Lack of a Role of Cytotoxic Necrotizing Factor 1 Toxin from Escherichia coli in Bacterial Pathogenicity and Host Cytokine Response in Infected Germfree Piglets

doi:10.1128/IAI.68.2.839-847.2000

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Infection and Immunity, February 2000, p. 839-847, Vol. 68, No. 2
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Lack of a Role of Cytotoxic Necrotizing Factor 1 Toxin from Escherichia coli in Bacterial Pathogenicity and Host Cytokine Response in Infected Germfree Piglets

S. Fournout,¹^,² C. M. Dozois,¹^, M. Odin,² C. Desautels,² S. Pérès,³ F. Hérault,³ F. Daigle,³^, C. Segafredo,¹ J. Laffitte,¹ E. Oswald,³ J. M. Fairbrother,² and I. P. Oswald¹^,^*

Laboratoire de Pharmacologie Toxicologie¹ and Laboratoire de Microbiologie Moléculaire Associé,³ Institut National de Recherche Agronomique, Toulouse, France, and GREMIP, Faculté de Médecine Vétérinaire, Saint-Hyacinthe, Québec, Canada²

Received 22 June 1999/Returned for modification 25 August 1999/Accepted 26 October 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Some Escherichia coli strains isolated from intestinal or extraintestinal infections in pigs produce cytotoxic necrotizingfactor 1 (CNF1). In order to analyze the role of CNF1 in the pathogenesisof porcine colibacillosis, newborn colostrum-deprived germfreepiglets were orally inoculated with a wild-type CNF1-producingstrain (M623) or with an isogenic cnf1 mutant (M623 $Delta$ CNF1). Thetwo isogenic strains induced a high mortality with similar lungand serosal inflammatory lesions, indicating that both strainswere pathogenic in these piglets. Bacterial counts in variousorgans of inoculated piglets revealed an intestinal predispositionof M623 and M623 $Delta$ CNF1 strains for the cecum and colon. Extraintestinalorgans (lungs, liver, spleen, and kidney) were also colonizedby both strains. Similar colonization of intestinal and extraintestinaltissues in animals inoculated with either strain was observed,except in the ileum, where M623 showed a higher colonization thanM623 $Delta$ CNF1. Intestinal (ileum and colon), extraintestinal (lungand kidney), and immune (mesenteric lymph nodes and spleen) tissueswere sampled at 1 day postinoculation and analyzed for cytokineexpression by a reverse transcriptase PCR technique. Inoculationwith E. coli M623 induced an enhanced expression of inflammatorycytokines (interleukin-1 $alpha$ [IL-1 $alpha$ ], tumor necrosis factor $alpha$ , andIL-12p40) in the intestinal organs compared to uninoculated pigletsor piglets inoculated with nonpathogenic intestinal E. coli 862B,which is also able to colonize the intestinal tract. There waslittle difference in cytokine transcript levels in the intestinaland extraintestinal organs in piglets inoculated with E. colistrains M623 or M623 $Delta$ CNF1, except in the ileum, where IL-1 $alpha$ andIL-8 mRNA levels correlated with bacterial colonization. Expressionof regulatory cytokines (gamma interferon and IL-4) was weak inimmune tissues from piglets inoculated with M623 or M623 $Delta$ CNF1.Taken together, our data indicate that the CNF1-producing strain,M623, is pathogenic and induces inflammatory cytokine expressionin germfree, colostrum-deprived piglets. Nevertheless, in thismodel, the CNF1 toxin does not appear to be a major factor forpathogenicity or cytokine response, as demonstrated by the useof an isogenic cnf1mutant.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Escherichia coli is a normal inhabitant of the intestinal tract but certain strains cause disease. Pathogenic E. coli belongto a restricted number of pathotypes defined by the presence ofvirulence factors which determine the host specificity and typeof disease produced by these pathotypes (43, 62). The virulencemechanisms of E. coli strains are complex and only partially understood.They include the ability to colonize mucosal surfaces, invadeextraintestinal tissues, survive and multiply in body fluids withlow concentrations of available iron (58), and escape phagocytosisand intracellular killing by phagocytes (46). E. coli strainsand/or their products modulate host cytokine responses (67).These cytokines, together with other inflammatory mediators areinvolved in the induction, persistence, or elimination of microbialinfection (29, 70).

The production of cytokines during bacterial infection has been extensively studied in human septic shock (50). In thismodel, the release of endotoxin-lipopolysaccharide (LPS) triggersthe synthesis of inflammatory cytokines such as tumor necrosisfactor (TNF), interleukin-1 (IL-1), and IL-6. These cytokinesinduce many changes which result in the failure of the major organsand rapid death of the patient (50). In addition to LPS, otherbacterial components have the capacity to induce cytokine production(for a review, see reference 72). Specific examples of pathogenicE. coli virulence factors that influence cytokine production includealpha-hemolysin, at nontoxic concentrations, which inhibits theproduction of TNF, IL-6, and IL-1 $beta$ by human peripheral blood cells(38); an as-yet-unknown protein from enteropathogenic E. coli(EPEC) that inhibits IL-2, IL-4, IL-5, and gamma interferon (IFN- $gamma$ )expression by peripheral and mucosal mononuclear cells (37,40); and Shiga-like toxin, which induces inflammatory cytokineproduction by murine macrophages (66). Adhesion to or invasionof epithelial cell monolayers by uropathogenic E. coli or EPECalso leads to the production of cytokines (19, 30, 59).Indeed, P fimbriae, which mediate attachment of uropathogenicE. coli to epithelial cells, enhance the host inflammatory responseto infection and increase virulence (10, 31). Similarly, EPECstimulate intestinal epithelial cell lines to produce IL-8 throughthe activation of NF- $kappa$ B (55).

