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Infection and Immunity, May 2000, p. 2484-2492, Vol. 68, No. 5
Max von Pettenkofer-Institut für
Hygiene und Medizinische Mikrobiologie,
Ludwig-Maximilians-Universität München, Munich, Germany
Received 14 December 1999/Returned for modification 18 January
2000/Accepted 1 February 2000
Yersinia enterocolitica infection of epithelial cells
results in interleukin-8 (IL-8) mRNA expression. Herein we demonstrate that besides IL-8, increased mRNA levels of five other cytokines, IL-1 Upon infection of the host, invasive
and noninvasive enteric pathogens first encounter the host's mucosal
surfaces lined by epithelial cells. The function of these cells in host
defense goes far beyond the mere mechanical barrier that separates the host's internal milieu from the external environment. In fact, epithelial cells can be considered an integral component of the mucosal
immune system, as they provide the underlying mucosa with the first
signals of an infection (22, 36). Thus, invasion by
enteropathogenic bacteria such as Salmonella enterica
serovar Dublin, Shigella dysenteriae, Yersinia
enterocolitica, Listeria monocytogenes, or
enteroinvasive Escherichia coli prompts a rapid cytokine
response in epithelial cells that orchestrates the early phase of
immune reactions, including the initiation of the cellular host
responses (20, 21, 24, 35).
On the other hand, cytokine responses by epithelial or phagocytic cells
can be disrupted by some pathogenic bacteria, eventually enabling their
escape of the host's immune system (for a review, see reference
62). For instance, inhibition of cytokine release in
macrophages by bacterial products has been reported for Y. enterocolitica, Brucella suis, Vibrio
cholerae, Bacillus anthracis, and Pseudomonas
aeruginosa (9, 11, 30, 37, 56, 59).
Y. enterocolitica causes various clinical syndromes ranging
from self-limited enterocolitis to potentially fatal systemic infection
(16). The virulence of Y. enterocolitica is
encoded by chromosomal (e.g., inv and yst)
(18, 31, 42, 46) and Yersinia virulence plasmid
(pYV)-encoded genes, including yadA and genes encoding
Yersinia outer proteins (Yops) (for reviews, see references
13 to 15).
After orogastic infection of mice, Y. enterocolitica
selectively invades M cells located in the follicle-associated
epithelium overlying Peyer's patches (1, 26, 27). After
transcytosis via M cells, Y. enterocolitica multiplies in
Peyer's patch tissue, thereby triggering an enormous recruitment of
polymorphonuclear and mononuclear phagocytes (3). This leads
to the formation of microabscesses and destruction of the
cytoarchitecture of Peyer's patches. Thereafter, yersiniae
disseminate, and abscesses appear in the mesenteric lymph nodes
(1). The massive influx of immune cells into the infected
mucosal tissue and their simultaneous activation might be due to the
activity of various cytokines released by epithelial cells.
Interleukin-8 (IL-8), which is released by intestinal epithelial cells
after exposure to Y. enterocolitica, is a potent
chemoattractant from the family of CXC chemokines (21).
Previous work from our laboratory suggested that
Yersinia-triggered IL-8 secretion depends on cell adhesion
rather than on bacterial invasion, suggesting that Yersinia
adhesion to epithelial cells via the bacterial outer membrane protein
invasin activates de novo synthesis and secretion of IL-8
(57). Other groups reported that secretion of IL-8 and other
cytokines after infection of epithelial cells with Helicobacter
pylori or S. enterica serovar Typhimurium was due to
the activation of the transcription factor NF- To obtain a more detailed view of the early cytokine network in
Yersinia-infected mucosa, we have now focused on other
proinflammatory cytokines which have been reported to be activated via
NF- Bacterial strains and growth conditions.
