p38 Mitogen-Activated Protein Kinase Mediates Lipopolysaccharide and Tumor Necrosis Factor Alpha Induction of Shiga Toxin 2 Sensitivity in Human Umbilical Vein Endothelial Cells

Escherichia coli O157:H7 Shiga toxin 2 (Stx2), one of the causativeagents of hemolytic-uremic syndrome, is toxic to endothelialcells, including primary cultured human umbilical vein endothelialcells (HUVEC). This sensitivity of cells to Stx2 can be increasedwith either lipopolysaccharide (LPS) or tumor necrosis factoralpha (TNF- ${alpha}$ ). The goal of the present study was to identifythe intracellular signaling pathway(s) by which LPS and TNF- ${alpha}$ sensitize HUVEC to the cytotoxic effects of Stx2. To identifythese pathways, specific pharmacological inhibitors and smallinterfering RNAs were tested with cell viability endpoints.A time course and dose response experiment for HUVEC exposureto LPS and TNF- ${alpha}$ showed that a relatively short exposure to eitheragonist was sufficient to sensitize the cells to Stx2 and thatboth agonists stimulated intracellular signaling pathways withina short time. Cell viability assays indicated that the p38 mitogen-activatedprotein kinase (MAPK) inhibitors SB202190 and SB203580 and thegeneral protein synthesis inhibitor cycloheximide inhibitedboth the LPS and TNF- ${alpha}$ sensitization of HUVEC to Stx2, whileall other inhibitors tested did not inhibit this sensitization.Additionally, SB202190 reduced the cellular globotriaosylceramidecontent under LPS- and TNF- ${alpha}$ -induced conditions. In conclusion,our results show that LPS and TNF- ${alpha}$ induction of Stx2 sensitivityin HUVEC is mediated through a pathway that includes p38 MAPK.These results indicate that inhibition of p38 MAPK in endothelialcells may protect a host from the deleterious effects of Stx2.

INTRODUCTION

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INTRODUCTION

Escherichia coli O157:H7 is a food-borne pathogen mainly associatedwith undercooked contaminated beef products (1). Most casesof E. coli O157:H7 infection are sporadic; however, numerousoutbreaks have been reported in temperate areas of the world(5, 6, 67). Once ingested, the bacteria form attaching and effacinglesions on colonic intestinal epithelial cells (46). It is herethat the bacteria release many different agents, including Shigatoxin 1 (Stx1) and Stx2 (3). Stx1 and Stx2 are the causativeagents of hemolytic-uremic syndrome (HUS) (70), which is themost frequent cause of acute renal failure in young children.HUS involves a combination of symptoms, including hemolyticanemia, thrombocytopenia, and acute renal failure, appearingmost frequently in children less than 4 years of age (9).

The Stxs consist of an enzymatically active A subunit proteinbound noncovalently to a pentamer of B-subunit proteins thatare responsible for binding to cells (13). Stx1 and Stx2 bindto the glycolipid receptor Gal ${alpha}$ 1-4Galβ1-4GlcCeramide, alsoknown as globotriaosylceramide (Gb₃), CD77, P^k antigen, or GL-3(50), and enter the target cell via receptor-mediated endocytosis.Once the toxin is within the endosomes, various mechanisms havebeen proposed for retrograde transport through the Golgi networkand endoplasmic reticulum and into the cytosol (49). Once thetoxin is in the cytosol, the Stx A subunit removes a specificadenine from rRNA and inhibits protein synthesis (16).

Gb₃ is a neutral glycosphingolipid that is either expressedconstitutively or induced under inflammatory conditions by typesof cells within the kidney. These cells include human glomerularendothelial cells, glomerular visceral epithelial cells (podocytes),proximal tubule cells, and mesangial cells (22, 65). Gb₃ levelsare increased on brain microvascular endothelial cells (15)after treatment with tumor necrosis factor alpha (TNF- ${alpha}$ ), providinga rationale for Stx-induced brain injury (51). Finally, Gb₃can be induced on human umbilical vein endothelial cells (HUVEC)with lipopolysaccharide (LPS), TNF- ${alpha}$ , or interleukin-1β(IL-1β) and has been widely used as an in vitro model forendothelial damage by Stx (27, 29, 37-39, 60, 68).

