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Infection and Immunity, March 1999, p. 1025-1033, Vol. 67, No. 3
Biophysics Division, Indian Institute of
Chemical Biology, Calcutta 700 032, India
Received 2 September 1998/Returned for modification 9 November
1998/Accepted 8 December 1998
The dnaK gene of Vibrio cholerae was
cloned, sequenced, and used to construct a dnaK insertion
mutant which was then used to examine the role of DnaK in expression of
the major virulence factors of this important human pathogen. The
central regulator of several virulence genes of V. cholerae
is ToxR, a transmembrane DNA binding protein. The V. cholerae
dnaK mutant grown in standard laboratory medium exhibited
phenotypes characteristic of cells deficient in ToxR activity. Using
Northern blot analysis and toxR transcriptional fusions, we
demonstrated a reduction in expression of the toxR gene in
the dnaK mutant strain together with a concomitant increase
in expression of a htpG-like heat shock gene that is located immediately upstream and is divergently transcribed from toxR. This may be due to increased heat shock induction in
the dnaK mutant. In vivo, however, although expression from
heat shock promoters in the dnaK mutant was similar to that
observed in vitro, expression of both toxR and
htpG was comparable to that by the parental strain. In both
strains, in vivo expression of toxR was significantly
higher than that observed in vitro, but no reciprocal decrease in
htpG expression was observed. These results suggest that
the modulation of toxR expression in vivo may be different from that observed in vitro.
Vibrio cholerae, a
noninvasive, gram-negative bacterium, is the causative agent of the
diarrheal disease cholera. For successful infection of the human host,
orally ingested V. cholerae cells must colonize the
intestine and produce cholera toxin (CT), a potent enterotoxin that
causes the severe watery diarrhea characteristic of the disease. A
toxin-coregulated pilus (TCP) coordinately expressed with CT greatly
enhances colonization of the intestinal epithelium by the bacterium.
Additional factors, including those necessary for survival of V. cholerae cells in the intestine, those required for evasion of the
host defense system, adhesins, and accessory colonization factors, and
other potential toxins, may also contribute to the virulence of this
important human pathogen (17).
One regulatory pathway, controlling the expression of a subset of
virulence factors of V. cholerae, that has been most
extensively characterized is the ToxR-ToxT system (10).
ToxR, a transmembrane DNA binding protein, directly activates
expression of toxT, and the resulting enhanced level of ToxT leads to
increased expression of other genes of the ToxR regulon, including
those coding for CT and TcpA, the major subunit of TCP. Thus, in the
virulence regulatory cascade of V. cholerae, ToxR is at the
top of the hierarchy, ToxT is at the next level, and a number of
virulence genes under control of ToxT are at the lowest level
(10). However, it has recently been shown that production of
OmpU, an osmoregulated outer membrane porin of V. cholerae,
is independent of ToxT, although OmpU is a member of the ToxR regulon
(5). Interestingly, in addition to its role as a
transcriptional activator, ToxR can also function as a negative
regulator, as suggested by the increased motility (12) and
higher levels of production of an outer membrane protein OmpT in
toxR mutants (28).
It has been hypothesized that the ToxR protein, probably by virtue of
its location in the cytoplasmic membrane (29), can sense
certain environmental parameters, leading to modulation of the
ToxR-dependent expression of virulence genes in response to the
external environment of the bacteria (40). It is now evident
that a common strategy among pathogenic organisms is the exploitation
of physical and chemical parameters that distinguish host from external
environments as signals for the coordinate expression of virulence
factors. This regulation presumably allows the bacteria to avoid
unnecessary expenditure of energy resources to produce virulence
factors under conditions where they would not be required. Thus, in
most pathogens environmental conditions characteristic of the
physiological sites of infection activate central regulators of
virulence determinants (6, 23). However, in the case of
V. cholerae biotype classical, a paradoxical situation exists, in that the intestinal environment may be presumed to display
parameters similar to the nonpermissive conditions for induction of the
ToxR regulon. The ToxR regulon is maximally expressed in cells grown at
30°C in media with a starting pH of 6.6 and osmolarity equivalent to
66 mM NaCl (28, 40). In the intestinal lumen, the
temperature is 37°C, pH is alkaline, and osmolarity is thought to be
equivalent to 300 mM NaCl or higher (42), conditions that
repress the expression of ToxR-activated virulence factors in the
laboratory. Although there is no doubt that ToxR is essential for
successful infection, the mechanism for activation of the ToxR regulon
in vivo is not clear. The possibility remains that the intestinal
environment induces the production of additional virulence regulatory
factors which could not be detected during in vitro growth of the cells
simply because the conditions necessary for their induction are not
known and hence could not be reproduced in the laboratory. Recently, a
factor which is induced specifically after infection of the small
intestine has been identified, although its precise role in virulence
has not been determined (21).
