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Infection and Immunity, August 2000, p. 4673-4680, Vol. 68, No. 8
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Role of Phosphoglucomutase of Bordetella
bronchiseptica in Lipopolysaccharide Biosynthesis and
Virulence
Nicholas P.
West,1
Heidrun
Jungnitz,2
John T.
Fitter,1,
Jason D.
McArthur,1
Carlos A.
Guzmán,2 and
Mark J.
Walker1,*
Department of Biological Sciences, University
of Wollongong, New South Wales, Australia,1 and
Department of Microbial Pathogenicity and Vaccine Research,
Division of Microbiology, GBF-National Research Centre for
Biotechnology, Braunschweig, Germany2
Received 8 November 1999/Returned for modification 3 January
2000/Accepted 5 May 2000
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ABSTRACT |
The phosphoglucomutase (PGM)-encoding gene of Bordetella
bronchiseptica is required for lipopolysaccharide (LPS)
biosynthesis. An insertion mutant of the wild-type B. bronchiseptica strain BB7865 which disrupted LPS biosynthesis was
created and characterized (BB7865pgm). Genetic analysis of
the mutated gene showed it shares high identity with PGM genes of
various bacterial species and forms part of an operon which also
encompasses the gene encoding phosphoglucose isomerase. Functional
assays for PGM revealed that enzyme activity is expressed in both
bvg-positive and bvg-negative strains of
B. bronchiseptica and is substantially reduced in
BB7865pgm. Complementation of the mutated PGM gene with
that from BB7865 restored the wild-type condition for all
phenotypes tested. The ability of the mutant BB7865pgm to
survive within J774.A1 cells was significantly reduced at 2 h
(40% reduction) and 24 h (56% reduction) postinfection.
BB7865pgm was also significantly attenuated in its ability
to survive in vivo following intranasal infection of mice, being
effectively cleared from the lungs within 4 days, whereas the wild-type
strain persisted at least 35 days. The activities of superoxide
dismutase, urease, and acid phosphatase were unaffected in the
PGM-deficient strain. In contrast, the inability to produce wild-type
LPS resulted in a reduced bacterial resistance to oxidative stress and
a higher susceptibility to the antimicrobial peptide cecropin P.
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INTRODUCTION |
Of the Bordetella genus,
Bordetella bronchiseptica is the principle effector of
respiratory disease in a wide range of mammals (16).
However, B. bronchiseptica only rarely infects humans (18, 46, 54). B. bronchiseptica is credited as
being the primary etiological component of tracheobronchitis in dogs
from as early as 1910 (14) and is known to be associated
with atrophic rhinitis, a common bronchial affliction of swine
(40). B. bronchiseptica infections are mediated
by the controlled expression of a number of virulence factors, such as
the adhesin filamentous hemagglutinin (10) and the toxins
adenylate cyclase hemolysin and dermonecrotic toxin (7, 50).
The regulation of these virulence determinants is under the control of
a two-component signal transduction system known as the
Bordetella virulence gene (bvg) locus. Genetic
control is observed in response to environmental conditions such as
temperature and chemical modulators, i.e., sulfate anions (1,
27).
Lipopolysaccharide (LPS) is a highly toxic and immunogenic molecule
that constitutes a major component of the cell membranes in
gram-negative bacteria (37). LPS has now emerged as having an integral role in the infection process, being responsible for resistance to serum, antibiotics (39), and naturally
occurring antimicrobial peptides termed defensins (5). The
role of LPS as an important adhesin molecule also seems likely;
however, its role in the pathogenesis process still remains largely
unknown. It has recently been stated that the LPS of some strains of
B. bronchiseptica is regulated by the bvg system
(48).
The LPS of the related bacterium Bordetella pertussis
displays a structure that generally typifies that of nonenteric
bacteria. This consists of a lipid A region anchored in the cell
membrane, being linked to a branched oligosaccharide domain
constituting the core, by a single keto-deoxyoctulosonic acid (2,
17, 48). These glycolipids lack long repeating oligosaccharide
units as are found in the Enterobacteriaceae and are
therefore sometimes termed lipooligosaccharides (37).
