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Previous Article | Next Article 
Infection and Immunity, September 2000, p. 5183-5189, Vol. 68, No. 9
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Shiga Toxin-Induced Tumor Necrosis Factor Alpha
Expression: Requirement for Toxin Enzymatic Activity and Monocyte
Protein Kinase C and Protein Tyrosine Kinases
Gregory H.
Foster,
Cassandra
S.
Armstrong,
Ramesh
Sakiri, and
Vernon L.
Tesh*
Department of Medical Microbiology and
Immunology, Texas A&M University Health Science Center, College
Station, Texas 77843-1114
Received 2 December 1999/Returned for modification 6 March
2000/Accepted 20 June 2000
 |
ABSTRACT |
Infections with Shiga toxin (Stx)-producing bacteria cause bloody
diarrhea which may progress to life-threatening complications, including acute renal failure and neurological abnormalities. The
precise mechanism of disease progression is unclear, although evidence
suggests that the localized production of the host proinflammatory cytokines tumor necrosis factor alpha (TNF-
) and interleukin-1 may
exacerbate toxin-mediated vascular damage. Purified Stxs have been
demonstrated to elicit proinflammatory cytokine synthesis from human
peripheral blood mononuclear cells and monocytic cell lines in vitro.
To understand toxin-monocyte interactions required for cytokine
synthesis, we have treated differentiated THP-1 cells with purified
wild-type toxins, enzymatic mutants, or B subunits and measured TNF-
production. Our data suggest that A subunit enzymatic activity is
essential for cytokine production. THP-1 cells were treated with a
series of protein kinase C (PKC), PKA, and protein tyrosine kinase
inhibitors to examine the role of intracellular signaling molecules in
Stx-mediated cytokine production. Treatment of cells with PKC and
tyrosine kinase inhibitors blocked TNF- secretion by Stx-stimulated
THP-1 cells. Stx treatment directly activated PKC, which occurred at a
point upstream of transcriptional activation of the gene encoding
TNF-.
| |
INTRODUCTION |
Shiga toxins (Stxs) are a group of
antigenically and functionally related protein toxins produced by the
enteric pathogens Shigella dysenteriae serotype 1 and
Escherichia coli serotypes categorized as enterohemorrhagic
E. coli. All members of the Stx family are AB5
holotoxins composed of an approximately 32-kDa A subunit protein in
noncovalent association with a pentameric ring of identical B subunit
proteins, each with a molecular mass of ~7.7 kDa. The A subunit is
the enzymatic component of the toxins and acts as a highly specific
N-glycosidase enzyme hydrolyzing the bond between ribose and
a single adenine residue found on a prominent loop structure in the 28S
rRNA component of eukaryotic ribosomes (6, 30). The
depurination reaction results in the rapid inhibition of protein
synthesis. Toxin binding to cells is mediated by B subunits which
primarily associate with the membrane neutral glycolipids
globotriaosylceramide (Gb3;
Gal1
4Gal
14GlcCer) (16, 18) and
globotetraosylceramide (Gb4;
GalNAc13Gal14Gal14GlcCer) (4,
29). S. dysenteriae serotype 1 produces the
prototypical Stx, whereas E. coli has been shown to
elaborate one or more toxins closely related to Stx, designated Stx1,
Stx2, Stx2c, Stx2d, and Stx2e (reviewed in reference
22).
Although infections with Stx-producing organisms generally cause
self-limited bloody diarrhea, patients are at increased risk for the
development of life-threatening complications. Chief among these
complications are progression to acute renal failure (hemolytic uremic
syndrome) and neurological abnormalities, such as seizures, stroke, and
coma (17, 34). A frequent pathologic finding in these
sequelae is damage to capillaries in the colon, kidneys, and central
nervous system (12). Thus, Stxs appear to selectively damage
microvascular endothelial cells. This concept was supported by work
demonstrating that human vascular endothelial cells were killed when
exposed to purified Stx in vitro (23). It was subsequently shown that human endothelial cells were sensitized to the cytotoxic action of Stxs by treatment of the cells with the proinflammatory cytokines tumor necrosis factor alpha (TNF-) or interleukin 1 (IL-1)
(19, 38, 42). The mechanism of sensitization involved increased endothelial cell Gb3 biosynthesis through TNF
receptor p55 signaling and protein kinase C (PKC) activation (20,
41). Thus, the proinflammatory cytokine response to Stxs may
contribute to pathogenesis by sensitizing endothelial cells to the
direct toxic effects of Stxs.
