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Infection and Immunity, October 2001, p. 6217-6224, Vol. 69, No. 10
Biotechnology Laboratory, University of
British Columbia, Vancouver, British Columbia V6T 1Z3,
Canada
Received 20 February 2001/Returned for modification 24 April
2001/Accepted 28 June 2001
Enteropathogenic Escherichia coli (EPEC) is an
extracellular bacterial pathogen that infects the human intestinal
epithelium and is a major cause of infantile diarrhea in developing
countries. EPEC belongs to the group of attaching and effacing (A/E)
pathogens. It uses a type III secretion system to deliver proteins into
the host cell that mediate signal transduction events in host cells. We
used gene array technology to study epithelial cell responses to EPEC
infection at the level of gene expression. We found that EPEC induces
the expression of several genes in infected HeLa cells by a
lipopolysaccharide (LPS)-independent mechanism, including cytokines and
early growth response factor 1 (Egr-1). The transcription factor
Egr-1 is an immediate-early-induced gene that is activated in most cell
types in response to stress. EPEC-induced upregulation of
egr-1 is mediated by the activation of the
MEK/extracellular signal-regulated kinase signal transduction pathway
and is dependent on the type III secretion system. egr-1 is
also induced during infection of mice by the A/E pathogen
Citrobacter rodentium, suggesting that both Egr-1 and
the activation of this mitogen-activated protein kinase signal
transduction pathway may play a role in disease.
Intestinal epithelial cells are the
first physical barrier that pathogens encounter in the gastrointestinal
tract. As a consequence of constant exposure to such pathogens, the
epithelium has evolved mechanisms to discriminate between pathogenic
and nonpathogenic bacteria. In the case of infection, epithelial cells
become activated to express and secrete proinflammatory and
chemoattractant cytokines, including interleukin 8 (IL-8), GRO One of the best-studied extracellular intestinal pathogens is
enteropathogenic Escherichia coli (EPEC). EPEC infects the
human small intestinal epithelium and is a prominent cause of diarrhea in infants in developing countries. EPEC uses a type III secretion system to deliver bacterial effectors into host cells. Among the EPEC-secreted proteins (Esp), EspA, EspB, and EspD are constituents of
the translocation machinery, with EspB and EspD being inserted in the
host cell membrane. EPEC attaches to intestinal epithelial cells by the
interaction of an outer membrane protein, intimin, and a type III
secreted protein that is translocated into the host cell membrane, Tir.
This interaction induces the polymerization of actin into
characteristic pedestal-like structures (reviewed in reference
31). Two other type III secreted proteins have been
described: EspF, a proline-rich protein recently shown to be
translocated into the host cell cytoplasm and involved in disrupting epithelial barrier function (20), and open reading frame
19, which has recently been shown to be translocated to the host
mitochondria (17). EPEC's secreted proteins induce signal
transduction events within the host cell, including inositol phosphate
fluxes and protein kinase C and phospholipase C Recent studies have shown that some bacterial pathogens are able to
activate mitogen-activated protein (MAP) kinase pathways in the host
cell (13, 23, 32, 33) to alter processes such as cell
differentiation, growth, and death. MAP kinase signaling pathways
described thus far include the extracellular signal-regulated kinases
(ERK), c-Jun N-terminal kinases (JNK) (also known as stress-activated protein kinases) and p38 MAP kinases. The activation of these pathways proceeds through a cascade of phosphorylation events leading
to the phosphorylation of downstream kinases and to the transcriptional
activation of several genes. MEK1 (MAPKK1) kinase activation leads to
phosphorylation of ERK1 and ERK2, resulting in their translocation to
the nucleus and phosphorylation of other proteins, including the
transcription factor Elk-1. This event induces the transcription of
genes like fos and egr-1. The early growth
response factor 1 (Egr-1) is an 80- to 82-kDa zinc finger transcription
factor that belongs to the early growth response gene family that
participates in several cellular processes such as differentiation and
proliferation. egr-1 is an immediate-early gene induced in
response to changes in the local cell environment, including exposure
to growth factors and cytokines, hypoxia, tissue damage, UV, or LPS
(18, 19). egr-1 can also be induced by the p38
MAP kinase pathway.