B. bronchiseptica and Bordetella parapertussis
do, however, produce an O-antigen of a single sugar polymer, consisting
of 2,3-dideoxy-di-N-acetylgalactosaminuronic acid (4,
13). There is considerable variation in glycolipid structure
within the genus Bordetella (48).
Two distinct bands, i.e., band A and band B (35), are
evident upon electrophoresis of purified B. pertussis LPS.
Band B consists of the core region of the molecule, whereas the
slower-migrating band A is this same core with the addition of a distal
trisaccharide comprised of N-acetylglucosamine,
N-acetyl-N-methylfucosamine, and
2,3-di-deoxy-2,3-di-N-acetylmannosaminuronic acid
(2). It is understood that all three elements of the LPS
molecule, i.e., lipid A, core, and O-antigen, are required for
virulence of Escherichia coli (23). Viability of
the organism is not necessarily disrupted by the absence of the
O-antigen or several of the core sugars, but the keto-deoxyoctulosonic
residues of the core and the lipid A are essential for growth
(23). So important is the lipid A component of LPS to the
viability of the cell that it has been described as a suitable
pharmaceutical target (34).
A gene cluster for LPS production in B. pertussis and
B. bronchiseptica has been identified, and the
probable functions of the gene products have been discussed (2,
36); however, the role of LPS in the B. bronchiseptica
infection process remains largely undescribed. We describe here an LPS
mutant of B. bronchiseptica, designated
BB7865pgm, resulting from an insertion in the
phosphoglucomutase (PGM)-encoding gene. This gene appears to be
organized into an operon with the phosphoglucose isomerase
(PGI)-encoding gene. Regulation of pgm is constitutive and
is therefore controlled independently of the bvg system.
Loss of PGM activity due to insertional mutation of the gene resulted
in a truncation of the LPS. Resistance to oxidative stress was
reduced in the mutants as was the ability to resist cecropin P. Finally, BB7865pgm was unable to survive within the mouse
macrophage-like cell line J774.A1 or colonize mouse lungs following
intranasal inoculation.
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MATERIALS AND METHODS |
Bacterial strains, plasmids, and growth conditions.
B.
bronchiseptica wild-type strain BB7865 and its isogenic
bvg-negative derivative BB7866 have been characterized
in a previous study (33). E. coli strain
SM10
pir (32) containing pUTmini-Tn5 lacZ1
(11) was used in mutagenesis experiments. E. coli
JM109 (55) was used in standard cloning experiments while
E. coli 294 Rifr (51) was used for
cosmid cloning. B. bronchiseptica strains were grown on
Bordet Gengou (BG) agar (Difco) containing defibrinated horse
blood (10%, vol/vol) and Stainer and Scholte medium (SS-X) (45) or a modulating version of SS-X containing 40 mM
MgSO4 replacing NaCl (SS-C). Liquid cultures were also
grown in SS-X or SS-C. E. coli strains were grown on Z agar
(51) or in LB broth (41). The following
antibiotics were used at the indicated concentrations: cephalexin, 50 µg/ml; kanamycin, 50 µg/ml; ampicillin, 100 µg/ml; rifampin, 100 µg/ml; nalidixic acid, 50 µg/ml; trimethoprim, 50 µg/ml.
Isopropyl-
-D-galactopyranoside (IPTG) (0.04 mM) and 5-bromo-4-chloro-3-indolyl--D-galactopyranoside (X-Gal)
(0.004%, wt/vol) were used where appropriate.
Mini-transposon mutagenesis.
Conjugation between B. bronchiseptica BB7866 and the donor E. coli SM10pir
containing the suicide plasmid (pUTmini-Tn5 lacZ1) was
performed. Equal amounts of each bacterial strain were mixed in 0.7%
saline and plated onto BG agar. Transconjugants were selected from the
resultant growth on SS-X at 37°C containing cephalexin, kanamycin,
X-Gal, and IPTG.
In vivo chromosome transfer.
The method by which the
mini-transposon was transferred from BB7866pgm to the
homologous location on the wild-type chromosome (BB7865pgm)
was that described by Smith and Walker (44). E. coli Q358(pR715::Tn813) was mated with
BB7866pgm. This resulted in the plasmid being introduced
into BB7866pgm. A permanent cointegration of the plasmid
into the chromosome occurred, catalyzed by the transposase encoded by
Tn813. This recombinant strain of BB7866pgm (Tpr Kmr) was then conjugally mated with BB7865
(Nalr Rifr). Chromosome transfer is then
promoted by the integrated tra genes of pR751, and the
recipient strain thus received the original Kmr cassette
following homologous recombination.