Cellular sources of proinflammatory cytokines produced in vivo in
response to Stxs remain to be characterized. However, it has been shown
that human monocytes and monocytic cell lines respond to the toxins by
synthesizing and secreting TNF-, IL-1, and IL-6 (26,
43). Using Northern blot analyses, we showed that Stxs affect
cytokine expression, at least in part, at the transcriptional level via
mechanisms that may involve activation of the DNA-binding proteins
nuclear factor 
B (NF-B) and activator protein-1 (28). The precise mechanisms by which Stxs, potent protein synthesis inhibitors that interact with membrane glycolipids, transduce signals
in monocytes necessary to activate cytokine gene expression are not
known. The experiments reported here are designed to elucidate the
toxin components necessary for proinflammatory cytokine induction and
to initially characterize host cell signaling pathways involved in
cytokine expression.
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MATERIALS AND METHODS |
Toxins and cytokine inducers.
Purified Stx1 and Stx2e were
prepared from recombinant E. coli strains expressing toxin
operons under control of thermoinducible promoters. Toxins were
purified from bacterial sonicates by sequential DEAE-Sepharose and
chromatofocusing column chromatography or MonoQ high-performance liquid
chromatography as previously described (10, 29, 38). At each
step, fractions were tested for Vero cell cytotoxicity by using the
assay of Gentry and Dalrymple (8). A purified Stx1 enzymatic
mutant, in which glutamate at position 167 and arginine at position 170 in the A subunit were replaced with glutamine and leucine, respectively
(Stx1-E167Q-R170L), by oligonucleotide-directed site-specific
mutagenesis, was the kind gift of Yoshifumi Takeda, National Institute
of Infectious Diseases, Tokyo, Japan. The preparation and purification
of Stx1-E167Q-R170L has been described previously (24). The
mutant Stx1 holotoxin exhibited high-performance liquid chromatography
and sodium dodecyl sulfate-polyacrylamide gel electrophoresis
(SDS-PAGE) profiles similar to those of the wild-type toxin.
Ouchterlony double gel diffusion with antisera raised against the
mutant toxin showed a line of identity between Stx1-E167Q-R170L and
wild-type Stx1, and both toxin preparations were shown to bind
Gb3 by thin-layer chromatography (24, 45). A
purified Stx2e enzymatic mutant in which glutamate at position 167 was
replaced with glutamine (Stx2e-E167Q) was the kind gift of James E. Samuel, Texas A&M University Health Science Center, College Station,
Tex. Stx2e-E167Q mutagenesis and purification procedures have been
published (10). The E167Q-R170L and E167Q point mutations
reduce verocytotoxicity approximately 105- to
106-fold compared to the verocytotoxicities of wild-type
Stx1 and Stx2e, respectively (10, 24). Purified pentameric
Stx1 B subunits were the kind gift of David Acheson, Tufts University
School of Medicine (Boston, Mass.). Molecular biology and purification
procedures for the Stx1 B subunit preparation have been reported
(1). Endotoxin contamination of all toxin preparations was
tested by Limulus amoebocyte lysate assay (Pyrotell,
Associates of Cape Cod, Inc., Falmouth, Mass.) prior to use in cytokine
induction experiments. Ricin and purified E. coli O111:B4
lipopolysaccharide (LPS) were purchased from Sigma Chemical Co., St.
Louis, Mo. Murine monoclonal immunoglobulin M antibody pK002 directed
against Gb3 was purchased from Accurate Chemical Corp.
(Westbury, N.Y.).
Cells.
The human myelogenous leukemia cell line THP-1
(40) was purchased from American Type Culture Collection
(Manassas, Va.) and maintained in RPMI 1640 (Gibco BRL, Grand Island,
N.Y.) supplemented with penicillin (50 U/ml), streptomycin (50 µg/ml), and 10% fetal bovine serum (FBS; Hyclone Laboratories,
Logan, Utah). Vero cells were grown in Minimum Essential Medium (Gibco
BRL) with Earle's salts, 10 mM L-glutamine, and the
supplements listed above. L929 cells were cultured in Iscove's
modified Dulbecco's medium with 10% FBS. All cells were maintained at
37°C in humidified 5% CO2.
