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Infection and Immunity, March 1999, p. 1194-1200, Vol. 67, No. 3
Departments of
Neurology1 and Hygiene and
Microbiology,
Received 13 July 1998/Returned for modification 16 September
1998/Accepted 24 November 1998
Campylobacter jejuni is a leading cause of infectious
diarrhea throughout the world. In addition, there is growing evidence that Guillain-Barré syndrome, an inflammatory demyelinating
disease of the peripheral nervous system, is frequently preceded by
C. jejuni infection. In the present study, the
hrcA-grpE-dnaK gene cluster of C. jejuni was
cloned and sequenced. The dnaK gene consists of an open
reading frame of 1,869 bp and encodes a protein with a high degree of
homology to other bacterial 70-kDa heat shock proteins (HSPs). The
overall percentages of identity to the HSP70 proteins of
Helicobacter pylori, Borrelia burgdorferi,
Chlamydia trachomatis, and Bacillus subtilis
were calculated to be 78.1, 60.5, 57.2, and 53.8%, respectively.
Regions similar to the Escherichia coli Campylobacter jejuni is a
bacterial enteric pathogen of increasing medical interest. It is
currently regarded as a leading cause of infectious diarrhea throughout
the world (35). Particularly, Campylobacter
infection is endemic in developing countries, where it contributes
considerably to diarrheal disease among young children (38).
There is growing evidence that Guillain-Barré syndrome (GBS), a
rare but potentially devastating disease of the peripheral nervous
system, is frequently preceded by a C. jejuni infection (27). It has been estimated that in the United States about 1 in every 1,000 cases of C. jejuni infection is followed by
GBS (23). In spite of the obvious importance of this
microorganism, remarkably little is known about the molecular
mechanisms involved in virulence, pathogenesis, and immune response
during Campylobacter-host interaction (20). Only
a few definite protein antigens have been characterized so far.
Reconvalescent-phase sera usually react with the 65-kDa flagellin, the
44-kDa major outer membrane protein, and 25- to 29-kDa surface proteins
(7, 12, 24, 43). PEB1, which has been proposed to function
as an adhesin for adherence of the bacterium to eukaryotic cells, is
highly immunogenic (26), and Campylobacter
trigger factor has recently been revealed to be a humoral antigen in
the human host (16).
GroEL- and GroES-like heat shock proteins (HSPs) of C. jejuni have been shown to elicit a serum immunoglobulin G (IgG) as well as a secretory IgA response in experimentally infected rabbits (46). HSPs are synthesized in virtually all cells under
conditions of stress, e.g., as a result of temperature or nutrient
change. The best-characterized HSPs belong to the 60-kDa (GroEL) and
70-kDa (DnaK) families and are the most conserved proteins known.
Bacterial HSPs have aroused the interest of microbiologists for many
years, since they represent major targets of the host's immune
response (19). Although less extensively studied than GroEL,
DnaK homologues of many bacterial pathogens have been found to be
immunogenic in humans or animals (1, 2, 5, 8, 10, 47).
Furthermore, as has been shown by the experimental infection of mice
with Borrelia burgdorferi, immunization with proteins
containing DnaK-specific sequences may protect against microbial
infection (4).
Growing evidence suggests that there are two paradigmatic mechanisms in
bacterial heat shock regulation. In the gram-negative species
Escherichia coli, heat induction is mediated by the
alternative sigma factor We are interested in the heat shock response of C. jejuni
and in the role of this organism's heat shock proteins as putative immune targets in infectious and autoimmune diseases. As a part of this
work, the hrcA-grpE-dnaK gene cluster from C. jejuni was cloned and sequenced. The protein encoded by
dnaK was expressed in E. coli, and the humoral
response against this protein in C. jejuni-infected patients
and in healthy individuals was examined.
Bacterial strains, vectors, and reagents.
The C. jejuni strain used in this study was isolated in the Department of
Hygiene and Microbiology of the University of Würzburg and
serotyped as Lior 11. E. coli BL21(DE3) and plasmid
pET-22b(+) were purchased from Novagen (Madison, Wis.). pCR-Script
SK(+) plasmid and XL-1 blue MRF' Kanr supercompetent cells
were purchased from Stratagene (La Jolla, Calif.). Vent polymerase and
restriction enzymes were obtained from New England Biolabs (Beverly,
Mass.).