In the course of the transition from the external environment to the
human body, V. cholerae cells are exposed to a series of
environmental changes, some of which are known to be stressful for
bacteria, such as a sudden increase in temperature or heat shock, low
pH in the stomach, bile salts in the intestine, and also perhaps
anaerobiosis and starvation. Several of these stressful stimuli are
known to trigger the enhanced synthesis of the evolutionarily conserved
and abundant heat shock protein DnaK, a member of the Hsp70 family
(22). Although primarily induced by heat shock (2), increased DnaK synthesis has also been reported in
response to oxidative stress (30), osmotic stress
(24), and starvation (13). In addition to its
fundamental role as a molecular chaperone in protein folding with the
functional cooperation of two other heat shock proteins, DnaJ and GrpE,
DnaK is involved in DNA replication, RNA synthesis, ribosome assembly,
protein transport, and cell division (15). In
Escherichia coli, DnaK, DnaJ, and GrpE negatively modulate
the induction of the heat shock response by decreasing the stability,
and perhaps also the synthesis, of the heat shock sigma factor Bacterial strains, plasmids, and media.
All bacterial
strains and plasmids used in this study are listed in Table
1. The V. cholerae and
E. coli strains were maintained at
0019-9567/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Role of DnaK in In Vitro and In Vivo Expression of
Virulence Factors of Vibrio cholerae
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
32,
which is specifically required for transcription from heat shock
promoters (4, 46). Of particular interest in the study of
microbial pathogenesis is evidence that DnaK may be involved in the
survival of bacterial pathogens in their hosts and pathogenicity in
vivo. It has been reported that DnaK is required for multiplication of
the intracellular bacterium Brucella suis in a human
macrophage-like cell line (19). DnaK has also been shown to
be among the dominant antigens recognized in immune response to a broad
spectrum of pathogens, including V. cholerae (34, 45). It was in this context that the V. cholerae dnaK
gene was cloned and a dnaK mutant was constructed and
characterized in the present study to elucidate a potential role of
DnaK in the survival of V. cholerae in the intestinal
environment and in the regulation of expression of virulence determinants.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
70°C in LB medium
containing 20% (vol/vol) glycerol. E. coli cells were grown
in LB medium, and V. cholerae cells were grown in LB, M9, or
Syncase (11) medium. Ampicillin (100 µg
ml
1), streptomycin (150 µg ml1),
chloramphenicol (30 µg ml1), and kanamycin (30 µg
ml1) were used where appropriate. Plasmids were
introduced into V. cholerae strains either by transformation
(32) or by triparental mating using E. coli
MM294(pRK2013) as a donor of mobilization factors.
TABLE 1.
Bacterial strains and plasmids used in the study
except pGP704,
which was maintained in E. coli SM10 (28).
DNA preparation and manipulation.
Genomic DNA from V. cholerae 569B was prepared from proteinase K-digested and
cetyltrimethylammonium bromide-precipitated cell lysates by using
standard procedures (1). Plasmid DNA was prepared by the
alkaline lysis method (36). Restriction enzymes and
DNA-modifying enzymes were purchased from New England Biolabs Inc.
(Beverly, Mass.) and used according to the manufacturer's recommendation. For Southern blotting, restriction enzyme-digested chromosomal or plasmid DNA was electrophoresed on 1% agarose gels and
blotted onto nylon membranes (Nytran; Schleicher & Schuell), using 10×
SSC (1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate) (36). The blots were hybridized with DNA fragments labelled with [32P]dCTP (Amersham International, Amersham, United
Kingdom) prepared by using a random-primed labelling kit (New England
Biolabs). Subgenomic libraries of V. cholerae DNA were
constructed in plasmid pACYC177. Genomic DNA was digested with an
appropriate restriction enzyme, and the fragments within the size range
of interest were excised from agarose gels, purified, ligated with
linearized and dephosphorylated plasmid pACYC177, and transformed into
E. coli DH5 according to standard recombinant DNA
techniques (36).
Construction of a V. cholerae dnaK mutant
strain.
A 0.6-kb HincII fragment of the V. cholerae dnaK gene (Fig. 1) was
cloned at the EcoRV site of the suicide vector pGP704 and transformed into a 
pir lysogen of E. coli
SM10 (28). Ampicillin-resistant transformants containing
recombinant plasmids were selected and mated with V. cholerae O395 (Smr) on LB agar plates. Transconjugants
resistant to both ampicillin and streptomycin were selected, and
Southern blot analysis was used to confirm that integration had
occurred into the chromosomal dnaK gene.