Among the putative virulence factors produced by E. coli, cytotoxic necrotizing factors (CNFs) are produced by strains involvedin diarrhea and septicemia in humans and in domestic animals (4,6, 12). Necrotizing E. coli producing CNF1 have also beenisolated from piglets with diarrhea and with edema disease (27)and have been associated clinically with lesions of polyserositisand septicemia in young pigs (22). CNF toxins are lethal whenadministrated intravenously to mice or sheep and are dermatonecroticwhen inoculated into the rabbit skin (13-15). In addition, experimentaloral inoculation of neonatal calves and pigs has shown that CNF-positiveE. coli causes septicemia and enteritis (57, 73). S. Clément,B. Martineau-Doizé, I. P. Oswald, E. Oswald, M. Odin, and J.M. Fairbrother (submitted for publication) have also examinedthe dynamics of infection of CNF1-producing E. coli in experimentallyinoculated conventional piglets of various ages and immune orweaning states. They demonstrated that CNF1-producing E. colicolonizes predominantly the large intestine and disseminates tomesenteric lymph nodes and internal organs, particularly in colostrum-deprivedpiglets. CNF1 and CNF2 are 110- to 115-kDa monomeric toxins thatcovalently interact with Rho (24, 48), resulting in its activationthrough the deamidation of a glutamine residue (25, 56). Thisactivation of Rho GTPases results in polymerization of F actin,increased formation of stress fibers and multinucleation of cells(6, 23, 48). In addition to being implicated in the regulationof cytoskeletal structure, the Rho family of small GTP-bindingproteins is also involved in the gene transcription and activationof the NF- $kappa$ B (41). Since this nuclear transcription factor playsa major role in the transcriptional regulation of many acute phaseproteins and inflammatory cytokines (1, 2), we could anticipatethat CNF induces cytokinesynthesis.

Even if several lines of evidence implicate CNF1 and CNF2 in the pathogenesis of colibacillosis, their exact role still needsto be determined. Indeed, CNF1-producing E. coli strains oftenexpress other virulence factors (17, 34) and have also beenfound in the intestine of healthy piglets (27). Moreover, inactivationof the cnf1 gene in diarrhea-associated E. coli did not lead toa decrease in diarrhea and inflammation in a rabbit intestinalligated loop model (20).

In the present study, we orally inoculated germfree colostrum-deprived newborn piglets with either E. coli M623, a wild-typeCNF1-producing strain, an isogenic cnf1 derivative of M623, ora nonpathogenic E. coli strain. Our aim was to investigate thepathogenicity of a CNF1-producing strain in this model and toelucidate the role of CNF1 in bacterial pathogenicity and hostcytokine response. In addition, we analyzed in vivo cytokine levelsby reverse transcriptase PCR (RT-PCR) in the tissues of piglets.Herein, we demonstrated that M623 is pathogenic in germfree pigletsand induces an inflammatory cytokine response in intestinal organs.Nevertheless, there were few differences at the level of pathogenicity,colonization, and cytokine levels elicited by M623 or its isogeniccnf1 mutant M623 $Delta$ CNF1. Overall, our results suggest that CNF1is not essential for pathogenicity, nor does it greatly influencethe induction of host inflammatory cytokines by strain M623 inexperimentally inoculated germfreepiglets.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains, plasmids, and media. Bacterial strains and plasmids used throughout this study are summarized in Table 1. Wild-type E. coli 862B (O115:K $-$ ) isnonpathogenic and serum sensitive and was isolated from the intestinalcontents of a pig (21, 45). E. coli M623 (O2:K+), isolatedfrom the intestine of a pig with enteritis (C. Wray, Central VeterinaryLaboratory, Surrey, England) was used for inoculation studies.This strain is serum resistant and produces cytotoxin CNF1, alpha-hemolysin,and P and S fimbriae (17) but does not produce cytolethal distendingtoxin. Cosmid 2CO2 (also called cosmid 10) contains the cnf1 andhly gene clusters from uropathogenic strain E. coli J96 and waskindly supplied by D. E. Berg (64). Cloning vector pBluescriptKSII⁺ was obtained from Stratagene (La Jolla, Calif.) and cloning vectorpILL570 was kindly supplied by A. Labigne (39). Plasmid pKNG101is a positive selection suicide vector containing strAB, sacBRand a pir-dependent R6K replicon (35). Plasmids were maintainedin laboratory strain DH5 $alpha$ (54), except for suicide plasmids(pKNG101 and derivatives), which were maintained in SM10 $lambda$ pir (32).Bacteria were isolated on Luria-Bertani (LB) agar and culturedin LB broth. Prior to piglet inoculation, strains were grown intryptic soy broth (TSB). Media were supplemented with appropriateantibiotics at the following concentrations: ampicillin, 100 µg/ml;kanamycin, 50 µg/ml; streptomycin, 50 µg/ml; and spectinomycin,100 µg/ml.

