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Flagellin, a Novel Mediator of Salmonella-Induced Epithelial Activation and Systemic Inflammation: IB Degradation, Induction of Nitric Oxide Synthase, Induction of Proinflammatory Mediators, and Cardiovascular Dysfunction¹

Tonyia Eaves-Pyles, Kanneganti Murthy^*, Lucas Liaudet^2,,¶, László Virág^*, Gary Ross, Francisco Garcia Soriano^3,¶, Csaba Szabó^*,¶ and Andrew L. Salzman^4,*,,

^* Inotek Corporation, Beverly, MA 01915; Critical Care Medicine, Pulmonary Biology, and Pulmonary Medicine, Allergy, and Clinical Immunology Division, Children’s Hospital Medical Center, Cincinnati, OH 45229; and ^¶ Department of Surgery, New Jersey Medical School, University of Medicine and Dentistry of New Jersey, Newark, NJ 01703

	Abstract

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Gram-negative sepsis is mediated by the actions of proinflammatory genes induced in response to microbes and their products. We report that flagellin, the monomeric subunit of flagella, is a potent proinflammatory species released by Salmonella. Flagellin (1 µg/ml) induces IB degradation, NF-B nuclear translocation, and inducible NO synthase expression in cultured intestinal epithelial cells (IEC). Aflagellic Salmonella mutants do not induce NF-B activation or NO production by cultured IEC. Antiserum to flagellin blocks NO production in IEC induced by medium conditioned by a variety of motile Gram-negative enteric pathogens (Escherichia coli, Salmonella muenchen, Serratia marcescens, Proteus mirabilis, and Proteus vulgaris). Flagellin, when injected systemically (10 µg/mouse), induces systemic inflammation characterized by the systemic expression of a range of proinflammatory cytokines and chemokines and of inducible NO synthase. At higher doses (300 µg/mouse), flagellin induces shock, characterized by hypotension, reduced vascular contractility in mice, and death. The effects of flagellin do not diminish in C3H/HeJ LPS-resistant mice, indicating that the Toll-like receptor-4 receptor is not involved in flagellin’s actions. In LPS-resistant mice, i.p. injection of S. dublin flagellin or medium conditioned by wild-type S. dublin induces serum IFN- and TNF-, whereas medium conditioned by aflagellic mutants has no effect. Flagellin can be detected in the blood of rats with septic shock induced by live bacteria at approximately 1 µg/ml. We propose that flagellin released by Gram-negative pathogens may contribute to the inflammatory response by an LPS- and Toll-like receptor-4-independent pathway.

	Introduction

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Salmonellae are Gram-negative, pathogenic micro-organisms that gain entrance to the human host by penetrating enterocytes in the intestinal mucosa. Enteroinvasion elicits a complex genetic response in the gut mucosa, inducing the expression of free radicals, cytokines, and chemokines associated with inflammation, tissue injury, and shock (1, 2, 3, 4, 5). Translocation of Salmonellae into the mesenteric lymphatics and the systemic circulation further activates proinflammatory gene expression in mononuclear cells, resulting in constitutional symptoms and hemodynamic alterations of septic shock (6). These effects are mediated by a broad range of cytotoxins, among them NO, a reactive free radical synthesized from L-arginine by inducible NO synthase (iNOS)⁵ (7). At nanomolar concentrations, NO functions as an endogenous antimicrobial factor, inhibiting oxygen consumption by disrupting the catalytic activity of the iron center in aconitase (8). Bacterial resistance to NO is dependent upon the inducible up-regulation of NO dioxygenase, a microbial flavohemoglobin that oxidizes NO via a peroxynitrite-like intermediate (9, 10).

De novo expression of iNOS in gut epithelial cells occurs in response to direct microbial interaction (1) and indirectly through the actions of proinflammatory cytokines induced by microbes and their products (11). Despite marked species variation in the organization of proinflammatory cis response elements of the iNOS promoter, the transcription of both murine and human iNOS genes is dependent upon the nuclear translocation of the cytosol-sequestered heterodimer p50/p65 (NF-B) of the Rel family (11, 12, 13). Intestinal epithelial cells (IEC) stimulated by Gram-negative bacteria readily induce degradation of the cytosolic inhibitor IB, resulting in the nuclear translocation and activation of NF-B (14) and the transcriptional up-regulation of nuclear iNOS mRNA (15). We now report that flagellin, a monomeric constituent of bacterial flagella, represents a crucial proinflammatory activity released by Salmonella dublin, a monophasic serotype making flagella (and so flagellin) of antigenic type g,p.

	Materials and Methods

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In vitro experiments

Bacterial culture. Salmonella dublin (SD), Salmonella typhimurium, Salmonella muenchen, Proteus vulgaris, Proteus mirabilis, and Serratia marcescens (American Type Culture Collection, Manassas, VA), Pseudomonas aeruginosa, and Escherichia coli (clinical isolates provided by Ian Holder, Ph.D., of the Shriners Burns Institute, Cincinnati, OH) were inoculated into 25 ml of brain heart infusion broth (BHI; Difco, Detroit, MI) and incubated overnight at 37°C in a shaking incubator (New Brunswick Scientific, Edison, NJ) to a stationary phase (10¹² CFU/ml). The cultures were centrifuged at 10,000 rpm for 10 min, and the broth was sterile-filtered through a 0.45-µm pore size filter.

Cell culture and infection. DLD-1 and Caco-2BBe cells (American Type Culture Collection) between passages 5 and 15 were cultured in DMEM supplemented with 10% FBS, 2 mM glutamine, 1% nonessential amino acids, and antibiotics. RAW cells (American Type Culture Collection) between passages 5 and 15 were cultured in DMEM supplemented with 10% FBS, 4 mM glutamine, 1.5 g/l sodium bicarbonate, 4.5 g/L glucose, 1.0 mM sodium pyruvate, and antibiotics. Cells were seeded onto 6- and 96-well plates and 10-cm tissue culture plates and cultured to confluence. The growth medium was replaced by DMEM without FBS or antibiotics immediately before studies.

NO₂^-/NO₃^- determination. The combined concentration of nitrite and nitrate, the degradation products of NO in the culture medium, was determined by the Griess reaction following nitrate reduction as previously described (11). Total nitrite/nitrate production is referred to in the text as NO production.