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Construction of transcriptional fusions to promoterless reporter genes. The heat shock promoter of the V. cholerae dnaK gene was isolated as a 550-bp EcoRI-HincII fragment from plasmid pSC350 (Fig. 1) and cloned at the BamHI-HindIII site of plasmid pKK232.8 by using appropriate linkers to give plasmid pSChs. A 220-bp BamHI-EcoRV fragment carrying the V. cholerae htpG-toxR intergenic region was excised from plasmid pVM7 (27) and cloned at the BamHI-StuI site of plasmid pTAC3704 to give plasmid pSCGR (Fig. 8). To construct a toxR-cat transcriptional fusion, the BamHI-EcoRV fragment of plasmid pVM7 was cloned at the BamHI-HindIII site of plasmid pKK232.8 with appropriate linkers, to give plasmid pNS1. To construct htpG-cat transcriptional fusion, the BamHI-EcoRV fragment was cloned in an inverse direction at the SmaI-SalI site of plasmid pKK232.8 to give plasmid pNS2.
RNA isolation and analysis. For isolation of RNA, cells were grown to the late logarithmic phase in LB (pH 6.6) at 30°C, conditions optimum for production of CT, TcpA, and ToxR. Total RNA was extracted and purified by using guanidinium isothiocyanate as described elsewhere (1). RNA samples (15 to 25 µg/well) were electrophoresed in duplicate in 1% agarose-2.1 M formaldehyde-morpholinepropanesulfonic acid gels, and one part was stained with ethidium bromide and visualized with UV light to confirm equal loading of all samples. The other part of the gel was blotted onto nylon membranes by using 20× SSC and hybridized with labelled probes as described elsewhere (14).
Assays for 
-galactosidase, alkaline phosphatase, and CAT
activities.
-Galactosidase and alkaline phosphatase activities
were assayed in permeabilized cells or culture supernatants by
measuring the hydrolysis of o-nitrophenyl galactopyranoside
or p-nitrophenyl phosphate, respectively (26).
Chloramphenicol acetylphosphatase (CAT) activity was measured in
sonicated cell lysates by using a Quan-T-CAT kit (Amersham) according
to the manufacturer's instructions and expressed as milliunits of
enzyme. The results presented represent the average of at least five
independent experiments.
Isolation of outer membrane proteins.
V. cholerae O395
and O395K1 were grown in LB medium to about 109 CFU
ml1, and cell lysates were separated into subcellular
fractions as described previously (34). The outer membrane
fraction was solubilized, and outer membrane proteins were analyzed by
sodium dodecyl sulfate-12.5% polyacrylamide gel electrophoresis
(SDS-PAGE) followed by staining with Coomassie blue (20).
Swarm plate assay. V. cholerae cells were stabbed into semisolid agar plates containing LB (pH 6.6 or 8.6) with 0.3% Bacto Agar (Difco). The plates were incubated at 30 or 37°C for 16 to 18 h, and swarm diameters were measured.
GM1-ganglioside dependent ELISA for assay of CT. CT production was assayed in V. cholerae culture supernatants, sonicated cell pellets, or fluid collected from rabbit ileal loops by GM1 enzyme-linked immunosorbent (ELISA) using polyclonal rabbit serum directed against purified CT. Dilutions of purified CT of known concentration (Sigma) were used to estimate the amount of CT in the samples.
Western blot procedure. Western immunoblot analysis was performed by the electrophoretic separation of total cellular proteins by SDS-PAGE followed by transfer to nitrocellulose membranes in a Transblot apparatus (Bio-Rad) (44). The DnaK protein was detected by using rabbit anti-E. coli DnaK polyclonal antisera and the Proto Blot system (Promega).
DNA sequencing.
Nucleotide sequence was determined with
double-stranded plasmid DNA as the template either by the dideoxy-chain
termination method (37) or by cycle sequencing using the
Applied Biosystems Prism dye system (Perkin-Elmer). For dideoxy
sequencing, [-35S]dATP and a Sequenase 2.0 DNA
sequencing kit (U.S. Biochemical Corp.) were used according to the
manufacturer's instructions. In some experiments, oligonucleotides
designed from sequences obtained previously were used as primers.
Ligated rabbit ileal loop model.