Macrophage differentiation.
THP-1 cells (106
cells/ml) grown in 60-mm-diameter culture dishes were induced to
differentiate to a mature macrophage-like state by treatment with
phorbol-12-myristate-13-acetate (PMA; Sigma) at 50 ng/ml for 48 h.
Plastic-adherent, differentiated cells were then washed twice in cold
Dulbecco's phosphate-buffered saline (PBS) and incubated with fresh
medium lacking PMA for 72 h with daily medium changes prior to use
in experiments. Unless otherwise noted, differentiated THP-1 cells were
used in all experiments.
Analysis of protein synthesis.
Stx enzymatic activity was
examined by measuring the inhibition of [3H]leucine
incorporation into nascent polypeptides. Briefly, THP-1 or Vero cells
grown in 24-well microtiter plates were incubated with purified Stxs
(400 ng/ml) for various time points. At each time point, toxins were
removed from the cells by three washes with cold sterile PBS. Forty
microliters of labeling medium containing 10 µCi of
[3H]leucine (DuPont New England Nuclear, Boston, Mass.)
in leucine-free RPMI 1640 plus 10% FBS was added to each well, and the
cells were incubated for 30 min at 37°C. The plates were then placed
on ice, and excess radiolabel was removed by washing with cold PBS.
Twenty microliters of RIPA buffer (0.15 M Tris-HCl [pH 7.4], 0.5%
sodium deoxycholate, 0.5% NP-40, and 0.1% SDS) was added to each
well. Lysates were transferred to microcentrifuge tubes. An additional 20 µl of RIPA buffer was added to the wells to collect any residual lysates. Lysates were centrifuged at 12,700 × g for 15 min at 4°C. Resultant supernatants were transferred to Whatman GF/C
filter papers and allowed to dry. Filters were treated twice with 10% trichloroacetic acid and once with 100% ethanol and were allowed to
air dry. Filters were placed in scintillant, and radioactivity was
measured using a scintillation counter (Beckman LS8000; Beckman Instruments Inc., Fullerton, Calif.).
Analysis of TNF- expression.
Amounts of immunoreactive
TNF- in culture supernatants were measured by enzyme-linked
immunosorbent assay (Quantikine, R&D Systems, Minneapolis, Minn.)
according to the manufacturer's instructions. The sensitivity of the
assay is 4.4 pg/ml. TNF bioactivity in culture supernatants was
measured by the lysis of actinomycin D-treated L929 cells as previously
described (37). We have previously shown that purified
toxins at 400 to 800 ng/ml induce optimal signals in these assays.
Kinase inhibitors.
PKC inhibitors H-7 and K252a, PKA
inhibitor H-89, and protein tyrosine kinase inhibitor genistein were
purchased from Calbiochem, La Jolla, Calif. H-7 and H-89 were dissolved
in sterile water and stored at 4°C. K252a was dissolved in dimethyl
sulfoxide (DMSO)-ethanol (50:50 [vol/vol]) at 500 µg/ml. Genistein
was dissolved in DMSO at 500 µg/ml. K252a and genistein were stored
at 
20°C before use. Differentiated THP-1 cells were treated with
the indicated concentrations of inhibitors for 2 h (genistein) or
3 h (H-7, H-89, and K252a). The cells were then washed twice in
cold PBS and treated with the inhibitors in the presence or absence of Stx1, LPS, PMA, or vehicle control. Trypan blue exclusion studies showed no loss of cell viability in response to treatment of the cells
with inhibitors alone. For all experiments, the percentage of organic
solvents did not exceed 0.2% and had no effect on TNF- expression.
Determination of PKC activity.