Bacterial cultivation and DNA purification.
C.
jejuni was routinely grown on agar plates at 37°C in a
microaerophilic environment (5% O2, 10% CO2).
To induce heat shock, surface-grown bacterial cells were harvested,
subcultured to brain heart broth supplemented with 1% yeast extract
(BHIYE) (46), and subsequently shifted to 48°C for 5 to 60 min. E. coli strains were grown at 37°C on Luria-Bertani
agar or in Luria-Bertani broth supplemented with ampicillin at a final
concentration of 50 µg ml Molecular cloning of the dnaK gene cluster.
Two
degenerate oligonucleotide primers,
5'-GG(A/T)AT(A/T)GA(C/T)(C/T)T(A/G/T)GGIACIAC(A/C/T)AA(C/T)TC-3'
and
5'-CC(A/T)GC(A/G/T)ATI(C/T)(G/T)(A/G/T)CCIGC(A/G)TC(C/T)TT-3', were synthesized according to highly conserved regions of bacterial HSP70 proteins (corresponding to amino acids [aa] 6 to 14 and aa 155 to 162 of E. coli DnaK, respectively). PCR was conducted with a GeneAmp 9600 PCR system (Perkin-Elmer), using the following cycle parameters: 94°C for 30 s, 52°C (42°C during the first
5 cycles) for 30 s, and 72°C for 1 min for 40 cycles. PCR
products were ligated with pCR-Script SK(+), cloned into XL1-Blue MRF' Kanr supercompetent cells, and sequenced. One 480-bp
fragment, which exhibited high nucleotide sequence homology to
bacterial dnaK sequences, was 32P labeled by
random priming (14). A plasmid library was constructed by
digesting C. jejuni genomic DNA with BglII and
cloning the resulting fragments into pET-22b(+). The library was
screened with the radiolabeled 480-bp PCR product in accordance with
standard procedures (30). Sequencing revealed that one
recovered clone (pdnaK1) with a 1.6-kb insert contained the 3' end of
the putative hrcA gene, the entire grpE gene, and
the 5' end of the dnaK gene. The missing parts of the
hrcA and the dnaK genes were obtained by a
PCR-based genomic walking strategy as recently described (39). Briefly, seminested PCRs were performed by using two
sequence-specific oligonucleotides oriented toward the unknown 3' end
and a random oligonucleotide as the reverse primer, which was used in
both the inner and outer PCRs. For each genomic walking step, 10 to 15 arbitrarily chosen primers previously available in our lab were tested.
To obtain the missing dnaK 3' end, two rounds of randomly
primed PCR (with random primers 5'-CTCCAAAAACTCATCCTGTACCTT-3' and 5'-CCTAAATCTCCAGACAAAGCTCAC-3', respectively) were
necessary. A PCR product containing the 5' end of hrcA was
amplified by using random primer 5'-CACGGGAGACTTGGAAAACAC-3'.
The resulting amplicons were cloned into pCR-Script SK(+) vectors
and sequenced.
DNA sequence analysis.
The DNA sequence was determined on
both strands by using a ABI Prism Dye Terminator Cycle Sequencing Kit
(Applied Biosystems, Foster City, Calif.). DNA sequencing was performed
on an ABI model 373A automated sequencer (Applied Biosystems). Nucleic
acid and predicted amino acid sequence data were analyzed by using the DNASIS software package (Hitachi, Tokyo, Japan). The Helicobacter pylori DNA sequences were obtained from the Institute for Genomic Research website (18a).
Northern blot analysis.
Total RNA was isolated by using
TRIzol reagent (Gibco BRL, Gaithersburg, Md.) as recommended by the
manufacturer. To generate a probe, a 539-bp DNA product internal to
dnaK was amplified by using oligonucleotide primers
5'-TCACGCAAATCATCAAGAGCT-3' and 5'-ACTTGATGTTACTCCGCTCTCT-3' and then 32P
labeled. Ten micrograms of total RNA was size separated in a formaldehyde-containing denaturing 1.2% agarose gel. Northern blotting
and hybridization were performed according to standard procedures
(3). Filters were autoradiographed at Primer extension analysis.
