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Infection and Immunity, July 2000, p. 4102-4107, Vol. 68, No. 7
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Identification of Genes Required for Chronic
Persistence of Brucella abortus in Mice
Priscilla C.
Hong,
Renée M.
Tsolis,* and
Thomas A.
Ficht
Department of Veterinary Pathobiology,
College of Veterinary Medicine, Texas A&M University, College
Station, Texas 77843-4467
Received 8 December 1999/Returned for modification 1 February
2000/Accepted 19 April 2000
 |
ABSTRACT |
The genetic basis for chronic persistence of Brucella
abortus in lymphoid organs of mice, cows, and humans is currently
unknown. We identified B. abortus genes involved in chronic
infection, by assessing the ability of 178 signature-tagged mutants to
establish and maintain persistent infection in mice. Each mutant was
screened for its ability to colonize the spleens of mice at 2 and 8 weeks after inoculation. Comparison of the results from both time
points identified two groups of mutants attenuated for chronic
infection in mice. The first group was not recovered at either 2 or 8 weeks postinfection and was therefore defective in establishing
infection. Mutants in this group carried transposon insertions in genes
involved in lipopolysaccharide biosynthesis (wbkA), in
aromatic amino acid biosynthesis, and in type IV secretion
(virB1 and virB10). The second group, which was
recovered at wild-type levels 2 weeks postinfection but not 8 weeks
postinfection was able to establish infection but was unable to
maintain chronic infection. One mutant in this group carried a
transposon insertion in a gene with homology to gcvB of
Mycobacterium tuberculosis, encoding glycine dehydrogenase, an enzyme whose activity is increased during the state of
nonreplicating persistence. These results suggest that some mechanisms
for long-term persistence may be shared among chronic intracellular
pathogens. Furthermore, identification of two groups of genes, those
required for initiating infection and those required only for long-term persistence, suggests that B. abortus uses distinct sets of
virulence determinants to establish and maintain chronic infection in mice.
| |
INTRODUCTION |
Bacteria causing chronic infections,
such as Mycobacterium tuberculosis, Chlamydia
trachomatis, and Brucella abortus are able to evade the
host's immune system throughout the infection by colonizing an
intracellular niche. This lifestyle may require adaptations other than
the brief survival in phagocytic cells observed for well-characterized
intracellular pathogens such as Salmonella serotypes which
cause an acute infection. While M. tuberculosis and C. trachomatis are difficult to manipulate genetically, the genetic
manipulation of the Brucella genome can be performed routinely, using tools such as plasmid vectors and systems for Tn5 mutagenesis (20-22). Thus, identification of
the genes required by B. abortus to cause infection may
reveal virulence mechanisms of chronic disease caused by other
intracellular pathogens. A recent improvement in Tn5
mutagenesis, known as signature-tagged transposon mutagenesis (STM),
has been developed for the in vivo selection of Tn5 mutants
that are defective in colonization (18). This method uses
experimentally infected animals to identify mutants that are attenuated
in vivo from a large, mixed pool of mutants (29). Since
Tn5 can be used in B. abortus, STM can be used to identify genes that are necessary for chronic intracellular infection.
Brucellosis is endemic in Mediterranean countries and Central and South
America and is manifested as an undulant fever in humans that, if
untreated, can develop into a chronic infection with symptoms
persisting for several months (32). Chronic infections may
result in infection of secondary tissues, including heart and brain, if
the infection is left untreated. Symptoms may also recur years after
the original infection. B. abortus infection is
acquired by humans through contact with infected livestock and
consumption of unpasteurized dairy products. Bacteria cause a systemic
infection and localize preferentially to organs that are rich in
elements of the reticuloendothelial system, such as liver, spleen, and
lymph nodes, where they survive and multiply within host macrophages.