THP-1 cells were treated with
Stx1 in the presence or absence of kinase inhibitors. The cells were
washed twice in cold PBS and pelleted by centrifugation at 100 × g for 5 min at 4°C. Cells were resuspended in 50 mM
Tris-HCl (pH 7.5) containing 0.3% (wt/vol) -mercaptoethanol, 1.0 mM
EDTA, 2.5 mM EGTA, 50 µg of phenylmethylsulfonyl fluoride per ml, and
10 mM benzamidine. The cells were disrupted by sonication, and the
homogenates were cleared by centrifugation at 135,000 × g
for 45 min. Total cellular PKC activity in sonicates was examined by
measuring the phosphorylation of a synthetic PKC-specific substrate in
the presence of a [
-32P]ATP donor (Biotrak PKC System;
Amersham Corp., Arlington Heights, Ill.) per the manufacturer's
instructions. PKC activity (picomoles of phosphate
transferred/minute/106 cells) is expressed as a percentage
of basal (untreated cells) levels.
Northern blot analysis of TNF- mRNA.
Total cellular RNA
was extracted from THP-1 cells by the acid guanidinium isothiocyanate
method (2) using Ultraspec II RNA isolation kits (Biotecx
Laboratories, Houston, Tex.). RNA purity was assessed by optical
density readings at 260 and 280 nm. Ten micrograms of RNA per lane was
subjected to electrophoresis using 0.8% agarose-2.0 M formaldehyde
gels in 1× MOPS (morpholinepropanesulfonic acid) running buffer at 50 V for 2 to 3 h. RNA was transferred to positively charged nylon
membranes (GeneScreen Plus; NEN DuPont, Boston, Mass.) by using a
Turboblotter Rapid Downward Transfer System (Schleicher and Schuell,
Keene, N.H.) and was cross-linked by exposing the membrane to UV light
(254 nm) for a total dose of 120 mJ/cm2 (UV Crosslinker;
Bio-Rad, Hercules, Calif.). A human TNF- probe, 5'-ATC TCT CAG CTC
CAC GCC ATT GGC CAG GAG-3' (Clontech, Palo Alto, Calif.), was 5'-end
labeled with [-32P]ATP. An 18S RNA antisense control
template (Ambion Inc., Austin, Tex.) was random prime labeled using
MegaPrime DNA labeling kits (Amersham). After labeling, unincorporated
nucleotides were removed using G-25 Sephadex columns. Membranes were
treated with 7 to 10 ml of Rapid-Hyb hybridization buffer (Amersham)
for 15 min at 42°C for the TNF- probe or 65°C for the 18S RNA
probe. Approximately 106 cpm of TNF- probe was added per
milliliter of hybridization buffer and hybridization was carried out at
42°C for 2 to 4 h. Membranes were washed in 2× SSC-0.1% SDS
for 10 min at room temperature and were exposed to a phosphorimager
screen overnight (1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate).
The screen was analyzed by a phosphorimager (Molecular Dynamics,
Sunnyvale, Calif.), and sums of counts above the background were
calculated using ImageQuant software (Molecular Dynamics). Membranes
were stripped by boiling in 0.1× SSC-0.1% SDS twice for 15 min and
hybridized with 18S RNA probe at 65°C as an internal control for RNA
loading. Ratios of counts of TNF- transcripts to 18S RNA were
calculated. To minimize interassay variability, relative levels of
TNF- mRNA from three separate experiments are shown by expressing
the ratios as percentages above basal (unstimulated) levels by using
the following formula:
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Phosphotyrosine analysis.
Eighteen hours prior to
stimulation, differentiated THP-1 cells were serum starved in medium
containing 0.5% FBS. The cells were then exposed to 1.0 µM genistein
or an equivalent volume of DMSO vehicle control for 2 h prior to
stimulation. The medium was replaced with medium containing purified
Stx1 (400 ng/ml) with or without the kinase inhibitor. Following 1 h of incubation at 37°C, cells were washed twice with cold PBS and
lysed with modified RIPA buffer (1.0% NP-40, 1.0% sodium
deoxycholate, 150 nM NaCl, 10 mM Tris-HCl [pH 7.5], 5.0 mM sodium
pyrophosphate, 1.0 mM NaVO4, 5.0 mM NaF, 1.0 µg of
aprotinin/ml, 1.0 µg of leupeptin/ml, and 0.1 mM phenylmethylsulfonyl
fluoride) for 15 min at 4°C. DNA was sheared by passing cell lysates
through 22 1/2- and 26 3/8-gauge needles. Lysates were cleared by
centrifugation at 14,900 × g for 15 min at 4°C.