Plasmid-harboring
(pYV+) and plasmid-cured (pYV
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Yersinia enterocolitica Invasin Protein Triggers
Differential Production of Interleukin-1, Interleukin-8, Monocyte
Chemoattractant Protein 1, Granulocyte-Macrophage Colony-Stimulating
Factor, and Tumor Necrosis Factor Alpha in Epithelial Cells:
Implications for Understanding the Early Cytokine Network in
Yersinia Infections
ABSTRACT
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
, IL-1
, monocyte chemoattractant protein 1 (MCP-1),
granulocyte-macrophage colony-stimulating factor (GM-CSF), and tumor
necrosis factor alpha (TNF-), can be detected upon infection of HeLa
cells with Yersinia. Yersinia-triggered
cytokine production was not affected by blocking
phosphatidylinositol-3-phosphate kinase with wortmannin, which
inhibited bacterial invasion. Comparable cytokine mRNA responses were
triggered by Escherichia coli expressing Yersinia
inv, while no response was triggered by an
inv-deficient Yersinia mutant. Moreover,
cytokine responses were independent from metabolic activity of the
bacteria, as killed bacterial cells were sufficient for triggering
cytokine responses in HeLa cells. Semiquantitative reverse
transcription-PCR analysis was used to assess the kinetics of cytokine
mRNA expression in infected HeLa cells. IL-8, IL-1, IL-1, MCP-1,
GM-CSF, and TNF- mRNA expression increased within 1 h
postinfection, reached a maximum after 3 to 4 h, and then declined
to preinfection levels within 3 h. IL-8, MCP-1, and GM-CSF were
secreted by HeLa cells, whereas IL-1 and IL-1 were not secreted
and thus were found exclusively intracellularly. TNF- protein could
not be detected in cell lysates or supernatants. Stimulation of HeLa
cells with IL-1 was followed by increased IL-8 mRNA expression,
whereas stimulation with IL-8 did not induce cytokine production.
Likewise, MCP-1 and GM-CSF did not induce significant cytokine
responses in HeLa cells. Our results implicate that the initial host
response to Yersinia infection might be sustained by IL-8,
MCP-1, and GM-CSF produced by epithelial cells.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
B in epithelial cells
(29, 45).
B (for reviews, see references 5, 8, and
39). By comparing the kinetics of cytokine mRNA
expression, production, and secretion, we gained insight into their yet
unclear role in Yersinia host defense. We further
investigated the function of the Yersinia invasin protein in
this process.
MATERIALS AND METHODS
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
) Y. enterocolitica WA314 (28), inv mutant
Y. enterocolitica (pYV) WA314 (52),
noninvasive E. coli HB101, and the E. coli
HB101(pInv1914) strain expressing Y. enterocolitica inv
(57) were routinely grown in Luria-Bertani broth (LB).
For infection experiments, overnight bacterial cultures were diluted to
an optical density at 600 nm (OD600) of 0.2 in LB and
incubated for another 3 h at 27°C (Y. enterocolitica
pYV) or 37°C (E. coli and Y. enterocolitica pYV+). Bacteria were collected by
centrifugation and washed twice with sterile phosphate-buffered saline
(PBS), pH 7.4. After determination of the OD600,
appropriate dilutions of the bacteria in PBS were performed to infect
the cells with a multiplicity of infection (MOI) of 150 bacteria/cell.
The actual number of bacteria administered was determined by plating
serial dilutions on Mueller-Hinton agar and counting of CFU.
Cell lines. Human cervical epithelial cells (HeLa; ATCC CCL-2.1) and T84 epithelial colon carcinoma cell line were obtained from the American Type Culture Collection, Manassas, Va. Cells were grown in RPMI 1640 (Biochrom KG, Berlin, Germany)-10% heat-inactivated fetal bovine serum (Gibco BRL, Karlsruhe, Germany) supplemented with 2 mM L-glutamine (Gibco BRL), penicillin (100 U/ml), and streptomycin (100 µg/ml) (Biochrom KG) in a humidified 5% CO2 atmosphere at 37°C.
Stimulation of epithelial cells by infection or cytokines.
Confluent monolayers of cells, grown in six-well plates, were washed
twice with PBS, and incubated in medium containing heat-inactivated fetal bovine serum without antibiotics. After 1 to 2 h of
equilibration, bacterial samples were added. Monolayers and bacteria
were incubated for 1 h to allow bacterial adherence and entry.
After removal of the medium, cultures were washed three times with PBS
to remove extracellular bacteria and further incubated for up to 4 h in the presence of 100 µg of gentamicin per ml of medium to
kill remaining extracellular bacteria. Then culture supernatants were removed and centrifuged for 10 min at 15,000 × g to
pellet residual bacteria and cells before cytokine determination. For
the determination of intracellular cytokines, cells were lysed with
double-distilled water in the presence of proteinase inhibitors
(phenylmethylsulfonyl fluoride and Complete protease inhibitor
cocktail tablets; Boehringer, Mannheim, Germany) and by freezing at
80°C and thawing; cells were then centrifuged for 20 min at
15,000 × g to pellet nonsoluble cell fragments. For
reverse transcription-PCR (RT-PCR) analysis, cells were washed twice
with PBS before total RNA extraction. We used bacterial
lipopolysaccharide (LPS) derived from E. coli O55:B5 and
Salmonella serovar Typhimurium (Bacto Lipopolysaccharides; Difco, Detroit, Mich.) in some stimulation experiments. Stock solutions
of wortmannin (Sigma), 10 mM, were prepared in dimethyl sulfoxide.
