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Infection and Immunity, March 2000, p. 1207-1214, Vol. 68, No. 3
Department of
Bacteriology1 and Department of Medicine
II,2 Nara Medical University, Kashihara,
Nara 634-8521, Japan
Received 1 October 1999/Returned for modification 29 October
1999/Accepted 12 November 1999
In a previous study, we showed that infection with Shiga toxin
(Stx)-producing Escherichia coli O157:H7 (strain
SmrN-9) caused neurologic symptoms in malnourished mice
with positive immunoreactions of Stx2 in brain tissues. The present
study explores the mechanism of how Stx injures the vascular
endothelium to enter the central nervous system in mice. Oral infection
with strain SmrN-9 elicited a tumor necrosis factor alpha
(TNF- Shiga toxin (Stx)-producing
enterohemorrhagic Escherichia coli strains of serotype
O157:H7 cause hemorrhagic colitis, which is often followed by
hemolytic-uremic syndrome (HUS) and/or acute encephalopathy (8,
12). Stx plays a critical role in the pathogenesis of diarrhea
caused by Stx-producing E. coli O157:H7, which has
been demonstrated by several animal studies (13, 23, 33,
35). However, the pathogenesis of these severe combined diseases is not well understood. Based on several experimental findings
(2, 26), one possible mechanism for the development of such
complications has been proposed: Stx produced by E. coli O157:H7 hematogenously disseminates from the gut to the kidney (36) or the brain (32).
Our previous study (16) showed that when mice with protein
calorie malnutrition (PCM) by feeding on a low-protein diet were infected intragastrically with a clinical isolate of
Stx-producing E. coli O157:H7, they died from brain
damage but not from renal damage. In only mice developing neurologic
symptoms, Stx was detectable in the blood, and immunoreactions of Stx
were demonstrated in the brain tissues by immunocytochemical staining.
Such findings may support the assumption that Stx hematogenously enters
the brain. Since the enhanced susceptibility of mice with PCM to
Stx-producing E. coli O157:H7 is explained by the
nondevelopment of an intestinal physical barrier (16), a
relatively large amount of Stx may be absorbed into the bloodstream in
such animals compared to well-nourished ones. However, the mechanism
whereby Stx enters the central nervous system (CNS) from the
bloodstream is not known.
Stx is known to induce apoptosis in group I Burkitt's lymphoma
(20) and a subset of germinal center B cells (30)
expressing Gb3/CD77 as a functional receptor for Stx. Moreover, Fujii
et al. (2) have reported that Stx exhibits a direct effect
on brain nerve cells and also demonstrated (3, 4) that in
rabbits Stx2 may leak from the bloodstream into the cerebrospinal
fluid, which leads to an increase in the paracellular
permeability through the blood-brain barrier (BBB) around the
third ventricle. If this is the case, Stx must first injure the
vascular endothelium in order to enter the CNS. However, vascular
endothelial cells, unlike Vero cells, are resistant to Stx
cytotoxicity (31). Moreover, it was demonstrated that
tumor necrosis factor alpha (TNF- Thus, the aim of this study was to examine how inflammatory cytokines
and Stx exert the synergistic effect on injury of vascular endothelial
cells and also to determine whether infection with Stx-producing
E. coli O157:H7 causes apoptosis in the mouse brain. In addition, we attempted to demonstrate the presence of Stx
receptors in mouse brain tissues. Results obtained here support
the concept that hematogenously disseminated Stx causes damage to the
vascular endothelium in cooperation with circulating TNF- Microorganisms.
E. coli O157:H7 strain
SmrN-9, which is resistant to streptomycin (100 µg/ml)
and is able to produce Stx1 and -2, was used (16). E. coli NP-4 isolated from the stool of a healthy adult was used as a
control strain (16). Both strains were preserved in
gelatin-charcoal disks at Mouse infection.
Specific-pathogen-free, 3-week-old female
C57BL/6 mice that had been weaned were purchased from Charles River
(Tokyo, Japan). Animals were fed a low-protein diet (5% protein)
(Oriental Bio Service Inc., Kyoto, Japan) for 2 weeks to achieve PCM as
described previously (16).