Western blotting. Cells grown in six-well culture plates were washed once in PBS and lysed in cold buffer containing 50 mM Tris (pH 8.0), 110 mM NaCl, 5 mM EDTA, 1% Triton X-100, and 0.1 mM PMSF. The Bradford assay (Bio-Rad, Hercules, CA) was used to determine protein concentrations of each sample. Cell lysates were boiled in an equal volume of loading buffer (4% SDS, 20% glycerol, 125 mM Tris-HCl (pH 6.8), and 10% 2-ME), and 50 µg of each protein sample was loaded per lane on an 8–16% Tris-glycine gradient gel (NOVEX, San Diego, CA). Electrophoresed proteins were transferred to a nitrocellulose membrane (NOVEX) using the NOVEX Xcell MiniGel system. Membranes were blocked with 10% nonfat dried milk in TBS for 1 h before exposure to rabbit polyclonal anti-IB antiserum (Santa Cruz Biotechnology, Santa Cruz, CA) and anti-iNOS antiserum (gift from Robert Webber, Research Diagnostic Antibodies, San Francisco, CA) at a dilution of 1/200 for 45 min. Blots were washed twice in TBS containing 0.1% Tween-20, followed by the addition of peroxidase-conjugated anti-rabbit IgG (Sigma, St. Louis, MO) at a dilution of 1/10,000 for 30 min. Blots were washed three times for 5 min per wash in TBS containing 0.1% Tween-20, incubated in commercial ECL reagents (Amersham, Aylesbury, U.K.), and exposed to photographic film.

Nuclear protein extraction. Nuclear protein extracts were prepared after cells were incubated with medium conditioned by SD (CM). Cells were washed twice with ice-cold PBS and harvested by scraping into 1 ml of PBS. After pelleting at 6,000 rpm for 5 min, cells were washed twice with cold PBS, resuspended in one cell pellet volume of lysis buffer (1.5 mM MgCl₂, 0.2% (v/v) Nonidet P-40, 10 mM HEPES (pH 7.9), 10 mM KCl, 0.1 mM EDTA, 1 mM DTT, and 0.1 mM PMSF), and incubated on ice for 5 min with intermittent vortexing. Nuclei were collected from the cell lysates by centrifugation (6,000 rpm for 5 min), then resuspended in one cell pellet volume of extraction buffer (1.5 mM MgCl₂, 25% (v/v) glycerol, 20 mM HEPES (pH 7.9), 420 mM NaCl, 0.1 M EDTA, 1 mM DTT, and 0.5 mM PMSF). After incubation on ice for 15 min with intermittent vortexing, nuclear proteins were collected by centrifugation (14,000 rpm for 15 min). Supernatants also were collected to ensure the elimination of nuclear debris.

EMSA. An NF-B oligonucleotide probe (5'-AGT TGA GGG GAC TTT CCC AGG-3'; Santa Cruz Biotechnology) was labeled with [-³²P]ATP using T4 polynucleotide kinase (Life Technologies, Gaithersburg, MD) and then purified on a Bio-Spin chromatography column (Bio-Rad, Hercules, CA). Ten micrograms of nuclear protein extracts were preincubated with EMSA buffer (1 mM EDTA, 1 mM DTT, 12 mM HEPES (pH 7.9), 4 mM Tris-HCl (pH 7.9), 5 mM MgCl₂, 25 mM KCl, 12% glycerol, 50 ng/ml poly[d(I-C)], and 0.2 mM PMSF) on ice for 10 min, followed by the addition of the radiolabeled probe for 20 min. The specificity of the binding reaction was determined by incubating duplicate nuclear protein samples with a 100-fold molar excess of unlabeled probe. Samples were resolved on a nondenaturing polyacrylamide gel containing 5% acrylamide and run in 0.5x TBE (1 mM EDTA, 45 mM boric acid, and 45 mM Tris-HCl) at a constant current (30 mA) for 1 h. Gels were transferred to Whatman 3M paper (Clifton, NJ) and dried under a vacuum at 80°C for 1 h, followed by film exposure to using an intensifying screen at -70°C for approximately 3 h.

Purification and preparation of flagellins. Flagellin was purified from SD and a congenic flagellin-deficient mutant according to well-established methods (16). Bacterial isolates were used to incubate 1-l Erlenmeyer flasks containing BHI infusion broth. Flasks were incubated at 35°C in an orbital shaker incubator at 80 rpm for 16 h. Bacterial cells were harvested by centrifugation at 5,000 x g for 30 min and then mixed with saline solution to form a moderately thick suspension. The suspension was adjusted to pH 2.0 with 1 M HCl and maintained at that pH under constant stirring for 30 min at room temperature. The bacterial cells, devoid of flagella, were separated by centrifugation at 5,000 x g for 30 min. The supernatant, which contained detached flagellin in monomeric form, was further centrifuged at 100,000 x g for 1 h at 4°C to sediment the pH 2.0-insoluble material. The pH of the supernatant was adjusted to 7.2 with 1 M NaOH. Ammonium sulfate was added slowly with vigorous stirring to achieve two-thirds saturation (2.67 M). The mixture was centrifuged at 15,000 x g for 15 min at 4°C. The precipitate was dissolved in approximately 5 ml of distilled water and then transferred to dialysis tubing (m.w. cutoff, 50,000). Dialysis was conducted for 18 h at 4°C with constant stirring in 4 l of distilled water. The dialyzed flagellin preparations were then lyophilized and stored at -70°C.

Recombinant flagellins of S. muenchen, E. coli, P. vulgaris, P, mirabilis, and S. marcescens were prepared as follows. The gene fragment corresponding to aa 1–156 of the flagellin gene of S. muenchen was generated by PCR amplification with a sense primer designated 1S (5'-CGCGGATCCCAATGGCACAAGTCATTAATACAAACA) and an antisense primer designated 468A (5'-TCCGCTCGAGTTAAATAGTTTCACCGTCGTTGGCACC). The entire flagellin gene was amplified with primers 1S and 1530A (5'-TCCGCTCGAGTTAACGCAGTAAAGAGAGGACGTTTTG). Underlined nucleotides represent adaptor sequences added to the ends of primers to maintain proper reading frame and facilitate cloning (BamHI recognition sites on sense primers and XhoI sites on antisense primers). Template DNA for PCR reactions was plasmid CL402, a clone of pBR322 containing a 3.8-kb EcoRI fragment of S. muenchen chromosomal DNA that harbors the 1.5-kb flagellin gene. PCR-generated flagellin DNA was digested with BamHI plus XhoI, gel purified, and subcloned into the BamHI/XhoI sites at the 3' end of the GST gene in expression vector pGEX-5X-2 (Pharmacia Biotech, Piscataway, NJ) and pET 30C (Novagen, San Diego, CA). Similarly DNA sequences corresponding to flagellin coding region of E. coli, P. vulgaris, P. mirabilis, and S. marcescens were amplified by PCR and cloned into pRSET C vector (Invitrogen, San Diego, CA). The correct reading frame and integrity of subcloned DNA were verified by DNA sequence analysis.