Tumor necrosis factor alpha (TNF-) was a gift from Bender, Vienna,
Austria; phorbol myristate acetate was obtained from
Calbiochem. Human recombinant cytokines were obtained from R&D Systems,
Wiesbaden-Nordenstadt, Germany (IL-1, IL-1,
granulocyte-macrophage colony-stimulating factor [GM-CSF], and
monocyte chemoattractant protein 1 [MCP-1]) and Pharmingen, San
Diego, Calif. (IL-8). For cell stimulation, the cytokines were added to
HeLa cell cultures at various concentrations. After 1 h, the
medium was removed, the cell monolayers were washed extensively, and
fresh medium without cytokines was added. After various intervals, the
supernatants were harvested for enzyme-linked immunosorbent assay
(ELISA), and the cells were harvested and RNA was prepared as described below.
Determination of cytokine production by ELISA.
The amounts
of cytokines released into the culture supernatant or remaining in the
cells were determined by ELISA. For IL-1, IL-1, GM-CSF, and
MCP-1, assay kits from R&D Systems were used. An ELISA for IL-8 was
established with optimal concentrations of a mouse anti-human IL-8
monoclonal antibody (MAb) and a biotinylated mouse anti-human IL-8 MAb
as detecting antibody as described previously (57). ELISA
microtiter plates (Nunc, Roskilde, Denmark) were coated overnight with
anti-human IL-8 MAb (G265-5; Pharmingen). After nonspecific binding
sites were blocked, supernatants were added to the wells and incubated
overnight. After several washing steps, biotin-labeled anti-human IL-8
MAb (G265-8; Pharmingen) was added. Finally, an avidin-biotin-alkaline
phosphatase complex (Strept ABC-AP kit; Dako, Glostrup, Denmark) was
used. For signal development, the wells were incubated with
p-nitrophenylphosphate disodium (Sigma), and the OD was
determined at wavelengths of 405 and 490 nm. IL-8 concentrations were
calculated from the straight-line portion of standard curves revealed
by means of recombinant human IL-8 (Pharmingen).
RT-PCR analysis.
As previously described (57),
total RNA of infected HeLa cells in six-well plates was extracted using
1 ml of TRIzol reagent (Gibco BRL). RNA (5 µg) was reverse
transcribed as described by Bohn et al. (10). cDNA products
were amplified by PCR in 50 µl of a mixture containing 10 mM Tris (pH
8.3), 50 mM KCl, and 2.5 mM MgCl2 plus 200 mM each dATP,
dCTP, dGTP, and dTTP in the presence of 25 pmol each of 5' and 3'
primer (35) and 2.0 U of AmpliTaq DNA polymerase or AmpliTaq
Gold DNA polymerase (for IL-8 and TNF-; Perkin-Elmer,
Überlingen, Germany). Temperature profiles for the amplification
were as described in reference 35; 1 min of
denaturation at 95°C and 2.5 min of annealing and extension at 60°C
(IL-1, IL-1, IL-8, and MCP-1), 65°C (GM-CSF), or 72°C
(TNF- and -actin). The number of PCR cycles was adjusted as
appropriate to maximize the differences between samples (-actin, 22 cycles; IL-8, IL-1, and MCP-1, 25 cycles; IL-1 and GM-CSF, 30 cycles; TNF-, 35 cycles). Negative controls were performed by
omitting RNA from the cDNA synthesis and specific PCR amplifications. PCR products were separated in 2% agarose gels and stained with ethidium bromide. Primers were obtained from Roth (Karlsruhe, Germany);
primer sequences (35) are shown in Table
1.
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-actin mRNA level. The
points of time of half-maximum cytokine expression were calculated to
assess the kinetics of cytokine mRNA expression.
Statistical analysis. Data were analyzed using Student's t test. P values of <0.05 were considered statistically significant. All experiments were repeated several times and yielded comparable results.