The aims of this study were to use genomic arrays to determine if
epithelial cells respond to EPEC infection by altering global gene
expression and to identify novel factors and pathways involved in this
process. Our findings show that EPEC infection of epithelial cells
causes upregulation of expression of cytokines. We also demonstrate
that EPEC activates the MEK/ERK signal transduction cascade that leads
to the expression of the transcription factor Egr-1. In vivo studies of
Citrobacter rodentium-infected mice confirmed
egr-1 induction and suggest that the induction of
egr-1 may play a role in disease.
Bacterial strains, mammalian cell lines, and culture
conditions.
EPEC strain E2348/69 (6) and the mutants
escC (see below) and espB (8) were
grown overnight in Luria-Bertani (LB) broth at 37°C without shaking
prior to infection. "Preactivated" bacteria were prepared by
diluting LB overnight cultures 1:50 in Dulbecco's modified
Eagle medium (DMEM) without serum and incubating at 37°C with 5%
CO2 for 3 h. C. rodentium
(formerly Citrobacter freundii biotype 4280) strain DBS100
was grown overnight in LB prior to mouse infection.
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.10.6217-6224.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Enteropathogenic Escherichia coli Infection
Induces Expression of the Early Growth Response Factor by Activating
Mitogen-Activated Protein Kinase Cascades in Epithelial Cells
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
,
GRO
, monocyte chemoattractant protein 1, tumor necrosis
factor alpha, granulocyte-macrophage colony-stimulating factor,
or IL-1 (reviewed in reference 15). Moreover, activated
epithelial cells play an important role in the initiation of
inflammatory and immune responses by transmitting signals to underlying
cells of the reticuloendothelial system. Bacterial lipopolysaccharide
(LPS) induces the production of inflammatory cytokines by immune cells
such as macrophages and monocytes. However, intestinal
epithelial cells do not normally respond to LPS from extracellular
pathogens to prevent exaggerated responses to the LPS of normal flora.
activation (2,
10, 16). EPEC also triggers IL-8 secretion through NF-
B
activation in T84 epithelial cells and recruitment of polymorphonuclear
cells in a coculture system (28, 29). These changes in
signaling may contribute to disease. However, the molecular mechanisms
by which EPEC causes diarrhea or induces pedestal formation are still unknown.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
Animal experiments. C57BL/6J mice (Jackson Laboratory, Bar Harbor, Maine) were infected by oral gavage with 0.1 ml of standing LB overnight cultures of C. rodentium (2.5 × 108 CFU). Mice were killed at days 6 and 10 postinfection, and colons were dissected for RNA isolation.
Construction of a nonpolar escC deletion
mutant.
The oligonucleotides ESCC-01F
(5'-GTTAACCTCGAGGCGGTTCCGATAG-3') (XhoI
restriction site) and ESCC-02R
(5'-GATGCGAGCTCTGTTGCTATCCAATG-5') (SacI
restriction site) were used to amplify escC from chromosomal DNA from EPEC E2348/69. The amplification product was cloned into pCR2.1 TOPO (Invitrogen), generating pCR-escC. Primers
ESCC-03R (5'-GGCGACGCGTGTATACCGCTGTTAAGCGACATTCC-3') and
ESCC-04F (5'-GGCGACGCGTCATTACACAATTCGTCCTATATCAG-3') were
used to create an in-frame deletion of 1,408 bp between bp 2 and bp
1410 of the escC gene in pCR-escC using inverse
PCR amplification. Both oligonucleotides ESCC-03R and ESCC-04F
introduced an MluI restriction site. The 2,049-bp
SacI-XhoI escC deletion fragment was
cloned into the positive-selection suicide vector pCVD442 (7), digested with SacI-SalI. The
resulting plasmid, pCVD442-
escC, was used to construct
the escC deletion mutant in EPEC E2348/69 (streptomycin
resistant) by allelic exchange as described (7), generating the EPEC escC strain.
RNA isolation.