A single colony of E. coli DH5 (Life Technologies) containing the desired plasmid was grown at 37°C in Luria broth containing 100 µg of ampicillin/ml to an A600 of 0.5 and then induced for 3 h with 0.5 mM isopropyl--D-thiogalactoside. Following induction, bacteria were harvested and washed with STE buffer (10 mM Tris (pH 8), 50 mM NaCl, and 1 mM EDTA). Cells were suspended in STE buffer containing 100 µg/ml lysozyme, incubated 45 min on ice, and then adjusted to 5 mM DTT. After two freeze-thaw cycles, the cell suspension was sonicated and clarified by centrifugation at 10,000 x g. The soluble lysate was applied to a glutathione-agarose column, washed with STE plus 5 mM DTT, and then eluted with STE plus 5 mM DTT buffer containing 10 mM reduced glutathione. The purity of each eluted fusion protein was analyzed by SDS-PAGE. Purified proteins were dialyzed against PBS, quantified by the Bradford method, and stored at -70°C.

Antiserum. Polyclonal lapine antiserum directed against a recombinant S. muenchen flagellin was prepared by Protein Express (Cincinnati, OH) as follows. Serum was collected from New Zealand rabbits immunized with a GST fusion of the N-terminus of recombinant S. muenchen flagellin, corresponding to aa 1–156. The Ag was prepared by expression of a cDNA clone obtained by PCR amplification of DNA from S. muenchen using a sense primer designated 1S (5'-CGCGGATCCCAATGGCACAAGTCATTAATACAAACA) and an antisense primer designated 468A (5'-TCCGCTCGAGTTAAATAGTTTCACCGTCGTTGGCACC). Underlined nucleotides represent adaptor sequences added to the ends of primers to maintain proper reading frame and facilitate cloning (BamHI recognition sites on sense primers and XhoI sites on antisense primers). The template DNA for PCR was plasmid CL402, a clone of pBR322 containing a 3.8-kb EcoRI fragment of S. muenchen chromosomal DNA that harbors the 1.5-kb flagellin gene. PCR-generated flagellin DNA were digested with BamHI plus XhoI, gel purified, and subcloned into the BamHI/XhoI sites at the 3' end of the GST gene in expression vector pGEX-5X-2 (Pharmacia Biotech). The correct reading frame and integrity of subcloned DNA was verified by DNA sequence analysis.

In vivo and ex vivo experiments

Effect of flagellin and conditioned medium on inflammatory mediator and iNOS expression in vivo. To test whether flagellin is capable of inducing the systemic inflammatory alterations characteristic of Gram-negative sepsis, C57BL/6 mice were challenged with 10 µg (400 µg/kg i.p.) of purified SD flagellin. Mice were sacrificed at various time points (2, 4, 8, and 24 h postflagellin), and serum concentrations of TNF-, IL-6, IL-12p40, macrophage inflammatory protein-1 (MIP-1), and IL-10 were measured with ELISA (see below), and nitrite/nitrate levels were measured with the modified Griess reaction (see above). In addition, at 24 h ileal samples were obtained and processed for iNOS immunohistochemistry. In an additional set of experiments, LPS-resistant C3H/HeJ mice were treated with vehicle, 10 µg/mouse purified flagellin, SD-conditioned medium (0.3 ml), or conditioned medium from aflagellic SD mutants (0.3 ml). Mice were sacrificed at 3 h, and serum TNF- and IFN- levels were measured. The presence of serum cytokines was detected by enzyme immunoassay. Enzyme immunoassay plates (Corning Costar, Cambridge, MA) were coated with 100 µl of 5 µg/ml goat anti-murine cytokine neutralizing Abs (R&D Systems, Minneapolis, MN) diluted in 0.1 M carbonate buffer (pH 9.6) and incubated at 4°C for 16 h. The plates were washed three times with washing buffer (1x PBS (pH 7.4) and 0.5% Tween-20). After washing, plates were incubated with blocking buffer (1x PBS (pH 7.4), 0.5% Tween-20, and 2% BSA) at 37°C for 2 h. To prepare a standard curve, serial dilutions of standard purified recombinant cytokines (R&D Systems) were prepared in blocking buffer and added to the plates. Samples (100 µl) or standards were added to the plates followed by incubation for 2 h at 37°C, washing three times, and blocking for 15 min at room temperature. Plates were incubated with 100 µl of 10 µg/ml rabbit anti-murine cytokine Ab at 37°C for 2 h. After incubation, plates were washed three times with washing buffer and incubated with 100 µl of 2 µg/ml goat anti-rabbit IgG (whole molecule) HRP-conjugated Ab (Calbiochem, San Diego, CA) at 37°C for 2 h. Plates were washed three times with washing buffer and then incubated with 150 µl of K Blue Substrate (Neogen, Lexington, KY), and the color was developed for 20 min at room temperature. Following color development, the plates were read using an automated microplate reader (Molecular Devices, Menlo Park, CA) at a wavelength of 650 nm. For iNOS immunohistochemistry, ileum was fixed and processed for immunohistochemistry as previously described (17). Tissue samples were fixed for 3 h in 4% paraformaldehyde and cryoprotected by a 1-h incubation in 10, 20, and 30% sucrose in 0.1 M sodium cacodylate buffer. The tissues were then placed on tissue holders covered with a thin layer of OCT (a water soluble glycol & resin compound; Tissue-Tek) and frozen in distilled freon 22 in liquid nitrogen. Eight-micron thin sections were placed onto slides and stained with the anti-nitrotyrosine Ab. The blocking solution consisted of 4% fatty acid-free BSA, 10% goat serum, and 3% Triton X-100 in 0.1 M PBS, pH 7.2. The iNOS immunoreactivity was detected using iNOS mAb (provided by Robert Webber, Research Diagnostic Antibodies). Samples were incubated with Ab at 2 µg/ml for 3 h. The Ab binding on tissue sections was visualized by a 1-h incubation with an anti-murine IgG conjugated to Texas Red (1/100 dilution in PBS). Slides were examined under a Nikon Diaphot-TND epifluorescence inverted microscope (Melville, NY).

Hemodynamic studies. Male C3H/OuJ mice and C3H/HeJ (25 g) were anesthetized i.p. with ketamine (50 mg/kg) and xylazine (5 mg/kg). Maintenance doses of ketamine (10 mg/kg) and xylazine (1 mg/kg) were given when necessary (interdigital reflex). Under deep anesthesia, polyethylene catheters (PE 10) were inserted into the left jugular vein for the i.v. administration of compounds and into the right carotid artery. The carotid artery catheter was connected to a pressure transducer for blood pressure measurement. Pressure signals were recorded using a MacLab A/D converter and were continuously displayed on a Macintosh computer (Cupertino, CA). Following a 20-min stabilization period, baseline hemodynamic parameters were recorded. The animals were then randomized to the i.v. injection of recombinant S. muenchen flagellin (10 mg/kg), E. coli LPS (10 mg/kg), or vehicle (10 mM PBS), given as a slow bolus over 1 min (200 µl), and were then observed for the next 4 h. At this time point, mice were euthanized by exsanguination, immediately followed by thoracolaparotomy to allow excision of the aorta. The aorta was cleared from periadventitial fat and cut into 1- to 2-mm-wide rings, mounted in organ baths filled with warmed (37°C) and oxygenated (95% O₂ and 5% CO₂) Krebs’ solution. Isometric forces were measured with isometric transducers (Kent Scientific, Litchfield, CT), digitized using a MacLab A/D converter, and stored and displayed on a Macintosh computer. A tension of 1 g was applied, and the rings were equilibrated for 60 min, followed by measurements of the concentration-response curves to phenylephrine (10^-10 to 3 x 10^-5 M) and acetylcholine (10^-9 to 3 x 10^-5 M).