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TABLE 1. Strains and plasmids

Recombinant DNA, genetic techniques, and nonpolar mutations in cnf1. Routine recombinant DNA techniques were performed by using standard procedures (54). A 13-kb EcoRI fragment from 2CO2 wascloned into pILL570. A 4.1-kb EcoRI/BamHI fragment bearing onlycnf1 was subcloned into pBluescript KSII⁺. The aphT gene devoid of its transcription terminator was retrievedfrom pSB315 (26) by BamHI restriction and cloned at the BglIIsite within cnf1. The ApaI fragment bearing cnf1 disrupted byaphT was cloned into pKNG101 vector, resulting in pKNGcnf::aphT.Suicide plasmid pKNGcnf::aphT was introduced into strain M623by conjugation. Mutants that had undergone allelic exchange leadingto the replacement of the wild-type locus with the locus disruptedby aphT were selected on LB plates without NaCl and containing5% sucrose and kanamycin, as previously described (35). Mutationswere confirmed by Southern blots and cytotoxic assay as previouslydescribed (15).

Experimental inoculation of piglets. Piglets were delivered from four specific-pathogen-free Yorkshire hybrid gilts by Caesarian delivery. Piglets were immediatelypassed through an iodine bath, placed in germfree isolators, andfed condensed milk ad libitum, as previously described (45).We confirmed the absence of bacteria in the feces of piglets inisolators prior to inoculation. At 2 days of age, piglets received10 ml of 1.2% NaHCO₃ through an intragastric tube to neutralizegastric acid. Piglets, chosen at random, were then similarly intubatedwith 1 ml of 0.9 to 2.1 × 10⁹ CFU in 19 ml of TSB of the wild-type parent strain M623 (n =12) or with its isogenic cnf1 derivative M623 $Delta$ CNF1 (n = 14) orwith the nonpathogenic strain 862B (n = 2). Piglets were examinedfor mortality for up to 7 days postinoculation. An additionalgroup of three uninoculated piglets served as controls for thedetermination of baseline cytokine mRNAlevels.

Necropsy procedure. Piglets were killed by an intracardiac injection of Euthanyl Forte (sodium pentobarbital at 540 mg/ml diluted in 0.20 ml ofpropylene glycol; Pharmacie, Faculté de Médecine Vétérinaire,Saint-Hyacinthe, Québec, Canada) at 1 or 7 days postinoculationor ifmoribund.

Tissues were sampled from the lung, liver, spleen, kidney, duodenum, jejunum, ileum, cecum, colon, and mesenteric lymph nodesdraining the corresponding jejunal and ileal segments of euthanizedanimals. These samples were consistently taken from the same areafrom respective organs in all animals. Lung samples were obtainedfrom nonconsolidated areas. Portions of each sample were usedimmediately for bacteriological and histopathological examination.Another portion of each tissue was frozen in 1 ml of Trizol (Gibco-BRL,Burlington, Ontario, Canada) for RNA extraction and analysis ofcytokine geneexpression.

Bacteriological counts. Tissues were evaluated quantitatively for the presence of E. coli. Samples were weighed and suspended in 2 ml of phosphate-bufferedsaline (PBS), homogenized at 5,000 rpm by using a Cat homogenizerx120 (PolyScience, Niles, Ill.), and 10-fold serially dilutedin sterile PBS. Dilutions were plated on tryptic soy agar forthe parental strain and on the same medium with kanamycin (50µg/ml) for the mutant strain by using a Spiral Plater System ModelC (Meyer Service and Supply Ltd., Long Sault, Ontario, Canada)as recommended by the manufacturer. After overnight incubationat 37°C, bacterial counts were determined. Several colonies fromeach individual were confirmed as being the infecting strain byPCR and agglutinationtests.

Histopathology. Tissue samples were fixed in 10% neutral buffered formalin, embedded in paraffin, sectioned at 6 µm, and stained with hematoxylinand phloxin saffron for examination by light microscopy. Bacteriallocalization in intestinal and extraintestinal tissues was determinedby immunocytochemistry. Sections were stained by Vector red (VectorLaboratories, Burlington, Ontario, Canada) as already described(52) by using rabbit polyclonal anti-O2 serogroup serum whichwas prepared as previously described (47).

RNA extraction. Samples from each organ, maintained in Trizol at $-$ 80°C, were homogenized by using a Cat homogenizer. Total RNA was extractedas recommended by the manufacturer. The RNA was resuspended in50 to 500 µl of ultrapure water containing 0.02% (wt/vol) diethylpyrocarbonate (Sigma, St. Quentin Fallavier, France) and 1 mMEDTA. Total RNA was quantified by using a spectrophotometer atan optical density of 260 nm (OD₂₆₀), and the purity was assessedby determining the OD₂₆₀/OD₂₈₀ ratio. All of the samples had anOD₂₆₀/OD₂₈₀ ratio above 1.8.