These in vitro agonists have a potential role in HUS. Increasedconcentrations of TNF- ${alpha}$ in serum have been associated with HUSpatients (36) along with increased concentrations of the solubleTNF receptors p55 and p75 (61). In addition, the urinary TNF- ${alpha}$ level was elevated in patients in the acute phase of HUS comparedto controls (26), suggesting a renal origin for this cytokine.Finally, when Stx was presented systematically to a transgenicmouse, TNF- ${alpha}$ promoter activity was observed exclusively withinthe kidney (21). LPS has also been implicated in the pathogenesisof HUS. Anti-LPS antibodies belonging to the O157:H7 serotypehave been found in the serum of HUS patients (2) along withclinical evidence of endotoxemia (31). It has also been shownthat in a primate model LPS is required in combination withStx1 to induce the clinical hallmarks of HUS (52). Finally,a complete murine model of HUS requires LPS in addition to Stx2(28).

The goal of the present study was to determine the intracellularpathways that LPS and TNF- ${alpha}$ utilize in HUVEC to induce Gb₃ andsubsequent Stx2 sensitivity. Different pharmacological inhibitors,along with RNA interference, were employed to test known pathwaysused by these two agents in HUVEC to determine which of thesepathways are involved in induction of Stx2 sensitivity. Theresults indicate that both stimuli use a p38 mitogen-activatedprotein kinase (MAPK)-dependent pathway to stimulate Stx2 sensitivity.

MATERIALS AND METHODS

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MATERIALS AND METHODS

Materials. Recombinant human TNF- ${alpha}$ ( $~$ 600 pg/U) was a gift from DainipponPharmaceutical Co., Ltd. (Osaka, Japan). Stx2 was immunoaffinitypurified from E. coli DH5 ${alpha}$ (pJES120) lysates obtained from A.D. O'Brien as described previously (41). Neutral red dye, cycloheximide,and E. coli O55:B5 LPS which was purified by gel filtrationchromatography and gamma irradiated were purchased from SigmaAldrich (St. Louis, MO). Wortmannin, Bay11-7082, SN50, SN50M,SB202190, SB203580, 2-phenyl-1,2-benzisoselenazol-3(2H)-one(Ebselen), SP600125, Jak inhibitor 1, U0126, and myristoylatedprotein kinase C ${zeta}$ (PKC ${zeta}$ ) pseudosubstrate were purchased from EMDBiosciences (San Diego, CA). A CCK-8 cell viability kit waspurchased from Dojindo Molecular Technologies (Gaithersburg,MD). The RNAiFect transfection reagent was purchased from Qiagen(Valencia, CA). SMARTpool small interfering RNA (siRNA) duplexesfor PKC ${iota}$ were purchased from Dharmacon (Lafayette, CO). Anti-PKC ${iota}$ ,anti-p38, and anti-phospho-p38 antibodies were purchased fromBD Biosciences (San Jose, CA). PD98059, anti-c-Jun, anti-phospho-c-Jun,anti-IRF-1, anti-Akt, anti-phospho-Akt, anti-phospho-CREB, andanti-I- ${kappa}$ B ${alpha}$ antibodies were purchased from Cell Signaling Technology(Danvers, MA). Anti-β-actin antibody was purchased fromAbcam (Cambridge, MA). A DuoSet human IL-6 enzyme-linked immunosorbentassay (ELISA) kit and anti-ICAM-1 antibody were purchased fromR&D Systems, Inc. (Minneapolis, MN). Anti-mouse immunoglobulinG and horseradish peroxidase (HRP)-tagged antibody were purchasedfrom Amersham (Piscataway, NJ). Anti-rabbit HRP-tagged antibodywas purchased from Zymed (San Francisco, CA). Anti-CREB andanti-sheep HRP-tagged antibodies were purchased from Upstate(Lake Placid, NY). All inhibitor targets are listed in Table1.

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TABLE 1. Effects of various signal transduction inhibitors on TNF- ${alpha}$ – or LPS-induced Stx2 cytotoxicity^a

Cell culture. Primary HUVEC were purchased from VEC Technologies (Rensselaer,NY) and grown in MCDB 131 medium (Mediatech/CellGro) supplementedwith 1 µg/ml hydrocortisone (Sigma Aldrich), 10 ng/mlepidermal growth factor (Collaborative Biomedical Products),100 µg/ml endothelial cell mitogen (Biomedical TechnologiesInc.), 2 mM L-glutamine (Gibco), 10% fetal bovine serum (HyClone),100 IU/ml penicillin, and 100 µg/ml streptomycin (Mediatech/CellGro).Cells were incubated at 37°C with 5% CO₂ and 90% humidityin Falcon 75-cm² flasks (BD Biosciences). All experiments wereperformed using HUVEC at passages 2 to 5.