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RESULTS |
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Introduction
Materials and Methods
Results
Discussion
References
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Y. enterocolitica-induced mRNA expression in HeLa
cells.
To assess the role of epithelial cells in generating
signals for the underlying mucosa and circulating immune cells in
Yersinia infections, we treated HeLa cells with Y. enterocolitica pYV at an MOI of 150 bacteria/cell
and analyzed mRNA extracted 3 h after infection. As shown in Fig.
1A, mRNA levels of the six proinflammatory cytokines, IL-8, TNF-, IL-1, IL-1, MCP-1, and GM-CSF, were markedly increased upon Yersinia infection
compared with noninfected cells. In keeping with previous
results (55, 56), infection of HeLa cells with Y. enterocolitica pYV+ did not significantly induce
expression of any of these cytokines, as secreted Yops suppress
cytokine production. Furthermore, infection of other epithelial cell
lines including T84 revealed similar results for IL-8 as infection with
HeLa cells (data not shown). Cytokine mRNA induction could not be
attributed to bacterial LPS since HeLa cells were completely
unresponsive to LPS derived from E. coli or
Salmonella serovar Typhimurium (not shown). This observation was made in both the presence and the absence of normal human serum.
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Adhesion of Yersinia to HeLa cells is sufficient to
trigger proinflammatory cytokine responses.
Recently we
showed that the phosphatidylinositol-3-phosphate kinase (PI3-K)
inhibitor wortmannin blocks invasion of Y. enterocolitica into epithelial cells but does not affect
Yersinia-induced IL-8 expression and secretion
(57). In accordance with these results, inhibition of
Yersinia invasion by wortmannin (not shown) did not alter
the Yersinia-induced mRNA expression of IL-8, TNF-, IL-1, IL-1, MCP-1, and GM-CSF (Fig. 1B). Wortmannin itself
did not induce cytokine mRNA expression or modulate phorbol myristate acetate-induced cytokine mRNA expression in HeLa cells (not shown). From these data we conclude that bacterial adhesion, rather than invasion, triggers IL-8, TNF-, IL-1, IL-1, MCP-1, and
GM-CSF mRNA production in epithelial cells.
Yersinia invasin protein triggers cytokine mRNA
expression.
In previous work we found that induction of IL-8 mRNA
in HeLa cells after Yersinia infection was dependent on
expression of the Y. enterocolitica outer membrane protein
invasin (57). Invasin mediates bacterial invasion by binding
to 1 integrins on the host cell surface (32). To
evaluate the contribution of invasin to
Yersinia-induced cytokine expression, we used a
Yersinia mutant deficient in the inv gene
(Y. enterocolitica pYV inv), which
is unable to invade epithelial cells (not shown). As shown in Fig. 1,
the Yersinia inv mutant was unable to induce cytokine mRNA
expression in HeLa cells. Likewise, a recombinant E. coli(pInv1914) strain expressing Y. enterocolitica inv,
but not E. coli, was able to induce IL-8, TNF-, IL-1,
IL-1, MCP-1, and GM-CSF mRNA expression. Furthermore, although
treatment with the PI3-K inhibitor wortmannin blocked E. coli pInv1914 invasion (not shown), this treatment did not affect
cytokine mRNA production. These results suggest that invasin-mediated
bacterial adhesion is sufficient to induce expression of
proinflammatory cytokines in epithelial cells.
Killed Yersinia induce cytokine responses in HeLa
cells.
For several pathogens, including Salmonella
spp., H. pylori, and Chlamydia spp., it has been
demonstrated that metabolic activity or an active type III protein
secretion system is necessary to induce cytokine responses in infected
cells (40, 48, 58). As the Yersinia invasin
protein appears to be essential for triggering cytokine responses in
epithelial cells, we wanted to investigate the potential of
metabolically inactive yersiniae expressing invasin to trigger cytokine
production. For this purpose, Y. enterocolitica pYV bacteria expressing invasin were killed by gentamicin
or heat treatment. Killed bacterial cell suspensions were added to HeLa cells, and cytokine production was determined. As shown in Fig. 2, killed Y. enterocolitica
pYV cells induced IL-8 mRNA expression and IL-8 protein
production to a similar degree as viable bacteria. Infection of
cells with different numbers of bacteria showed a dose-dependent
response in terms of IL-8 mRNA expression. Comparable results were
achieved by infection with heat-killed E. coli(pInv1914) expressing Yersinia invasin
(data not shown). These data show that metabolic activity of bacteria
is not necessary for invasin-mediated cytokine production and
secretion by HeLa cells.