RT-PCR detection of cytokine mRNA and densitometric quantification of PCR products. An RT-PCR procedure was performed as previously described (18). Briefly, 1 µg of RNA was reverse transcribed (SuperscriptII RNase H; Life Technologies, Eragny, France) and then amplified (Taq DNApolymerase; Promega, Charbonnières, France). Primer sequencesand the number of PCR cycles chosen for each cytokine are listedin Table 2. Amplified DNA was analyzed after electrophoresison 1.2% TBE (Tris-borate-EDTA) agarose gels, which were stainedwith ethidium bromide and photographed with Polaroid 665 film.The level of each PCR product was quantified by densitometry byusing Image Aquisition and Whole Band Analyzer software (Bioimage)on a Sun Sparc Station 5 (Cadrus, Ramonville St-Agne, France)as previously described (18). To compare the relative cytokinemRNA expression levels among samples, the values are presentedas the ratio of the band intensity of the cytokine-specific RT-PCRproduct over that of the corresponding constitutively expressed"housekeeping" gene, cyclophilin.

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TABLE 2. Oligonucleotides designed in this study to specifically detect porcine cytokine and cyclophilin cDNA

Statistical analysis. Student's t test and/or analysis of variance were used to analyze bacterial counts and cytokine production. P values of <0.05were considered significant. Macroscopic lesions were analyzedby use of the $chi$ ² test. $chi$ ² values of <3.84 were not consideredsignificant.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Pathogenicity of E. coli M623 in piglets. We first investigated the pathogenicity of E. coli M623 in germfree, colostrum-deprived piglets inoculated by the oral route.Of 12 piglets, 2 demonstrated respiratory distress and died suddenlyat less than 12 h postinoculation. At 24 h postinoculation, sixinoculated piglets were randomly chosen and euthanized for necropsy;of the four remaining piglets, only one survived up to 7 dayspostinoculation. Table 3 summarizes the macroscopic lesions notedin the 10 piglets necropsied after death or after euthanasia.Most of the piglets inoculated with M623 demonstrated congestionof the lung, and half of these piglets presented intestinal congestion.Fluid and fibrin were observed in the thoracic, pericardial, and/orperitoneal cavities of all piglets examined at more than 24 hpostinoculation but rarely in piglets examined at 24 h postinoculation.Microscopically, changes in piglets examined at 24 h postinoculationwere minimal, the most important being inflammatory changes inthe lung. These changes were characterized by a multifocal septalleukocytic infiltration composed of a mixed population of neutrophilsand mononuclear cells and by an occasional fibrinous to leukocyticalveolitis. Bronchioalveolar necrosis was observed in one piglet(Table 4). Of note, no significant lesions were observed in uninoculatedcontrols or piglets inoculated with strain 862B (data not shown).

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TABLE 3. Macroscopic lesions in germfree piglets inoculated with isogenic E. coli strains expressing or not expressing CNF1 toxin

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TABLE 4. Microscopic findings in germfree piglets inoculated with isogenic E. coli strains expressing or not expressing CNF1 toxin and then euthanized 24 h postinoculation

We examined the ability of strain M623 to colonize intestinal and extraintestinal organs as demonstrated by bacterial countsin different tissues of the piglets euthanized at 24 h postinoculation.At this time, M623 colonized the intestinal tract, mostly thelarge intestine and to a lesser extent the small intestine (Table5). Bacteria had translocated to the mesenteric lymph nodes anddisseminated to the lungs, liver, spleen, and kidney. Bacteriapersisted in all organs until 7 days postinoculation. As alreadydescribed (45), the control nonpathogenic strain 862B, whichdid not induce death in piglets, also colonized the intestinesand was recovered from the mesenteric lymph nodes and extraintestinalorgans at levels similar to strain M623 at 24 h postinoculation.This strain colonized the intestines and was recovered from themesenteric lymph nodes but not from other extraintestinal organsat 7 days postinoculation (data not shown).

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TABLE 5. Quantitative bacterial counts in tissues of piglets necropsied at 1 day postinoculation with E. coli M623 and M623 $Delta$ CNF1

Bacterial distribution in tissues was assessed by immunocytochemistry by using Vector red (52). In the digestive tract,most bacteria were found on the luminal aspect, occasionally inclose contact with the mucosa. Bacterial colonization was alsoobserved in the serosa and to a lesser extent in the submucosa.Bacteria were also found extraintestinally in the mesenteric lymphnodes (Fig. 1A), lung (Fig. 1B), kidneys, and, when present, themesentery. In the lung, bacteria were found in the interlobularand alveolar septa, lining the alveoli or within the alveolarlumen, associated with macrophages. Renal colonization was characterizedby the presence of O2-positive rods in the interstitium and occasionallyin the tubular lumen. Bacteria were scattered throughout the mesentery.