Immunoblotting. HUVEC were seeded at a concentration of 400,000 cells/well,allowed to attach and grow overnight to confluence in six-wellplates, and treated as indicated below. Following treatment,wells were aspirated, and 400 µl Laemmli sample buffer(Bio-Rad) with 5% 2-mercaptoethanol was added for lysis. Togenerate lysates for use in immunoblots, cells were harvestedby scraping, DNA was sheared by passing cells through a 28-gaugeneedle more than six times, and proteins were denatured at 95°Cfor 4 min. Equal volumes of lysate were separated using sodiumdodecyl sulfate (SDS)-polyacrylamide gel electrophoresis (PAGE),transferred to a polyvinylidene difluoride membrane, and probedwith primary and HRP-conjugated secondary antibodies. BoundHRP was detected by enhanced chemiluminescence according tothe manufacturer's instructions (Western Lightning, Perkin Elmer).To assess loading controls, membranes were stripped by washingthem thoroughly with phosphate-buffered saline (PBS)-Tween,incubating them in 62.5 mM Tris-HCl (pH 6.8)-2% SDS-100 mM 2-mercaptoethanolat 50°C for 30 min, and rewashing them prior to reprobing.

Cell viability assays. HUVEC were seeded at a concentration of 24,000 cells/well andallowed to attach and grow overnight to confluence in 96-wellplates, and then they were treated as indicated below. Followingtreatment, either neutral red (37) or CCK-8 cell viability assayswere performed according to the manufacturer's instructions(Dojindo Molecular Technologies).

Pharmacological inhibition of different pathways. HUVEC were seeded as described above for the cell viabilityassays. At different times prior to stimulation with eitherLPS or TNF- ${alpha}$ , the following inhibitors were diluted in mediaand added to the cells: at 1 h prior to stimulation, wortmannin(1, 10, or 100 nM), PKC ${zeta}$ pseudosubstrate (50, 60, or 80 µM),SN50 (100 µM), SP600125 (500 or 10 µM), Jak inhibitor1 (100 or 500 nM), and PD98059 (10, 25, or 100 µM); at45 min prior to stimulation, Bay11-7082 (20 µM) and U0126(40, 60, 100, or 500 nM or 1 µM); at 40 min prior to stimulation,SB202190 (1, 10, 20, 50, or 100 µM) and SB203580 (20 µM);at 30 min prior to stimulation, Ebselen (1, 10, or 100 µM);and at the time of stimulation, cycloheximide (0.5, 2, or 5µg/ml). When appropriate, dimethyl sulfoxide diluent controlswere included. LPS and TNF- ${alpha}$ were then added to the cells inthe presence of the inhibitors for 24 h. The medium was thenreplaced with or without 1 nM Stx2 for 24 h, and cell viabilityassays were performed as described above. In separate experiments,HUVEC were incubated with the maximum tested dose of an inhibitorand treated with TNF- ${alpha}$ for 20 min or with LPS for 4 h; then theywere analyzed by immunoblotting as described above or fixedin 96-well plates for a cell-based ELISA, or supernatants wereanalyzed for secreted IL-6 by an ELISA performed according tothe manufacturer's instructions (R&D Systems).

Cell-based ELISA. Cells were treated with Bay11-7082 and SN50 as described above,treated with LPS or TNF- ${alpha}$ , and incubated for 4 h at 37°C.Following incubation, cells were fixed with a 1% glutaraldehydesolution for 20 min. Cells were then washed with PBS and blockedwith PBS containing 1% bovine serum albumin for 1 h. After blocking,cells were incubated with a 1:1,000 dilution of anti-ICAM-1antibody (overnight) and anti-sheep HRP (2 h). The signal wasvisualized with a 3,3',5,5'-tetramethylbenzidine substrate solutionand 2 N H₂SO₄ and quantified by determining the optical densityat 450 nm with a reference wavelength of 570 nm. Following collectionof ELISA data, cells were stained with crystal violet and valueswere normalized to the relative cell number. This protocol wasadapted from the protocol described in the general FACE kitmanual from Active Motif (Carlsbad, CA).