B. abortus has been found to inhibit the bactericidal
functions of phagocytes, including phagolysosomal fusion, neutrophil
degranulation, and the oxidative burst (5); however, as with
other intracellular pathogens which cause chronic infection, the
genetic basis for the interaction of Brucella with phagocytic cells is still poorly understood. B. abortus
virulence is conveniently studied in a mouse model that mimics the
chronic infection observed in humans. Here bacteria are found
intracellularly, within macrophages of infected organs (25).
Experimental infection of BALB/c mice has shown that the infection has
two phases: during the first 2 weeks, bacteria multiply rapidly. In the
second phase, bacterial numbers stabilize over the next 5 to 6 weeks
and then decrease slowly. Bacteria have been recovered from
spleens of infected mice as late as 24 weeks postinfection
(26, 28). The different phases of B. abortus
infection in mice raise the question whether this pathogen uses
different sets of virulence genes during the early and late stages of
this disease.
To address this question, we have performed a random screen of the
genome of B. abortus to identify genes required for
infection at an early (2 weeks postinfection) and a late (8 weeks
postinfection) time point postinoculation. Comparative analysis of
these results provided new insight into the genetic basis for chronic
intracellular infection and B. abortus pathogenesis.
Furthermore, our results suggest that a better understanding of the
mechanisms by which B. abortus is able to cause chronic
intracellular infection may ultimately reveal strategies that are
shared by other, less tractable pathogens.
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MATERIALS AND METHODS |
Construction of mutants and growth conditions.
B.
abortus strain 2308 (obtained from B. L. Deyoe, National
Animal Disease Center, Ames, Iowa) was used as a host for STM. A bank
comprising 240 signature-tagged B. abortus mutants (ST mutants) was constructed using a pool containing 10,000 uniquely tagged
miniTn5Km2 derivatives carried on suicide plasmids, which was obtained from David Holden (18). The transposons were
introduced into B. abortus S2308 by electroporation and
selected on tryptic soy agar (TSA; Difco) containing 100 mg of
kanamycin (Km) per liter (1). Approximately 20 mutants were
taken from each of 10 individual electroporations in order to minimize
the isolation of siblings. Mutants resistant to ampicillin were
eliminated from the pool, since they carry the suicide vector inserted
into the chromosome. For infection of mice, B. abortus
strains were grown on potato infusion agar (PIA; Difco) for 48 h
and resuspended at the appropriate concentration in phosphate-buffered
saline (PBS) (2). For determination of auxotrophy, the
chemically defined solid medium formulated by Gerhardt was used, which
contains glycerol, glutamate, lactate, thiamine, nicotinic acid,
biotin, calcium pantothenate, and inorganic salts (15). This
basal medium was supplemented with 10 groups of amino acids to perform
auxanography for attenuated mutants. All work with live B. abortus was performed in a biosafety level 3 containment facility
following Centers for Disease Control-National Institutes of Health guidelines.
Infection of mice.
For the mutant screen, pools of 46 mutants were used to infect groups of six 6- to 8-week-old BALB/c mice
intraperitoneally (i.p.) at a total dose of approximately
106 CFU. Groups of three mice were sacrificed at 2 and at 8 weeks postinfection, and bacteria were recovered from the spleens.
Spleens were homogenized in 3 ml of PBS, and serial 10-fold dilutions were plated on TSA-Km.
Signature-tagged screen and hybridization analysis.
Bacteria
recovered from murine spleens at 2 and 8 weeks postinfection were
pooled to obtain one output pool from each mouse. Total chromosomal DNA
was prepared from each output pool to serve as a template for
generating probes containing labeled tags, as described before
(18). Labeled tags used as probes were prepared by
incorporation of [
-32P]dATP during PCR amplification
of tags from total chromosomal DNA. Blots containing chromosomal DNA
from individual mutants in each pool were prepared by transferring
pools of B. abortus ST mutants from 96-well plates onto
nylon membranes laid on top of TSA plates with a 48-prong replicator.