Protein content of cell lysates was determined using the Micro BCA
assay kit (Pierce, Rockford, Ill.). Equivalent amounts of proteins were
separated by SDS-12% PAGE and analyzed by Western blotting using an
anti-phosphotyrosine monoclonal antibody (4G10; UBI, Lake Placid, N.Y.)
and anti-mouse immunoglobulin G-horseradish peroxide (HRP) as the
secondary antibody. Blots were developed using the ECL system
(Amersham) by following the manufacturer's instructions.
Statistics.
Two sample-paired t tests were
performed using Minitab Release 8 statistical software (Minitab, Inc.,
State College, Pa.).
| |
RESULTS |
Stx induction of TNF- requires A subunit activity.
Earlier
studies have shown that, in contrast to epithelial or endothelial
cells, human peripheral blood monocytes and differentiated monocytic
cell lines express low levels of membrane Gb3 and are relatively resistant to the cytotoxic action of purified Stxs, with
50% cytotoxic doses (CD50s) of >1.0 µg/ml
(26). However, monocytic cells are not unresponsive to the
toxins; they respond by internalizing toxins and synthesizing the
proinflammatory cytokines TNF-, IL-1, and IL-6 (26,
43). Our preliminary studies showed that toxin receptor binding
by purified Stx1 B subunits did not elicit monocyte cytokine
production. We hypothesized, therefore, that enzymatically active Stx A
subunits may be necessary for cytokine induction. We examined this
hypothesis by treating differentiated THP-1 monocytic cells for 18 h with purified Stx holotoxins or Stx holotoxin molecules containing
point mutations in the A subunit catalytic site (Stx1-E167Q-R170L,
Stx2e-E167Q). The ability of Stxs to induce TNF- production appeared
to require A subunit enzymatic activity (Table
1). To further link TNF- production with toxin enzymatic activity, THP-1 cells were treated with sublethal or lethal concentrations of ricin (CD50, ~5.0 ng/ml), the
Ricinus communis toxic lectin that shares
N-glycosidase activity with Stx A subunits. Ricin treatment
also elicited TNF- production. In contrast, reagents which bind to
Gb3 in the absence of enzymatic activity, i.e., purified
Stx A subunit mutants, purified Stx1 B subunits, or
anti-Gb3 monoclonal antibody, did not induce TNF- synthesis.
To correlate ribosomal inactivation with cytokine production, we
examined protein synthesis inhibition in cells treated with Stxs. When
toxin-sensitive Vero cells (CD50 = 1.0 pg/ml) were treated with purified Stx1 or Stx2e (400 ng/ml), the incorporation of
3[H]leucine into nascent polypeptides was inhibited by
approximately 90% within 1 h of toxin treatment (Fig.
1). We previously showed that
undifferentiated THP-1 cells express relatively high levels of membrane
Gb3, are sensitive to Stx1 (CD50 = 18 pg/ml), and fail to produce TNF- when stimulated with Stxs
(26). Within an hour of treatment with purified Stx1 (400 ng/ml), undifferentiated THP-1 cells manifested an approximate 75%
reduction in protein synthesis. In contrast, when differentiated THP-1
cells were treated with an equivalent dose of Stx1, we noted transient
increases in total protein synthesis 1 to 2 h after toxin
treatment. Following treatment of cells with Stx2e, protein synthesis
was inhibited by, at most, 20% over a 4-h time period. Thus, the
sublethal amounts of Stxs used in these experiments to induce TNF-
expression from differentiated monocytic cells only marginally affected
total protein synthesis.
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FIG. 1.
Protein synthesis inhibition mediated by purified Stxs.
Differentiated THP-1 cells were treated with 400 ng of purified Stx 1 ( ) or Stx2e ( ) per ml, and undifferentiated THP-1 cells ( ) and
Vero cells ( ) were treated with 400 ng of Stx1/ml. At the indicated
time points, cells were washed and incubated an additional 30 min in
medium containing [3H]leucine. Following lysis of the
cells and trichloroacetic acid precipitation of proteins, incorporation
of radiolabeled leucine into nascent polypeptides was measured by
scintillation counting. The data are expressed as percentages of basal
protein synthesis (untreated cells) and are derived from at least three
independent experiments.
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Stx induction of TNF- requires serine/threonine kinase
activity.