RNA interference knockdown of PKC ${iota}$ . Transfections were performed using the RNAiFECT handbook guidelines,with the following modifications. HUVEC were seeded at a concentrationof 12,000 cells/well in 96-well plates and allowed to attachovernight. The 25-µl (total volume) transfection mixtureconsisted of 0.125 µg siRNA, 0.75 µl RNAiFECT reagent,and 23.75 µl medium (control cells received PBS in placeof the siRNA suspension). Transfection was carried out for 4h, and then the transfection mixture was replaced with 200 µlmedium and the cells were incubated at 37°C for 24 h. Thenthe assay was performed as described above for the cell viabilityassay.

TLC of Gb₃. Equal amounts of HUVEC were seeded in Falcon 75-cm² flasks,and the cells were allowed to grow to confluence. Cells werethen treated as described in the figure legends, trypsinized,and counted. Neutral glycolipids were then isolated from thecells and analyzed by the thin-layer chromatography (TLC)-Stx1subunit B overlay method as described previously (47). TLC plateswere analyzed by densitometry, and the amounts were normalizedto the cell number and Gb₃ amount interpolated by comparisonwith authentic glycolipid standards (Matreya LLC) on each plate.

Statistics. Cell viability data were expressed as means ± standarddeviations. Student's two-sample t tests were used to comparecell viability values where indicated. A P value of <0.01was considered significant.

RESULTS

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RESULTS

LPS and TNF- ${alpha}$ induce Stx2 sensitivity in HUVEC. HUVEC are relatively insensitive to the cytotoxic effects ofStx2 compared to other subtypes of endothelial cells; however,their sensitivity can be increased by preincubating the cellswith LPS or TNF- ${alpha}$ (27, 37-39, 48, 59, 60). We were able to confirmthese findings by preincubating HUVEC with 0.01 to 100 µg/mlLPS or 0.2 to 2,000 U/ml TNF- ${alpha}$ for 24 h prior to treatment ofthe cells with 1 nM Stx2. As shown in Fig. 1A and B, both LPSand TNF- ${alpha}$ had a dose-dependent effect on Stx2 sensitivity. Wefurther characterized the system by adding either 10 µg/mlLPS or 200 U/ml TNF- ${alpha}$ to HUVEC for various times prior to 24h of Stx2 challenge. Figure 1C shows both the LPS- and TNF- ${alpha}$ -inducedStx2 sensitivities after the first hour of incubation and thatinduction remained relatively constant throughout the 48-h timecourse. TNF- ${alpha}$ was slightly more potent than LPS at the 8-, 12-,16-, and 24-h time points at these doses. In all additionalexperiments described here 10 µg/ml LPS or 200 U/ml TNF- ${alpha}$ was used for 24 h prior to Stx2 addition.

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FIG. 1. TNF- ${alpha}$ and LPS induce Stx2 cytotoxicity in a dose- and time-dependent manner. (A and B) Confluent HUVEC were incubated with the indicated concentrations of (A) LPS or (B) TNF- ${alpha}$ for 24 h before treatment with 1 nM Stx2 for 24 h. (C) Confluent HUVEC were incubated with either 10 µg/ml LPS or 200 U/ml TNF- ${alpha}$ for the indicated times before treatment with 1 nM Stx2 for 24 h. Cell viability assays were performed, and the results were expressed as the percent viability for identical treatments for each concentration and time point without Stx2; the error bars indicate standard deviations (n = 4). An asterisk indicates that the value is statistically significantly (P < 0.01) different from the value for samples without LPS or TNF- ${alpha}$ .