Hybridization and washes were carried out under stringent conditions
(4). To identify potentially attenuated mutants,
hybridization signals on a blot probed with labeled tags prepared from
the input pool (inoculum) were compared with three identical blots
hybridized with tags prepared from the output pools recovered from the
three mouse spleens at each time point. Mutants giving a hybridization
signal with the input pool but no signal in the output pool of at least two mice were selected for further study. To confirm that each mutant
carried a single insertion of mini-Tn5 in the chromosome, mutants were analyzed by Southern blot (4). Chromosomal DNA was prepared (4) and digested with EcoRI, which
cuts once within the transposon, outside the kanamycin resistance gene.
After agarose gel electrophoresis and transfer to nylon membranes,
chromosomal DNA was analyzed by hybridization with a probe containing a
1.3-kb fragment of the Tn903 kanamycin resistance gene from
plasmid pUC4KSAC (Pharmacia). Mutants whose chromosomal DNA gave a
hybridization signal with a single band on the Southern blot were
determined to have only one copy of the transposon inserted into the chromosome.
Competitive infection assay.
For competitive infection
experiments, groups of four mice were inoculated i.p. with an
approximately 1:1 mixture of mutant and wild-type B. abortus, at a total dose of approximately 105 CFU.
Mice were sacrificed at 2 or 8 weeks postinfection, and bacteria were
recovered from infected spleens. The CFU of mutant and wild-type
B. abortus recovered from infected spleens were enumerated
by serial dilution in PBS and plating in parallel on TSA and TSA-Km.
Numbers of wild-type and mutant bacteria were calculated by subtracting
the CFU recovered on TSA-Km, on which only the Tn5 mutants
are able to grow, from the CFU recovered on TSA plates, representing
the total number of bacteria recovered. Data were normalized by
dividing the output ratio of (CFU [wild type]/CFU [mutant]) by the
input ratio of (CFU [wild type]/CFU [mutant]). All data were then
converted logarithmically for statistical analysis. A Student's
t test was used to determine whether the wild-type/mutant
ratio recovered from infected spleens was significantly different from
the wild-type/mutant ratio present in the challenge inoculum.
Cloning and sequence analysis.
Transposon-flanking DNA was
cloned by inverse PCR as described previously (6) using
RsaI for digestion of chromosomal DNA and the primer pair
SIGN-10 (5'-GCCGAACTTGTGTATAAGAGTCAG-3') and SIGN-11
(5'-AAAGGTAGCGTTGCCAATG-3'). The PCR products were ligated into cloning vector pCR II (Invitrogen), and plasmid DNA for sequencing was isolated from Escherichia coli strain DH5
(17) using ion-exchange columns from Qiagen. In addition,
larger DNA fragments flanking the transposon insertions in several of
the mutants were cloned by ligating PstI- or
EcoRI-restricted genomic DNA into cloning vector pBluescript
SK+ restricted with the appropriate enzyme and selection for the
kanamycin resistance marker of mini-Tn5Km2 (12).
Nucleotide sequences were analyzed using the MacVector 6.5 software
package (Oxford Molecular Group). Sequence homology was determined
using the BLAST2 search algorithm at the National Center for
Biotechnology Information (NCBI) (3).
| |
RESULTS |
Generation of signature-tagged mutants of B. abortus.
B. abortus 2308 was mutagenized with a pool
of signature-tagged mini-Tn5Km2 derivatives carried on
plasmid pUT by electroporation, and mutants were selected on
TSA-Km. These mutants were screened for susceptibility to
ampicillin to eliminate strains (fewer than 2% of mutants)
carrying cointegrates of the suicide vector pUT inserted in the
chromosome. To confirm that mutants obtained from the same
electroporation are not siblings but arise from independent transposition events, Southern hybridization was performed
using the 1.3-kb EcoRI fragment of pUC4KSAC, which contains
the Tn903 Kmr gene (12). Using this
probe, the hybridization profiles of EcoRI-digested
chromosomal DNA from 10 randomly chosen mutants from a single
electroporation were compared. Since EcoRI cuts only once
within miniTn5Km2, a mutant with a single transposon insertion should have only one band hybridizing with the probe. All of
the mutants examined had a single band of unique size hybridizing with
the probe, indicating that each mutant contained a single, unique
insertion of the transposon (data not shown).