Many studies have implicated serine/threonine kinases of
the PKC family as monocyte/macrophage signal transduction molecules required for cytokine production (reviewed in reference
36). We hypothesized that PKC may also participate
in Stx-mediated cell signaling. A series of PKC inhibitors was employed
to monitor the effects of blocking kinase activity on TNF production by
Stx1-treated THP-1 cells. Treatment of cells with the PKC inhibitor H-7
(Fig. 2A) or K252a (Fig. 2B) reduced TNF
secretion in a dose-dependent manner following stimulation of cells
with Stx1 for 12 h. Although H-7 and K252a are potent inhibitors
of PKC, they can also inhibit cyclic nucleotide-dependent protein
kinases (14). To exclude the involvement of PKA in
Stx-induced TNF production, the PKA inhibitor H-89 was used. H-89
inhibits PKA activity at nanomolar concentrations, whereas the
inhibitory concentration for PKC is several hundredfold higher.
Treatment of THP-1 cells with concentrations of H-89 ranging from 0.1 to 1,000 nM did not result in significant decreases in TNF production
in response to Stx1 (data not shown). These data suggest that members
of the PKC family of serine/threonine kinases are involved in Stx
signaling for cytokine production.
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FIG. 2.
Effect of PKC inhibitors on Stx1-mediated TNF production
by THP-1 cells. PMA-differentiated THP-1 cells were pretreated with
various doses of the PKC inhibitors H-7 (A) or K252a (B) for 3 h
prior to stimulation with 800 ng of purified Stx1/ml. Twelve hours
later, culture supernatants were collected and TNF bioactivity was
determined by lysis of actinomycin D-treated L929 cells. Results shown
are mean levels of TNF bioactivity (picograms/milliliter) ± standard errors of the means for three independent experiments.
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The capacity of Stx1 to activate PKC was directly assessed. Total
cellular PKC activity in lysates prepared from Stx1-treated monocytes
was examined by measuring the transfer of the -phosphate group from
[-32P]ATP to a PKC-specific substrate. Treatment of
THP-1 cells with Stx1 increased total cellular PKC activity to ~150%
above basal levels in untreated cells (Fig.
3). Treatment of cells with H-7 or K252a
prior to Stx1 exposure prevented elevated PKC activity, whereas H-89
treatment did not affect Stx1-mediated PKC activity. Short-term PMA
treatment was used as a positive control and increased THP-1 PKC
activity by ~350%.
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FIG. 3.
Effect of Stx1 on PKC activation in THP-1 cells.
PMA-differentiated THP-1 cells were treated with purified Stx1 (800 ng/ml) for 3 h or PMA for 1 h. Some cells were pretreated
with the PKC inhibitor H-7 (50 mM) or K252a (500 nM) or the PKA
inhibitor H-89 (1000 nM) for 3 h prior to stimulation with 800 ng
of purified Stx1/ml. PKC activation was assessed by measuring the
transfer of 32P to a synthetic PKC substrate. Data shown
are means ± standard errors of the means for three independent
experiments.
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PKC inhibitors block TNF- mRNA synthesis in Stx-treated THP-1
cells.
Northern blot analyses of Stx-treated THP-1 cells
demonstrated that the toxins act, at least in part, at the
transcriptional level to increase quantities of TNF- mRNA
transcripts extracted from the cells (28). We used Northern
blots to examine the role of PKC in Stx-induced TNF- mRNA synthesis.
Pretreatment of cells with the PKC inhibitors H-7 and K252a
significantly blocked TNF- transcript induction following
stimulation with Stx1, while the PKA inhibitor H-89 did not affect
toxin induction of TNF- mRNA (Fig. 4).
These data suggest PKC involvement in signaling events occurring
upstream of TNF- transcriptional activation. The positive control in
these experiments, short-term treatment of THP-1 cells with TPA,
triggered TNF- mRNA synthesis.
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FIG. 4.
Effect of PKC inhibitors on Stx1-mediated TNF- mRNA
synthesis by THP-1 cells. PMA-differentiated THP-1 cells were treated
with purified Stx1 with or without protein kinase inhibitors as
outlined in the legend to Fig. 3. Total RNA was isolated from the
cells, and TNF- mRNA was detected by Northern blot analysis. Ratios
shown are the means ± standard errors of the means for three
separate experiments.
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Stx induction of TNF- requires tyrosine kinase activity.