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Kinetics of Yersinia-induced proinflammatory
cytokine mRNA production in HeLa cells.
To obtain a more
detailed view of the early Yersinia-induced cytokine network
in epithelial cells, the kinetics of cytokine mRNA expression was
assessed semiquantitatively by means of fluoroimager analysis.
The data depicted in Fig. 3 show that
IL-8, TNF-, IL-1, IL-1, MCP-1, and GM-CSF mRNA expression was
upregulated within 1 h postinfection to reach a maximum
after 3 h. Only MCP-1 showed a slightly delayed peak between 3 and
4 h. mRNA levels then declined to levels before infection within
the following 3 to 5 h. Points of time of half-maximum mRNA levels
were calculated as indicators of the sequential order of cytokine mRNA
expression. As indicated in Fig. 3, IL-8 was expressed first, about 20 to 30 min before IL-1 and MCP-1, which were closely followed by
IL-1, TNF-, and GM-CSF.
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IL-8, MCP-1, and GM-CSF, but not IL-1 and IL-1, are secreted
by HeLa cells.
We next measured the amount of cytokine protein in
cell culture supernatants and cell lysates of
Yersinia-infected HeLa cells to gain additional information
on whether secreted cytokines might augment the bacterium-stimulated
cytokine responses of epithelial cells. The results shown in Table
2 demonstrate that 4 to 6 h postinfection considerable quantities of IL-8, MCP-1, and GM-CSF were
secreted into culture supernatants by HeLa cells, whereas IL-1 and
IL-1 could be detected intracellularly only in cell lysates. MCP-1
was detectable also in cell lysates, although in small quantities only.
TNF- was not detectable in culture supernatants or cell lysates by
ELISA. At 24 h after infection, IL-1 and IL-1 still remained
intracellular in gradually decreasing levels, and neither of the two
cytokines was secreted. In contrast, MCP-1, like IL-8, was detectable
only extracellularly in supernatants after 24 h. As observed after
4 to 6 h, TNF- was not detectable by ELISA or Western blotting
in all lysates or supernatants after 24 h (data not shown).
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IL-1, but not IL-8, stimulates cytokine responses in HeLa
cells.
To investigate whether IL-8, which was produced and
secreted by Yersinia-stimulated HeLa cells, might augment
epithelial cytokine production, HeLa cells were stimulated with various
quantities of IL-8, and at various intervals culture supernatants as
well as cell lysates were analyzed for the presence of cytokines by RT-PCR (Fig. 4) and ELISA (not shown). As
controls, Yersinia- or IL-1-stimulated HeLa cells were used.
The results in Fig. 4 show that IL-8 did not stimulate cytokine
production in HeLa cells, whereas Yersinia and IL-1
stimulated all of the cytokines investigated (IL-8, IL-1,
IL-1, and MCP-1) in a dose-dependent manner. Moreover, exposure of
HeLa cells to various concentrations of MCP-1 or GM-CSF did not induce
significant cytokine responses (data not shown).
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DISCUSSION |
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Abstract
Introduction
Materials and Methods
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Discussion
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Although several studies with detailed histologic approaches analyzed the inflammatory response of the infected mucosa to infection by Y. enterocolitica (2, 4), it is still unclear which pathogen and host signals may trigger and promote this reaction. Epithelial cells, the first cells to encounter yersiniae upon orogastric infection, are attributed a key role in generating signals to the underlying mucosa, thereby initiating the host's immune response. To evaluate the role of epithelial cells in intestinal inflammation upon Yersinia infection, we used an epithelial cell monolayer infection model and analyzed Yersinia-triggered cytokine production in these cells.
Infection of HeLa cells with Y. enterocolitica resulted in
mRNA expression of several proinflammatory cytokines,
including IL-8, TNF-, IL-1, IL-1, MCP-1, and GM-CSF.
However, only IL-8, MCP-1, and GM-CSF were secreted into the
extracellular environment, while IL-1 was produced but not
secreted. TNF- protein was not detectable at all. Although we cannot
exclude that the ELISA and Western blot assays used for detection of
TNF- protein production were not sensitive enough, TNF- mRNA
expression was detected only after 35 PCR cycles, suggesting that very
low quantities of TNF- mRNA (and possibly protein) were produced.