Signature-tagged screen of B. abortus mutants in
mice.
To identify mutants defective in establishing chronic
infection, we used the BALB/c mouse model of chronic brucellosis. Mice infected i.p. with B. abortus have been shown to harbor
bacteria in the spleen for up to 24 weeks postinfection (5,
9). The persistence of B. abortus in mice is similar
to chronic infection observed in other host species, including humans.
It has not been shown whether attenuated B. abortus
mutants exhibit competitive infection defects in mice when
coinoculated with a virulent strain. We therefore performed a
preliminary competitive infection experiment using B. abortus 2308 and CA180, a Tn5 mutant defective in the
synthesis of the O antigen of lipopolysaccharide (LPS), which was
characterized previously (1). Three mice were infected i.p.
with a mixture containing 6.4 × 104 CFU of B. abortus 2308 and 4.1 × 104 CFU of CA180. At 1 week postinfection, no mutant B. abortus could be recovered
from the spleens of any infected mouse, while the number of wild-type
B. abortus ranged from 6 × 103 to 2 × 106 CFU/spleen. This result showed that a mutant with a
defect in a known B. abortus virulence factor, LPS, exhibits
a competitive infection defect in the BALB/c mouse model of
brucellosis. Furthermore, it suggested that STM, which utilizes
competitive infection as the basis for screening pools of mutants,
could be used to screen for mutants defective in chronic infection.
For the screen in mice, pools of 46 mutants were grown individually in
tryptic soy broth (TSB) in 96-well plates for 48 h
and then
stamped with a 48-prong replicator onto PIA plates and
grown for
48 h. Bacteria were resuspended from PIA plates, and
the
concentration was adjusted to approximately 10
7 CFU/ml with
PBS. Of this suspension, 0.1 ml was injected i.p.
into each of six
BALB/c mice. In the pooled inoculum, the dose
of each individual mutant
was therefore approximately 10
4 CFU. At 2 and 8 weeks
postinfection, groups of three mice were
sacrificed. At necropsy, the
only sign of disease evident was
enlargement of the spleen. To recover
bacteria, spleens were homogenized
in PBS, and serial 10-fold dilutions
were plated on TSA-Km. After
incubation for 4 days, bacteria were
resuspended from plates containing
between 1,000 and 5,000 colonies,
and chromosomal DNA was prepared
from the recovered pool of mutants.
Probes of input and output
pools were generated by PCR amplification of
tags from chromosomal
DNA of pooled ST mutants as described before
(
18) and used for
hybridization with dot blots containing
individual mutants in
the corresponding pool. For each time point, a
fresh input pool
probe was prepared and a blot was hybridized for
comparison with
the output pools recovered from the mice. We found that
39 mutants
failed to give a reproducible hybridization signal when the
input
pool probe was prepared more than once from a chromosomal DNA
preparation. These mutants were eliminated from the screen. Thus,
a
total of 178 mutants with consistently hybridizing tags were
screened.
Mutants which gave weak or no hybridization signals on output pool
blots from at least two of the three mice at each time
point were
identified as putatively attenuated by comparison with
input pool blots
(Fig.
1). At 2 weeks postinfection, 28 mutants
exhibited a reduction in the hybridization signal, suggesting
reduced recovery from the mouse spleens. Of these 28 mutants,
11 exhibited a reduced hybridization signal in output pools recovered
at 8 weeks postinfection.
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FIG. 1.
Colony blots showing hybridization of B. abortus ST mutants with probes containing tags amplified from the
input pool and from output pools recovered from spleens of three mice
at 8 weeks postinfection. At the upper left and lower right corner of
each blot is the parent stain, B. abortus 2308. Arrows
indicate mutants (BA142, BA152, BA159, and BA184 [left to right])
which gave weak signals in the output pools of at least two of the
three mice inoculated and whose competitive infection defect was
confirmed subsequently. Open squares indicate mutants that gave
inconsistent hybridization results and were therefore eliminated from
the screen.