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Pathogenic Mechanism of Mouse Brain Damage Caused by Oral
Infection with Shiga Toxin-Producing Escherichia coli
O157:H7
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
) response in the blood as early as 2 days after infection,
while Stx was first detected at 3 days postinfection. In the
brain, TNF- was detected at day 3, and its quantity was increased
over the next 3 days. Frozen sections of the brains from moribound mice
contained high numbers of apoptotic cells. Glycolipids recognized by an
anti-Gb3 monoclonal antibody were extracted from the brain, and
purified Stx2 was able to bind to the glycolipids. In human umbilical
vascular endothelial cells (HUVEC) cultured with fluorescein-labeled
Stx2 (100 ng/ml), TNF- (20 U/ml) significantly facilitated the
intracellular compartmentalization of fluorescence during 24 h of
incubation, suggesting the enhanced intracellular processing of Stx2.
Consequently, higher levels of apoptosis in HUVEC were found at
48 h. Short-term exposure of HUVEC to Stx2 abrogated their
apoptotic response to subsequent incubation with TNF- alone
or TNF- and Stx2. In contrast, primary exposure of HUVEC to TNF-
followed by exposure to Stx2 alone or TNF- and Stx2 induced
apoptosis at the same level as obtained after 48-h incubation
with these two agents. These results suggest that the rapid production
of circulating TNF- after infection induces a state of competence in
vascular endothelial cells to undergo apoptosis, which
would be finally achieved by subsequent elevation of Stx in the blood.
In this synergistic action, target cells must be first exposed to
TNF-. Such cell injury may be a prerequisite to brain damage
after infection with Stx-producing E. coli
O157:H7.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
) could induce apoptosis in
endothelial cells in the presence of inhibitors of protein synthesis
(25, 39), although normally this cytokine does not injure
endothelial cells (24). In addition, many investigators have
shown that cooperation between Stx and inflammatory cytokines including
interleukin (IL)-1
(14, 18) and TNF- (9, 11, 18) are involved in injury of vascular endothelial cells and in
eliciting the pathologic changes in HUS. Since Stx is a strong protein
synthesis inhibitor for cells expressing Gb3/CD77, we speculated that
Stx may potentiate TNF--induced apoptosis in vascular
endothelial cells.
and
leaks into the cerebrospinal fluid. In this pathogenic process, TNF-
accelerates the intracellular processing of Stx, which in turn, may
potentiate TNF--induced apoptosis in vascular endothelial
cells. Furthermore, such a synergistic effect may occur in the brain,
since TNF- production and functional receptors for Stx were found in
brain extracts.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
20°C. Before use, one of the preserved disks was dissolved in 1 ml of tryptic soy broth (Difco Laboratories, Detroit, Mich.), and 100 µl of this bacterial suspension was
inoculated into 10 ml of fresh tryptic soy broth. For infection study,
bacteria were harvested by centrifugation from broth culture after
growth overnight at 37°C, washed, and resuspended in sterile
phosphate-buffered saline (PBS; 10 mM, pH 7.2) at a concentration of
2 × 107 CFU/ml.
Extraction of neutral glycolipids from mouse brains. The brain was removed from the bony skeleton after mice were sacrificed by intravenous injection of pentobarbital at 0.5 ml/kg of body weight. Brains obtained from three mice were washed in saline and homogenized in 5 ml of chloroform-methanol (2:1, vol/vol) by vigorous vortexing and sonication. The homogenate was heated at 60°C for 1 h and centrifuged at 2,000 × g for 20 min. The supernatant of chloroform-methanol was collected, and cell residue was reextracted with chloroform-methanol and centrifuged. These two extracts were combined and evaporated to dryness under a stream of nitrogen. The residue was heated at 60°C for 1 h in chloroform-methanol (2:1, 1:1, and then 1:2) and centrifuged. The supernatant of chloroform-methanol (total lipid extract) was collected and dried under a stream of nitrogen. This extract was then partitioned into aqueous and organic fractions with diisopropyl ether-1-butanol-100 mM NaCl (6:5:4, vol/vol/vol) by a modification of the technique of Ladisch and Gillard (17). The fractions were dried, and the aqueous fraction was resuspended in chloroform-methanol-water (1:10:10, vol/vol/vol). To remove salts and water-soluble contaminants, reversed-phase chromatography was performed on RP18 cartridges (Waters Associates, Milford, Mass.) (15). The desalted extract was separated into acidic and neutral fractions by chromatography on a column of DEAE-Sephadex A-25 (Pharmacia Biotechnology, Tokyo, Japan) (15, 27). Neutral fractions eluted with chloroform-methanol-water (30:60:8, vol/vol/vol) from the DEAE column were evaporated to dryness. Then dried materials were dissolved in a minimum amount of chloroform and incubated at 40°C for 30 min after addition of 6 N NH4OH in methanol. After incubation, treated samples were dried, dissolved in chloroform-methanol (2:1, vol/vol), and used as the brain neutral glycolipid extract.