Induction of bacterial sepsis in rats and quantification of serum levels of flagellin by enzyme immunoassay. S. marcescens was grown overnight in nutrient broth and then harvested by centrifugation. The cell pellet was washed twice with PBS and suspended in PBS at a concentration of 3.3 x 10⁵ CFU/ml. Three milliliters of bacteria (1 x 10⁹ CFU/ml) were injected into male 250-g Wistar rats (i.p.). Blood samples were collected at 0, 4, and 8 h. Serum was collected after centrifugation of blood at 14,000 rpm for 15 min. The centrifugation step was repeated three times to remove any contaminating bacteria. Plasma samples were tested negative for colony-forming viable bacteria after centrifugation. Serum samples were screened by ELISA using Immulon 2HB Microtiter plates (Dynex, Chantilly, VA). The plate wells were coated overnight at 4°C with 0.5 µg of murine anti-flagellin Abs in 50 mM sodium carbonate buffer (pH 9.3). After each step, unbound reagents in the wells were removed by repeated washing with PBS and 0.05% Tween 20. Wells were blocked with 5% nonfat dry milk (NFDM) and 1% BSA in PBS for 1 h. Following blocking, serum samples were diluted 1/1 with 1% BSA in PBS, and then 100 µl was added to each well. Bacterially expressed and purified recombinant Serratia marcescens flagellin protein serially diluted in 1% BSA was used as standard for quantitative measurements. Plates were incubated overnight at 4°C with gentle shaking. Rabbit anti-flagellin polyclonal Abs (1/2000) were added to the wells and incubated at room temperature with gentle shaking for 2 h. To detect Ag-Ab complexes, the wells were treated with 100 µl of peroxidase-conjugated goat anti-rabbit IgG used at a 1/2000 dilution in 1% NFDM/PBS. The peroxidase enzyme substrate 3,3',5,5'-tetramethylbenzidine was used at a volume of 100 µl/well. After 5 min at room temperature the reaction was stopped by adding 25 µl of 0.1 M H₂SO₄, and the absorbance was measured at 450 nm.

Statistical Analysis. Numerical results are reported as the mean ± SEM of three or more independent experiments. Gels or immunohistochemical pictures shown are representative of results obtained in three or more independent experiments. For analysis of the numerical data, ANOVA followed by Tukey’s test was used to compare mean values. Statistical differences were declared significant for p < 0.05.

	Results

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Flagellin influences inflammatory gene expression by Salmonella

Sterile-filtered CM grown overnight to a stationary phase (10¹² CFU/ml) was added to cultured human IEC, Caco-2BBe, and DLD-1. CM (1/100 dilution) induced IB degradation (Fig. 1A) and the nuclear translocation of NF-B (Fig. 1B) at 30 and 60 min poststimulation, respectively. Addition of CM (1/100–50,000 dilution) to DLD-1 cells primed for 2 h with IFN- (100 U/ml) induced high levels of NO production (64 µM nitrate/nitrite; EC₅₀ = 1/1,600 dilution) over 16 h of incubation.

View larger version (52K): [in this window] [in a new window]   FIGURE 1. Salmonella-conditioned medium induces IB degradation and NF-B activation in Caco-2BBe cells. A, IB degradation was induced in a time-dependent manner in Caco-2BBe cells stimulated with CM. Confluent Caco-2BBe cells were stimulated by CM for 20, 30, or 60 min. Total protein was extracted, and equal amounts of protein were subjected to SDS-PAGE gel electrophoresis, followed by immunoblotting for IB as previously described (14 ). Blots were probed with a lapine polyclonal anti-IB antiserum (Santa Cruz Biotechnology). Unconditioned medium (M) and unstimulated control cells (C) showed no degradation of IB at 30 min. Cells stimulated with CM showed a loss of immunoreactive IB at 20 and 30 min. At 60 min poststimulation, IB is resynthesized by the activation of NF-B released through the degradation of IB protein. B, Representative EMSA demonstrating NF-B activation in Caco-2BBe cells stimulated for 60 min with CM. Nuclear extracts from unstimulated cells showed no NF-B activation (C). NF-B activation was demonstrated in cells stimulated with flagellin for 60 min. To confirm the specificity of the NF-B signal, a 100-fold excess of cold oligonucleotide was used as a competitor to inhibit the binding activity of NF-B (COMP). Gels representative of three to five independent determinations are shown.

View larger version (44K): [in this window] [in a new window]   FIGURE 2. Purification of proinflammatory activity of Salmonella-conditioned media. A, SDS-PAGE gel demonstrating silver-stained SD-released protein(s) purified by standard protein purification methods. Equal amounts of total protein were loaded in each lane. B, IB degradation in Caco-2BBe cells stimulated with SD-released protein(s). Confluent Caco-2BBe cells were exposed for 20, 30, or 60 min to 1/200 dilution of purified fractions of CM. Unstimulated cells served as controls (C). Cells were washed, and total eukaryotic protein was extracted and equal amounts of protein were subjected to SDS-PAGE gel electrophoresis, followed by immunoblotting of IB as described in Fig. 1A. Lane 1, Sterile BHI. Lane 2, BHI medium inoculated with SD and grown for 18 h. Conditioned medium was filtered to eliminate intact bacteria and medium containing secreted proteins from SD was collected. Lane 3, Conditioned medium was run over an anion exchange column (fast protein liquid chromatography), and fractions that induced NO production in IFN- (100 U/ml)-primed DLD-1 cells were pooled and electrophoresed. Lane 4, Conditioned medium fractionated by fast protein liquid chromatography, followed by gel filtration. Fractions that induced NO production were pooled and electrophoresed. Lane 5, Purified SD flagellin as previously described (16 ). Gels representative of three to five independent determinations are shown.