Transcriptional start sites were
determined by primer extension analysis using 5'-IRD800-labeled
oligonucleotides (MWG-Biotech, Ebecsberg, Germany).
5'-CATACAC-AGCAACACAAGAATT-3' is complementary to
nucleotides +37 to +58 relative to the dnaK start codon,
5'-TATCTTGCAAATCATCCTGC-3' is complementary to nucleotides
+57 to +76 relative to the grpE translation start site, and
5'-ATAGGCGCATTATCCAAAAG-3' is complementary to nucleotides
+58 to +77 relative to the hrcA start codon. Total RNA was
isolated from C. jejuni cells that had been heat shocked for
20 min at 48°C. Contaminating DNA was removed by DNase I (Gibco BRL)
treatment. One picomole of each primer was annealed to 10 µg of RNA
for 20 min at 52°C and then for 10 min at room temperature. The
oligonucleotide primers were extended with 1 U of avian myeloblastosis virus reverse transcriptase (Promega, Madison, Wis.) at 42°C for 30 min. The samples were precipitated with ethanol and resuspended in a
solution containing 2 µl of H2O and 1.5 µl of formamide
loading dye (Promega). Nucleotide sequencing was carried out by using a
Thermo Sequenase Fluorescent Labelled Primer Cycle Sequencing Kit
(Amersham Pharmacia, Little Chalfont, United Kingdom). The extension
products and sequencing reactions performed with the same primer were
loaded onto a 6% polyacrylamide sequencing gel and analyzed on a model
4000 automated DNA sequencer (LI-COR, Lincoln, Nebr.).
Purification of recombinant C. jejuni DnaK
protein.
The full-length coding region of the dnaK gene
was amplified by PCR with primers
5'-AAAAGGATAACATATGAGTAAAGTTATAGGTA-3' and 5'-TCAACTTCAGCGTCGATTAC-3' (NdeI site is
underlined), using 1 U of Vent polymerase per 100-µl reaction volume.
The resulting DNA product was digested with NdeI and ligated
with pET-22b(+) which had been digested with XhoI, blunt
ended with mung bean nuclease, and then digested with NdeI.
Thus, the last codon of the dnaK open reading frame (ORF)
was fused in frame to the 5' end of the vector sequence encoding a
6-histidine tail. The nucleotide sequence of the insert was confirmed
by sequence analysis to be correct. The plasmid was transformed into
E. coli BL21(DE3). Large-scale expression and nondenaturing
purification by nickel-nitrilotriacetic acid (Qiagen) metal affinity
chromatography were performed as proposed by the manufacturer.
Fractions containing the recombinant protein were pooled and applied on
a Sephacryl S100-HiPrep 26/69 column (Pharmacia, Freiburg, Germany).
The N-terminal sequence of the purified protein was determined by the
Edman degradation technique (model 473A amino acid analyzer; Applied Biosystems).
Western blot analysis and ELISA.
For Western blot
experiments, the purified recombinant protein was subjected to sodium
dodecyl sulfate-polyacrylamide gel electrophoresis and transferred to
nitrocellulose membranes. Nonspecific binding sites were saturated for
2 h with a solution consisting of 10% fetal calf serum and 1%
bovine serum albumin in phosphate-buffered saline (PBS), pH 7.4. The
nitrocellulose sheet was cut into strips, which were incubated with
either human sera (diluted 1:200) or an anti-histidine tag monoclonal
antibody (Dianova, Hamburg, Germany). After the strips were washed with
PBS-0.05% Tween 20, bound antibodies were detected with anti-human
IgG and anti-mouse IgG peroxidase-conjugated secondary antibodies,
respectively. For the enzyme-linked immunosorbent assay (ELISA), 1 µg
of recombinant protein ml Nucleotide sequence accession number.
The nucleotide
sequence of the dnaK locus was assigned GenBank/EMBL
accession no. Y17165.
Molecular cloning of the dnaK gene cluster.