In situ DNA fragmentation analysis. DNA fragmentation was determined by the in situ TUNEL (terminal deoxynucleotidyltransferase (TdT)-mediated dUTP-biotin nick end labeling) technique (6), which is based on the specific binding of TdT to 3'-OH ends of DNA. For this assay, frozen sections of mouse brains obtained at 10 days postinfection and formalin-fixed monolayers of cultured human umbilical venous endothelial cells (HUVEC) were used. Frozen sections (3 µm thick) of brains or formalin-fixed HUVEC monolayers were treated with proteinase K (Boehringer Mannheim, Indianapolis, Ind.) at a concentration of 20 µg/ml for 20 min, rinsed, blocked with 1% bovine serum albumin and 0.003% Triton X-100 in 10 mM PBS for 30 min at room temperature, and then rinsed again. These treated preparations were immersed in TdT (0.5 U/µl) and 1 mM biotin-16-dUTP in reaction buffer (Boehringer Mannheim) and incubated in a humid atmosphere at 37°C for 1 h. The reaction was stopped with termination buffer (300 mM NaCl, 30 mM sodium citrate [pH 7.2]). These sections were washed with distilled water, blocked with 2% bovine serum albumin in PBS for 10 min, rinsed again with distilled water, immersed in PBS for 5 min at room temperature, and then incubated with an avidin-peroxidase complex (Boehringer Mannheim) diluted 1:600 in PBS for 30 min at 37°C. Color development was done with diaminobenzidine (DAB)-H2O2. The number of TUNEL-positive cells in experimental and control materials was counted under a light microscopy in a blinded fashion by three different investigators. Apoptotic cells were identified by dark-brown staining in the nucleus. On each slide, approximately 200 cells were evaluated for the presence of apoptotic cells. The background number of TdT-positive cells in controls was subtracted from the number of TUNEL-positive cells in experimental material.
TLC-blot analysis. Brain neutral glycolipids were spotted onto two Silica Gel 60 high-performance thin-layer chromatography (TLC) plates (0.2 mm thick; Merck AG, Darmstadt, Germany) and were developed in chloroform-methanol-water (65:25:4, vol/vol/vol) to 7 cm from the origin. TLC standards of neutral glycolipids (Accurate Chemical & Scientific Corporation, Westbury, Conn.) were used as reference. After chromatographic separation, the plates were dried, and one of them was sprayed with orcinol reagent (Sigma) to identify each glycolipid in brain samples and standard preparations. For immunoblotting, the other plate was coated with 0.1% polyisobutyl-methacrylate (Polyscience, Warrington, Pa.), air dried, and sprayed with 20 mM Tris-HCl-150 mM NaCl-5 mM MgCl2-0.15 mM CaCl2 (pH 7.4) (TNMC). The plate was covered with a polyvinylidene difluoride (PVDF) membrane (Atto Co. Ltd., Tokyo, Japan) and then glass membrane filters (GF/A, Whatman Paper Ltd., Maidstone, United Kingdom). This assembly was pressed with an electric iron at 180°C for 30 s. The blot membrane was dried, rehydrated by being placed on the surface of TNMC, and then incubated with 10% horse serum in TNMC for 1 h at 37°C to block excess binding capacity.
Immunodetection.
To examine Gb3, the blot membrane was
washed with TNMC after blocking and overlaid with an
anti-Pk monoclonal antibody (MAb) (specificity, Gal
1-4Gal 1-4 Glc1-1Cer moiety of Gb3; isotype, murine
immunoglobulin M [IgM]) (Accurate Chemical & Scientific Corporation)
(1) diluted 1:8 in 10% horse serum in TNMC. After overnight
incubation at 4°C, the membrane was washed five times with TNMC and
then incubated for 1 h with a 1:100 dilution of
peroxidase-conjugated goat anti-mouse IgM F(ab')2 (Organon
Teknika, Durham, N.C.). The membrane was washed five times with TNMC,
and the color reaction was performed with DAB-H2O2.
Cytokine assay.
IL-1, IL-6, IL-10, and TNF- in brain
homogenates and serum were quantified by enzyme-linked immunoassay
(EIA) using commercially available kits (Genzyme, Cambridge, Mass.).