Aflagellic Salmonella mutants do not induce NO production by cultured IEC

To establish the relative importance of flagellin to the CM-mediated induction of NO by IFN- primed DLD-1 cells, we compared the effect of CM obtained from wild-type SD (SL7276) and an aflagellic SD mutant (SL7276; Fig. 3). CM produced by wild-type SD potently induced synthesis of NO comparable to that stimulated by the cytokine combination of IL-1 and IFN-. In contrast, CM produced by the aflagellic SD mutant induced only slightly more NO than BHI alone. We also observed a high level of induction of NO production by CM obtained from clinical isolates of other flagellated Gram-negative bacillary pathogens, such as E. coli and P. aeruginosa (Fig. 3).

View larger version (49K): [in this window] [in a new window]   FIGURE 3. Bacteria-conditioned medium induces NO production in DLD-1 cells. Addition of CM (1/200 dilution) to DLD-1 cells primed for 2 h with IFN- (100 U/ml) induced NO production over 16 h of incubation, comparable to the level of induction produced by the cytokine combination of IL-1 and IFN-. Medium conditioned by an aflagellic SD mutant did not induce NO production. A similar induction of NO production was obtained with sterile-filtered medium conditioned by E. coli and P. aeruginosa (Ps. a.). The combined concentration of nitrite and nitrate was determined by the Griess reaction following nitrate reduction. There were seven to nine determinations per experimental group or time point.

Effect of purified flagellin on IB stability, NF-B activation, and NO production

Because NF-B activation regulates iNOS transcription (11, 12, 13), we tested the effect of SD CM and purified flagellin on the stability of IB expression. Caco-2BBe cells stimulated by 1 µg/ml of SD-purified flagellin underwent a loss of immunoreactive IB 20 and 30 min poststimulation, followed by its reappearance at 60 min (Fig. 4A). The loss of IB preceded NF-B binding activity, which was detected 30, 60, and 120 min after exposure of cells to flagellin (Fig. 4B). As predicted by the replenishment of IB protein at 60 min (Fig. 4A), NF-B binding activity was diminished at 120 min (Fig. 4B). The specificity of the binding activity was confirmed by competition with a 100-fold excess of cold oligonucleotide competitor (Fig. 4B).

View larger version (55K): [in this window] [in a new window]   FIGURE 4. Purified flagellin induces IB degradation, NF-B activation, and NO synthesis in Caco-2BBe cells. A, IB degradation was induced in a time-dependent manner in Caco-2BBe cells stimulated with SD-purified flagellin. Confluent Caco-2BBe cells were exposed for 10, 20, 30, or 60 min to 1 µg/ml of SD-purified flagellin, purified as previously described (16 ). Total protein was extracted, and equal amounts of protein were subjected to SDS-PAGE, followed by immunoblotting of IB as described in Fig. 1A. Unstimulated cells showed no loss of IB immunoreactivity (C). Cells exposed to SD-purified flagellin demonstrated IB degradation at 20 and 30 min, with a reappearance at 60 min. B, Representative EMSA demonstrating NF-B activation in Caco-2BBe cells stimulated for 30, 60, or 120 min with SD-purified flagellin. Nuclear extracts from cells stimulated with flagellin were incubated with 32P-labeled NF-B oligonucleotides to determine NF-B activation as described in Fig. 1B. Nuclear extracts from unstimulated cells showed no NF-B activation (C). NF-B activation was demonstrated in cells stimulated with flagellin at 30, 60, or 120 min. To confirm the specificity of the NF-B signal, a 100-fold excess of cold oligonucleotide was used as a competitor to inhibit the binding activity of NF-B (COMP). C, Addition of purified flagellin to Caco-2BBe cells primed for 2 h with IFN- (100 U/ml) dose-dependently induced NO production over 16 h of incubation. The combined concentration of nitrite and nitrate was determined by the Griess reaction following nitrate reduction. There were seven to nine determinations per experimental group or time point. D, Purified SD flagellin induces iNOS protein expression in cultured human intestinal epithelial cells. DLD-1 and Caco-2BBe cells were primed for 2 h with 0.5 ng/ml IL-1 or 100 U/ml IFN- followed by the addition of 1 µg/ml purified SD flagellin for approximately 16 h. Upper, IFN--primed DLD-1 cells exposed to flagellin or IL-1 showed induction of iNOS expression. Individual cytokines and flagellin alone did not up-regulate iNOS protein expression in either cell line. Lower, IFN--primed Caco-2BBe cells exposed to flagellin or IL-1 showed induction of iNOS expression. Individual cytokines and flagellin alone did not up-regulate iNOS protein expression in either cell line. There were three to five determinations per experimental group.

The effect of flagellin on iNOS protein expression was determined by Western analysis of extracts from DLD-1 and Caco-2BBe cells exposed to purified flagellin derived from SD. Stimulation by IFN-, IL-1, or flagellin alone did not induce the expression of detectable immunoreactive iNOS protein (Fig. 4D). In IFN--treated cells, in contrast, IL-1 and flagellin elicited increased iNOS expression in both cell lines. In addition, ELISA measurements of the supernatants of Caco-2BBe cells stimulated with purified SD flagellin (1 µg/ml) revealed secretion of IL-6 (from undetectable levels to 216 ± 12 pg/ml at 24 h). Purified SD flagellin, in the presence of IFN- (but not without IFN- costimulation), induced the production of IL-8 (from undetectable levels to 87 ± 3 pg/ml at 24 h). Thus, flagellin is able to elicit a general proinflammatory response from human epithelial cells (18, 19).

To establish the overall contribution of flagellin to the induction of IB degradation in intestinal epithelial cells, we compared the effect of CM obtained from wild-type SD (SL7276) and the aflagellic SD mutant (SL7276; Fig. 5). CM produced by wild-type SD (1/200 dilution) potently induced IB degradation by Caco-2BBe cells. In contrast, CM produced by the aflagellic SD mutant (1/200 dilution) had no effect on IB expression. We also observed that CM produced by E. coli and P. aeruginosa induced IB degradation comparable to the effect of CM from wild-type S. dublin (Fig. 5).

View larger version (38K): [in this window] [in a new window]   FIGURE 5. Conditioned bacterial medium induces IB degradation in Caco-2BBe cells. IB degradation was induced in a time-dependent manner in Caco-2BBe cells exposed for 30 or 60 min to BHI (lane A), medium conditioned by wild-type SD or aflagellic SD (lane B), and medium conditioned by E. coli or P. aeruginosa (lane C). Total protein was extracted, and equal amounts of protein were subjected to SDS-PAGE, followed by immunoblotting of IB as described in Fig. 1A. BHI-treated cells showed no loss of IB immunoreactivity (lane A). Cells exposed to CM demonstrated IB degradation at 30 min, with a reappearance at 60 min, whereas aflagellic SD did not induce IB degradation (lane B). Medium conditioned by E. coli and P. aeruginosa demonstrated a similar pattern as wild-type SD (lane C). Gels representative of three to five independent determinations are shown.