In vivo growth and CT
production by strains O395 and O395K1 were assayed by using the ligated
rabbit ileal loop model essentially as described by De and Chatterjee
(9). Briefly, rabbits fasted for 48 h were
anesthetized, and the small intestine was tied into consecutive 6- and
2-cm segments proximal to the mesoappendix. An inoculum of 0.5 ml of
V. cholerae strains containing about 5 × 106 CFU was introduced into each 6-cm segment, while one
loop was inoculated with saline as a negative control. The intestine
was returned to the peritoneal cavity, and the incision was closed. After 16 to 18 h, the animals were sacrificed and the small
intestine was removed. Fluid accumulated in each loop was separately
collected and measured, after which the loops were slit open and
scraped. The fluid and scrapings were centrifuged (8,000 × g, 5 min) to collect the bacteria as a pellet, washed twice
with normal saline, and finally resuspended in saline. Bacterial count
in the suspension was measured by plating on thiosulfate-citrate-bile
salt-sucrose (TCBS) agar plates containing appropriate antibiotics.
-Galactosidase, alkaline phosphatase, and CAT activities in a
measured amount of the in vivo-grown cells were assayed as described
above. CT in the fluid was measured by GM1 ELISA. Although no fluid
accumulated in the loops inoculated with saline, these loops were also
washed and scraped, and CFU, -galactosidase, alkaline phosphatase,
CAT, and CT were assayed in the scrapings and washings to determine whether the intestine contained any inhabitant flora and also to
estimate if the normal intestinal content interfered with the enzymatic
assays or GM1 ELISA. At least two loops in the same animal were
inoculated with each bacterial strain, and each strain was tested in at
least five individual animals.
Statistical analysis. Comparison among results obtained from in vitro and in vivo experiments were made by the two-sample t test.
Nucleotide sequence accession number. The nucleotide and deduced amino acid sequences of the V. cholerae dnaK gene appear in EMBL, GenBank, and DDBJ databases under accession no. Y14237.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The dnaK gene of V. cholerae: cloning,
nucleotide sequence, and complementation of E. coli
mutants.
The V. cholerae dnaK gene was cloned by
screening a subgenomic library, using an E. coli dnaK gene
fragment (31) as a probe. Construction of the plasmid
carrying the V. cholerae dnaK region is shown in Fig. 1.
Plasmid pSC830 could functionally complement the temperature-sensitive
and phage-resistant phenotypes of E. coli dnaK mutant
strains CG800 and GW4813 (31, 41) and also the E. coli
dnaJ mutant CG2682 (Fig. 1) (38). The recombinant V. cholerae DnaK protein coded by plasmid pSC830 was
detected by immunoblot analysis using anti-E. coli DnaK
sera. In heat-shocked cell lysates of E. coli GW4813
(
dnaK) carrying plasmid pSC830, anti-E. coli
DnaK sera cross-reacted with a 70-kDa protein that comigrated with the
E. coli and native V. cholerae DnaK proteins (Fig. 2). No immunoreactive band was
detected in the lysates of strain GW4813 carrying vector plasmid alone
(Fig. 2, lane a).
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32-specific
promoters P1 and P2 were identified by comparison with the consensus
35 and 10 sequences of E. coli heat shock promoters (Fig. 3) (8). The 13-bp spacer
region between the 35 and 10 sequences in both promoters is
characteristic of promoters of heat shock genes. Downstream of the
dnaK gene, we detected the 5' end of an ORF which has about
64% homology with the dnaJ gene of E. coli over
a stretch of 256 nucleotides at the 5' end (3). However, the
noncoding intergenic region was not conserved and was larger (200 nucleotides) than in E. coli (88 nucleotides). A weak
promoter-like sequence and ribosome binding site were detected in the
intergenic sequence. Analysis of the sequence upstream of the
dnaK gene revealed a region coding for 44 amino acids which has significant homology with the C-terminal end of GrpE proteins. Thus, the genomic organization of the dnaK, dnaJ,
and grpE genes in V. cholerae is
grpE-dnaK-dnaJ (Fig. 1B).
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Construction of V. cholerae dnaK mutant. Site-directed insertion mutation in the V. cholerae dnaK gene was constructed by chromosomal integration of the mobilizable suicide plasmid pGP704 (28), containing an internal 0.6-kb HincII fragment (Fig. 1) of the cloned dnaK gene. That the mobilized plasmid had integrated into the genome at the desired site in the dnaK gene was confirmed by Southern blot analysis (data not shown).