PCR on
genomic DNA, using two degenerate oligonucleotide primers derived from
highly conserved regions of bacterial HSP70 proteins, resulted in the
amplification of three DNA fragments of 480 to 500 bp. Nucleotide
sequence analysis revealed that one of the isolated fragments
(designated dnaK2) was highly homologous to bacterial
dnaK genes. A genomic plasmid library was constructed and
screened by colony hybridization with the 32P-labeled
PCR product. One recombinant plasmid (pdnaK1), carrying a 1.6-kb
BglII fragment, was recovered. A database homology search based on nucleotide analysis of the 1.6-kb insert showed that the 5'
end of the putative C. jejuni dnaK gene was present in pdnaK1. The missing 3' end was obtained by a PCR-based genomic walking
approach. After two rounds of randomly primed PCR, two overlapping DNA
products of 1.1 and 1.0 kb (dnaK3 and dnaK4,
respectively) were amplified, cloned, and sequenced. As was shown by
nucleotide sequence analysis, the missing 3' end of the dnaK
gene was contained within the two amplified fragments. To determine the
nucleotide sequence of the entire hrcA-grpE-dnaK gene
cluster, a 1.2-kb PCR product (hrcA1) was amplified by the
genomic walking approach. Cloning and sequencing of the relevant region
revealed that the amplicon contained the 5' end of hrcA and
the upstream flanking region.
Nucleotide sequences and analysis of the hrcA,
grpE, and dnaK genes.
By reconstruction of
the genomic DNA sequences from the insert of pdnaK1 and from the three
PCR products, the complete nucleotide sequence of the dnaK
gene cluster from C. jejuni was determined (Fig.
1B). The dnaK gene consists of
an ORF (ORF1) of 1,869 bp and encodes a polypeptide of 623 aa with a
predicted molecular mass of 67.3 kDa and a pI of 4.82. The
dnaK gene is preceded by a putative ribosome binding site
(AAGGAT) 5 nucleotides upstream of the AUG start codon. The average G+C
contents at positions 1, 2, and 3 of codons of the putative HSP70 gene
are 50.6, 33.2, and 22.0%, respectively, confirming the codon usage
commonly found in C. jejuni genes. The predicted protein
displayed a high degree of homology to members of the 70-kDa family of
HSPs. In particular, the overall degrees of identity to HSP70 proteins
of H. pylori (18), Borrelia
burgdorferi (2), Chlamydia trachomatis
(10), and Bacillus subtilis (44) were
calculated to be 78.1, 60.5, 57.2, and 53.8%, respectively. A second
ORF (ORF2), which is 525 bp long, was identified 22 bp upstream of
dnaK. ORF2 encodes a protein with a calculated molecular
mass of 20.0 kDa and a pI of 4.64. This protein exhibited a moderate
degree of homology to bacterial GrpE proteins, with overall degrees of
identity of 37.8% (H. pylori), 36.6% (Bacillus
subtilis), 36.2% (Borrelia burgdorferi), and 34.5%
(Chlamydia trachomatis). A third ORF (ORF3) was found
upstream of grpE. The stop codon TGA of ORF3 overlaps with
the start codon GTG of the grpE gene, and consequently the putative ribosome binding site of grpE (AAGGAG) located 5 bp
upstream of the start codon is a part of the preceding ORF. The
initiation codon GTG is seldom used in the A+T-rich genome of C. jejuni, and we observed that other strains of C. jejuni
used ATG as the grpE start codon. Interestingly, a similar
overlapping of grpE with the upstream gene has been reported
for the Chlamydia trachomatis hrcA-grpE-dnaK operon
(37) and as well as the H. pylori genome (41) (Fig. 1C). ORF3, which is 792 bp long, codes for a
protein with a molecular mass of 30.9 kDa and a pI of 5.1. The overall degree of identity of the encoded polypeptide to other bacterial HrcA
proteins is low. However, closer inspection revealed a region of
greater homology at the N-terminal end of the C. jejuni
protein. This region (aa 2 to 83) exhibits identities to HrcA
homologues of 35% (Clostridium acetobutylicum), 32%
(Chlamydia trachomatis and Lactococcus lactis),
28% (Bacillus subtilis), and 23% (Caulobacter crescentus) (Fig. 2). In some
bacterial species (e.g., Bacillus subtilis), dnaJ
is a part of the dnaK operon. Therefore, we searched for
dnaJ-homologous sequences downstream of dnaK, but
no such region could be identified within 600 bp.