Media conditioned by the aflagellic mutant of SD (SL7276) failed to induce NO production in IFN--primed DLD-1 cells, suggesting that flagellin may be the predominant proinflammatory exotoxin released by SD. Since LPS is a well-established Gram-negative endotoxin, we conducted the following series of investigations to exclude its contribution to the flagellin-induced inflammatory responses. 1) The level of immunoreactive IB was unaltered by exposure of Caco-2BBe cells to purified S. typhimurium LPS (1 µg/ml) (20), in contrast to the effect of purified SD flagellin. 2) Cotreatment of IFN- primed DLD-1 cells with an LPS binding agent, polymyxin B (10 µg/ml), blocked NO production induced by 1 µg/ml of LPS purified from S. typhimurium (Sigma, catalogue L-7261), but not by 1 µg/ml of purified SD flagellin (Fig. 6A). 3) The content of LPS in 1 µg of purified SD flagellin, as measured by the chromogenic Limulus amebocyte assay (1), was <20 pg. As we previously reported, S. typhimurium LPS at a concentration of <1 µg/ml is unable to induce iNOS expression and NO production in cultured human intestinal epithelial cells (1). 4) In C3H/HeJ LPS-resistant mice, i.p. injection of purified SD flagellin or conditioned medium of the wild-type parent strain of SL7276 induced serum IFN- and TNF-, whereas conditioned medium from SL7276 aflagellic mutants had no effect (Fig. 6B). In further support of the LPS-independent role of flagellin on proinflammatory gene expression, addition of recombinant S. muenchen flagellin (purified over a polymyxin B column) to IFN--primed DLD-1 and Caco-2BBe cells dose-dependently induced NO production (data for Caco-2BBe cells shown in Fig. 7A). 5) Full-length, but not truncated, recombinant N-terminal S. muenchen flagellin (aa 1–156) induced NO synthesis in IFN--primed DLD-1 cells (data not shown).

View larger version (49K): [in this window] [in a new window]   FIGURE 6. The proinflammatory effect of flagellin is independent of LPS. A, Polymyxin blocks LPS-induced, but not flagellin-induced, production of NO in Caco-2BBe cells. Cotreatment of IFN- (100 U/ml)-primed DLD-1 cells with an LPS-binding agent, polymyxin B (10 µg/ml), blocked NO production induced by 1 µg/ml of LPS purified from S. typhimurium, but not by 1 µg/ml of purified SD flagellin (n = 12; p < 0.01). B, Systemic flagellin injection induces serum cytokine expression in LPS-resistant mice. C3H/HeJ mice were treated with vehicle, 10 µg/mouse purified flagellin, SD-conditioned medium (broth), or conditioned medium from aflagellic SD mutants (aflagellic broth). Mice were sacrificed at 3 h, and serum TNF- and IFN- levels were measured. Purified flagellin and SD-conditioned medium, but not conditioned medium from aflagellic SD mutants, induced the production of IFN- and TNF-. There were three to five determinations per experimental group.

View larger version (35K): [in this window] [in a new window]   FIGURE 7. Antiserum to flagellin inhibits NO production induced by Caco-2BBe cells exposed to bacteria-conditioned medium or recombinant flagellin. A, Recombinant S. muenchen flagellin induced a concentration-dependent increase in NO production in IFN--primed (100 U/ml) Caco-2BBe cells. B, Medium conditioned by various motile Gram-negative pathogens (E. coli, S. muenchen, S. marcescens, and P. mirabilis) induced NO production in IFN- primed (100 U/ml) Caco-2BBe cells. C, Recombinant flagellins cloned from various motile Gram-negative pathogens (E. coli, S. muenchen, S. marcescens, and P. mirabilis) induced NO production in IFN- primed (100 U/ml) Caco-2BBe cells. NO production was inhibited by preincubation (1 h at room temperature) of recombinant flagellin (A and C) or conditioned medium (B) with a 1/100 dilution of lapine polyclonal antiserum generated against recombinant S. muenchen flagellin. Incubation with preimmune serum was not inhibitory. There were three to five determinations per experimental group.

Anti-flagellin antiserum blocks induction of NO production induced by flagellins of various motile Gram-negative bacteria

To further implicate flagellin as the relevant NO-inducing species, we next tested whether anti-flagellin Abs would neutralize the production of NO induced by conditioned medium or recombinant flagellin. As a positive control, lapine antiserum raised against the N-terminus of S. muenchen flagellin abolished the NO-inducing activity of recombinant Salmonella muenchen flagellin in IFN- primed Caco-2BBe cells (Fig. 7A). The antiserum also abolished the NO-inducing activity of recombinant flagellins (Fig. 7B) or conditioned medium (Fig. 7C) derived from a series of Gram-negative motile bacterial species (E. coli, S. muenchen, S. marcescens, P. mirabilis, and P. vulgaris). The latter data imply that flagellin may represent the crucial factor in the induction of NO production by CM obtained from flagellated Gram-negative bacilli.

Flagellin induces inflammatory gene expression in mice

Retention of the flagellin monomer within the growing polymeric filament is dependent upon the presence of the HAP2 cap protein, which is located at the distal terminus of the intact flagellum. HAP2 gene-deficient mutants produce and excrete flagellin monomers into the surrounding media at a high rate (>1/s) (21). Release of flagellin also appears to occur in wild-type Salmonella, as shown by its purification from SD CM.

To test whether flagellin, independent of live bacteria, is capable of inducing the systemic inflammatory alterations characteristic of Gram-negative sepsis, C57BL/6 mice were challenged with 10 µg (400 µg/kg i.p.) of purified SD flagellin. Flagellin induced a prototypic inflammatory response, demonstrated by up-regulated serum concentrations of TNF-, IL-6, IL-12p40, MIP-1, IL-10, and nitrite/nitrate (Fig. 8). Similar results were obtained in BALB/c mice injected with recombinant S. muenchen flagellin (data not shown).

View larger version (31K): [in this window] [in a new window]   FIGURE 8. A—H, Flagellin induces the production of inflammatory mediators in vivo. A–F, C57BL/6 mice were treated with vehicle or 10 µg/mouse flagellin at time zero, and plasma TNF-, MIP-1, IL-6, IL-12p40, IL-10, and nitrate levels were measured at 0–24 h. G and H, Dose-dependency of the flagellin-induced inflammatory response (0.3–10 µg/mouse flagellin). Dose-responses were determined at 4 h, except for TNF- and MIP-1, where dose-responses were determined at 90 min postflagellin injection. There were four to six mice per time point or experimental group.

View larger version (143K): [in this window] [in a new window]   FIGURE 9. Systemic flagellin injection induces iNOS expression in the intestinal epithelium in mice. C57BL/6 mice were treated with vehicle or 10 µg/mouse flagellin for 24 h, followed by immunohistochemical staining for iNOS of intestinal samples as previously described (43 ). While no iNOS staining was localized in vehicle-treated control animals (upper panel), flagellin induced a massive expression of iNOS, which almost exclusively localized to the basal intestinal epithelial cells (lower panel). Magnification, x100. Immunohistochemical pictures shown are representative of four to six slides per group.