DNA manipulations.
Plasmid DNA was extracted from host cells
using midi-prep columns in accordance with manufacturer's instructions
(Qiagen). Chromosomal DNA was extracted according to the method of
Priefer et al. (38). Restriction endonuclease digestion and
agarose gel electrophoresis were conducted using standard methods
(41). Cosmid cloning was achieved via the packaging of
recombinant cosmids (pHC79) (21) containing chromosomal DNA
fragments into lambda phage Max Plax kits (Epicentre Technologies) and
subsequent transduction into E. coli 294 Rifr
cells. Desired clones were selected and screened by colony
hybridization. Chromosomal DNA for Southern hybridization was
transferred to positively charged nylon membranes by way of alkaline
transfer. Probe DNA was either digoxigenin labeled (Roche) or
radiolabeled with [
-32P]dATP using a nick translation
kit (Gibco BRL). Blots were probed under stringent conditions (65°C
hybridization). Automated DNA sequencing was performed on plasmid DNA
with a Perkin Elmer ABI Prism 377 DNA sequencer. Reactions were
performed with Perkin Elmer BigDye terminator cycle sequencing ready
reaction mix. Contiguous sequences were constructed using AutoAssembler
software (Perkin-Elmer) and aligned with sequences in the GenBank
database located at the Australian National Genomic Information Service
by utilizing the Blastp algorithm.
PGM and phosphomannomutase (PMM) assays.
Crude lysates were
prepared from the strains to be tested for mutase activity using the
modified method from Sandlin and Stein (42). Cultures of the
strains were grown in either SS-X at 37°C or SS-C at 25°C to late
logarithmic phase and then centrifuged. The resultant pellets were
resuspended in 10 ml of sonication buffer (50 mM MOPS
[morpholinepropanesulfonic acid], pH 7.0; dithiothreitol, 1 mM; EDTA,
3 mM). The cells were again pelleted and resuspended in 1 ml of
sonication buffer and frozen at 
80°C. The cells were immediately
thawed and sonicated five times at maximum output for 15 s per
burst (Branson Sonifier 250) and allowed to cool on ice between bursts.
The sonicated sample was centrifuged at 68,000 × g for
20 min to remove cellular debris. The resulting supernatant is the
crude lysate used in both mutase assays and was stored at 80°C
until required. Protein concentration of the crude lysates were
determined in triplicate with a standard Bradford reagent assay
(Sigma). PGM and PMM activities were determined essentially as
previously described (25, 42). Specific activities were
expressed as milliunits per milligram of protein, where 1 µmol of
NADP (substrate) is reduced to NADPH (product) in 1 min by 1 U of
enzyme. NADPH production was calculated from its molar extinction
coefficient of 6,220. Lysates were tested in duplicate, and three
independent lysates were prepared.
LPS extraction.
Cells were grown to late log phase in SS-C
at 25°C or SS-X at 37°C to an A560 of 1.0 and concentrated to A560 1.5 in
phosphate-buffered saline (PBS). The resultant cell pellet from 500 µl of sample was resuspended in 100 µl of distilled
H2O. An equal volume of 2× sample buffer (6% sodium
dodecyl sulfate; 6% 2-mercaptoethanol; 10 mM dithiothreitol; 46%
glycerol; 60 mM Tris, pH 8.0; 0.1% bromophenol blue) was added, and
the samples were boiled for 10 min. Protein was digested by the
addition of proteinase K to a final concentration of 50 µg/ml at
37°C overnight. Samples were again boiled for 10 min, and a second
volume of proteinase K, equal to the first, was added and incubated at
55°C for 3 h. LPS samples were stored at 20°C until
required. LPS profiles were determined by Tricine-sodium dodecyl
sulfate-polyacrylamide gel electrophoresis. Gels of 16.5% were
assembled and electrophoresis was performed as described by Lesse et
al. (28). LPS was visualized by oxidative silver staining
(47).
Complementation of pgm.