Features of the noncoding regions.
Using oligonucleotides
complementary to the 5' ends of dnaK and grpE,
respectively, primer extension analyses revealed a putative transcription start (P1) site 46 bp upstream of the dnaK
start codon (Fig. 3A) and a second
putative transcription start site (P2) 184 bp upstream of the
grpE start codon (data not shown). However, no regions
convincingly compatible with
0019-9567/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Cloning and Expression of the dnaK Gene
of Campylobacter jejuni and Antigenicity of Heat Shock
Protein 70
and
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
70
promoter consensus sequence and to a cis-acting regulatory
element (CIRCE) are located upstream of the hrcA gene.
Following heat shock, a rapid increase of dnaK mRNA was
detectable, which reached its maximum after 20 to 30 min. A
6-His-tagged recombinant DnaK protein (rCjDnaK-His) was generated in
E. coli, after cloning of the dnaK coding
region into pET-22b(+), and purified by affinity and gel filtration
chromatography. Antibody responses to rCjDnaK-His were significantly
elevated, compared to those of healthy individuals, in about one-third
of the serum specimens obtained from C. jejuni enteritis patients.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
32, allowing for the coordinate
expression of genes that belong to the so-called 32
regulon (50). After enhancing transcription of heat shock
genes, 32 is sequestered by the DnaK chaperone machine
and degraded by ATP-dependent cellular proteases (22, 40).
Alternatively, in the gram-positive model organism Bacillus
subtilis, a highly conserved palindromic sequence is involved as a
cis-acting operator in the regulation of class I
(groE and dnaK) heat shock genes. As known so
far, this element, designated CIRCE (for controlling inverted repeat of
chaperone expression) by Zuber and Schumann (51), is located
at the groE and/or dnaK upstream regulatory region of more than 30 bacterial species (for a recent review, see
reference 34). CIRCE most probably acts at the DNA
level by binding a repressor encoded by the hrcA gene (hrc,
for heat shock regulation at CIRCE elements) and, if the inverted
repeat is a part of the transcript, by modulating mRNA stability
(31, 48, 49). Heat shock regulation in C. jejuni
is poorly understood. In front of the C. jejuni dnaJ heat
shock gene were observed sequences compatible with E. coli
32 as well as 70 consensus sequences
(21). We have recently demonstrated that heat-induced
transcription of the groESL operon, which is preceded by a
CIRCE element, is under the control of a 70-like
promoter (39).
MATERIALS AND METHODS
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
1, if required. Genomic DNA
was isolated as described elsewhere (3). Plasmid DNA was
purified by using a QIAprep plasmid kit (Qiagen, Hilden, Germany).
80°C overnight. A
0.24- to 9.5-kb RNA ladder (Gibco BRL) was used as a size marker.
1 was adsorbed onto 96-well
microtiter plates where were then incubated overnight at 4°C. After
the plates were washed with PBS-0.05% Tween 20, remaining binding
sites were blocked with a solution consisting of 5% fetal calf serum,
0.1% bovine serum albumin, and 0.03% gelatin in PBS, pH 7.4. Again,
the plates were washed and incubated with serially diluted human sera
overnight at 4°C. Detection of bound immunoglobulins was achieved by
incubation for 30 min at room temperature with peroxidase-coupled
anti-human IgG and IgA antibodies, respectively, diluted 1:5,000 in
blocking buffer. Antibody binding was visualized with 2 mM ABTS
[2,2'-azino-bis(3-ethylbenzthiazoline-6-sulfonic acid); Boehringer,
Mannheim, Germany] in ABTS substrate buffer (Boehringer). Optical
densities (ODs) was read at wavelengths of 405 and 450 nm.
RESULTS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
View larger version (17K):
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FIG. 1.
(A) The 5' flanking region and the 5' end of the
hrcA gene. Putative promoter regions are single underlined.