LPS and TNF- ${alpha}$ induce similar signal transduction pathways at different rates. LPS and TNF- ${alpha}$ stimulate a wide range of downstream effects throughmany different pathways (for reviews, see references 11, 40,and 64). To characterize a sample of these events in HUVEC,confluent monolayers of HUVEC were treated with either LPS orTNF- ${alpha}$ for up to 1 h, cells were lysed, and proteins were analyzedby immunoblotting. We found that TNF- ${alpha}$ (Fig. 2A) induced theNF- ${kappa}$ B and p38 MAPK pathways within 5 min and with between 10and 20 min of stimulation, respectively. I- ${kappa}$ B ${alpha}$ degradation wasobserved in a similar time frame, with the levels dropping belowthe detectable limits by 20 min poststimulation. In comparison,LPS showed a much slower induction profile with these pathways.LPS-induced phosphorylation of p38 MAPK reached maximal levelsat 1 h poststimulation and did not change throughout the remainingtimes tested (Fig. 2B). Additional experiments showed that therewere negligible changes in these proteins prior to 1 h poststimulation(data not shown). LPS-induced degradation of I- ${kappa}$ B ${alpha}$ showed a similartemporal response to p38 MAPK. In all cases, phosphorylationof p38 coincided with phosphorylation of the downstream transcriptiontargets CREB and ATF-1 (Fig. 2A and B).

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FIG. 2. TNF- ${alpha}$ and LPS induce intracellular pathway activation at different rates. Confluent HUVEC were incubated with (A) TNF- ${alpha}$ and (B) LPS for the indicated times and lysed. Lysates were processed by SDS-PAGE and analyzed by immunoblotting.

Differential inhibition of LPS- or TNF- ${alpha}$ -induced Stx2 sensitivity. Since LPS and TNF- ${alpha}$ stimulate many different pathways, pharmacologicalinhibitors and siRNAs were used to determine which of thesepathways was involved in LPS- or TNF- ${alpha}$ -induced sensitizationof HUVEC to Stx2 (Table 1; see Fig. S1 in the supplemental material).Of all the signal transduction inhibitors tested, only the p38MAPK inhibitors SB202190 and SB203580 fully inhibited both LPS-and TNF- ${alpha}$ -induced Stx2 sensitivity. However, the PKC ${zeta}$ pseudosubstrateadded prior to LPS or TNF- ${alpha}$ induction inhibited LPS-induced sensitivityby 50%. This inhibition was the same when the pseudosubstrateconcentration was increased to 80 µM. All pseudosubstrateconcentrations above 80 µM were cytotoxic. As expected,cycloheximide was also effective at inhibiting both LPS andTNF- ${alpha}$ induction of Stx2 sensitivity, which is consistent withprevious results (60).

p38 MAPK is required for Stx2 sensitization. p38 MAPK has been shown to be involved in Stx-mediated celldeath in other cell types (7, 24, 54). To determine which phase(i.e., induction or Stx2 challenge) of the experiment the p38inhibitors targeted, cells were treated with inhibitor beforeand/or after treatment with the inducer (Fig. 3A). As shownin Fig. 3B, both LPS and TNF- ${alpha}$ enhanced HUVEC sensitivity toStx2. The induction of sensitivity was reversed when a p38 inhibitorwas given prior to treatment with LPS or TNF- ${alpha}$ . Notably, thenoninduced cells were also more resistant to Stx2 challenge(P < 0.01). However, when the p38 inhibitor was given afterinduction and before Stx2 challenge, no significant changeswere observed. The cells that were exposed to the inhibitorthroughout the experiment were indistinguishable from the cellsthat were incubated with the inhibitor only prior to and concurrentlywith LPS or TNF- ${alpha}$ .

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FIG. 3. Inhibition of p38 reduces TNF- ${alpha}$ and LPS induction of Stx2 cytotoxicity. (B) HUVEC were treated with SB202190 (a p38 MAPK inhibitor) before or after induction and then challenged with Stx2. Details are as follows (A). For preinduction, one of the following was added to the cells for 40 min: 20 µM SB202190 or control medium. For induction one of the following was added to the cells for 24 h: SB202190, TNF- ${alpha}$ , LPS, TNF- ${alpha}$ plus SB202190, LPS plus SB202190, or control medium. For postinduction one of the following was added to the cells for 40 min: SB202190 or control medium. For challenge one of the following was added to the cells for 24 h: SB202190, 1 nM Stx2, SB202190 plus Stx2, or control medium. For the cytotoxicity assay after 24 h of incubation with Stx2, CCK-8 cell viability assays were performed, and the results were expressed as percentages of the viability of an identical treatment without Stx2; the error bars indicate standard deviations (n = 4). An asterisk indicates that the value is statistically significantly (P < 0.01) different from the value for samples not treated with SB202190. The data are representative of three independent experiments. The data obtained with a separate p38 MAPK inhibitor, SB203580, were similar.