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|
In addition to the 11 mutants reduced in colonization at both 2 and 8 weeks, we identified 16 mutants that were only defective
for
colonization at 8 weeks. While mutants identified from both
the 2- and
8-week output pools may be unable to establish infection,
those
identified only from the 8-week output pools may be defective
in
sustaining chronic infection. The 17 mutants identified only
from the
2-week output pools may represent mutants which are slow
to colonize
the spleen but are still able to persist. However,
infection defects in
these mutants were not characterized further,
since these mutants were
able to sustain chronic infection. Thus,
two groups of mutants, those
identified at both 2 and 8 weeks
and those identified only at 8 weeks,
were considered putatively
attenuated for chronic infection and were
chosen for further study
(Table
1).
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TABLE 1.
Confirmation of competitive defects of STM mutants by
competitive infection of mice with B. abortus S2308a
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|
Competitive infection of mice with mutants identified by STM.
Following our identification of mutants putatively attenuated for
chronic infection, we performed a quantitative assay to confirm their
colonization defect. To this end, each of the 27 mutants identified by
the STM screen was inoculated i.p. at a 1:1 ratio with wild-type
B. abortus at a total dose of approximately 105
CFU to groups of four mice (Table 1). As a control, mutant BA53, which
was recovered at both 2 and 8 weeks postinfection from mice, was
selected at random from the STM pool as a negative control and
administered to mice in a competitive infection experiment as described
above. During mixed-infection experiments, 15 mutants identified in the
STM screen were found to have a significant defect in persistence in
mouse spleens. One of these mutants, BA11, had a significant
colonization defect only at 2 weeks and therefore was not characterized
further. Thus, for 14 of 27 mutants identified in the preliminary STM
screen, the putative chronic infection defect could be confirmed by a
significant reduction in colonization during competitive-infection
experiments. Mutants which did not have significant colonization
defects in the competitive-infection assay either may have been
false-positives in the STM screen or may only display competitive
colonization defects when inoculated at a wild type-to-mutant ratio of
greater than 1. However, these possibilities were not investigated
further. Mutants with significant colonization defects during mixed
infections fell into two groups: those reduced in colonization at both
2 and 8 weeks, and those reduced at only 8 weeks (Fig.
2). Subsequent mouse infection
experiments showed that mutants with competitive colonization defects
are also attenuated when administered alone to mice (data not shown). To determine whether colonization of the spleen was reduced due to a
general growth defect, mutants displaying significant defects at both 2 and 8 weeks postinoculation were assayed for in vitro growth defects by
inoculating TSB with a mixture of wild-type and ST mutant strains
(Table 1). With the exception of BA100, which was outgrown almost
fivefold by the parent strain, none of the mutants displayed a strong
growth deficiency in laboratory medium.
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FIG. 2.
Mutants with statistically significant colonization
defects, as confirmed by individual competitive infections and
statistical analysis. Homologues of disrupted genes are given in
parentheses. nh, no homology.
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|
Identification of inactivated genes.
Genes inactivated by
mini-Tn5Km2 insertions were identified by cloning
transposon-flanking DNA, sequence determination, and comparison with
the GenBank database using the BLAST2 search program at NCBI.
Transposon-flanking DNA was cloned from eight mutants.
Mutants with defects in establishing chronic infection included
BA184, which carried a transposon insertion in a
B. abortus homologue of
Brucella melitensis wbkA, encoding a
mannosyltransferase
that functions in the biosynthesis of O antigen
(
16). LPS biosynthesis
is required for virulence in
Brucella species, and it has recently
been shown that
strains of
B. abortus and
B. melitensis carrying
defined mutations in genes required for LPS biosynthesis are unable
to
establish infection in mice (
1,
16,
24). Identification
of
this known virulence factor thus validated the STM
screen.
Two additional mutants with defects in establishing persistent
infection, BA41 and BA114, carried transposon insertions in
homologues
(
virB1 and
virB10, respectively) of the
Brucella suis virB locus (
27).