HeLa cells (1.5 × 106) were seeded in 10-cm-diameter tissue culture
plates in 10 ml of DMEM plus 10% FCS and cultured overnight. Culture
medium was changed to DMEM without FCS, and cells were infected
for 3 h with overnight bacterial cultures: EPEC wild type (wt) (30 µl), the espB mutant (100 µl), the escC
mutant (30 µl), or EPEC exposed to LPS from E. coli
O111:B4 (10 µg/ml; Sigma, St. Louis, Mo.). Cells were washed five
times with diethyl pyrocarbonate-treated phosphate-buffered saline and
scraped in 1 ml of diethyl pyrocarbonate-phosphate-buffered saline.
Cells were pelleted and resuspended in 1 ml of Trizol (Life
Technologies), and RNA was purified following the manufacturer's
instructions. RNA was treated with DNase I (Clontech, Palo Alto,
Calif.) to remove contaminant genomic DNA for 1.5 h in the
presence of RNase inhibitor (Ambion, Austin, Tex.), and the reaction
was stopped using 10× termination mix (0.1 M EDTA, pH 8; glycogen, 1 mg/ml). The enzyme was removed by phenol-chloroform extraction, and RNA was precipitated with 2 volumes of ethanol and a 1/10 volume of sodium
acetate, pH 5.2. RNA was resuspended in 15 µl of
H2O containing the RNase inhibitor and stored at
70°C. RNA was tested for the presence of remaining DNA
contamination by 35 cycles of PCR amplification using GAPDH
(glyceraldehyde-3-phosphate dehydrogenase)-specific primers (Table
1).
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Human cDNA expression arrays and image analysis. Atlas Human cDNA expression arrays 1.2 contain 1,176 partial human cDNAs (Clontech). 32P-labeled cDNA probes were synthesized by RT (according to the manufacturer's instructions) using 5 µg of total RNA, [32P]dATP (Amersham), and gene-specific primers. Array membranes were hybridized with 3 × 106 to 5 × 106 cpm of cDNA probe. Atlas Image 1.0 (Clontech) and Excel 5.0 (Microsoft) software was used for quantification and comparison of the hybridization signals. The intensity of the signals was corrected for background and normalized to the nonvariable genes coding for GAPDH, tubulin, and ubiquitin that are spotted on the membranes. Genes were considered to be induced when they gave a detectable signal and were induced by more than twofold in EPEC-infected cells in two independent experiments (9).
Northern blots.
RNA (10 µg/lane) was resolved by
electrophoresis on 1.5% agarose-formaldehyde gels and transferred to
positively charged nylon membranes (Ambion), cross-linked with
long-wave UV light, and baked at 80°C for 30 min. cDNA was
synthesized with Superscript II reverse transcriptase (Life
Technologies) using total RNA purified from EPEC-infected HeLa cells as
the template, with oligo(dT) for the GAPDH probe and with the
oligonucleotide egr for the egr-1 probe. Specific
double-stranded DNA (dsDNA) fragments of GAPDH and egr-1
were PCR amplified from the cDNA using the primers listed in Table 1.
Antisense cDNA was synthesized by PCR using the specific dsDNA
fragments as templates, the appropriate 3' primer and modified
nucleotides (Strip-EZ PCR; Ambion). The single-stranded DNA PCR
products were column purified (Qiagen, Mississauga, Ontario, Canada)
and labeled with biotin using psoralen-biotin (Ambion) and
cross-linking with 365-nm UV light. Northern blotting was performed
with the NorthernMax-Gly kit (Ambion). Hybridizations were performed in
5 ml of UltraHyb solution (Ambion)and incubated overnight at 45°C.
The BrightStar nonisotopic detection kit (Ambion) was used for probe detection.
RT-PCR analysis of mRNA levels.