To demonstrate that flagellin induces hemodynamic instability characteristic of septic shock, endotoxin-responsive C3H/OuJ mice were injected i.v. with recombinant S. muenchen flagellin (10 mg/kg; i.v.; n = 10) or a saline vehicle control (n = 5). In response to a challenge of 10 mg/kg flagellin (i.e., 300 µg/mouse), the mean arterial pressure remained at baseline levels for 2 h, followed by severe hypotension, respiratory distress, cyanosis, and death between 2–4 h (Fig. 10). Saline-treated vehicle controls, in contrast, were normotensive and free of respiratory distress for the duration of the 4 h period of observation. Thoracic aortae from flagellin-treated mice demonstrated an ex vivo loss of vascular contractility, a classic feature of Gram-negative bacilli induced systemic inflammation and shock (Fig. 10). A potential confounding effect of endotoxin contamination was investigated by also testing the flagellin responses in the LPS-resistant C3H/HeJ mice. This latter strain of mice is resistant to the LPS effects because it lacks functional Toll-like receptor-4 (TLR-4) receptors (25). In agreement with previous studies, i.v. injection of E. coli LPS (10 mg/kg) in the C3H/OuJ mice caused a time-dependent fall in mean arterial blood pressure (e.g., from 102 ± 4 to 78 ± 3 mm Hg at 4 h; n = 6), whereas no significant drop in blood pressure was observed in the C3H/HeJ mice (mean arterial blood pressure at 0 and 4 h after LPS injection, 89 ± 5 and 86 ± 7 mm Hg, respectively; n = 4). However, i.v. flagellin injection (10 mg/kg) induced similar effects on blood pressure, vascular responsiveness, and mortality, in both the LPS-responsive (C3H/OuJ) and the LPS-resistant (C3H/HeJ) mice (Fig. 10), indicating that 1) the effect of flagellin was not mediated by LPS contamination, and 2) the hypotensive and shock-inducing effects of flagellin are not mediated by activation of the TLR-4 receptor. Reduction of the flagellin challenge to 1 mg/kg i.v. produced moderate progressive hypotension without mortality and significant ex vivo vascular hypocontractility at 6 h (data not shown).

View larger version (30K): [in this window] [in a new window]   FIGURE 10. Flagellin induces shock in mice. Anesthetized, 8-wk-old male C3H/OuJ (A–C and G–H) and LPS-resistant C3H/HeJ (D–F and I–J) mice were treated with recombinant S. muenchen flagellin (10 mg/kg i.v.) or saline vehicle control (0.2 ml). Treatment with 10 mg/kg flagellin produced severe hypotension within 3 h. Representative tracings are shown of vehicle-treated mice (A and D) and flagellin-treated mice demonstrating hypotension (B and E) and mortality (C and F). g, Flagellin induces progressive hypotension (n = 10) and mortality (7 of 10 animals at 4 h) in BALB/c mice compared with saline-treated controls (n = 5; *, p < 0.05). H, Flagellin induces progressive hypotension (n = 7) and mortality (four of seven animals at 4 h) in C3H/HeJ mice compared with saline-treated controls (n = 4; *, p < 0.05). Hypotension was associated with a severe reduction in the ex vivo contractility of thoracic aortic rings harvested at 220–240 min from mice surviving flagellin treatment (10 mg/kg i.v.). Flagellin induced hypocontractility in C3H/OuJ (I) and C3H/HeJ (J) mice compared with saline-treated controls (p < 0.05). In the vascular ring studies, four or five rings per group were used.

The proinflammatory and shock-inducing effects of flagellin suggested that free circulating flagellin might mediate some of the septic responses to Gram-negative infection. To establish that free flagellin circulates in the early phase of sepsis, rats were challenged with a lethal i.p. dose of S. marcescens (3 x 10⁸ CFU). Before infection, the blood was sterile (Fig. 11A), and circulating serum flagellin was undetectable (Fig. 11B). Four hours after challenge, rats became bacteremic (Fig. 11A), and the serum flagellin concentration increased to approximately 400 ng/ml (Fig. 11B). Rats became morbidly ill at 8 h, with a 50% mortality rate at 12 h. Parallel to these observations, the level of bacteremia and flagellemia increased sharply at 8 h postchallenge.

View larger version (26K): [in this window] [in a new window]   FIGURE 11. Free flagellin circulates in septic rats. Wistar rats were injected i.p. with S. marcescens (3 x 109 CFU/rat). A, Quantitative blood cultures were obtained at 4 and 8 h postinfection. B, Serum flagellin concentrations were determined at 4 and 8 h postinfection. Before infection, the blood was sterile, and circulating serum flagellin was undetectable. Four hours after challenge, rats became bacteremic, and the serum flagellin concentration was about 400 ng/ml. Rats became morbidly ill at 8 h, with a 50% rate of mortality at 12 h. In parallel to these observations, the level of bacteremia and flagellemia increased sharply at 8 h postchallenge. There were four animals per determination.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Flagellin is a 55-kDa monomer obtained from bacterial flagella, a polymeric rod-like appendage extending from the outer membrane of Gram-negative bacteria that propels the organism through its aqueous environment (26). In addition to their role in motility, flagella may also act as a virulence factor. Flagella aid bacteria in attaching to epithelial cells, assisting bacterial invasion (27). Flagellin-deficient mutants of P. mirabilis invade renal epithelial cells less efficiently and fail to induce pyelonephritis, unlike wild-type strains (28). Flagella may also play a key role in up-regulating IL-8 secretion in gastric epithelial cells stimulated by Helicobacter pylori (29).

It is generally accepted that LPS released from the bacterial cell wall is the trigger of the inflammatory response to Gram-negative pathogens (30). This conclusion is based on substantial data revealing that 1) parenteral administration of LPS produces a lethal shock state in experimental animals; 2) LPS can be measured in the circulation of the majority of patients with symptomatic Gram-negative infection; and 3) LPS induces proinflammatory responses in cultured cells. However, several lines of recent evidence suggest that LPS may not be the sole proinflammatory stimulus of clinical inflammation induced by motile enteric Gram-negative bacilli. First, incontrovertible differences exist between LPS-induced shock and bacterial sepsis. LPS does not faithfully reproduce the kinetics, magnitude, and distribution of proinflammatory gene expression typical of experimental models of live Gram-negative infection or clinical sepsis (31, 32). Second, the passive immunization of anti-LPS antisera has not increased survival from sepsis in pivotal clinical trials (33, 34). Increasingly, it is proposed that inflammatory injury and shock in Gram-negative infection may also be triggered by microbial stimuli other than LPS.