The CXC chemokine IL-8, which could be detected in our model immediately after Yersinia infection, attracts and activates predominantly neutrophils but also monocytes and T lymphocytes (6). MCP-1, a CC chemokine, has a more specific chemotactic activity for monocytes and basophils (38; see reference 7 for a review). GM-CSF, which was also found after Yersinia infection of HeLa cells, is a strong chemoattractant for neutrophils and eosinophils (60). Moreover, GM-CSF stimulates the proliferation and differentiation of neutrophilic, eosinophilic, and monocytic cell lineages and functionally activates the corresponding mature forms of these cells by, e.g., enhancing phagocytosis of bacteria by neutrophils (17, 25, 41, 61). All of the aforementioned effects of IL-8, MCP-1, and GM-CSF might be involved in triggering cellular immune responses against Yersinia as observed in a mouse infection model. In Yersinia-infected mice, polymorphonuclear leukocytes are recruited into infected Peyer's patches 24 h after infection and give rise to microabscesses (1, 3). Several days thereafter, further inflammatory cells including mononuclear phagocytes are recruited into Yersinia-induced Peyer's patch lesions and promote tissue destruction.
While IL-8, MCP-1, and GM-CSF were secreted, both IL-1 and IL-1
were produced but not secreted by HeLa cells upon Yersinia infection and thus remained intracellular for more than 24 h. This observation argues for a special role of IL-1 in Y. enterocolitica infection. Similar to infections with other
pathogens such as Entamoeba histolytica (23), it
might well be that a second challenge to the epithelial cells (e.g.,
cytotoxicity) may be required for IL-1 release during
Yersinia infection. Trophozoites of the protozoan parasite
Entamoeba histolytica induce increased mRNA expression of
several proinflammatory cytokines in HeLa cells similar to that
observed after Y. enterocolitica infection (23).
However, cytokine production and secretion are predominantly due to the paracrine action of preformed, constitutively expressed IL-1 which
is released after Entamoeba-induced cytolysis
(23). After Chlamydia infection of epithelial
cells, mRNA expression and secretion of IL-8, GM-CSF, and other
proinflammatory cytokines is upregulated (48). Similar to
Entamoeba histolytica infection, cytokine mRNA upregulation
could be attributed mainly to the paracrine action of IL-1, which
was passively released by epithelial cells damaged by
Chlamydia infection (48). However, an additional
signaling pathway for direct induction of IL-8 production and secretion was postulated. In Shigella flexneri infection,
presynthesized IL-1 is released from macrophages as a stress signal
paralleled by apoptosis. However, Shigella itself is
incapable of inducing de novo synthesis of cytokines in macrophages
(53). Taken together, in infections with
Shigella, Entamoeba, or Chlamydia,
IL-1 is the actual inducer of proinflammatory cytokine production
and secretion leading to tissue inflammation.
Unlike infection with Entamoeba histolytica,
Chlamydia, or S. flexneri, production and
secretion of IL-8 in Yersinia infection was not linked to the release
of intracellular IL-1. In fact, in our experiments Y. enterocolitica pYV infected HeLa cells were not
damaged and did not undergo apoptosis consistent with other
publications (43, 44, 51). Therefore, both IL-1 and
IL-1 remained intracellular for more than 24 h after infection.
However, pathogenic yersiniae harbor a virulence plasmid which encodes
Yop effector proteins, e.g., YopE mediating cytotoxicity
(50). Therefore, it is conceivable that such events might
lead to the release of IL-1 from epithelial cells during Yersinia infection in vivo.
In contrast to IL-1, both IL-8 and MCP-1 as well as GM-CSF did not
augment the inflammatory response of epithelial cells. In keeping with
these observations, recent investigations (19, 34)
demonstrated a distinct pattern of CC/CXC receptor expression on human
colon epithelial cells such as HT29, Caco-2, and T84 cells. Hence,
CCR1-8 and CXCR4-5 are all constitutively expressed on these cells,
whereas CXCR1 and CXCR2 are little, if at all, expressed. As IL-8 binds
to CXCR1 and CXCR2, and GM-CSF and MCP-1 bind to CCR2 or CCR10, it is
evident that these cytokines do not act on epithelial cells. Although
HeLa cells have not been included in the aforementioned studies, our
results may suggest that HeLa cells do not express CXCR1, CXCR2, CCR2,
and CCR10. In keeping with these data, we found that IL-1, but not
IL-8, MCP-1, or GM-CSF, is a potent stimulus for transcription and
secretion in HeLa cells of proinflammatory cytokines such as IL-8,
MCP-1, and GM-CSF. Furthermore, IL-1 itself stimulates IL-1 and
IL-1 production in HeLa cells (this work) and other epithelial cells
(23, 35). Nevertheless, further work is required on cytokine
receptor expression on the various epithelial cell lines as well as on
intestinal epithelial cells in situ.