One of the earliest macrophage responses to LPS binding is the
phosphorylation of multiple proteins at tyrosine residues (reviewed in
reference 3). Treatment of THP-1 cells with purified
Stxs also results in tyrosine phosphorylation (and dephosphorylation) of multiple proteins. Following toxin stimulation, major phosphoprotein bands at approximately 73, 70, 60, and 20 kDa appeared, while a 33-kDa
band appeared dephosphorylated (Fig. 5).
Toxin-mediated changes in phosphorylation appeared to be sensitive to
the general tyrosine kinase inhibitor genistein, which reduced levels
of phosphorylation to levels detected in untreated controls (Fig. 5,
compare lanes 1 and 4). This finding led us to assess the role of
protein tyrosine kinases in Stx-mediated TNF- production. We treated
monocytes with the tyrosine kinase inhibitor genistein prior to Stx1
exposure and monitored TNF- secretion. Pretreatment of THP-1 cells
with genistein for 2 h inhibited Stx1- and LPS-mediated TNF-
production (Fig. 6). Exposure of the
cells to the carrier solvent DMSO or to genistein plus DMSO did not
induce TNF- production. Thus, Stx1 treatment of monocytic cells
induced tyrosine phosphorylation, the inhibition of which was
associated with the loss of cytokine expression.
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FIG. 5.
Stx1-induced phosphorylation of tyrosine residues in
THP-1 cells. Differentiated THP-1 cells were preincubated with 100 µM
genistein or vehicle for 2 h followed by exposure to Stx1 (400 ng/ml) with or without the kinase inhibitor. Cells were also treated
with the inhibitor or DMSO vehicle alone. Cells were lysed, and
extracts were cleared by centrifugation. Equal amounts of protein were
separated by SDS-12% PAGE and analyzed by Western blotting using an
anti-phosphotyrosine monoclonal antibody, 4G10, as described in
Materials and Methods. Closed arrows indicate phosphoproteins induced
by Stx1 treatment that are sensitive to genistein. The open arrow
indicates a phosphoprotein band of decreased intensity following Stx1
treatment that appears restored following inhibitor treatment.
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FIG. 6.
Effect of the tyrosine kinase inhibitor genistein on
Stx1-mediated TNF- production by THP-1 cells. PMA-differentiated
THP-1 cells were treated with purified Stx1 (400 ng/ml) or LPS (200 ng/ml) for 18 h. Some cells were pretreated with genistein (100 µM) for 2 h prior to stimulation with purified Stx1 or LPS.
Culture supernatants were collected, and soluble TNF- levels were
determined by enzyme-linked immunosorbent assay. Data shown are the
means ± standard errors of the means for three separate
experiments.
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DISCUSSION |
Data presented in this study and elsewhere (26, 43)
suggest that sublethal concentrations of Stxs induce TNF- and
IL-1 expression by human monocytes and monocytic cell lines. We
demonstrate that cytokine production in response to Stx treatment
correlates with toxin A subunit enzymatic activity, as mutants with
markedly reduced N-glycosidase activity, but retaining the
ability to form AB5 holotoxins and bind to the cells via
Gb3 or Gb4 receptors, fail to elicit TNF-
production. Furthermore, treatment of monocytes with ricin, a toxin
possessing an identical mechanism of action as Stx A subunits, elicits
TNF- production. Binding of Gb3 by Stx1 B subunits or
antibody against Gb3 was not sufficient to trigger cytokine production.
The precise mechanisms by which Stxs trigger increased cytokine
synthesis and secretion by monocytes is unknown. A number of
well-characterized transmembrane signaling pathways are triggered by
growth factor-growth factor receptor interactions (31). The lipid A component of LPS has been shown to bind to a number of monocyte/macrophage membrane proteins, including CD14,
2 leukocyte integrins (CD11a,b,c/CD18), and the
scavenger receptor (reviewed in reference 7).
Following LPS binding to membrane receptors, transmembrane signaling
may be initiated by toll-like receptors, a series of signal transfer
proteins. In contrast to growth factors or LPS, Stxs and ricin do not
appear to stimulate host cell signaling cascades solely through the
simple interaction of toxins with membrane receptors. Rather, it
appears that wild-type toxins must enter cells, undergo retrograde
intracellular routing, and initiate cell signaling cascades from within
the cell. A likely starting point for cell signal initiation is the
ribosome (15), and studies are under way to link
Stx-mediated ribosome inactivation with cytokine production by
monocytic cells.