A putative ribosome binding site is double underlined. The CIRCE-like
inverted repeat is depicted as a stem-loop structure. The putative
transcription start site is indicated by an arrow. (B) Restriction map
of the dnaK locus. Abbreviations for restriction sites are
as follows: Bc, BclI; Bg,
BglII; Pv, PvuII; Ec,
EcoRI; and Ba, BalI. Vertical arrows
indicate the insertion sites of plasmid pdnaK1 and the PCR products,
from which the nucleotide sequence was derived. Boxes indicate the
hrcA, grpE, and dnaK genes. (C)
Nucleotide and amino acid sequences of the hrcA-grpE
overlapping region from C. jejuni and corresponding
sequences from H. pylori and Chlamydia
trachomatis. Putative ribosome binding sites are double
underlined. Overlapping start and stop codons are indicated by ovals.
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FIG. 2.
Alignment of the deduced N-terminal amino acid sequence
of the C. jejuni (Cj) HrcA protein with those
from Chlamydia trachomatis (Ct; GenBank accession
no. P54306), Clostridium acetobutylicum (Ca;
P30727), Caulobacter crescentus (Cc; P54305),
Synechococcus sp. (Sy; P72795), L. lactis (Ll; P42370), Staphylococcus aureus
(Sa; P45556), and Bacillus subtilis
(Bs; P25499). Amino acid residues identical to those of
C. jejuni are indicated by colons, while conservative
replacements are indicated by dots. Amino acid residues identical or
conserved in all species are gray shaded. Gaps, indicated by dashes,
have been introduced to maximize similarity. The numbers indicate the
percentages of amino acid identity (id) and similarity (sim),
respectively, between the N-terminal end of the C. jejuni
HrcA protein and the corresponding region of the bacterial
homologues.
70 or heat shock promoter
consensus sequences (9) were identified upstream of P1 or
P2. Surrounding P2, a high-energy (
G0 = 24.2 kcal mol1) putative stem-loop structure was
detected within the hrcA coding region, ranging from
nucleotides 570 to 616 relative to the hrcA translation
start site. Therefore, the possibility that a secondary structure in
the RNA stopped the reverse transcriptase during the primer extension
reaction cannot be ruled out. A third putative transcription start site
(P3) was identified 34 bp upstream of the hrcA translation
initiation codon (Fig. 3B). The region in front of P3 exhibited a
nucleotide sequence identical to the E. coli
70 consensus promoter sequence
(TTGACA-N16-18-TATAAT). Furthermore, between
the putative 10 promoter hexamer and the hrcA translation start site, a putative stem-loop structure similar to the CIRCE inverted repeat was detected. P3 is located at the seventh position of
the 5' branch of the hairpin (Fig. 1A). The C. jejuni
sequence differs from the CIRCE consensus sequence
(5'-TTAGCACTC-N9-GAGTGCTAA-3') in that it
exhibits three mismatches in the stem and contains 8 nucleotides in the
loop of the putative hairpin structure.
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FIG. 3.
Mapping of the 5' end of the dnaK (A) and the
hrcA (B) genes by primer extension analysis. IRD800-labeled
oligonucleotides complementary to the 5' ends of dnaK and
hrcA, respectively, were hybridized with 10 µg of total
RNA (lanes P). The letters G, A, T, and C above the lanes represent
products of sequencing reactions using the same oligonucleotide as a
primer. Arrowheads indicate the main primer extension products.
G0 = 14.2 kcal mol1) 14 nucleotides downstream of the
dnaK stop codon, followed by a stretch of 6 T's, might
function as a rho-independent transcription terminator (11,
28).
Observation of dnaK mRNA levels under conditions of heat stress. The in vivo transcripts of the dnaK locus were detected by Northern analysis with total RNA obtained from normally grown or heat-stressed bacteria. A 32P-labeled PCR product internal to dnaK hybridized with two mRNA species with molecular sizes of about 2.0 and 2.8 kb (Fig. 4). The 2.8-kb mRNA might correspond lengthwise to a grpE-dnaK transcript, whereas the 2.0-kb mRNA species might correspond to the dnaK gene or constitute a degradation product of the larger transcript. Following heat shock, there was a rapid increase in both mRNA species, with levels reaching a maximum after 20 to 30 min. Even after 60 min, the amount of mRNA was clearly augmented. Under the conditions described in Materials and Methods (growth at 37°C in a microaerobic environment) no dnaK-specific transcripts were detected in C. jejuni cells. However, after longer times of exposure, a signal of low intensity corresponding to a 2.8-kb mRNA species could be detected (data not shown). The possibility of nonspecific degradation of the mRNA was excluded because rehybridization of the blot with a groEL-specific probe yielded a distinct signal (data not shown). Since heat shock experiments were performed in an aerobic-atmosphere environment, C. jejuni cells were cultivated for 60 min at 37°C in BHIYE as a control. Under these conditions, specific mRNA was increased; however, the increase was weaker than that after 5 min of heat shock. This observation is in concordance with published results showing that expression of a putative HSP60 homologue of C. jejuni is induced under aerobic growth conditions (36).