B. suis
mutants carrying disruptions at this
locus show a reduced ability to
multiply in vitro within macrophages
and HeLa cells. Our data suggest
that this locus is required for
establishing chronic infection in
organs of the
mouse.
We could obtain no clone from DNA flanking the transposon insertion of
the fourth mutant (BA100) defective in establishing
chronic infection.
However, BA100 was unable to grow on
Brucella minimal medium
unless supplemented with a combination of aromatic
amino acids. These
auxanography data indicated that this mutant
was defective in an early
step of the aromatic amino acid biosynthesis
pathway.
Sequences obtained from the transposon insertion site in three mutants
defective in sustaining chronic infection showed homology
to metabolic
genes. BA159 was interrupted at the
gluP locus, encoding
a
putative transporter for glucose and galactose (
14). Mutant
BA152 carried a transposon insertion in a homologue of
Rhizobium etli gltD, encoding the small subunit of glutamate synthase
(
10).
The identification of these two mutants in the STM
screen suggests
that glucose, galactose, or glutamate may serve as
carbon and/or
nitrogen sources during growth of
B. abortus
in the host. BA102
carried an insertion in a putative glycine
dehydrogenase or glycine
cleavage system. Since BA102 did not have a
competitive growth
defect in TSA and was able to grow on minimal medium
without glycine,
the virulence defect of BA102 is likely not due to
auxotrophy.
Interestingly, the activity of glycine dehydrogenase has
been
shown to increase 10-fold upon entry of
M. tuberculosis
into a
state of nonreplicating persistence (
30,
31). Since
B. abortus,
like
M. tuberculosis, is able to
persist chronically in infected
hosts, glycine dehydrogenase may play a
similar role in the entry
of these pathogens into a latent state in the
host.
Finally, DNA flanking two insertions in mutants defective for
maintaining chronic infection showed either no homology to genes
in the
database (BA73) or homology to an open reading frame of
unknown
function (BA87) (Table
2).
| |
DISCUSSION |
The goal of the STM screen was to identify and compare B. abortus genes required for establishment and maintenance of
chronic persistence in the mouse. Since fewer than 200 genes have been sequenced in Brucella species, we reasoned that screening a
small number of mutants would be sufficient to identify new B. abortus genes required for chronic infection. The STM screen
identified 27 mutants putatively attenuated for chronic infection. A
statistically significant competitive-infection defect could be
detected in 14 of these mutants. Thus, statistically significant
evidence for attenuation was obtained for 8% (14 of 178) of the
mutants screened. Assuming that our mutagenesis was random and that the coding density of the 3,200-kb B. abortus genome is similar
to that of the E. coli genome, our data suggest that an
estimated 257 genes may be required for establishing and maintaining
chronic persistence in mice after i.p. infection. In contrast, i.p.
infection of mice with an STM bank of Salmonella enterica
Typhimurium revealed that only 3% of its 4,400-kb genome, or an
estimated 153 genes, is required for the acute infection caused by this
intracellular pathogen (18). The greater number of virulence
genes required for chronic infection versus acute disease may reflect
the requirement for additional adaptations to ensure long-term
persistence, such as those which prevent clearance of B. abortus by the host immune system.