The mini-transposon
insertion into BB7865pgm was complemented by the conjugal
transfer into BB7865pgm of plasmid pBBR1MCS-4 (26), which harbored a 1.5-kb SacII fragment
containing the complete pgm gene of BB7865. This
plasmid was designated pBBR1MCS-4/pgm+.
Resistance to oxidative stress.
A disk diffusion assay was
utilized to determine sensitivity to paraquat (methyl viologen; Sigma)
(22). Approximately 106 cells of BB7865, BB7866,
BB7865pgm, and BB7866pgm were plated onto SS-X or
SS-C. A filter with a pore size of 0.22 µm, presoaked in 10 mM
paraquat, was placed onto each plate, and this was followed by
incubation at 30 or 37°C. Sensitivity to paraquat was measured by the
zone of inhibition surrounding the disk. The zone was measured in two
axes, and the mean values were calculated.
SOD, acid phosphatase, and urease assays.
For superoxide
dismutase (SOD) assays, sonicated cell samples (100% output; four 15-s
bursts) were cleared by centrifugation (12,000 × g for
2 min). A total of 115 µg of protein from each sample was loaded onto
an 8% native polyacrylamide gel and electrophoresed according to
standard procedures (52). Nitroblue tetrazolium was used to
reveal regions of enzyme activity as outlined by Beauchamp and
Fridovich (6). Acid phosphatase and urease activities were determined as previously described (22, 24, 31).
Cecropin P radial diffusion and liquid killing assays.
The
sensitivity of the mutant strains to cecropin P, a bioreactive peptide,
was tested. Radial diffusion assays were performed essentially as
described previously (5). Bacteria were cultured on BG agar
before being resuspended to a final optical density of 0.2 at
A600 in SS-C or SS-X. Low-gelling-temperature
agarose (1%) in either SS-X or SS-C was prepared and when cool was
supplemented with bovine serum albumin (final concentration, 0.15%).
To 10-ml aliquots, 200-µl aliquots of the cell suspensions were added
and allowed to set in a standard 90-mm-diameter petri dish. Cecropin P
(5 µg; 1 µg/µl in H2O; Sigma) was added to
3-mm-diameter wells made in the agarose. Following incubation at room
temperature for 4 h, the plates were transferred to 37°C (SS-X
plates) until zones were clearly visible. For liquid killing assays,
BB7865 and BB7865pgm were cultured on SS-X at 37°C and
suspended in PBS. Equal volumes of the cell suspension and cecropin P
were combined, giving a final peptide concentration of 50 µg/ml.
Following 1.5 h of incubation at 37°C, serial dilutions were
performed on BB7865 and BB7865pgm, with and without cecropin
P; plated onto SS-X; and incubated at 37°C.
Tissue culture.
The mouse macrophage-like cell line J774.A1
(ATCC TIB 67) was maintained in Dulbecco's modified Eagle medium
supplemented with 10% fetal calf serum (vol/vol) and 5 mM glutamine in
an atmosphere containing CO2 (5%, vol/vol) at 37°C.
Approximately 5 × 104 cells were seeded per well in
24-well tissue culture plates, incubated for 18 h, and then washed
twice with complete medium. For invasion assays the method essentially
followed that described by Guzmán et al. (19). The
results reported are mean values of three independent assays with
standard deviations. Incubation of B. bronchiseptica
bacteria, resuspended to an optical density equal to that used in the
invasion assays in Dulbecco's modified Eagle medium supplemented with
gentamicin at 50 mg/ml for 2 h resulted in >6 orders of magnitude
of reduction in CFU.
Murine respiratory infection model.
Female BALB/c mice at 6 to 10 weeks of age were used as a model of in vivo respiratory
infection by B. bronchiseptica. Following treatment with
Ketamine (50 mg/kg) and Xylazine (10 mg/kg) in sterile PBS, two
12.5-µl aliquots of a bacterial suspension were delivered
intranasally to each mouse via an air-displacement pipette and the
mouse was allowed to recover. The total number of viable bacteria
administered was approximately 105 cells. At each time
point four mice from each group were sacrificed and their lungs were
removed aseptically. Lungs were homogenized in sterile physiological
saline, and appropriate dilutions were plated onto nutrient agar to
determine the number of viable bacteria present in the lungs.
Statistics.
The results tested for statistical significance
were subjected to Student's t test. Differences were
considered significant if P was 
0.05.