RT was performed with
Superscript II reverse transcriptase following the manufacturer's
instructions. cDNA was synthesized in 20-µl reaction mixtures using
oligo(dT) or specific reverse primers for Egr-1 and MIP-2 and 3 µg
of total RNA as the template. PCR amplification was performed in 0.5 µl of cDNA using gene-specific primers and the number of cycles as
listed in Table 1. For all PCRs, the following conditions were used: a
10-min denaturing step at 94°C; cycles of 40 s at 94°C,
40 s at 61°C (68°C for mouse Egr-1), and 50 s at 72°C;
and 10 min at 72°C. The PCR cycle number was optimized for each gene
to prevent saturation of the reaction. PCR products were analyzed by
1.5% ethidium bromide-agarose gel electrophoresis.
Preparation of protein extracts and Western blots. HeLa cells (3 × 105) were seeded in 60-mm-diameter tissue culture plates and incubated overnight. The medium was changed to DMEM without serum 2 h prior to infection. Overnight standing LB bacterial cultures were diluted 1:50 in prewarmed DMEM without serum and incubated for 3 h in a 37°C, 5% CO2 incubator. Aliquots (10 µl) of these cultures were used for infections. Infected cells were scraped in 100 µl of 1× boiling sodium dodecyl sulfate-polyacrylamide gel electrophoresis loading buffer. Total protein lysates were resolved by sodium dodecyl sulfate-10% polyacrylamide gel electrophoresis, electrotransferred to a nitrocellulose membrane, and blocked with 5% skim milk in Tris-buffered saline-0.1% Tween 20. The following antibodies were used at the indicated concentrations: rabbit anti-ERK1 (New England Biolabs, Beverly, Mass.), 1:2,000; monoclonal phosphospecific anti-p44/p42 (ERK1/2; New England Biolabs), 1:1,000; rabbit anti-Egr-1 (Santa Cruz Biotechnology, Santa Cruz, Calif.), 1:300; monoclonal anti-TirA2, 1:500 (4). Primary antibodies were incubated on blots overnight at 4°C.
Cells were pretreated with MAP kinase inhibitors for 30 min prior to infection with the following at the indicated concentrations: PD 98059 (Calbiochem) at 50 µM and SB 203580 (Calbiochem) at 20 µM.| |
RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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EPEC induces changes in gene expression in epithelial cells. It is believed that EPEC infection of epithelial cells initiates a complex chain of events that ultimately result in disease. It is likely that many of these changes originate at the gene expression level. Therefore, we used DNA array technology to investigate transcriptional responses of epithelial cells to EPEC infection.
HeLa cells provide a well-established model to study EPEC interactions with human epithelial cells (26). Monolayers were infected with wt EPEC for 3 h, and total RNA was purified. This time was chosen because after 3 h of infection effectors have been delivered and actin has been rearranged into pedestals. Radiolabeled cDNA was synthesized from infected and uninfected cells as described in Materials and Methods and used to hybridize two array membranes in parallel, containing spotted cDNAs for 1,176 human genes. The data were analyzed by phosphorimaging, and the intensities of the signals were normalized to each other using the housekeeping genes coding for GAPDH, ubiquitin, and tubulin that were also on the membranes. The majority of the genes showed no significant variation in mRNA levels following infection. Genes that had detectable signal and were induced more than twofold in EPEC-infected cells in two independent experiments are listed in Table 2. They include the transcription factors Egr-1 and ETR101, the neutrophil chemoattractants MIP-2 (GRO) and IL-8, the antideath factor IEX-1L, and the
cytoskeleton protein zyxin.
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, and IL-8 was confirmed by
this method (Fig. 1). Our array
hybridization data, supported by RT-PCR analysis, also confirm an
earlier report that EPEC induced IL-8 secretion (28).
These results also identified egr-1 as a previously
unrecognized gene upregulated by EPEC in vitro.
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Confirmation of egr-1 induction by Northern blotting
and RT-PCR.