The working hypothesis of this study was that different sets of genes
may be required for the initial steps or the establishment of chronic
infection, which is characterized by rapid bacterial growth, than for
maintenance of chronic infection, in which little or no growth is
observed (5, 9). Indeed, the 14 attenuated mutants
identified in this study fell into two classes (Fig. 2). Four mutants
were unable to establish infection by either 2 or 8 weeks
postinfection. In contrast, the remaining 10 mutants were able to
establish infection at 2 weeks postinfection but displayed a defect in
chronic persistence at 8 weeks postinfection. The first class included
mutants with transposon insertions in genes required for O antigen
biosynthesis (BA184), type IV secretion (BA41 and BA114), and
biosynthesis of aromatic amino acids (BA100). The genes inactivated in
these mutants are predicted to play a role early during infection. For
example, BA184, a wbkA mutant, was the most highly
attenuated and was outcompeted by the wild type by 1,000-fold at 2 weeks postinfection, suggesting that it was eliminated early in the
infection process. Since rough mutants are sensitive to the
bactericidal action of complement, it is possible that BA184 is cleared
by complement-mediated lysis and may reach the spleen only in small
numbers (1, 11, 13). The transposon insertion in BA100
rendered this mutant defective in the biosynthesis of aromatic amino
acids, as determined by auxanography. This biosynthesis pathway is also
required for the biosynthesis of 2,3-dihydroxybenzoic acid, the only
siderophore known to be produced by B. abortus
(23). However, since this siderophore has been shown to be
dispensable for growth in mice (7), it is more likely that
attenuation of this mutant is the result of its inability to acquire
aromatic amino acids in the host. Salmonella aro mutants are
unable to survive and replicate within macrophages and are attenuated
for virulence (19). Thus, some of the virulence genes
required in an early phase during chronic B. abortus
infection may be similar to those used by intracellular pathogens, such
as S. enterica serovar Typhimurium, which cause an acute
infection. Two mutants (BA114 and BA41) defective for initiation of
chronic infection carried insertions in a putative type IV secretion
system of B. abortus, encoded by the virB
genes (27). Mutant BA114 (virB10) displayed a
greater competitive colonization defect in murine spleens at 2 weeks
postinfection than BA41 (virB1) (Table 1). A similar effect
has been described for the homologues of the B. abortus
virB10 and virB1 genes present in the genome of the
plant pathogen Agrobacterium tumefaciens. Inactivation of
virB1 in A. tumefaciens causes a lower degree of
attenuation than a mutation in virB10 (8).
Mutations in the virB locus render B. suis unable
to multiply in HeLa cells or macrophage cell lines in vitro
(27). These data, together with our findings that B. abortus virB1 and virB10 mutants are unable to persist
in mouse spleens after i.p. inoculation, suggest that attenuation in
the animal model is due to an inability of these strains to grow intracellularly.
The second class of mutants, which were unable to maintain chronic
infection, included strains defective in production of glutamate
synthase (BA152), glycine cleavage (BA102), nutrient uptake (BA159),
and several unknown functions (BA31, BA38, BA73, BA87, BA63, BA122, and
BA142). While the inactivated genes in these mutants were not required
for initiation of infection, they were required for chronic
persistence. Mutant BA102 carried a transposon insertion in a gene with
homology to gcvB, encoding glycine dehydrogenase, from
M. tuberculosis. The activity of this enzyme has been found
to increase 10-fold upon entry of M. tuberculosis into a
state of nonreplicating persistence in vitro (31). The finding that glycine dehydrogenase is required for persistence of
B. abortus in the mouse spleen suggests that M. tuberculosis and B. abortus may depend on similar
metabolic pathways for chronic persistence in the host. This result
underscores the potential for research on host pathogen interactions of
B. abortus to elucidate mechanisms of intracellular
persistence which are shared by other chronic intracellular pathogens.
| |
ACKNOWLEDGMENTS |
We thank Andreas Bäumler for critical comments on the
manuscript and Garry Adams for helpful discussions throughout the
course of this work.
Work in T.A.F.'s laboratory is supported by USDA/BARD Project No.
US-2781-96 and Animal Formula Health AH8675. P.C.H. was supported by
Food and Agriculture Science Fellowship 96-38420-3059 from USDA.
R.T. was supported by National Research Service Award AI10050 from
NIH/NIAID.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Veterinary Pathobiology, College of Veterinary Medicine, Texas A&M
University, College Station, TX 77843-4467. Phone: (979) 862-4779. Fax:
(979) 862-1088. E-mail: rtsolis{at}cvm.tamu.edu.
Editor:
A. D. O'Brien
| |
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Infection and Immunity, July 2000, p. 4102-4107, Vol. 68, No. 7
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Abstract
Introduction