Nucleotide sequence accession number.
The nucleotide
sequence data for PGM and PGI have been submitted to the GenBank
database under the accession number AF171632.
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RESULTS |
Identification of a novel LPS genetic locus in B. bronchiseptica.
A mini-Tn5 mutant of the BvgS mutant
strain BB7866 was produced (designated BB7866pgm) that
demonstrated an inability to synthesize a complete LPS molecule, as
demonstrated by oxidative silver staining of LPS extracts. Initial DNA
sequence data obtained from a cosmid clone positive for the
mini-Tn5 in Southern blots (data not shown) allowed the
production of PCR primers adjacent to the insertion site. These primers
enabled the amplification of a 300-bp gene fragment which was
utilized to probe a BB7865 cosmid library. The result of these
investigations, following cosmid cloning and subcloning, was a 3.4-kb
NotI fragment shown to contain a complete gene (Fig.
1A) with an amino acid sequence identity
of 55% (72% similarity) with the PGM gene from Neisseria
gonorrhoeae (Fig. 1B). The PGM gene was shown via Southern
blotting to hybridize with DNA fragments of B. pertussis and B. parapertussis but not with
Bordetella avium (Fig. 2).
Separated by just 10 bp and downstream of the PGM-encoding gene, a
second open reading frame was identified which exhibits high homology
with the PGI gene from several organisms. These two genes appear to be
organized into an operon (Fig. 1A) based on their spatial
organization and the absence of an intervening promoter-like sequence.
PGI is also found in a similar genetic organization in B. pertussis and shares 99.3% nucleotide sequence homology with the
B. bronchiseptica pgi gene as sequenced thus far (the
B. pertussis genome is found on line at
http://www.sanger.ac.uk/Projects/B_pertussis/). This operon has
not been previously described in Bordetella. An open reading
frame located downstream of the pgi gene from B. pertussis has been identified as encoding a possible galactosyl transferase; however, this gene is not included within the
pgm operon. The identical gene was mutated in
BB7865, the parental strain of BB7866, by way of an in vivo chromosome
transfer technique (44). This allowed for the effects of
such a mutation to be observed in a bvg-positive background.
The resultant mutant was designated BB7865pgm.
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FIG. 1.
Genetic organization and sequence homology of
pgm. (A) Spatial orientation of the operon from
B. bronchiseptica containing pgm and
pgi. The equivalent genes were found to exist in
B. pertussis in the same orientation and with high DNA
sequence homology (98.6 and 99.3%, respectively). A gene downstream of
B. pertussis pgi was located and shown to have the
highest homology with other galactosyl transferases. The dashed line
indicates the fragment of DNA cloned into pBBR1MCS-4 (26)
and thereafter utilized for complementation of BB7865pgm.
Arrows indicate the direction of transcription. Arrowheads indicate
putative promoter sequences. (B) ClustalW alignment of B. bronchiseptica (Bbro) pgm gene and the following
homologous sequences (pgm and pmm) (abbreviations
and accession numbers are given in parentheses): Neisseria
meningitidis pgm (Nmen; P40391), N. gonorrhoeae pgm
(Ngon; P40390), P. aeruginosa pmm (Paer; P26276),
Azospirillum brasilense pmm (Abra; P45632), and
Prochlorothrix hollondica pmm (Phol; U23551). Identical
residues are depicted by dots. Dashes indicate gaps introduced in the
amino acid sequence for optimal alignment.
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FIG. 2.
Characterization of the pgm insertion
mutation. (A) The mini-Tn5 insertion (5.0 kb) was found to
have occurred 604 bp downstream of the pgm methionine start
codon. (B) Southern blot analysis of pgm mutants and other
Bordetella spp. utilizing the 300-bp PCR fragment (PCR-1),
amplified adjacent to the mini-transposon insertion (see panel A). The
pgm gene exists in an EcoRI fragment of 8.4 kb.
An EcoRI site located on the transposon results in a
restriction fragment 539 bp shorter than that of the wild type. Lane 1, BB7865; lane 2, BB7866; lane 3, BB7865pgm; lane 4, BB7866pgm; lane 5, B. pertussis; lane 6, B. parapertussis; lane 7, B. avium.