The early growth response factor egr-1 is
an immediate-early-induced gene that is activated in most cell types in
response to stress. The induction of egr-1 was assessed by
Northern blot analysis and RT-PCR in two independent experiments: a
time course infection in which HeLa cells were infected with wt EPEC
for 3, 4 and 5 h and for 3 h with wt EPEC and the
espB mutant. mRNA levels were normalized to GAPDH
expression, which is unaffected by EPEC infection. EspB is a type III
secreted protein that is inserted into the host cell membrane during
infection. A mutant in this protein is unable to deliver type III
effectors into the host cell (34). Similar results were
obtained with both techniques (Fig. 2),
showing that egr-1 mRNA increases after 3 h of
infection with wt EPEC and is still induced after 4 h but
decreases after 5 h. While egr-1 is induced after a 3-h
infection with wt EPEC, the espB mutant stimulated a reduced
transcription of this gene. These results show that egr-1
expression is induced over time, with high levels observed at 3 to
4 h after infection, and then decreases. EspB contributes to this
induction, suggesting that the type III secretion system may be
involved in this event. Since both Northern blotting and RT-PCR yielded
similar results, only RT-PCR was used for further gene expression
studies.
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LPS does not trigger egr-1 or IL-8 gene expression
in epithelial cells, but the type III secretion system is necessary for
full induction.
egr-1 is induced by several stimuli in
a variety of cell lines, including bacterial LPS in
macrophages. In order to investigate whether the induction of
egr-1 and IL-8 genes is triggered by LPS or by some
EPEC-specific factor, transcriptional levels of these genes were
analyzed in cells exposed to LPS from E. coli (10 µg/ml).
To test if the reduced transcription observed with the espB
mutant is EspB or type III dependent, cells were infected with the type
III secretion mutant escC. EscC is a structural component
of the type III secretion system believed to be the outer membrane
secretin, and a mutant in this gene is unable to secrete or translocate
any of the Esp, while complementation of this mutant with
escC on a plasmid restores translocation (data not shown).
As shown in Fig. 3, egr-1 and
IL-8 gene expression is not induced by exposure to E. coli
LPS. Densitometric quantification of the RT-PCR products and
normalization relative to GAPDH expression indicated a (4.2 ± 0.3)-fold induction of egr-1 and (2.5 ± 0.4)-fold induction of IL-8 by wt EPEC relative to uninfected cells
(n = 3). By the same analysis, the type III secretion
mutant caused no significant change in expression of egr-1
or IL-8 genes ([1.1 ± 0.4]- and [0.9 ± 0.2]-fold
induction relative to uninfected cells, respectively). Therefore, in
cells infected with the escC mutant, expression of these
genes is significantly decreased compared to wt EPEC. The same result
was obtained for MIP-2 expression (data not shown). These
experiments show that a functional type III secretion system is needed
for full induction of egr-1, IL-8, and MIP-2 genes.
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EPEC infection induces egr-1 expression by
activation of the MEK signal transduction pathway in HeLa cells.
We focused our research on egr-1 expression because it is a
previously undescribed host response to EPEC infection. Activation of
MAP kinase signal transduction pathways mediates egr-1
induction in response to extracellular stimuli. Of the three MAP kinase cascades described (MEK/ERK, p38, and stress-activated protein kinase-Jun-N-terminal protein kinase), both MEK/ERK and p38 have been
shown to upregulate egr-1 expression (5, 24).
Therefore, we investigated which of these two signal transduction
pathways is involved in EPEC-induced transcription of egr-1.
HeLa cells were pretreated with specific inhibitors of these pathways
prior to infection with EPEC. PD 98059 inhibits MEK activation by
blocking its phosphorylation, and SB 203580 selectively inhibits
p38-stress-activated protein kinase 2. The presence of PD 98059 abolished EPEC-mediated egr-1 induction, while SB 203580 only slightly decreased egr-1 mRNA levels (Fig.
4A). Both inhibitors decreased IL-8
expression partially, but neither abrogated it.
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EPEC-mediated ERK1/2 phosphorylation occurs before Egr-1 synthesis
and is type III dependent.
MEK mediates phosphorylation of ERK1/2
(p44/p42) kinases, which then phosphorylate other factors such
as Elk-1, which ultimately activates egr-1 transcription.