p38 is required for LPS or TNF- ${alpha}$ induction of Gb₃. It has been shown that Gb₃ is the cellular receptor for Stx2(63) and that Gb₃ levels correlate with Stx sensitivity (48,59, 60, 62). Therefore, to determine the effects of p38 inhibitionon levels of Gb₃ on HUVEC, cells were treated with LPS or TNF- ${alpha}$ alone and after pretreatment with SB202190. Figure 4 shows thatpretreatment with the p38 inhibitor SB202190 reduced LPS andTNF- ${alpha}$ induction of relative Gb₃ levels, a trend that was observedconsistently. Note that although the fold change values aredifferent for the individual replicates, in each case the p38inhibitor reduced LPS- and TNF- ${alpha}$ -induced Gb₃ levels.

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FIG. 4. p38 inhibition reduces TNF- ${alpha}$ and LPS induction of Gb₃ in HUVEC. (A) Confluent HUVEC were treated with 20 µM SB202190 40 min prior to and concurrently with 200 U/ml TNF- ${alpha}$ or 10 µg/ml LPS for 24 h. Cells were trypsinized and counted, and neutral glycolipids were extracted. Glycolipids were separated by TLC and visualized by using Stx1 subunit B overlay. TLC plates were analyzed by densitometry, and amounts were interpolated by comparison with authentic standards on each plate. (B) Results for TLC-Stx1 subunit B overlay from replicate 2.

Specificity of SB202190. SB202190 has been shown to be a selective inhibitor of p38 MAPK(12). To verify this specificity under our conditions, HUVECwere treated with 10 and 20 µM SB202190, followed by 200U/ml TNF- ${alpha}$ (Fig. 5A) or 10 µg/ml LPS (Fig. 5B) for 20 minand 1 h, respectively, and the cells were lysed and analyzedby immunoblotting. SB202190 inhibited both TNF- ${alpha}$ and LPS inductionof CREB and ATF-1 phosphorylation but not degradation of I- ${kappa}$ B ${alpha}$ .This result is consistent with published data showing that CREBand ATF-1 are exclusively downstream of p38 (20).

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FIG. 5. Specificity of SB202190. Confluent HUVEC were treated with the indicated concentrations of SB202190 for 40 min prior to treatment with (A) TNF- ${alpha}$ for 20 min or (B) LPS for 1 h and lysed. Lysates were processed by SDS-PAGE and analyzed by immunoblotting.

DISCUSSION

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DISCUSSION

We show here for the first time that LPS and TNF- ${alpha}$ use a p38MAPK-dependent pathway to sensitize endothelial cells to Stx2-inducedcell death. p38 MAPK has been identified as a signaling factorin both Stx-induced cell death (54) and TNF- ${alpha}$ induction of Gb₃(55) in other cell types, so we examined if one or both of theseroles were evident in HUVEC. Since LPS and TNF- ${alpha}$ have been shownto increase Gb₃ levels over a 24-h time period (48), p38 inhibitorswere used to treat HUVEC before, during, and/or after 24 h ofinduction using LPS or TNF- ${alpha}$ . We found that p38 MAPK inhibitorswere effective at reducing LPS- or TNF- ${alpha}$ -induced Stx2-mediatedcell death only when given prior to the inducer, indicatingthat in HUVEC, p38 is principally involved in the inductionof the Stx2 receptor and not in toxin-mediated cell death. Thisconclusion is supported by the TLC data which showed that oneof the p38 inhibitors, SB202190, reduced LPS- and TNF- ${alpha}$ -inducedGb₃ levels.

We show here that both LPS and TNF- ${alpha}$ induce Stx2-mediated celldeath in a dose-dependent manner. These inflammatory mediatorshave been shown to increase Gb₃ and/or Stx sensitivity in kidneycell types such as mesangium (53), tubular epithelial cells(10), and glomerular microvascular endothelial cells even thoughTNF- ${alpha}$ does not affect the retrograde transport of the Stx B subunitin these cells (65). We also show that these cells requiredminimal times of exposure to LPS or TNF- ${alpha}$ in order to have increasedsensitivity to Stx2.

Signal transduction of HUVEC in response to LPS and TNF- ${alpha}$ israpid, with TNF- ${alpha}$ causing effects in as little as 5 min and LPScausing effects after 1 h of stimulation. This explains whyLPS and TNF- ${alpha}$ can sensitize HUVEC to the cytotoxic effects ofStx2 after only 1 h of stimulation. Our results are in concertwith previous findings that showed that I- ${kappa}$ B ${alpha}$ degradation occursmore rapidly in the presence of TNF- ${alpha}$ than in the presence ofLPS (69).