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Analysis of PGM enzyme activity from BB7865, BB7866, and their
respective pgm-deficient mutants.
PGM assays were
performed to determine the level of enzyme activity in parental and
mutant strains. These assays demonstrate that the mutation eliminates
the ability to produce functional enzyme, as BB7865pgm and
BB7866pgm are shown to have a PGM activity below the
detection limits of the assay (i.e., <2 mU/mg). This was shown to be
statistically significant (P 0.01) for strains grown in
either SS-C at 25°C or SS-X at 37°C (Table
1). PMM assays were also performed, as
the mutated gene also shared high amino acid homology to PMM from
Pseudomonas aeruginosa. Similar results were obtained for
this enzyme, with PGM mutants again displaying low levels of activity,
whereas the wild type expressed levels closer to 8.12 mU/mg.
Complementation of BB7865pgm with the wild-type pgm gene restored PGM and PMM activity to levels observed in
BB7865. It is of interest that PGM is known to be a bifunctional enzyme (42) capable of using either glucose or mannose as a
substrate. Mannose, however, is not reported as a component of the
B. pertussis LPS (3); it therefore seems
likely that the affected enzyme acts as PGM in B. bronchiseptica.
Electrophoretic profiles of LPS extractions clearly demonstrate the
physical alterations caused by the mutation of PGM (Fig.
3A). The band A and band B core
structures (
35) and the O-antigen
are all seen to be present
in the parental strains (Fig.
3A).
However, O-antigen is absent from
BB7865
pgm and BB7866
pgm, and
the core structure
is considerably truncated, migrating faster
than the band B of the
parental strains. Complementation with
pgm from the parental
BB7865 strain restored the wild-type LPS
phenotype to
BB7865
pgm (Fig.
3A). The influence of the
bvg
locus
on the expression of PGM was analyzed. At 37°C and in the
absence
of chemical modulators such as MgSO
4, virulence
factors are expressed.
There exists a separate class of genes that are
repressed by the
bvg locus, including the genes encoding
flagellum biosynthesis
(
1). This occurs with growth in
modulating medium, i.e., containing
MgSO
4, at
lower temperatures (25°C). The size of the LPS molecule
from the
mutant strains is unaffected by growth under either modulating
or
nonmodulating conditions, as is the case for the wild type,
indicating
that the
bvg locus elicits control only over the distal
region of the molecule including the O-antigen. PGM and PGI are
both
required early in the pathway for production of sugar nucleotides
destined for LPS synthesis. In fact they both catalyze the same
substrate, glucose 1-phosphate, converting it to the respective
precursors (Fig.
3B).
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FIG. 3.
LPS phenotypes and biosynthesis pathway. (A)
Electrophoretic profiles of LPS extracted from BB7865 (lanes 1 and 5),
BB7866 (lanes 2 and 6), BB7865pgm (lanes 3 and 7), and
BB7866pgm (lanes 4 and 8); lanes 9 and 10 contain the
complemented mutant, BB7865pgm
(pBBR1MCS-4/pgm+). Strains represented in lanes
1 to 4 and 9 were cultured in SS-C at 25°C, whereas those shown in
lanes 5 to 8 and 10 were cultured in SS-X at 37°C. O-antigen and core
band A and B are indicated to the left. (B) Biosynthesis of nucleotide
sugars via pgm and pgi for production of LPS.
(Modified from reference 56 with permission of the publisher.)
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Intracellular survival of parental and PGM-deficient
B. bronchiseptica.
In vitro invasion and survival
assays utilizing J774.A1 cells demonstrated a significantly
reduced ability of the mutant strains to survive. Compared to the CFU
of the respective parental strains, only 43% of
BB7865pgm and 40% of BB7866pgm remained after
24 h (Fig. 4). Complementation of
BB7865pgm with the wild-type pgm gene
restored survival rates to levels above those observed in BB7865.
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FIG. 4.
Intracellular survival of B. bronchiseptica strains in J774.A1 cells at 2 and 24 h.
Results shown are represented as mean percentages of CFU recovered of
the respective parental strains. Error bars indicate the standard error
of the mean.
