.B. pertussis and B. parapertussis, which have independently shiftedtheir host ranges to infect humans but do not cause persistentinfections, appear to have modified their distal LPS structuresto perform different roles. These functions are still requiredin SCID-beige mice, indicating that they are not limited to interactionswith adaptive immunity. For B. pertussis, distal LPS structuresare required for colonization of the nasal cavity of every mousestrain examined. For B. parapertussis, the $Delta$ wlb strain was severelydefective (1/10,000 of wt levels) in colonization of the lungsof some mouse strains but not others. Together, these data suggestthat the different distal structures modifying the LPS moleculeson these three closely related subspecies serve different purposesin respiratory tract infection. Exchange of the genes involvedin LPS assembly between the three subspecies will elucidate theirroles in either common properties of respiratory tract colonizationor subspecies-specific characteristics such as persistence, hostspecificity, andvirulence.

	ACKNOWLEDGMENTS

This work was supported by USDA grant 960-1856 (to E.T.H.), USDA grant 1999-02298 (to J.F.M.), NIH grant AI38417 (to J.F.M.),NIH grant AI43986 (to P.A.C.), Wellcome Trust Project Grant 045666(to D.J.M.), and Wellcome Trust Programme Grant 054588 (to D.J.M.).

	FOOTNOTES

^* Corresponding author. Present address: Department of Veterinary Science, Pennsylvania State University, 125 Henning Building,University Park, PA 16802. Phone: (814) 863-8522. Fax: (814) 863-6140.E-mail: harvill{at}psu.edu.

Editor: D. L. Burns

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