HeLa cells were infected with EPEC in a time course experiment in the
presence or absence of 50 µM PD 98059. The role of the type III
secretion system in this induction was also examined by infecting with
the escC mutant. Because PD 98059 degrades over time, and to
minimize the time that cells are exposed to this inhibitor, infection
conditions were changed to the preactivation method (27).
Overnight EPEC cultures were subcultured for 3 h at 37°C with
5% CO2 in cell culture medium without shaking
before being used to infect epithelial cells. Under these culture
conditions EPEC becomes activated and attachment to cultured cells
occurs faster. Total protein extracts prepared from infected cells at
different time points were assayed by Western blotting and probed with
antibodies recognizing phosphorylated ERK1/2. As shown in Fig.
5A, EPEC induces phosphorylation of
ERK1/2 after 1 h of infection, peaking at 2 h and decreasing
afterwards. Anti-Egr-1 antibodies detected this protein at 2.5 h
after infection. When cells were pretreated with the inhibitor PD
98059, only a small amount of ERK1/2 was phosphorylated and no Egr-1
protein was detected (Fig. 5B). The type III mutant escC was
also unable to induce ERK1/2 phosphorylation to wt levels, and Egr-1
was undetectable (Fig. 5C). To prove that the inhibitor does not impair
type III secretion, the same protein extracts were probed with anti-Tir antibodies. The presence of PD 98059 did not interfere with Tir delivery into the host cell membrane as the phosphorylated 90-kDa form
of Tir, which is only observed after Tir delivery into host cells, was
present in both infections and follows the same time course. The 78-kDa
form of Tir, which corresponds to the bacterial form of the protein
before being translocated into the host cell membrane, is observed due
to the bacteria attached to infected cells. The phosphorylated 90-kDa
form of Tir is absent in cells infected with the escC
mutant, as a result of the inability of this mutant to translocate Tir
into the host cell, where it undergoes phosphorylation. Furthermore,
the amount of total Tir protein appeared to be the same, indicating
that PD 98059 does not affect attachment or bacterial growth. Samples
were also probed with anti-ERK1 antibodies which cross-react with ERK2
to show that similar amounts of ERK1/2 were present in the different
samples, suggesting that neither EPEC infection nor PD 98059 affects
ERK expression. When the same experiment was performed with the normal infection method (where bacteria were not preactivated), ERK1/2 phosphorylation peaked at 3 h and Egr-1 synthesis was observed after 4 h (data not shown).
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Egr-1 is induced in C. rodentium-infected mice. C. rodentium is an enteric bacterial pathogen of mice that causes attaching and effacing (A/E) lesions on the mouse intestinal epithelium, similar to those caused by EPEC on human cells. Although infected mice do not get diarrhea, they develop hyperplasia and inflammation in the colon. C. rodentium also uses a type III secretion system to deliver effectors into epithelial cells that share high homology with EPEC's virulence factors. C. rodentium-infected mice have been previously used as an in vivo model to study EPEC effectors (11).
We investigated whether the equivalent mouse egr-1 gene is induced during C. rodentium infection. C57BL/6J mice were orally infected with C. rodentium, and gene expression was examined in colons dissected after 6 and 10 days. While at day 6 little, if any, sign of inflammation was observed, after 10 days the infected mice had developed hyperplasia and an immune and inflammatory cell infiltrate (12). Total RNA was isolated from these colons, and egr-1 expression was analyzed by RT-PCR. As shown in Fig. 6, egr-1 mRNA was increased at both time points, indicating that in vivo the colon responds to Citrobacter infection by increasing egr-1 expression even at very early time points, resembling the in vitro response of human epithelial cells to EPEC infection.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Gene array technology is increasingly being used to study host
cell responses at the gene expression level to different kinds of
stimuli, including bacterial infection (1, 9, 25). In this
study, we have used array analysis to gain new insights into how
epithelial cells respond to EPEC infection at the molecular level.