Similar to the E. coli dnaK mutants (31), the dnaK mutant of V. cholerae designated O395K1 was temperature sensitive for growth at 42°C, and prolonged incubation at 42°C rendered the mutant nonviable, as it was no longer capable of growth even at 30°C. The growth defects of the mutant could be complemented by plasmid pSC830, carrying the V. cholerae dnaK gene and also by plasmid pKP31, carrying the E. coli dnaK gene. The mutant could not be complemented by plasmid pSC510, carrying the V. cholerae dnaJ gene (Fig. 1). Unlike E. coli dnaK null mutants, in which growth at 30 and 37°C has been reported to be slower than in the wild-type strains (31), the growth rate of the V. cholerae dnaK insertion mutant at 30 and 37°C was comparable to that of the parental strain.CT and TcpA production is reduced in the V. cholerae dnaK mutant. To examine if DnaK has any role in virulence of V. cholerae, production of CT, the major virulence factor of the organism, was examined in the dnaK mutant strain O395K1. When grown in LB medium (pH 6.6) at 30°C, conditions optimum for CT production (28), although the parental strain O395 produced about 1 mg of CT per unit of optical density at 600 nm, only about 100 ng of CT could be detected in culture supernatants of the dnaK mutant strain. Practically no CT was detected in culture supernatants of V. cholerae toxR mutant strain JJM43 (16), used as control. Thus, CT in culture supernatants of strain O395K1 was reduced by more than 90% compared to the parental strain O395 when both strains were grown under conditions favorable for optimum CT production (Fig. 4). Similar results were obtained when the cells were grown in M9 or Syncase medium. Upon growth at 37°C, only about 20% of the amount of CT produced at 30°C was detected in strain O395, whereas a negligible amount of CT was produced by strain O395K1 (Fig. 4). The amount of CT in sonicated cell pellets of the parental and mutant strains was determined, and in both cases no CT was detected in the cell pellets by GM1 ELISA, indicating that production and not secretion of CT is drastically reduced in the dnaK mutant, even under conditions that normally promote high levels of CT production.
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and
O395K1 
. Cells were grown in LB (pH 6.6) at 30°C, in LB (pH 8.6)
at 37°C, or in rabbit ileal loops, and CFU per milliliter was
assayed. CT was measured in culture supernatants or intestinal fluids
corresponding to 109 CFU and expressed as a percentage of
the amount obtained in culture supernatants of strain O395 grown at pH
6.6, 30°C.
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Outer membrane proteins. The two major outer membrane porins of V. cholerae are OmpU (38 kDa) and OmpT (40 kDa). OmpU, together with CT and TcpA, is positively regulated by ToxR, whereas OmpT expression is apparently under negative regulation of ToxR (28). Since expression of both ctxAB and tcpA is significantly reduced in the dnaK mutant of V. cholerae, the levels of OmpU and OmpT were examined in the mutant. SDS-PAGE of outer membrane proteins indicate that OmpU is the major porin in strain O395, and OmpT was not detectable in the outer membrane of this strain under conditions used in this study (Fig. 6). Under the same conditions, however, we detected a substantial amount of OmpT in the dnaK mutant (Fig. 6). The other outer membrane proteins were unaffected in the dnaK mutant strain except for a 23-kDa minor protein, the level of which was slightly increased. A 23-kDa minor outer membrane located protein has previously been identified as a heat shock protein (34).
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Swarm plate assays. It has recently been reported that expression of the major virulence factors and motility are reciprocally regulated in V. cholerae (12). Since production of both CT and TcpA is drastically reduced in the dnaK mutant of V. cholerae, the swarming ability of these cells in semisolid motility medium was examined. Under ToxR-inducing conditions at 30°C, the parental strain O395 displayed little motility in the swarm plates (Fig. 7A). However, the dnaK mutant strain O395K1 was significantly more motile, and a 150% increase in swarm diameter was observed (Fig. 7A). The motility of strain O395 was somewhat higher at 37°C than at 30°C. A further 150% increase in swarm diameter was observed in strain O395K1 (Fig. 7B).
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CT production in vivo.
In view of the fact that a mutation in
the dnaK gene significantly reduced expression of the major
virulence genes of V. cholerae cells grown in the
laboratory, we used the ligated rabbit ileal loop model (9)
to examine the in vivo effect of the mutation. A major advantage of
this model is that it allows comparative studies between parental and
mutant strains simultaneously in the same animal, thus avoiding
variations among individual animals. Strains O395 and O395K1 were
injected separately into ligated ileal loops (about 5 × 106 CFU), and after 16 to 18 hours, the animals were
sacrificed and the loops were examined. Almost equal amounts of fluid
accumulated in loops inoculated with either strain O395 or O395K1. The
contents of each loop were separately collected, and the number of
bacteria as well as amounts of CT present in each loop was determined
as described in Materials and Methods. Both strains grew to a density of 2 × 109 to 3 × 109 CFU
ml1 the ileal loops. In contrast to the results obtained
from in vitro experiments, estimation of CT in intestinal fluids
indicate that on a per-cell basis, the amounts of CT produced in the
intestinal loops by strains O395 and O395K1 were almost equal and about
160% of the amount produced by strain O395 in LB medium (pH 6.6) at 30°C (Fig. 4).