LPS and TNF- ${alpha}$ are known to stimulate multiple pathways in HUVEC(11, 40, 64), so we examined each pathway individually usingvarious inhibition methods in order to either include or excludea pathway's role in Stx2 sensitization. The pharmacologicalinhibitors that almost completely inhibited LPS and TNF- ${alpha}$ inductionof Stx2 sensitivity were SB202190 and SB203580, which are closelyrelated inhibitors of p38 MAPK, and cycloheximide, a generalinhibitor of protein synthesis. Cycloheximide has been shownto reduce the amount of TNF- ${alpha}$ -induced Stx1 binding to human femoralvein endothelial cells and HUVEC (60), theoretically by inhibitingtranslation of one or more of the biosynthetic enzymes requiredto make the functional Stx receptor, Gb₃. Our hypothesis includedthe possibility that multiple pathways could be utilized toincrease Gb₃, and thereby Stx2, sensitization. If multiple pathwayswere involved, then inhibition of any one of the necessary pathwaysshould partially block LPS- or TNF- ${alpha}$ -induced sensitivity to Stx2.Indeed, a PKC ${zeta}$ pseudosubstrate reduced LPS-induced Stx2 sensitivityby 50% in HUVEC. No other inhibitor tested partially reducedLPS-induced Stx2 sensitivity; however, it was shown previouslythat myristolated PKC ${zeta}$ pseudosubstrate nonspecifically causedthe phosphorylation of p38 MAPK, ERK1/2, Akt, and endothelialnitric oxide synthase in porcine pulmonary artery endothelialcells (32), making interpretation of these data difficult. Inhibitionof p38 MAPK did not completely reverse LPS- or TNF- ${alpha}$ -inducedStx2 sensitivity; however, the negative results obtained withall other signal transduction inhibitors tested imply that ifan additional pathway is involved, it is not one of the pathwaysidentified in endothelial cells.

p38 MAPK has been implicated at multiple stages in Stx-mediatedHUS. Upon release from the bacterium, Stx interacts with theintestinal epithelium, where p38 MAPK mediates Stx-induced releaseof IL-8 (58), eIF4E phosphorylation (8), caspase 3 cleavage,and cell death (54). After crossing the intestinal epithelium(23) and entering the vasculature, Stx stimulates circulatingmonocytes to secrete TNF- ${alpha}$ in a p38-dependent manner (4, 18).Once in the vasculature, the main targets of Stx are the brainand kidneys (56). Stricklett et al. showed that p38 MAPK isrequired for TNF- ${alpha}$ induction of Gb₃ and Stx1 sensitivity in humanbrain endothelial cells (55); moreover, Morigi et al. implicatedp38 in Stx2-mediated expression of endothelin-1, which is involvedin glomerular hemodynamics (45). It is noteworthy that in allcases, inhibiting p38 MAPK would theoretically benefit the host.Thus, p38 MAPK may represent a therapeutic target for reducingthe harmful host response to Stx2 if these in vitro resultscan be verified in an animal model.

In conclusion, p38, a common pathway intermediate, was shownto be involved in sensitization of HUVEC to Stx2 by both LPSand TNF- ${alpha}$ . p38 MAPK is required by both agonists to increasecellular Gb₃ levels and subsequent Stx2 sensitivity but notfor the Stx2-induced cytotoxicity that follows. These findingssupport the hypothesis that p38 MAPK is an effective targetin patients exposed to Stx2 for minimizing symptoms associatedwith HUS.

ACKNOWLEDGMENTS

We acknowledge Regina Seaner for expert technical assistance.

Funding for this work was provided by USPHS award AI024431 (T.G.O.).

FOOTNOTES

* Corresponding author. Mailing address: Department of Medicine, Division of Nephrology, University of Virginia, Box 800133, Charlottesville, VA 22908. Phone: (434) 982-1063. Fax: (434) 924-5848. E-mail: to3e{at}virginia.edu

Published ahead of print on 17 December 2007.

Supplemental material for this article may be found at http://iai.asm.org/.

Editor: B. A. McCormick

REFERENCES

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