Although EPEC infection does not induce as dramatic changes in gene
expression in infected cells as have been described for the invasive
pathogen Salmonella (9, 25), several genes
showed increased transcription that could be confirmed by RT-PCR,
including IL-8, MIP-2, and egr-1 genes. While LPS is a
potent inducer of macrophages' transcriptional responses to
gram-negative bacteria, it is not the principal inducer of the
upregulation of these genes in epithelial cells, as shown by exposing
cells to a high concentration (10 µg/ml) of purified E. coli LPS. Other groups have demonstrated that intestinal
epithelial cells are not responsive to LPS from pathogenic and
nonpathogenic bacteria under normal conditions (14),
presumably to prevent chronic inflammation within the intestine.
IL-8 and MIP-2 participate in the initiation of immune responses by
attracting neutrophils to the sites of infection. Both are induced by
other pathogens such as Salmonella in epithelial cells,
indicating that the initiation of an inflammatory process is a general
response of epithelial cells to bacterial infections. Savkovic et al.
have shown that EPEC infection of the intestinal epithelial cell line
T84 induces NF-B activation, leading to IL-8 secretion and
transmigration of polymorphonuclear leukocytes in a coculture system by
an EspB-dependent mechanism (28, 29). The data presented
here confirm those observations by showing that EPEC's type III
secreted virulence factors contribute to the increase in IL-8 mRNA
levels in infected HeLa cells, presumably through NF-B activation.
We have identified the transcription factor egr-1 as a novel
gene that is highly induced by EPEC in epithelial cells. Increased egr-1 expression was observed in two independent array
experiments and confirmed by Northern blot and RT-PCR. Immediate-early
genes like egr-1 act as connectors between membrane-linked
signal transduction pathways and downstream effectors, expanding and
diversifying the response by inducing different genes. We hypothesize
that in vivo egr-1 expression leads to the induction of
other genes that participate in host defense. Egr-1 can regulate the
expression of several genes in different cell lines, including those
encoding platelet-derived growth factor, tumor necrosis factor alpha,
transforming growth factor , intracellular adhesion molecule
1, CD44, macrophage colony-stimulating factor, C-ets2, tissue
factor, urokinase-type plasminogen activator, and metalloproteinases
(18). Among these genes, we have analyzed the expression
of intracellular adhesion molecule 1, CD44, C-ets2, and tissue factor
in HeLa cells after 5 h of infection. No significant changes were
observed in their levels of transcription (data not shown). However,
this result does not exclude these genes from being upregulated in vivo
during infection or in vitro at other time points. Furthermore,
promoters of many Egr-1-controlled genes have additional binding sites
for other factors such as Sp1 that contribute to their transcription. The role of Egr-1 in the host response to infection is unclear. One
must be cautious in directly translating in vitro findings into the in
vivo situation as the increased expression of egr-1 seen in
the infected colon may involve other cell types beyond just epithelial
cells. However, the demonstration that EPEC infection in tissue culture
and C. rodentium infection in mice both lead to increased
egr-1 expression does suggest a potential role for this gene
in the host response to infection by A/E pathogens.
The fact that these genes were expressed 3 h after infection
suggests that IL-8 and MIP-2 may be involved in an early host response aimed at attracting neutrophils to the site of infection, while genes regulated by Egr-1 may be responsible for later events such
as secretion of other cytokines or upregulation of adhesion molecules.
Gene expression was analyzed at 3 h after infection, because at
this time point bacteria are intimately attached to the host cell
through the Tir-intimin interaction and type III effectors that could
have some role in altering cellular processes have been delivered.
The use of MAP kinase cascade inhibitors revealed that the MEK/ERK pathway is involved in EPEC-mediated egr-1 induction. The inhibitor PD 98059 prevented egr-1 expression in a dose-dependent fashion, and Western blot analysis showed that Egr-1 is produced after ERK1/2 phosphorylation. However, it cannot be excluded that other signaling pathways, including the p38 kinase pathway, contribute to egr-1 activation. MAP kinases transmit signals from the cell surface to the nucleus to regulate cell survival, cytokine production, and cell responses to stress and growth factors. MAP kinases represent a conserved target for a variety of bacterial pathogens: ERK2 activation is required for Listeria monocytogenes invasion into HeLa cells (30); the Yersinia pseudotuberculosis effector YopJ inhibits the three MAP kinase pathways by targeting the superfamily of MAP kinase kinases and blocking their activation (22); Helicobacter pylori activates the ERK/MAP kinase cascade, which induces c-fos transcription, leading to epithelial hyperproliferation (21); and p38 MAP kinase is involved in IL-8 activation in Salmonella enterica serovar Typhimurium-infected intestinal cells (13) and Clostridium difficile toxin A-treated monocytes (32).