Our data suggest that flagellin, the subunit of bacterial flagella, may be an additional proinflammatory factor induced by motile Gram-negative bacilli. This hypothesis is supported by the following observations. 1) Flagellin is a potent stimulus of inflammation and shock in LPS-resistant mice. 2) Flagellin appears to act as an exotoxin; free flagellin is released by motile Gram-negative bacteria in vitro and appears in the blood of septic rats. The concentration of flagellin detected in vivo in septic rats was several orders of magnitude in excess of that required to induce NF-B activation and inflammatory mediator production in cultured cells in vitro. 3) Flagellin induces alterations in key proinflammatory signaling pathways and in the expression of free-radical generating enzymes. 4) Flagellin injection potently induces the expression of iNOS and proinflammatory cytokines in vivo and at higher doses induces a shock-like state, associated with hypotension, vascular dysfunction, and mortality. 5) Flagellated bacteria, purified flagellin, and medium conditioned by flagellated bacteria all readily induce IB degradation, NF-B activation, and iNOS expression in transformed human epithelial cells and murine macrophages. 6) Medium conditioned by a flagellin-deficient mutant has no effect on IB stability, NF-B activation, and iNOS expression. 7) Parenteral administration of medium conditioned by aflagellic mutants has no proinflammatory effect in LPS-resistant mice. 8) Polyclonal antiserum to flagellin eliminates the NO-inducing activity of medium conditioned by multiple motile Gram-negative bacillary pathogens.

The eukaryotic receptors responsible for flagellin-induced NF-B activation and proinflammatory gene expression remain to be identified. Based on the results of the study in the C3H/HeJ mice, TLR4 (a crucial receptor involved in LPS signaling) does not play a role in flagellin signaling. Recent data show that a broad variety of Gram-positive and Gram-negative bacterial proteins stimulate proinflammatory signaling pathways in IECs in a TL4-independent manner via binding to TLR2 (35, 36, 37, 38, 39, 40, 41). Studies in our laboratory are currently underway to assess the role of TLR2 in flagellin-induced NF-B degradation and iNOS expression in human cells.

The majority of infections in the critical care setting are produced by flagellated Gram-negative bacilli, such as E. coli, Pseudomonas aeruginosa, Enterobacter cloacae, S. marcesens, Campylobacter jejuni, Yersinia enterocolitica, Citrobacter freundii, and P. mirabilis. The relative contribution of flagellin to sepsis-induced shock and mortality induced by these organisms remains to be determined. Presumably, multiple virulence factors, in particular LPS, trigger the systemic proinflammatory host response to motile Gram-negative pathogens. It should be additionally noted that sepsis is readily induced by nonflagellated infectious species, in which flagellin clearly does not play a role, including Rickettsia, fungi, yeast, Babesia, Gram-positive bacteria, hemorrhagic viruses, P. falciparum, and Gram-negative diplococci and nonmotile Gram-negative bacilli.

Given its considerable potency and its probable release in the host during active infection, flagellin may be an important stimulus of in vivo inflammation and shock induced by motile Gram-negative enteric bacilli. However, the doses of flagellin needed to induce hypotension and shock were orders of magnitude higher than the doses of flagellin required to induce proinflammatory mediator expression. In this respect, flagellin behaves similar to LPS. Nevertheless, the causative role of flagellin in bacteremic shock remains to be clarified. The possibility that flagellin induces systemic inflammation and shock in synergy with LPS or other bacterial components must also be investigated in further studies. We hypothesize that differences in the rate of flagellin release at sites of infection might represent a clinically relevant virulence factor. It may also be expected that antibiotics might influence the rate of release of monomeric flagellin, akin to their well-established effect on LPS release. Further work must determine whether neutralization of flagellin represents a novel anti-inflammatory or anti-sepsis strategy.

While our current manuscript was in review, a related study appeared, identifying flagellin as a novel factor of enteroaggregative E. coli (EAEC)–induced epithelial cell activation (42). Similar to our findings, the soluble, heat-stable, IL-8-inducing factor released by these EAEC bacteria in culture was identified as flagellin. It was found that flagella purified from EAEC isolates potently induce IL-8 release from Caco-2 cells, while an engineered aflagellar mutant did not induce the release IL-8. Finally, it was found that cloned EAEC flagellin expressed in nonpathogenic E. coli as a polyhistidine-tagged fusion protein maintained its proinflammatory activity. These findings coupled with our present findings demonstrate that flagellin production and release may be a novel mechanism by which various bacteria induce intestinal and systemic inflammation. Our findings have obvious implications for diagnosis and vaccine development.

	Acknowledgments

 
We acknowledge Paul Hake (Children’s Hospital Medical Center, Cincinnati, OH) for assistance with in vivo studies, Dr. Carol Beach (University of Kentucky, Lexington. KY) for assistance with microsequence analysis, and Alvin Denenberg (Children’s Hospital Medical Center, Cincinnati, OH), Dr. Al Comb, and Dr. Kenneth Blumenthal (University of Cincinnati College of Medicine, Cincinnati, OH) for assistance with analytical separations. We thank Prof. Bruce Stocker (Department of Microbiology, Stanford University, Stanford, CA) for providing the aflagellic S. dublin mutant strains. Animal care was conducted in accordance with institutional guidelines at Children’s Hospital Medical Center (Cincinnati, OH) and Inotek Corp. (Beverly, MA).

	Footnotes

 
¹ This work was supported in part by National Institutes of Health Grant R01GM57407 and a grant from the American Heart Association (to A.L.S.), National Institutes of Health Grant R29GM54773 (to C.S.), a fellowship (to F.G.S.) from Fundaçao de Amparo à Pesquisa do Estado de Sao Paulo (Brazil). Part of this work represents a Ph.D. thesis by T.E.-P. in fulfillment of her graduate degree at the Department of Cell Biology, Neuroscience, and Anatomy, University of Cincinnati.

² On leave from the Critical Care Division, Department of Internal Medicine, University Hospital (Lausanne, Switzerland).

³ On leave from Department of Critical Care Medicine, Hospital das Clinicas da Universidade de Sao Paulo (Sao Paulo, Brazil).

⁴ Address correspondence and reprint requests to Dr. Andrew L. Salzman, Inotek Corporation, Suite 419E, 100 Cummings Center, Beverly, MA 01915.

⁵ Abbreviations used in this paper: iNOS, inducible NO synthase; IEC, intestinal epithelial cell; SD, Salmonella dublin; BHI, brain heart infusion broth; STE buffer, 10 mM Tris (pH 8), 50 mM NaCl, and 1 mM EDTA; MIP-1, macrophage inflammatory protein-1; CM, medium conditioned by SD; TLR, Toll-like receptor; NFDM, nonfat dry milk.

Received for publication April 20, 2000. Accepted for publication October 11, 2000.

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