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FIG. 1. In situ visualization of bacteria in tissues by immunohistochemistry with an anti-O2 serum by Vector red staining. Piglets were inoculated with M623 and were euthanized 24 h postinoculation. (A) Clusters of bacteria are found extracellularly close to the hilus of mesenteric lymph node (arrow). Bar, 25 µm. (B) Bacteria are observed along the pulmonary epithelium (arrow facing right) and are occasionally found in the alveolar lumen, associated or not with alveolar macrophages (arrow facing left). A focal septal leukocytic infiltration composed of a mixed population of neutrophils and mononuclear cells can be seen (arrowhead). Bar, 10 µm.

Role of cnf1 on these effects. In order to understand the role of CNF1 in pig colibacillosis, a derivative of strain M623 unable to produce CNF1 (M623 $Delta$ CNF1)was constructed by allelic exchange. As expected, bacterial lysatesfrom M623 $Delta$ CNF1 did not induce stress fibers and multinucleationin cultured HeLa cells, in contrast to lysates obtained from thewild-type M623 strain (data notshown).

We then examined the pathogenicity of the cnf1 mutant in orally inoculated piglets. Of 14 inoculated piglets, 3 demonstratedsevere respiratory distress and died at between 14 and 24 h postinoculation.At 24 h postinoculation, seven piglets inoculated with M623 $Delta$ CNF1were randomly chosen and euthanized for necropsy. Overall, strainM623 $Delta$ CNF1 tended to be slightly less pathogenic than M623. Twoof four piglets inoculated with M623 $Delta$ CNF1 survived for up to 7days postinoculation compared to only one of four piglets inoculatedwith M623. Piglets inoculated with either strain demonstratedsimilar macroscopic lesions on necropsy at 24 h postinoculation(Table 3). However, pulmonary inflammatory changes were observedsignificantly (P = 0.05) more often in piglets inoculated withstrain M623 than in those inoculated with the CNF1 mutant at 24h postinoculation (Table 4). The bronchioalveolar necrosis, althoughonly observed in one M623 inoculated piglet, was not observedat all in piglets inoculated with the CNF1 mutant. Finally, thoracic,pericardial, and/or peritoneal fluid and fibrin were observedmore frequently in piglets inoculated with M623 than in thoseinoculated with the CNF1 mutant, at 36 h or more following inoculation(Table 3).

M623 $Delta$ CNF1 colonized the examined tissues, except for the ileum, to the same extent as strain M623 (Table 5). Indeed, aboutfive times more CFU per gram were recovered from the ileum ofpiglets inoculated with strain M623 than from piglets inoculatedwith strain M623 $Delta$ CNF1. Bacteria persisted in all organs until7 days postinoculation, and no difference in bacterial persistencewas observed for the surviving piglets belonging to either theM623 $Delta$ CNF1 or M623 inoculated groups (data notshown).

E. coli M623 and M623 $Delta$ CNF1 induce an enhanced production of inflammatory cytokines in the intestine. The ability of E. coli M623 and M623 $Delta$ CNF1 to induce inflammatory cytokines such as IL-1 $alpha$ , IL-6, IL-8, IL-12p40, and TNF- $alpha$ at the transcriptional level was then compared in piglets necropsiedat 24 h postinoculation. Cytokine mRNA expression was measuredby semiquantitative RT-PCR in samples from various organs. Sincepiglets were inoculated by the oral route, we first investigatedthe mRNA expression of inflammatory cytokines in the small intestine(ileum) and in the large intestine (colon). In the ileum, IL-1 $alpha$ ,TNF- $alpha$ , and IL-12p40 mRNA levels were significantly higher in pigletsinoculated with M623 than in control piglets (Fig. 2). On theother hand, IL-8 mRNA production was only slightly higher in theileum of M623-inoculated piglets than in uninoculated controls.In the colon, IL-1 $alpha$ and TNF- $alpha$ mRNA levels for M623-inoculatedpiglets were significantly greater than for control piglets, whereasIL-12p40 mRNA production was only weakly enhanced. IL-8 mRNA wasnot detected in the colon of any of the piglets. The expressionof IL-6 was not detected in the two intestinal organs investigated.Expression of the different cytokines by a piglet inoculated withthe strain 862B was similar to that observed in uninoculated piglets,except in the case of IL-1 $alpha$ in the colon (Fig. 2).

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FIG. 2. Inflammatory cytokine production in intestinal samples from inoculated piglets. Piglets were inoculated with M623 (wild type [WT]) or with its isogenic cnf derivative (M623 $Delta$ CNF1) (CNF $-$ ) and were euthanized 1 day postinoculation. Untreated piglets were used as controls (Cont.). Tissues from the ileum and colon were sampled and homogenized. Total RNA was then isolated and assayed for expression of inflammatory cytokine (IL-1 $alpha$ , TNF- $alpha$ , IL-12p40, and IL-8) and the cyclophilin housekeeping genes by RT-PCR. Quantification of these cytokine mRNAs from the ileum and the colon in different animals (closed triangles) and the mean (± the standard error of the mean [SEM]) of these results for each group are shown (vertical bars). Opened triangles in the controls represent the values of piglets inoculated with nonpathogenic strain 862B. Student's t tests were performed to compare M623-inoculated piglets with control ones or M623 $Delta$ CNF1-inoculated animals. *, P < 0.05; **, P < 0.01.