|
Antigenicity of the recombinant DnaK protein. The full-length coding region of the dnaK gene was amplified by PCR and ligated into the prokaryotic expression vector pET-22b(+). Large-scale expression and nondenaturing purification by metal affinity chromatography revealed that in addition to the recombinant DnaK protein (rCjDnaK-His), a polypeptide with an apparent molecular mass of ~18 kDa, which might be translated from an in-frame ATG codon, was coexpressed and copurified (Fig. 5, lanes B and C). Therefore, fractions containing rCjDnaK-His were pooled and further purified by size exclusion chromatography. The final purified fraction showed a single band with an apparent molecular mass of about 68 kDa (Fig. 5, lane D). The N-terminal sequence of the purified protein was determined by the Edman degradation technique to be SKVIGIDLGT and agreed perfectly with the predicted amino acid sequence.
|
-D-thiogalactopyranoside (IPTG)-induced
E. coli lysate; C, elute from an Ni2+ chelating
column; D, rCjDnaK-His after gel filtration. Sizes of protein standards
(low molecular weight marker; Pharmacia) are shown to the left (in
thousands).
|
|
) and 16 healthy controls
(
). Means ± SDs are indicated. ODs were read in an ELISA
reader at 405 and 450 nm.
| |
DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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In this study, we have cloned, sequenced, and characterized the hrcA-grpE-dnaK gene cluster of C. jejuni. Whereas the polypeptides encoded by the dnaK and grpE genes exhibited distinct homology to the respective proteins of other bacterial species, only a low overall degree of similarity was seen between C. jejuni HrcA and its bacterial homologues. However, at the N-terminal end, a stretch of approximately 85 aa residues exhibited significant homology (~32% identity and ~50% similarity) to the corresponding region of other HrcA proteins. This region encompasses two amino acid sequences of extended homology (designated boxes A and B [Fig. 2]), which might be involved in HrcA activity (31). Although the organization of the dnaK gene cluster, unlike the groE operon, differs considerably among bacterial species, the basic structure seems to be hrcA-grpE-dnaK-dnaJ and derivatives thereof (e.g., dnaK-dnaJ in E. coli) (34). In C. jejuni, dnaJ does not appear to be a part of the dnaK operon, a finding that is corroborated by the recently published nucleotide sequence of the dnaJ gene (21). Hence, the organization of the C. jejuni dnaK operon (hrcA-grpE-dnaK without dnaJ) is most similar to those seen in Chlamydia trachomatis (37) and L. lactis (13). Also, in the genome of H. pylori, dnaK and dnaJ are separated (41). In C. jejuni, as well as in Chlamydia trachomatis and H. pylori (between grpE and the preceding gene), but not in the gram-positive species L. lactis, an overlap of translational regulatory signals at the hrcA-grpE intergenic boundary was observed. Therefore, these two genes might be translationally coupled, which would ensure balanced synthesis of HrcA and GrpE proteins.
The hrcA gene is supposed to code for a repressor of the
groE and dnaK heat shock genes that acts by
binding to a highly conserved inverted repeat designated CIRCE. A
putative stem-loop structure very similar to the CIRCE consensus
sequence was detected in front of the hrcA start codon. A
CIRCE element was found upstream of the C. jejuni groE
operon, located as well between the 10 promoter box and the
translation initiation site (39). In contrast to L. lactis, in which a CIRCE stem-loop structure is involved in dnaJ expression (42), C. jejuni's
dnaJ gene did not appear to have a CIRCE element in front of
it (21).