Yersinia-induced cytokine production could be attributed to
the activity of a virulence factor, the Yersinia outer
membrane protein invasin, which is known to bind to 1 integrins of
mammalian cells, thereby mediating, e.g., bacterial internalization
into host cells (32). As a further pathogenic effect of
invasin, we found that binding of bacteria via invasin to 1
integrins on epithelial cells leads directly to the expression of
proinflammatory cytokines including IL-8. For several other bacteria
infecting epithelial surfaces (e.g., Salmonella spp.
[29, 40], H. pylori [45,
58], or Chlamydia [48]), it was
shown that bacterial protein synthesis or a type III or IV protein
secretion system was necessary to induce a cytokine responses. In
Yersinia infection, however, the type III protein secretion
system might counteract invasin-triggered cytokine production
(56). Moreover, in contrast to other enteropathogenic
bacteria like Salmonella serovar Dublin or enteroinvasive E. coli (21), we could show that Yersinia invasin-mediated cytokine induction did not require bacterial invasion,
as inhibition of bacterial entry with the PI3-K inhibitor wortmannin
did not alter the Yersinia-induced cytokine pattern. Furthermore, killed invasin-expressing bacterial cells trigger cytokine
production comparable to that induced by viable bacteria.
Based on these and previous results, we propose the following scenario
for Yersinia infection in vivo. Invasin-expressing yersiniae
are translocated efficiently through M cells, and invasin plays an
important role in the early phase of Peyer's patch infection (1,
12, 47). Via interaction with 1 integrins on host cells,
invasin might trigger production and release of
proinflammatory cytokines and chemokines. Thereafter, yersiniae
express plasmid-encoded pathogenicity factors (1, 33) in
order to evade the innate host immune response. Yersiniae might
translocate effector proteins such as YopE, YopH, YopM, and YopJ into
the cytosol of host cells (for a review, see reference
15). YopE may disrupt host cells by destroying the
actin cytoskeleton (49), and YopJ/YopP may induce
apoptosis of macrophages (43, 44). It is tempting to speculate that these events might lead to release of both
preformed as well as invasin-induced de novo-produced IL-1. In turn,
this process might augment the inflammatory response initially
triggered by invasin-induced IL-8, MCP-1, and GM-CSF release.
Whether the inflammatory response induced by Yersinia invasin has protective (anti-Yersinia) or deleterious (destruction of Peyer's patches by the inflammatory response) effects is a matter of ongoing research in our laboratory. Current investigations in our laboratory focus on the chemokine production including production of IL-8-like chemokines in the early phase of the Yersinia infection in mice. Moreover, we have to take into account that in vivo cells other than epithelial cells (e.g., dendritic cells) might also contribute to chemokine production (54).
In summary, our observations may have implications for understanding the early cytokine network operating in mucosal Yersinia infections and further define the role of Y. enterocolitica invasin as an important outer membrane protein with a high contribution to Yersinia pathogenicity in the early phase of mucosal infection.
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ACKNOWLEDGMENTS |
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This work was supported by a grant from the Deutsche Forschungsgemeinschaft.
We thank Nicole Bücheler and Sonja Preger for expert technical assistance.
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FOOTNOTES |
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* Corresponding author. Mailing address: Max von Pettenkofer-Institut für Hygiene und Medizinische Mikrobiologie, Ludwig Maximilians-Universität, Pettenkoferstrasse 9a, D-80336 Munich, Germany. Phone: 49-89-51605280. Fax: 49-89-51605223. E-mail: Autenrieth{at}m3401.mpk.med.uni-muenchen.de.
Editor: J. D. Clements
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REFERENCES |
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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| 1. |
Autenrieth, I. B., and R. Firsching.
1996.
Penetration of M cells and destruction of Peyer's patches by Yersinia enterocolitica: an ultrastructural and histological study.
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