Expression of toxR in vitro and in vivo.
To
investigate the mechanism behind the dramatic difference in CT
production by the V. cholerae dnaK mutant under in vitro and
in vivo conditions, the expression of toxR was examined in cells grown in vitro or in vivo. Northern blot analysis revealed that
expression of the toxR gene was substantially reduced in the
dnaK mutant strain O395K1 grown in vitro even under
ToxR-inducing conditions (Fig. 5C), which may account for the decrease
in CT production observed in vitro (Fig. 4). Since Northern blot
experiments with RNA isolated from cells grown in the rabbit intestine
did not give clear results, a reporter plasmid (pNS1) carrying a
toxR-cat transcriptional fusion was constructed as described
in Materials and Methods. The plasmid as well as the control vector
pKK232.8 were conjugally transferred into V. cholerae O395
and O395K1, and CAT activity was assayed in the transconjugants grown
either in LB medium or in rabbit ileal loops. In agreement with a
previous report that an increase in growth temperature is accompanied
by a decrease in toxR expression (33), in LB
medium the parental strain O395 carrying plasmid pNS1
(toxR-cat) showed 1.5-fold-lower CAT activity at 37°C than
at 30°C. A twofold decrease in toxR expression was
observed between cells of strain O395K1 and strain O395 grown in LB
medium (pH 7.2, 37°C [Table 2]),
although a higher magnitude of reduction was observed by Northern blot
analysis (Fig. 5C). In contrast, when CAT activity was assayed in
strains O395 and O395K1 harboring plasmid pNS1 (toxR-cat)
grown in rabbit ileal loops, no statistically significant difference in
toxR expression was observed between the two strains
(P 
0.2 [Table 2]). Furthermore, a comparison of
CAT activity between in vivo- and in vitro-grown cells clearly
indicated a statistically significant (P = 0.001) increase in toxR expression in cells grown in vivo. On a
per-cell basis, we observed nearly 2.5-fold-higher CAT activity in
cells of strain O395 grown in LB medium (pH 7.2) at 37°C than in
cells grown in rabbit ileal loops. In strain O395K1, the increase in toxR expression between cells grown in vitro and in vivo was
even higher (Table 2).
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0.025). On a per-cell
basis, both cells O395 and O395K1 expressed comparable amounts of CAT
(Table 2).
Results were similar in assays using a reporter plasmid pSCGR in which
the htpG-toxR intergenic region was cloned in the promoter probe vector pTAC3734, which has an MCS between promoterless
phoA and lacZ genes. Plasmid pSCGR was
constructed in such a manner that the promoter of the toxR
gene directs transcription of the lacZ gene whereas
phoA expression is under the control of the htpG
promoter (Fig. 8A). With this plasmid,
the relative amounts of toxR and htpG expression
could be determined simultaneously under different conditions. Alkaline
phosphatase and -galactosidase activities were measured in cells
carrying plasmid pSCGR (htpG-phoA toxR-lacZ)
grown at either 37 or at 30°C in LB medium. We observed about
2-fold-higher alkaline phosphatase activity but 1.5-fold-lower -galactosidase activity in cells grown at 37°C than in cells grown
at 30°C. Thus, the temperature-dependent coordinate and reciprocal
effect on expression from toxR and htpG promoters
reported previously (33) was clearly demonstrated with
plasmid pSCGR. However, such coordinated expression of toxR
and htpG was not observed in vivo. When cells were grown in
rabbit ileal loops, although htpG expression was only
slightly higher than that observed in vitro at 37°C, toxR
expression was found to be about threefold higher (Fig. 8B). The
differences were statistically significant (P 
0.001).
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Heat shock induction in cells grown in vitro or in vivo.