When cytokine mRNA expression was compared in intestinal samples from M623- and M623 $Delta$ CNF1-inoculated piglets, a higher expressionwas observed in animals inoculated with the wild-type strain (Fig.2). However, these differences were only significant for IL-1 $alpha$ and IL-8 in the ileum. Cytokine expression was also assayed intwo extraintestinal organs: the lungs and kidney. No significantdifferences were observed between animals inoculated with eitherM623 or M623 $Delta$ CNF1 except for an increase in TNF- $alpha$ expression inthe lungs of piglets inoculated with M623 $Delta$ CNF1 (Table 6).

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TABLE 6. Cytokine mRNA levels in the lungs and the kidney of infected piglets

Expression of Th1 and Th2 cytokines by M623 and M623 $Delta$ CNF1. In order to determine whether the immune response elicited by M623 and M623 $Delta$ CNF1 was of the Th1 or Th2 type, we examined theproduction of a Th1 (IFN- $gamma$ ) and a Th2 (IL-4) cytokine, by RT-PCR,in two immune organs (the spleen and the intestinal lymph nodes).As we only observed a weak production of these cytokines, probablydue to the immaturity of the immune system of the piglets, wedetermined the frequency of detection of these two cytokines fromcontrols and from piglets inoculated with M623 or M623 $Delta$ CNF1 (Fig.3). Control animals did not express these two cytokines in theirintestinal lymph nodes. In inoculated animals, IFN- $gamma$ was not expressedin the spleen and was expressed in only a low proportion of thelymph nodes. By contrast, IL-4 was expressed in a much higherproportion (up to 100%) of spleen and intestinal lymph node samplesfrom inoculated animals, suggesting that these piglets displaya Th2 response.

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FIG. 3. Regulatory cytokine gene expression in immune organs from inoculated piglets. IL-4 and IFN- $gamma$ mRNA production by spleen and intestinal lymph nodes from uninoculated controls (Cont.,

) or from M623 (M623,

)- and M623 $Delta$ CNF1 (CNF $-$ ,

)-inoculated piglets. Frequencies of detection of IL-4 and IFN- $gamma$ mRNAs are expressed as the percentage of positive samples observed by RT-PCR assays. Student's t tests were performed to compare M623-inoculated piglets with control ones or with M623 $Delta$ CNF1-inoculated animals. *, P < 0.05; ND, not done.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In this study, we demonstrated the pathogenicity of the CNF1-producing E. coli strain M623 in colostrum-deprived germfreepiglets. This strain induced pulmonary interstitial and exudativeinflammation and subsequently typical lesions of polyserositiswhich are observed in natural cases of E. coli septicemia in thepig (22, 46). E. coli isolates from such cases are often CNF1positive. Rapid death (>24 h postinoculation) was observed intwo piglets inoculated with the CNF1-producing E. coli strainand three piglets inoculated with the CNF1 mutant. These pigletsdemonstrated nonspecific lesions of pulmonary and intestinal congestionmacroscopically, which may have been due to endotoxic shock ratherthan to trauma or injury due to the inoculation, since no evidenceof inoculum aspiration was observed during the removal of thestomach tube and this phenomenon has not been observed in pigletssimilarly inoculated with other septicemic or nonpathogenic E.coli (45). Only one piglet examined at 24 h postinoculationwith M623 demonstrated a pulmonary lesion, i.e., bronchoalveolarnecrosis, which could have been related to the inoculation procedurewith secondary aspiration of remaining bacteria during extubation.The bacteria not present at the site of inflammation may havealready been eliminated by the inflammation. Hence we feel that,in general, this route was not a contributing factor in bacterialcolonization of thelung.

Strain M623 colonizes intestinal and extraintestinal organs from at least 1 day postinoculation and persists up to 7 dayspostinoculation (Table 5). The colonization is predominantlyin the intestine and particularly in the cecum and colon. Theseresults are in agreement with the fact that the gastrointestinaltract would act as a reservoir for bacteria that can cause extraintestinalinfections (63). Bacteria probably pass through the epithelialcells lining the intestines and are carried in the lymph to themesenteric lymph node and possibly to the systemic complex (3),allowing bacterial establishment in extraintestinal organs. Ofnote, as already demonstrated (45), the nonpathogenic strain862B was also able to colonize the intestine and to translocateinto the mesenteric lymph nodes in colostrum-deprived germfreepiglets. However, this strain did not persist in other extraintestinalorgans nor did it induce any lesions or mortality. Hence, strainM623 possesses additional virulence attributes which may not berequired for translocation from the intestine but which permitbacteria to persist and induce lesions in extraintestinal sites,at least in this model. In conventional, 2-day-old colostrum-deprivedpiglets (S. Clément, submitted), we also found that M623 wasable to translocate to the draining lymph nodes and to the extraintestinalorgans. However, in this model the strain did not induce any lesionsor mortality. The difference in the pathogenesis observed in thetwo cases is probably due to the absence of intestinal barrierin germfree piglets. Indeed, newborn germfree piglets lack theability to transfer maternal regulatory factors, both antigensand immunoglobulins, which have been shown to inhibit bacterialadherence to receptors on the intestinal epithelial cells andto neutralize the activity of the cytotoxins produced by E. coli(68). Using other CNF1-producing strains and higher doses ofbacteria, Wray et al. (73) observed bacterial colonization ofthe intestine and extraintestinal organs, diarrhea, and respiratorysigns in inoculated piglets, although clinical signs appearedto vary widely depending on the bacterial strain used and evenwithin a group of animals given the samestrain.