Whole brains were removed from mice killed by exsanguination and were
minced in 10 mM phosphate buffer (pH 7.2) containing 0.5 mM
phenylmethylsulfonyl fluoride (Sigma) and 0.05% Triton X-100. Then
they were homogenized with a sonicator (Tomy Handy Sonicator; Tomy
Seiko Co. Ltd., Tokyo, Japan) at 4°C. These homogenates were
centrifuged at 30,000 × g for 20 min, and supernatants
were collected for cytokine assay. A standard curve for each cytokine
was constructed with the appropriate recombinant murine cytokine
(Genzyme) incorporated into normal mouse serum or brain extract. For
measurement of serum cytokines at each time point, serum was collected
from three mice, and individual samples were divided into three
100-µl aliquots. Data were obtained from three different experiments.
With these EIA kits, the limits of detection for IL-1, IL-6, IL-10,
and TNF- in serum were 15, 18, 13, and 14 pg/ml, respectively. The
limit of detection for cytokines in brain extracts was 30 pg/100 mg of
protein, irrespective of the cytokine used for measurement. The protein
content of each homogenate was determined by the dye-binding assay
using a DC protein assay kit (Bio-Rad Laboratories, Hercules, Calif.).
Measurement of Stx antigen. Stx levels in the blood were determined with an EIA kit (Premier EHEC; Meridian Diagnostic, Inc., Cincinnati, Ohio) as described previously (16). Blood was obtained from the ophthalmic arteries of infected mice. Serum was separated from clotted blood by centrifugation and then concentrated 20-fold by ultrafiltration before assay. Twenty microliters of each concentrated serum sample was mixed with 4 volumes of the sample dilution buffer, and then 100 µl of each mixture was assayed with the EIA kit reagents. A standard curve was constructed with the purified Stx1 incorporated into normal mouse serum, and results were expressed as Stx1 amounts (picograms) per milliliter of neat serum (16). With this EIA kit, the limit of detection for Stx1 was 20 pg/ml of neat serum.
Labeling of Stx2 with fluorescent dye. Lyophilized Stx2 was dissolved at a concentration of 1.2 mg/ml in 200 µl of PBS and labeled with Oregon Green 488 (37), using a FluoReporter protein labeling kit (F-6153; Molecular Probes, Inc., Eugene, Oreg.). Labeling was done exactly as instructed by the manufacturer. The molar ratio of Oregon Green 488 to Stx2 was 20, and the fluorescent dye-Stx2 conjugate was recovered using a spin column provided by the manufacturer. The labeled Stx2 was dialyzed against PBS, and the final labeled preparation was confirmed to retain the same degree of verocytotoxicity as the unlabeled material.
Determination of uptake of Stx2 by HUVEC. HUVEC were purchased from Dainipon Pharmaceutical Co. (Tokyo, Japan). Basal culture medium was alpha minimal essential medium (GIBCO, Grand Island, N.Y.) with 20% heat-inactivated fetal bovine serum (HyClone Laboratories, Logan, Utah), 100 µg of heparin (Sigma) per ml, 50 U of penicillin per ml, and 50 µg of streptomycin per ml (defined as complete medium [CM]). HUVEC were suspended at a concentration of 103/ml in CM supplemented with 10 µl of bovine retinal extract per ml (CM-BRE) prepared as described previously (7, 29). HUVEC were seeded in culture dishes (6-cm diameter; Falcon; Becton Dickinson Labware, Oxnard, Calif.) coated with human fibronectin (1 µg/cm2) and incubated at 37°C in humidified 5% CO2.
The cells were fed every other day with fresh CM-BRE and were detached with a mixture of 0.5% collagenase S-1 (Nitta Gelatin, Osaka, Japan) and 0.02% EDTA in Ca2+- and Mg2+-free balanced salt solution when the culture became subconfluent. Washed detached cells were distributed into fibronectin-coated chambers of Lab-Tek chamber slides (eight-chamber type; Nunc Inc., Naperville, Ill.) at a concentration of 5 × 104 per chamber in a volume of 400 µl of CM-BRE. After 12 h of incubation, fluorescent dye-labeled Stx2 was added to each chamber at a concentration of 100 ng/ml. This dose of the labeled toxin was equivalent to about 105 CD50, where CD50 is defined as the dose required for 50% death of Vero cells. After 12 and 24 h, cell monolayers were washed three times with PBS before microscopic observation. Fifty randomly selected HUVEC were observed under an Olympus (Tokyo, Japan) BX50 fluorescence microscope. The intensity of fluorescence per cell was quantified with a computer-assisted confocal laser microscope (InSIGHT plus-IQ; Meridian Instruments Inc., Okemos, Mich.) as described elsewhere (10, 31), and the mean intensity per cell was determined by measuring the fluorescence intensity of 50 individual cells in three different fields on a slide.Synergistic effect of cytokines and Stx2 on cell damage to
HUVEC.