Northern blot analysis led to the detection of two mRNA species, of 2.8 and 2.0 kb, both of which were strongly heat inducible. The amount of
specific mRNA in C. jejuni cells growing microaerobically at
37°C was very small. Similarly, in the closely related species H. pylori, no dnaK transcript was observed in
cells grown under nonstressed conditions, although the gene product,
the HSP70 protein, was synthesized (18). A possible
explanation is that minute amounts of mRNA are sufficient for
maintenance of HSP70 protein levels in nonstressed cells.
Alternatively, for reasons yet unknown, dnaK mRNA may be
prone to specific degradation. Transcript mapping by primer extension
identified three putative transcription start points, in front of the
hrcA, grpE, and dnaK start codons. The putative 10 and 35 promoter boxes upstream of hrcA
perfectly match the E. coli 70 consensus
sequence (17), which is an interesting finding because the
consensus sequence for the C. jejuni vegetative promoter in the 35 portion is completely different from that of E. coli (45). Putative promoter regions similar or
identical to the E. coli 70 consensus
promoter have been found in front of the dnaJ
(21), groE (39), and clpB
(38a) heat shock genes from C. jejuni. It can be
speculated that a primary hrcA-grpE-dnaK transcript of
C. jejuni is initiated from the 70-like
promoter upstream of hrcA. As could be demonstrated for the
dnaK operon of Chlamydia trachomatis, methods
like reverse transcription-PCR and RNase protection assay, which are
considerably more sensitive than standard Northern blot hybridization,
were necessary to detect the polycistronic transcript (37).
No regions similar to 70 or heat shock
(32) consensus promoters were found corresponding to P1
and P2. Therefore, it may be possible that P1 and/or P2 is an mRNA
processing site instead of a transcription start site. Regulation of
dnaK expression appears to be complex and may differ among
eubacterial species. There has been discussion of posttranscriptional
processing of the dnaK operons of Bacillus
subtilis and Chlamydia trachomatis giving rise to mRNA
species smaller than the primary polycistronic transcript (32, 37,
44). High-energy stem-loop structures, like that surrounding P2,
have been described in bacterial polycistronic operons as
transcriptional terminators or attenuators or sites crucial for mRNA
processing or degradation (15, 29).
Western blot analyses as well as ELISA studies indicate that DnaK is immunoreactive in the human host, though only in a minority of C. jejuni-infected patients. However, when interpreting these data, the fact that serological tests using convalescent-phase sera from C. jejuni-infected patients may produce ambiguous results must be taken into account. First, in some patients, no antibody response to Campylobacter antigens is observed (6), and second, sera from healthy individuals sometimes react with Campylobacter proteins (12). Furthermore, antibodies reacting with epitopes shared by microbial DnaK homologues may contribute to the seropositivity among healthy individuals observed in Western blot experiments. Due to the extensive homology between bacterial HSPs and their mammalian counterparts, the humoral and/or T-cell response against these proteins has been proposed to influence the pathogenesis of autoimmune diseases (19). Cloning of C. jejuni heat shock genes and overexpression of the encoded proteins are first steps in studying their roles, if any, in the pathogenesis of C. jejuni-associated GBS. Since heat shock proteins are currently being discussed as promising candidates for subunit vaccines (25) and a Campylobacter vaccine is urgently needed (33), efforts to rule out the possibility or to demonstrate that C. jejuni HSPs can trigger or support autoimmune mechanisms must be increased.
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ACKNOWLEDGMENTS |
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F.L.T. held a postgraduate training grant from the Deutsche Forschungsgemeinschaft, Graduiertenkolleg "Infektiologie." This work was supported in part by the Sander-Stiftung (95.038.1).
We thank Uwe Enders for helpful discussions, S. Lukas for technical assistance, and D. Palm for peptide sequencing.
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FOOTNOTES |
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* Corresponding author. Present address: Department of Neurology, Universität Regensburg, Universitätsstr. 84, D-93053 Regensburg, Germany. Phone: 49-941-944-8950. Fax: 49-941-944-8998. E-mail: gerhard.giegerich{at}klinik.uni-regensburg.de.
Present address: Department of Neurology, Karl Franzens University,
A-8036 Graz, Austria.
Editor: P. E. Orndorff
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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