Several studies have investigated the action of CNF toxin in vitro. Based on these studies, the effect of CNF appears to bevery different depending on the model used. For example, CNF1increases intestinal permeability in Caco-2 cells (28), whereasit does not affect tight junction permeability in T84 monolayer(33). Similarly, this toxin induced a phagocytic behavior inhuman epithelial HEp-2 cells (23) but downmodulated integrinactivation-dependent phagocytosis in human monocytes (5). Inaddition, CNF1 does not seem to have any effect on the abilityof hemolytic E. coli to damage human bladder cell monolayers invitro (34), but CNF1 effaced cell microvilli and decreased transepithelialmigration of polymorphonuclear leukocytes on polarized T84 epithelialintestinal cell monolayers (33).

In the present study we investigated the in vivo role of CNF1 in the pathogenicity of colibacillosis. CNF1-positive E. coliare associated clinically with lesions of polyserositis and septicemiain young pigs (22). Initial experiments carried out in conventionalpiglets of different ages (10-day-old weaned or unweaned and 2-day-oldcolostrum fed or colostrum deprived) in an attempt to reproducethese lesions were not able to demonstrate any pathogenicity forE. coli M623 (Clément et al., submitted). Indeed, even in thepresence of bacterial colonization of the intestine and disseminationto mesenteric lymph nodes and internal organs, we did not observeany mortality or significant lesions. Hence, we chose the moresensitive colostrum-deprived, germfree piglet, with which we havehad considerable experience in the study of the pathogenesis ofporcine E. coli septicemia (45), as our model for the studyof the pathogenesis of M623 infection. We constructed a CNF1-isogenicmutant of a wild-type pathogenic E. coli strain, and we orallyinoculated germfree neonatal piglets with either the M623 parentalstrain or the M623 $Delta$ CNF1 mutant strain. We hypothesized that inactivationof cnf1 would decrease the ability of E. coli to colonize theintestine and/or to translocate to and cause lesions in internalorgans in swine. However, inactivation of cnf1 did not reducethe pathogenicity of the wild-type M623 strain except for a weakercolonization of the ileum (Table 5), a slight decrease in mortality,and a slight decrease in inflammatory response in the lungs andserosal surfaces. Our results confirm and extend those of Elliotet al. (20), who used CNF1 mutants in a rabbit model of intestinalligated loops and did not observe a significant effect on theonset, duration, or severity ofdiarrhea.

The inability to find significant differences in the pathogenicity of the M623 and the M623 $Delta$ CNF1 can be interpreted in severaldifferent ways. First, CNF1 may play no role in bacterial pathogenicityand the fact that CNF-positive strains are pathogenic may resultsolely from a genetic linkage of the cnf1 gene with other virulencefactors genes, such as those encoding alpha-hemolysin (hly) andP-related adhesin (prs) located on the same pathogenicity islandon strain J96 (64) as well as strain M623 (E. Oswald, unpublisheddata). Second, our germfree piglet model may be insufficientlysensitive for the detection of the effect of CNF1. Moxley et al.found that inactivation of hemolysin did not reduce the incidenceof septicemia in gnotobiotic piglets inoculated with isogenicenterotoxigenic E. coli strains after oral inoculation (42).Similarly, expression of heat-stable enterotoxin STb by adherentE. coli is not sufficient to cause severe diarrhea in neonatalpigs (7). Finally, other virulence factors may obscure theeffects of CNF1. Indeed, strain M623 produces P and S fimbriaeand hemolysin, which may contribute to the development of infection(17). In light of the results presented here, we tend to favorthe last two hypotheses. Indeed, necrotoxigenic E. coli strainscould be considered as pathogens of an opportunistic nature (Clémentet al., submitted), and we have demonstrated that in vitro CNFpotentiates the effect of another toxin, CDT (S. Pérès, F. Daigle,N. Ghichemerre, O. Marchés, F. Hérault, J. De Rycke, and E.Oswald, submitted for publication). Thus, using another infectiousmodel, such as an immunocompromised piglet and/or E. coli strainsthat express other virulence factors, we would expect to increasethe slight differences observed in the present study between isogenicstrains expressing or not CNF1 toxin, in terms of mortality, inflammatorylesions, and cytokineresponse.