Purified Stx2 was added at a final concentration of 100 ng/ml to HUVEC monolayers in the presence or absence of human
recombinant TNF-, IL-1, or IL-6 (Genzyme). Incubation was carried
out at 37°C for 72 in 5% CO2, and the number of
apoptotic cells was determined by the TUNEL method. The optimal
doses of these three cytokines were initially determined by their
ability to stimulate HUVEC to release soluble intercellular adhesion
molecule I (sICAM-1) without cell damage twice as much as unstimulated
cells produce in culture supernatants: 20 U of TNF- per ml, 15 U of
IL-1 per ml, and 35 U of IL-6 per ml, respectively. A human sICAM-1
EIA kit (Endogen, Woburn, Mass.) was used to measure sICAM-1 in culture supernatants. Anti-Stx2 MAb (Toxin Technology) and anti-human TNF-
MAb (Genzyme) were used to neutralize the activity of Stx2 and TNF-, respectively.
target spontaneous-background)/(target
maximum target spontaneous-background)} × 100. Maximum
LDH release from target HUVEC was determined after complete lysis of
the cells with 0.8% Triton X-100.
To confirm the nucleosomal ladder pattern of DNA degradation in HUVEC,
DNA was extracted from the cells cultured in 24-well culture plates at
48 h of incubation using a DNA extraction kit (Stratagene, La
Jolla, Calif.). Precipitated DNA was air dried and suspended in 10 mM
Tris-1 mM EDTA, pH 7.4. The DNA solution was subjected to conventional
electrophoresis (2% agarose for 1.5 h at 10 V/cm). DNA was
visualized with ethidium bromide.
Sequential treatment of HUVEC with Stx2 and TNF-.
HUVEC
monolayers were pulsed with either Stx2 (100 ng/ml) or TNF- (20 U/ml) and incubated at 37°C for 6 h in 5% CO2. At
the end of pulsing, monolayers were washed four times with CM-BRE. Thereafter, TNF- (20 U/ml) was added to the monolayers pulsed with
Stx2, and Stx2 (100 ng/ml) was added to those pulsed with TNF-.
After 42 h of incubation, TUNEL assay was performed. Monolayers of
HUVEC incubated with Stx2 (100 ng/ml) and TNF- (20 U/ml) for 48 h were used as a positive control, and 44.9% ± 6.4% (mean ± standard deviation [SD]) of cultured cells became TUNEL positive.
Statistics. The significance of differences observed was assessed by the Kruskal-Wallis one-way analysis of variance in comparison of percentage of TUNEL-positive cells, cytotoxicity, and fluorescence intensity. P < 0.05 was considered significant.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Measurement of Stx and cytokines in mouse serum.
Stx was
elevated to detectable levels in the serum from days 3 through 5 when
PCM mice were infected intragastrically with 2 × 106
CFU of strain SmrN-9 (Fig.
1); serum levels peaked at day 4 (mean,
34.8 ± 4.6 pg/ml). In contrast, Stx was not detected from days 1 through 8 in well-nourished mice inoculated with the same dose of
SmrN-9.
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, P < 0.05 compared to days 2 and 3; was first elevated to detectable levels in the
sera of PCM mice at day 2 (mean, 135.2 ± 40.2 pg/ml); the peak
serum level was as much as 300 pg/ml. Thereafter, serum levels of
TNF- decreased gradually over 4 days. On the other hand, the IL-10
level slowly increased in the sera of infected PCM mice. In contrast,
serum IL-1 levels remained lower than the limit of detection from
days 1 through 8. None of these cytokines was detected in the sera of
PCM mice after infection with 2 × 106 CFU of E. coli NP-4. In addition, neither Stx, TNF-, IL-1, nor IL-10
was detected in the sera of well-nourished mice inoculated with 2 × 106 CFU of SmrN-9 from days 1 through 8.
Determination of cytokine levels in the brain.
Cytokine levels
in the brain tissues of infected PCM mice were measured at 3 and 6 days
after infection. Only TNF- was detected (54 ± 25 pg per 100 mg
of tissue protein) in the brain tissues of PCM mice at 3 days
postinfection: there was no TNF- response in the brain during the
first 2 days of infection. Levels of TNF- in the brain were
increased approximately by twofold (98 ± 34 pg per 100 mg of
tissue protein) at 6 days after infection. Among other cytokines, only
IL-10 was measurable in the brain tissues of infected PCM mice at 6 days postinfection (45 ± 9 pg per 100 mg of tissue protein), but
neither IL-1 nor IL-6 was detected on days 3 and 6 of infection.