It is likely that EPEC activation of the MEK pathway leads to other
cellular responses in addition to egr-1 induction that may
also be relevant in infection. Blocking of the MEK or p38 kinase
cascades did not abrogate EPEC-induced IL-8 expression, although it was
slightly reduced. Furthermore, when cells were treated with increasing
concentrations of the MEK inhibitor PD 98059, IL-8 expression was not
significantly altered. Our results suggest that activation of NF-B
leading to IL-8 induction occurs through alternate signal transduction
pathways to egr-1 upregulation. A recently published report
by Czerucka et al. (3) showed that EPEC infection of T84
cells induces activation of the MAP kinase pathways MEK/ERK, p38, and
Jun N-terminal protein kinase in a type III-dependent fashion. The
results presented here further characterize those observations using a
different cell system by examining MEK activity at later time points.
While Czerucka et al. show that ERK phosphorylation is completely type
III dependent after 1 h of infection with preactivated bacteria,
we see an attenuated yet reproducible phosphorylation of ERK1/2 that is
maximal at 2 h in cells infected by the type III bacterial mutant.
Furthermore, we show how the MEK/ERK and p38 kinase pathways activated
by EPEC infection (3) diverge in their downstream targets,
by providing evidence that MEK/ERK activation results in
egr-1 induction.
The type III secretion system is required for many EPEC-induced signal
transduction events. We present data to show that this system is also
needed for MEK/ERK activation. At the gene expression level,
escC- and espB-infected HeLa cells show
markedly decreased egr-1 expression compared to the
increased expression caused by wt EPEC infection. The fact that
egr-1 expression was not abolished suggests that other
bacterial factors may also participate in this process. When protein
levels were analyzed, very low phosphorylation levels of ERK1/2 were
detected in cells infected with the escC mutant, which could
account for the lower egr-1 mRNA levels found. We also
investigated whether the type III secreted proteins EspF and Tir are
responsible for MEK activation, because, unlike the type III secretion
mutants espB and escC, they are not
involved in the translocation of other effectors. HeLa cells were
infected with the mutants in espF and tir, and
ERK1/2 phosphorylation was analyzed by Western blotting at different
infection times. Both of these mutants were able to activate the
MEK/ERK cascade (data not shown), suggesting that they are not crucial
for the activation of this pathway and that another type III effector
may be involved.
In conclusion, our observations provide evidence that EPEC activates MAP kinase signaling pathways in epithelial cells, which then leads to the upregulation of egr-1. Further studies are needed to address the functional consequences of egr-1 induction in infected cells, as well as in C. rodentium-infected mice.
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ACKNOWLEDGMENTS |
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We thank the entire Finlay laboratory and José Luis Puente for their encouragement and support.
This work was supported by operating grants to B.B.F. from the Medical Research Council of Canada (MRC) and the Canadian Bacterial Disease Network. C.M.R. is supported by a Natural Sciences and Engineering Research Council of Canada postgraduate scholarship, A.G. is supported by an MRC doctoral research award, and B.A.V. is funded by an MRC postdoctoral fellowship. B.B.F. is a Howard Hughes International Scholar and is an MRC Scientist.
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FOOTNOTES |
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* Corresponding author. Mailing address: Biotechnology Laboratory, University of British Columbia, Room 237 Wesbrook Building, 6174 University Blvd., Vancouver, British Columbia V6T 1Z3, Canada. Phone: (604) 822-2210. Fax: (604) 822-9830. E-mail: bfinlay{at}interchange.ubc.ca.
Editor: A. D. O'Brien
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Infection and Immunity, October 2001, p. 6217-6224, Vol. 69, No. 10
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.10.6217-6224.2001
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