Stx-mediated cytokine induction by monocytes was dependent on cell
differentiation and toxin dose. Treatment of toxin-sensitive undifferentiated THP-1 cells with Stxs (400 ng/ml) resulted in cell
death without cytokine release (26). In contrast, cytokine production manifested in differentiated THP-1 cells following treatment
with an identical dose of Stx1 which was sublethal and did not
drastically alter protein synthesis. The cytokine induction ability of
sublethal doses of Stxs may not be limited to proinflammatory cytokine
production by myeloid cells. Recently, it was shown that human
intestinal epithelial cells, although relatively sensitive to Stxs,
secreted the chemokine IL-8 when treated with doses of purified Stxs
that mediated only ~10% of the cell killing (39, 45).
Interestingly, IL-8 production by the human colonic epithelial cell
line Caco2 also required A subunit activity (45). These data
suggest that cytokine and chemokine induction within localized tissues
may occur in the presence of concentrations of Stxs that are sublethal
for cells in vitro.
To determine signaling components involved in Stx-mediated TNF-
production, we examined the role of PKC, PKA, and protein tyrosine
kinases in induction. The PKC family of serine/threonine kinases
contains at least 12 isoforms that are involved in signal transduction,
regulation of gene expression, and myeloid differentiation (21). The PKC family is subdivided into three groups: (i)
the conventional PKC group containing isoforms requiring both
Ca2+ and diacylglycerol (DAG), phosphoserine, or phorbol
esters for activation, (ii) the Ca2+-independent PKC group,
requiring only DAG, phosphoserine, or phorbol esters for activation,
and (iii) the atypical PKC isoforms, which require neither
Ca2+ nor lipids for activation and are insensitive to
phorbol esters. Various PKC isoforms have been implicated in
LPS-mediated signaling, but their role in induction of TNF- remains
controversial (25, 32, 33). Shapira et al. (33)
showed that LPS-stimulated human monocyte production of TNF- and
IL-1 was blocked by both tyrosine kinase and PKC inhibitors. However, a
DAG-dependent kinase inhibitor did not affect LPS-induced TNF-
production, suggesting that atypical PKC isoforms may be involved in
LPS signaling. Herrera-Velit et al. (13) showed that LPS
treatment of human monocytes resulted in the selective activation of
the atypical PKC-
isoform. Atypical PKC isoforms may, in turn, be
linked to activation of downstream kinases, such as the extracellular
signal-regulated kinase cascade, involved in LPS-mediated signaling
(9, 27, 44). The results presented here suggest that PKC
activation in differentiated THP-1 cells is essential in Stx-mediated
signaling for TNF- production. The position of PKC in the signaling
pathway and the identity of the PKC isoform(s) involved in Stx
signaling remain to be determined.
Using the tyrosine kinase inhibitor genistein, TNF- production by
THP-1 cells stimulated by Stx1 was decreased. Thus, protein tyrosine
kinases are also involved in Stx-mediated signaling. Several possible
candidate kinase pathways that contain tyrosine kinase activity have
been characterized in LPS-treated monocytes, including the
extracellular signal-regulated kinase, c-Jun N-terminal kinase, and p38
mitogen-activated protein kinase cascades (5, 12, 35, 44).
It will be necessary to screen specific components of these pathways to
establish their role in Stx signaling since the parallels between LPS-
and Stx-induced signaling are currently unknown.
| |
ACKNOWLEDGMENTS |
We thank Anastasia Green and Belakere Ramegowda for excellent
technical assistance. We thank David Acheson, Jim Samuel, and Yoshifumi
Takeda for kindly sharing reagents essential for the completion of this study.
This work was supported by Public Health Service grant AI-34530 from
the National Institute of Allergy and Infectious Diseases.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Medical Microbiology and Immunology, 407 Reynolds Medical Building,
Texas A&M University Health Science Center, College Station, TX
77843-1114. Phone: (409) 845-1313. Fax: (409) 845-3479. E-mail:
tesh{at}medicine.tamu.edu.
Editor:
R. N. Moore
| |
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Abstract
Introduction