Neither PCM mice given 2 × 106 CFU of E. coli NP-4 nor well-nourished mice infected with the same dose of
SmrN-9 showed cytokine responses in the brain.
Detection of Stx receptors in the brain.
To test for the
presence of Stx-binding glycolipids (Gb3) in the mouse brain, neutral
glycolipid extracts of brain tissues were prepared, separated by
TLC (Fig. 2, lane B), and compared to TLC
of standard neutral glycolipids (lane A). Gb3 was identified by
TLC-blot assay using an anti-Pk MAb recognizing the
specific epitope of Gb3. Immunostaining demonstrated the presence of
glycolipids recognized by an anti-Pk MAb in the brain
neutral glycolipid fraction (lane D) and the standard neutral
glycolipids (lane C). In addition, a TLC-blotted PVDF membrane (the
same as used for lane D) was incubated with the purified Stx2, and the
glycolipid-Stx complexes were identified by immunostaining with an
anti-Stx2 MAb (lane E) at the position corresponding to Gb3 on the
TLC-blotted membrane as seen in lanes C and D.
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Apoptosis in the brain after infection.
Frozen sections of
brain tissues from six PCM mice infected with SmrN-9 were
prepared for in situ TUNEL experiments at 10 days postinfection. Widespread apoptosis was observed in brain tissues in five out of six infected PCM mice, one of which is presented in Fig.
3. The mice whose brain tissues had many
TUNEL-positive cells exhibited neurologic symptoms after day 5 of
infection, and all were in a moribound state on day 10 postinfection.
Approximately 28% of brain cells (56 ± 12/200 cells) in the
sections from individual mice were TUNEL positive; such
apoptotic cells were detected in the cerebellum, hippocampus,
and brain stem samples from mice infected with
SmrN-9. In contrast, only a background level of
apoptosis (4 ± 2/200 cells; about 2%) was found in these
areas of PCM mice inoculated with 2 × 106 CFU of
E. coli NP-4 and in those of well-nourished mice infected with the same dose of SmrN-9.
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Cytotoxicity to HUVEC of Stx and cytokines.
To explore the
cooperation between Stx and inflammatory cytokines in causing cell
damage to HUVEC, the effect of cytokines on the intracellular
processing of fluorescein-labeled Stx2 was examined. HUVEC were
incubated with the fluorescein-labeled toxin (100 ng/ml) in the
presence or absence of TNF- (20 U/ml), IL-1 (15 U/ml), or IL-6
(35 U/ml). As shown in Fig. 4, only
TNF- at 20 U/ml decreased the intensity of fluorescence per cell
during 24 h of incubation. But none of these cytokines altered the
binding of Stx2 to the surface of HUVEC during the first 12 h of
incubation, since the mean fluorescence intensity per cell at 12 h
of incubation remained at the same level, irrespective of the
cytokines used. Microscopic observation, however, showed that the
fluorescence intensity varied with individual cells in each culture
group during the first 12 h of incubation, suggesting
heterogeneity of cultured HUVEC with respect to Stx binding (Fig.
5A). Interestingly, the decrease in the
fluorescence intensity of HUVEC cultured with Stx2 and TNF- was
associated with intracellular compartmentalization of the labeled
toxin during the next 12 h of incubation (Fig. 5B). In contrast,
neither IL-1 nor IL-6 microscopically enhanced the intracellular
compartmentalization of Stx2 in HUVEC (data not shown).
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) or in the presence of TNF-
), IL-1
), or IL-6 (35 U/ml) (
). At
12 and 24 h of incubation, the cells were washed three times with
PBS, 50 cells were randomly selected, and the fluorescence intensity of
each cell was quantified with a computer-assisted fluorescence scanning
confocal microscope. Data were obtained from three independent
experiments, each performed in triplicate. Results are expressed as the
mean ± SD for nine determinants. Each bar represents SD.
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(20 U/ml) induced only 7% ± 3% positive cells (Fig. 6). However, simultaneous
addition of Stx2 (100 ng/ml) and TNF- (20 U/ml) to cultures of HUVEC
resulted in about 47% ± 6% of the cells becoming TUNEL positive.