To
examine the induction of the heat shock response in cells grown under
in vitro or in vivo conditions, we constructed a reporter plasmid,
pSChs, containing a heat shock promoter derived from the V. cholerae dnaK gene, fused to a promoterless cat gene in
plasmid pKK232.8. Very little CAT activity could be detected in the
E. coli rpoH mutant strain K165 (7) containing
plasmid pSChs, indicating that expression from the heat shock promoter in plasmid pSChs is dependent on 32. The plasmid was transferred to
V. cholerae O395 or O395K1 by conjugation, and CAT activity was assayed in the transconjugants grown either in LB medium at 37°C
or in rabbit ileal loops. A twofold increase in CAT activity was
observed between cells of strain O395 and O395K1 grown in LB medium at
37°C. Identical results were obtained when the cells were grown in
rabbit ileal loops (Table 2). Thus, the universal heat shock response
was not repressed in cells grown in the intestine, nor did we observe
any significant increase in heat shock induction in these cells.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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In this study, we present evidence that the highly conserved and
abundant heat shock protein DnaK influences the expression of
toxR and ToxR-regulated virulence factors of V. cholerae grown in standard laboratory media but has no effect on
toxR expression in cells grown in the intestine. The
dnaK gene was cloned from V. cholerae 569B, and
the identity of the cloned gene was confirmed by (i) phenotypic
complementation of E. coli dnaK mutants (Fig. 1), (ii)
immunological reactivity of the gene product with anti-E. coli DnaK sera (Fig. 2), and (iii) comparison of the nucleotide sequence with those of other dnaK and hsp70
genes. To study the role of DnaK in V. cholerae virulence, a
site-directed insertion mutation in the dnaK gene of the
wild-type strain O395 was constructed. The mutation produced phenotypes
characteristic of dnaK mutants, including sensitivity to
elevated growth temperatures and increased expression from promoters of
heat shock genes (Table 2) (31). Furthermore, the following
evidence suggests that mutation in dnaK has profound effects
on the expression of ToxR-regulated virulence factors: (i)
transcription of the ToxR-activated genes ctxAB and
tcpA (10) is drastically reduced in the
dnaK mutant strain O395K1 (Fig. 5), (ii) the level of the
ToxR-repressed outer membrane porin OmpT (28) is
significantly higher in the mutant than in the parental strain (Fig.
6), and (iii) motility of the cells which is negatively regulated by
ToxR (12) is also higher in the dnaK mutant (Fig.
7). Analysis of the expression of toxR-specific mRNA and of
a plasmid carrying a toxR-cat transcriptional fusion in the
wild-type O395 and mutant O395K1 strains confirmed that expression of
toxR was substantially reduced in the dnaK mutant (Fig. 5; Table 2). It is attractive to hypothesize that the control exerted by DnaK on transcription of the toxR gene is
indirect and possibly due to the negative modulatory effect of DnaK on the production and stabilization of 32, the heat shock sigma factor
(4, 46). The increased expression of a reporter
cat gene fused to a consensus heat shock promoter in the
V. cholerae dnaK mutant strain O395K1 suggested that as in
E. coli dnaK mutants, the level of active 32 in the
V. cholerae dnaK mutant strain O395K1 might be higher than
in the parental strain. It has previously been shown that an increase
in the level of 32 resulted in reduced toxR expression
(33). This effect was postulated to be due to an increase in
the divergent transcription of a htpG-like heat shock gene
by 32-RNA polymerase, which leads to a proportionate decrease in the
expression of the toxR gene by 70-RNA polymerase, due to
competition between RNA polymerase containing 32 or 70 for access
to the short region between htpG and toxR
(33). Consistent with this hypothesis, the higher levels of
active 32 in the dnaK mutant strain of V. cholerae may be correlated with increased htpG and
reduced toxR expression in the mutant compared to the wild-type strain. The increase in htpG expression was almost
proportional to the decrease in expression of toxR, further
confirming the coordinate but reciprocal relationship between
toxR and htpG expression proposed by Parsot and
Mekalanos (33).
Although this model very elegantly explains the low levels of CT
observed in cells grown in standard laboratory media at 37°C, it
raises fundamental questions regarding expression of the ToxR regulon
in vivo. In this study we demonstrate that toxR expression is significantly higher during growth at 37°C within the intestinal environment than in laboratory media (Table 2; Fig. 8). What could be a
possible mechanism for increased toxR expression in vivo?
Although many factors affect ToxR activity, the only parameter known to
control expression of toxR is temperature, and it is only a
decrease in the level of 32 that is known to produce an increase in
toxR expression, and vice versa. To address the possibility that the level of 32 at 37°C is actually lower in cells grown in
vivo than in cell grown in vitro, we have measured expression from a
standard heat shock promoter in cells grown either in LB medium at
37°C or within rabbit ileal loops. Since it has been shown that
expression of V. cholerae heat shock genes is dependent on
32 (33, 35), the results obtained clearly indicate that there is no difference in 32 levels between cells grown to the steady state at 37°C in vitro or in vivo (Table 2). Furthermore, when
cells were grown in the intestine, expression from the heat shock
promoter was about two times higher in the dnaK mutant
strain than in the wild-type strain, which is comparable to the results obtained from in vitro studies (Table 2). From these results, it may be
concluded that there is no mechanism that can specifically antagonize
the heat shock response during intraintestinal growth of V. cholerae which may account for the increased toxR
expression observed in these cells.