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Highly reactive oxygen anion radicals are an effective intracellular
defense mechanism employed by the host. Intracellular
bacteria can
utilize various enzymes such as SOD for the conversion
of these
radicals to more stable forms, i.e., O
2
to
H
2O
2 and O
2. Of interest here is
the effect of a compromised
physical barrier to free radical attack;
therefore, sensitivity
of PGM mutants to oxidative stress was measured.
BB7865
pgm was
notably more sensitive to paraquat (Table
2), a superoxide radical-generating
compound, exhibiting a zone of inhibition of 8.5 mm on SS-C at
25°C
and 7 mm on SS-X at 37°C compared to 0 mm for BB7865 under
both
conditions. Complementation of BB7865
pgm with the wild-type
pgm gene restored the wild-type phenotype. SOD activity
levels
remained unchanged for BB7865
pgm (results not shown),
suggesting
a role for LPS as a physical barrier. Other phenotypes
tested
that are suggested to participate in intracellular survival
within
eukaryote cells are acid phosphatase (
9) and urease
(
31).
These phenotypes remained unaffected in the
BB7865
pgm mutant (results
not shown).
Resistance to the cationic peptide cecropin P.
LPS is
credited as being responsible for conferring some
protection against antibiotics and serum (53) as a
mode of protection from host defenses. Another naturally occurring
class of molecules are the defensins. These are cationic peptides found
in a wide variety of vertebrate and invertebrate organisms
(15) on the surface of skin, trachea, and tongue among
others (20, 43). The sensitivity of BB7865pgm to
the defensin cecropin P in a radial diffusion assay was shown to
be significantly increased (P 0.01) compared
to that of the wild-type strain (Table
3). Complementation of
BB7865pgm with the wild-type pgm gene restored
the wild-type phenotype in radial diffusion assays. It was also
established that 90% of BB7865pgm, compared to
BB7865 cells, were killed when incubated with a 50-µg/ml
solution of cecropin P for 1.5 h in liquid killing assays (results
not shown).
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TABLE 3.
Sensitivity of B. bronchiseptica
wild-type and mutant strains to cecropin P as measured by
radial diffusion
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Survival of BB7865pgm within the murine respiratory
tract.
In vitro survival assays demonstrated a marked reduction in
the ability of the PGM mutant to invade or persist within J774.A1 cells
(Fig. 4). This result led to the investigation of the effect the
B. bronchiseptica pgm mutation would have within a
murine respiratory infection model. Nonlethal doses of BB7865 or
BB7865pgm were administered to BALB/c mice intranasally, and
the numbers of CFU present in the lungs were measured at various time
points following infection. Although the wild-type strain showed
a classic pattern of infection (22), the mutant strain was
unable to survive, being effectively cleared within 4 days. This
was the result observed in two independent trials. The reduction in
BB7865pgm CFU was found to be consistently significant from
day 2 (P 0.05). Mice infected with the wild-type
strain still had an average of 1,000 CFU/lung persisting 35 days
following inoculation (Fig. 5).
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FIG. 5.
In vivo persistence of wild-type BB7865 and the
pgm mutant, BB7865pgm, in a murine respiratory
model. Lungs were taken at different time intervals, and the number of
viable bacteria per lung was determined. The results are averages of
values for four mice.
|
|
| |
DISCUSSION |
A new gene cluster critically involved in the production of LPS in
B. bronchiseptica is described here. The operon
includes genes identified as encoding PGM and PGI, which are utilized
in the synthesis of nucleotide sugars for inclusion into growing LPS
molecules. Abolition of PGM activity will lead to the loss of glucose
and all other components distal to the heptose residue of the
B. bronchiseptica inner core (i.e., band A, band B, and O-antigen). Of further interest is the fact that the abolition of PGM
activity renders the bacteria more susceptible to antimicrobial peptides and oxidative stress, reduces bacterial ability to survive within J774.A1 cells, and results in an inability to colonize the
murine respiratory tract. Complementation of the PGM mutant B. bronchiseptica pgm with the wild-type pgm
gene restored the wild-type condition for all phenotypes tested,
indicating that the mutation of pgm was responsible for the
altered phenotypes observed in this study.