Agarose gel electrophoresis demonstrated the nucleosomal ladder pattern
of DNA extracted from HUVEC incubated with Stx2 and TNF- for 48 h (Fig. 7), indicating that these
TUNEL-positive cells underwent apoptosis. DNA preparations extracted from HUVEC treated with Stx2 alone or TNF- alone presented less or no DNA fragmentation. Cytotoxicity as determined by the LDH
release assay at 72 h of incubation was significantly increased (P < 0.01) in the presence of Stx2 and TNF-: from
14.3% (Stx2 alone) or <5.0% (TNF- alone) to 63.5% (Stx2 plus
TNF-) (Table 1). In contrast, neither
IL-1 (15 U/ml) nor IL-6 (35 U/ml) displayed the synergistic effect
when added to HUVEC monolayers at the initiation of incubation with
Stx2 (data not shown). An anti-TNF- MAb (50 ng/ml) significantly
reduced both apoptosis (P < 0.05) (Fig. 6) and
cytotoxicity (P < 0.01) (Table 1) caused by the
synergistic effect of Stx2 and TNF-. Twenty units of IL-10 also
reduced both apoptosis (P < 0.05) (Fig. 6) and
cytotoxicity (P < 0.01) (Table 1) induced by Stx2 and
TNF-, and its antiapoptotic activity was nearly comparable
to that of anti-TNF- MAb (50 ng/ml).
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Relationship between Stx2 and TNF- in induction of
apoptosis in HUVEC.
The relationship between Stx2 and
TNF- in induction of apoptosis in HUVEC was examined by
systematically varying the order in which cells were exposed to each
agent. HUVEC first exposed to Stx2, TNF-, or medium (for 6 h)
and subsequently cultured with medium (for 42 h) manifested
baseline levels of apoptosis only after 48 h of incubation
(3.0 to 3.5%) (Table 2). Cultures first
exposed to TNF- and then to Stx2 demonstrated apoptosis in
about 43.8% of HUVEC, the level of which was nearly comparable to the
magnitude of apoptosis in response to 48-h incubation after simultaneous addition of Stx2 and TNF- (44.9% ± 6.5%). In
contrast, HUVEC first exposed to Stx2 manifested a significantly
reduced apoptotic response to subsequent exposure to TNF-
(9.8% ± 3.3%) (P < 0.01 compared to positive
controls), the level of which was similar to that obtained with
subsequent exposure to Stx2 (11.4% ± 3.9%). In addition, initial
exposure to Stx2 significantly (P < 0.01) suppressed
the apoptotic response to subsequent exposure to Stx2 and
TNF- (14.9% ± 4.8%) compared to cultures exposed first to medium
and then to Stx2 and TNF- (42.8% ± 6.7%, positive controls). In
contrast, initial exposure to TNF- did not affect the
apoptotic response of HUVEC subsequently incubated with Stx2 and TNF- (46.7% ± 5.9%).
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Several investigators have shown that inflammatory cytokines,
particularly TNF- and IL-1, are capable of enhancing Stx toxicity to vascular endothelial cells expressing Gb3 (14, 18, 31, 34). Isogai et al. (11) have reported that TNF- in
the tissue but not in the serum may contribute to the pathogenesis of
brain damage caused by Stx. We attempted to identify Stx receptors
in the mouse brain and also to examine how HUVEC are injured by the synergistic effect of inflammatory cytokines and Stx.
Although Stx has not been detected in sera of HUS patients, the toxin
was measurable by EIA in the sera of PCM mice from days 3 through 5 after infection. Because of its molecular size, Stx must first damage
the BBB in order to reach the CNS. This would possibly occur in the
presence of TNF- and/or IL-1 (18). In this study,
serum levels of TNF- were increased in infected PCM mice before Stx
was detected in the serum. Our preliminary study has shown that PCM
mice manifest higher levels of TNF- response after an injection of
bacterial endotoxin than do well-nourished animals. Such an
immunological disposition in PCM mice seems to account for the early
production of TNF- in the blood after infection.