Cytokines are important in the regulation of the immune response and in the control of inflammation, but they can also contributeto immunopathological changes in the host after bacterial infection.In the current study, we investigated the cytokine response inboth the intestinal tract and the immune tissues. In the spleenand intestinal draining lymph nodes, we particularly investigatedthe Th1-Th2 balance by measuring IFN- $gamma$ and IL-4. These two cytokineswere weakly expressed, probably due to the age of the animalswhose lymphoid organs were not totally developed. However, ininoculated animals the higher frequency of IL-4 mRNA detectionin the lymphoid organs compared to that of IFN- $gamma$ argue in favorof a Th2 response following E. coli inoculation. This is in agreementwith the shift toward the Th2-cell-type response observed in volunteersgiven a low dose of E. coli endotoxin (74) and may reflect thefact that E. coli, as do other extracellular bacteria, stimulatesa stronger humoral than cellular immuneresponse.

We also determined the cytokine response in intestinal tissues from control animals and from piglets inoculated with M623,M623 $Delta$ CNF1, or 862B strains. In contrast to control uninoculatedor 862B inoculated animals, piglets inoculated with M623 or M623 $Delta$ CNF1strains produced increased levels of mRNA encoding for inflammatorycytokines in their intestinal tract. Bacterial LPS did not seemto trigger this local synthesis of cytokines since strain 862B,which colonizes the intestine to the same extent as the two otherstrains, did not induce any inflammatory response in the ileumor in the colon (Fig. 2). Inoculation with either of the pathogenicstrains M623 and M623 $Delta$ CNF1 induces an inflammatory response inthe intestinal tract, as measured by the production of IL-1 $alpha$ andTNF- $alpha$ (Fig. 2). These cytokines play a major role in the courseof bacterial infection and in sepsis (16), and local inductionof these inflammatory cytokines has been detected in murine modelsof pyelonephritis (36, 53) and epididymitis (65) inducedby E. coli. Recombinant IL-1 and TNF have also been shown to increasethe colonization of EPEC in the rabbit small bowel (71). Thus,the local induction of these inflammatory cytokines during oralinoculation by pathogenic E. coli may create a microenvironmentthat facilitates their own colonization of the intestine. Surprisingly,we did not find any increase in IL-6 and IL-8 mRNA levels in theintestine of inoculated piglets, although these cytokines havebeen detected in clinical patients or in experimental animalsinoculated with E. coli (11, 61).

Similar responses were observed in piglets inoculated with either M623 or M623 $Delta$ CNF1 E. coli strains, except in the ileum whereanimals inoculated with the mutant strain displayed lower inflammatorycytokine transcript levels than animals inoculated with the parentalstrain (Fig. 2). In the ileum, the bacterial colonization alsodiffered between the two groups of animals (Table 5). We believethat the lower cytokine production reflects the lower bacterialcolonization of this organ and is not directly related to a putativeeffect of CNF1 on NF- $kappa$ B (1, 2). This hypothesis is substantiatedby the observation of Capo and coworkers (5), who did not findany specific inflammatory cytokine production in macrophages stimulatedby purified CNF1 toxin. However, we cannot exclude an alternativeexplanation, i.e., that higher levels of IL-1 and TNF- $alpha$ expressionin M623-inoculated piglets compared to M623 $Delta$ CNF1-inoculated onescould facilitate bacterial colonization of the wild-type E. colistrain, as has already been demonstrated for EPEC (71).

Possible sources of the inflammatory cytokines induced by M623 strains include macrophages (9, 44), as well as dendriticcells (8, 69), and epithelial cells (19, 30, 60). Thelatter cells which line the intestine are continuously in contactwith bacteria and their products and are known to play an activerole in the mucosal immune system (19, 30). Of note, mostof the inflammatory cytokine mRNAs that we investigated were detectedby RT-PCR, although at low levels, in samples from control piglets(Fig. 2). This has been described in other studies and may reflectthe dynamic nature of immune regulation even in the absence ofmicrobial invasion (49, 51).

In conclusion, our results showed that the CNF1-producing strain M623 is pathogenic in germfree piglets and specifically inducesthe production of inflammatory cytokines. The CNF1 toxin doesnot seem to be the essential factor of virulence since the isogenicmutant is alsopathogenic.

	ACKNOWLEDGMENTS

Sylvie Fournout and Charles M. Dozois were supported by the Natural Sciences and Engineering Research Council (NSERC) of Canadagrant GPG0181728 and by an INRA postdoctoral fellowship, respectively.This work was supported in part by NSERC of Canada grant GPG0181728,by a grant from the European Community program FAIR (number 1335),and by programme prioritaire "Génomes et Fonctions" (INRA)grant.

	FOOTNOTES

^* Corresponding author. Mailing address: Laboratoire de Pharmacologie Toxicologie, INRA, 180 Chemin de Tournefeuille, 31931Toulouse Cedex 9, France. Phone: 33 (0) 561285480. Fax: 33 (0)561285310. E-mail: ioswald{at}toulouse.inra.fr.

Present address: Department of Biology, Washington University, Saint Louis, MO63130.

Editor: P. E. Orndorff

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