The role played by the bvg locus in regard to the regulation
of the PGM operon was investigated and was not found to be
required for expression. The bvg locus has been shown in
this study and in others (48) to influence the expression of
LPS in response to a modulating environment (i.e., reduced temperature
and increased sulfate anions). This is exemplified by the identical LPS
profile of the bvg-negative mutant BB7866 and BB7865 grown
in SS-C at 25°C compared to the contrasting LPS profile seen in
BB7865 when grown in SS-X at 37°C. It has been observed that LPS
expressed by B. bronchiseptica can change during an
infection (17). This type of expression has been suggested
to be a mechanism of adaptation to the host environment in other
mucosal pathogens such as P. aeruginosa and N. gonorrhoeae (12, 49). The length of the O-antigen has
been demonstrated to be an important factor for resistance to
complement (8). It is therefore feasible that regulation of
the LPS composition includes one form required for colonization or
invasion and another for survival in a particular niche protected from
host humoral defenses. The bvg-repressed form of LPS may
also be advantageous to the cell during transmission between hosts.
Other evidence existing for bvg-regulated LPS expression includes monoclonal antibodies specific for band B LPS of B. pertussis, which only react with B. bronchiseptica
LPS in a bvg-repressed state (30).
However, pgm is not regulated by bvg. There is
not a significant difference in the activity of the enzyme produced by
bvg-positive or bvg-negative parental strains
under any growth condition. This result is mirrored in the LPS profiles
of the mutant strains that indicate the same size LPS molecule is
produced for both, irrespective of growth conditions. A possible
explanation for this observation is that the early core biosynthesis is
not bvg-regulated. These genes are likely to be expressed as
housekeeping genes rather than being controlled by the virulence
regulator. Genes utilized for the synthesis of the LPS molecule distal
to the core glucose are not required for growth but are utilized for
virulence and thus may be regulated by the bvg locus. This
hypothesis also seems likely given that the genes of the PGM
operon are distinct from the other LPS biosynthesis genes, such
as the wlb genetic locus responsible for band A biosynthesis
and also involved in O-antigen production. Strengthening this point is
the existence of the waaA and waaC genes
(required for synthesis of the deep inner core), which are not
incorporated in the wlb locus (3, 36).
The importance of LPS to pathogenesis can be inferred by the
B. bronchiseptica pgm mutant. The results obtained from
the murine respiratory infection model demonstrate that although lipid
A and the deep inner core are sufficient for viability, this truncated form of LPS is inadequate for colonization and survival of
B. bronchiseptica in vivo. The absence of the O-antigen
is likely to be a major factor in the behavior of BB7865pgm
mutant in vivo. The increased sensitivity to defensins is probably due
to the lack of the O-antigen and may offer some reason as to why
bacterial clearance was so efficient. The antimicrobial peptide tested
in this study was of the cecropin class. These, like the defensins, are
cationic peptides and play an important role in the innate immunity of
the host respiratory tract. The mode of action of the peptides is the
destabilization of the cellular membrane by binding with anionic
phospholipids (29). The O-antigen of B. bronchiseptica is thought to constitute a protective barrier, thereby concealing the negative charge of the membrane (5).
Resistance to superoxide anions is an important factor in terms of
bacterial intracellular survival. Evidence to suggest that LPS is in
some way responsible for a level of protection from intracellular
superoxide radicals may come from the fact that the mutants were more
susceptible to paraquat despite SOD levels remaining at wild-type
levels (results not shown). Again, the high charge of B. bronchiseptica O-antigen may be able to shield the cell from the
destructive O2 radicals, at least at the
concentration tested in this study.
The bvg regulation of the distal portion of the LPS molecule
is in response to the environment in which the bacterium finds itself.
The pathogen must be capable of expressing an O-antigen of the correct
length and composition. Sequential mutagenesis of the LPS molecule from
the distal region would be required to highlight which portion of the
molecule is specifically required for pathogenesis.
| |
ACKNOWLEDGMENTS |
We acknowledge support from the Australian Research Council
(grant A09231658). N. P. West is the recipient of a
University of Wollongong postgraduate research award.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Biological Sciences, University of Wollongong, New South Wales,
Australia 2522. Phone: 0061-242213439. Fax: 0061-242214135. E-mail:
mwalker{at}uow.edu.au.
Present address: Endocrine Unit, Department of Medicine, John
Hunter Hospital, Newcastle, New South Wales, Australia.
Editor:
S. H. E. Kaufmann
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Abstract
Introduction