Stx2 did not equally bind to cultured HUVEC in this study; the
intensity of fluorescence microscopically varied with individual cells
during 12 h of incubation. Obrig et al. (22) have
reported that basal levels of Gb3 are approximately 50 times higher in human renal endothelial cells than in HUVEC. Moreover, HUVEC obtained from individual umbilical cords differ in their sensitivities to
Shiga toxin (22). Thus, the expression levels of
Gb3 may differ among individual cultured HUVEC. Nevertheless,
TNF- rapidly decreased the fluorescence intensity of the cells. Stx
bound to Gb3 has been shown to be taken up intracellularly through
coated vesicles and transported in a retrograde manner to the
endoplasmic reticulum via the trans-Golgi network
(28), and Stx is processed by a trypsin-like cleavage to
generate A1 and A2 subunits for full expression of its cytotoxicity
(5). Thus, both the decrease in fluorescence intensity and
the increased intracellular compartmentalization of labeled Stx2 may
result from the acceleration of intracellular processing of Stx2 by
TNF-. Since the degree of cytotoxicity at 72 h almost
paralleled that of apoptosis as determined by TUNEL assay at
48 h, death of HUVEC caused by Stx2 and TNF- is likely to
result mainly from apoptosis. This assumption is supported by
the nucleosomal ladder pattern of DNA extracted from HUVEC stimulated
with Stx2 and TNF- for 48 h. IL-1 is also a potent stimulant
for HUVEC to induce Gb3 expression (14, 18), but such an
effect is not apparent unless the cells are preincubated with IL-1
at least for 24 h before exposure to the toxin (14).
In contrast, IL-10 reduced apoptosis in HUVEC cultured with
Stx2 and TNF-. The reason why the present study dealt with IL-10 is
that serum levels of IL-10 were elevated to a significant extent in HUS
patients (21). In fact, IL-10 levels were elevated in sera
of infected PCM mice. However, IL-10 has a variety of biological activities, and its role in infection with E. coli O157:H7
remains to be determined.
Recently, endothelial cell apoptosis by TNF- was shown to be
enhanced by inhibitors of protein synthesis (25, 38).
Normally, TNF- does not injure human endothelial cells, but it can
cause apoptosis of the cells cocultured with either the protein
synthesis inhibitor cycloheximide or the lipid mediator ceramide
(24). Moreover, TNF receptors are required for
TNF-induced apoptosis in microvascular endothelial cells
(19). Taking these findings together, we hypothesized that
Stx can potentiate TNF--induced apoptosis in HUVEC, rather
than TNF- enhancing Stx cytotoxicity, since HUVEC are at least
106-fold less susceptible to Stx than Vero cells
(31). In this study, short-term exposure of HUVEC to Stx
significantly suppressed the apoptotic response to subsequent
culture with TNF-. In contrast, initial exposure to TNF- induced
apoptosis in HUVEC during subsequent incubation with Stx, the
level of which was comparable to that induced by 48-h continuous
culture with these two agents. These results were consistent with the
report by Polunovsky et al. (25) showing the synergistic
effect of TNF- and cycloheximide on endothelial cells. Commitment to
apoptosis in HUVEC by TNF- therefore may be manifest only
after subsequent inhibition of protein synthesis by Stx2. In addition,
the present study has proved the hypothesis (18) that TNF
treatment of HUVEC influences the uptake or activation of Stx. In fact,
injury of HUVEC was completely blocked by an anti-TNF- MAb.
Moreover, the present findings are in agreement with the report
(11) showing that a TNF- inhibitor (protease inhibitor)
reduced the pathological symptoms in mice after infection with
Stx-producing E. coli O157:H7.
Neutral glycolipid fraction of mouse brains contained Gb3 which was
functionally active. Moreover, frozen sections of the brain from
infected PCM mice contained higher numbers of TUNEL-positive cells
compared to those from control PCM mice infected with a nonpathogenic
E. coli strain. Although a TNF- response in the blood was
detected on day 2 of infection, circulating TNF- normally does not
enter the CNS unless the BBB is injured. Nevertheless, this cytokine
was detected in brain tissues of infected PCM mice as early as 3 days
after infection. At present, it is most probable that TNF- enters
the CNS through the BBB damaged by circulating TNF- and Stx.
In conclusion, the rapid production of TNF- after infection is
crucial to the injury of vascular endothelial cells; TNF- promotes
the rapid intracellular activation of Stx, and in turn, activated Stx
potentiates TNF--induced apoptosis in the cells. In this
synergistic action, the cells should be first exposed to TNF-.
Such cell damage must be a prerequisite to the initiation of brain
damage after infection with Stx-producing E. coli.
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ACKNOWLEDGMENTS |
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This work was supported in part by a Research Grant for International Medical Cooperation and also by Grant-in-Aid for Scientific Research 10670359 from the Ministry of Education, Science, Sports and Culture, Japan.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Bacteriology, Nara Medical University, 840, Shijyocho, Kashihara, Nara 634-8521, Japan. Phone: 81-744-29-8839. Fax: 81-744-29-7375. E-mail: eijikita{at}nmu-gw.cc.naramed-u.ac.jp.
Editor: J. T. Barbieri
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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