We next considered the possibility that access of 32-RNA polymerase
to the htpG-toxR intergenic region is specifically reduced during intraintestinal growth of V. cholerae. Using reporter
gene fusions to the htpG-toxR intergenic region, we have
shown that under in vitro conditions, expression from the
htpG promoter was significantly greater in the V. cholerae dnaK mutant O395K1 than in the parental strain O395,
consistent with the increased 32 level in strain O395K1. In vivo,
however, although the 32 level remained higher in strain O395K1 than
in strain O395, expression from the htpG promoter in strain
O395K1 was lower than that observed in vitro. These results indicate
that the access of 32-RNA polymerase to the htpG promoter
was specifically reduced in cells grown in vivo. It is likely that this
may be mediated by as yet unknown factors induced specifically during
in vivo growth of the cells. It may be noted that an essential feature
of the Parsot and Mekalanos model for heat shock control of
toxR expression is that any change in the level of
toxR expression should be coordinated with a reciprocal alteration in htpG expression. We observed that although
toxR expression was significantly increased between cells
grown in vitro and in vivo, the increase in toxR expression
is not accompanied by a reciprocal decrease in htpG
expression (Table 2; Fig. 8). We do not know whether, in addition to
increased expression, activity of ToxR is also altered during
intraintestinal growth of V. cholerae. Since experiments
were performed with cells grown overnight in rabbit ileal loops, we
have not been able to determine at which stage of the infection process
the increase in toxR expression actually occurs. Also, only
the steady-state level of heat shock induction in cells grown in vitro
or in vivo was considered. It is likely that immediately after
infection, stressful intestinal conditions may strongly induce the heat
shock response. Even if this were the case, it is doubtful whether the
higher level of heat shock induction could reduce toxR
expression in the early stages of infection, since in the
dnaK mutant, constitutively higher levels of heat shock
induction had no effect on toxR expression in vivo. If
expression of the ToxR-activated genes is indeed turned off at the
early stages of infection, as has been proposed, it is likely to be due
to a decrease in ToxR activity rather than a reduction in
toxR expression. In this context it may be mentioned that
bile, a major constituent of the intestinal lumen, drastically decreases the expression of several ToxR-activated genes without affecting expression of toxR itself (14). Similar
results have been reported for growth of V. cholerae cells
in media of alkaline pH or high osmolarity, parameters characteristic
of the intestinal environment (28).
Examination of virulence regulatory processes in many pathogenic bacteria has revealed that results obtained from laboratory analysis are often difficult to explain in the context of the in vivo situation (23, 25). In this study, we show that the model proposed for heat shock regulation of toxR expression from in vitro studies cannot be extrapolated to the in vivo situation. These studies reinforce a growing awareness that the regulation of virulence gene expression or environmental modulation of the regulatory processes in the complex and largely undefined environment of the animal body may be different from that observed under laboratory conditions.
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ACKNOWLEDGMENTS |
|---|
We are grateful to J. Das, Indian Institute of Chemical Biology, for generous advice and all members of the biophysics division for helpful discussions. We thank John J. Mekalanos, Department of Microbiology and Molecular Genetics, Harvard Medical School, Boston, Mass., for the generous gift of plasmids pGP704, pVM7, and pSC 18.1 and V. cholerae JJM43; Costa Georgopoulos, Department of Medicine, University of Geneva, Geneva, Switzerland, for kindly providing E. coli CG2682 and CG800; and Graham Walker, Biology Department, Massachusetts Institute of Technology, Cambridge, for the kind gift of E. coli GW4813, plasmid pKP31, and anti-E. coli DnaK antisera. We thank I. Guhathakurta for excellent technical support.
The work was supported by research grants SP/SO/D-56/96 from the Department of Science and Technology and BT/PRO411/Med/09/086/96 from the Department of Biotechnology, Government of India. S.C. is grateful to the Council of Scientific and Industrial Research for a research fellowship.
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FOOTNOTES |
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* Corresponding author. Mailing address: Biophysics Division, Indian Institute of Chemical Biology, 4 Raja S.C. Mullick Road, Calcutta 700 032, India. Phone: 91 33 473 0350. Fax: 91 33 473 0350/5197. E-mail: iichbio{at}giascl01.vsnl.net.in.
Present address: Department of Cell Biology, Yale University School
of Medicine, New Haven, Conn.
Editor: D. L. Burns
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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