Inoculum Composition and Salmonella Pathogenicity Island 1 Regulate M-Cell Invasion and Epithelial Destruction by Salmonella typhimurium

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Infect Immun, February 1998, p. 724-731, Vol. 66, No. 2
0019-9567/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Inoculum Composition and Salmonella Pathogenicity Island 1 Regulate M-Cell Invasion and Epithelial Destruction by Salmonella typhimurium

M. Ann Clark,¹^,^* Barry H. Hirst,¹ and Mark A. Jepson²

Department of Physiological Sciences, Medical School, University of Newcastle upon Tyne, Newcastle upon Tyne NE2 4HH,¹ and Cell Imaging Facility and Department of Biochemistry, School of Medical Sciences, University of Bristol, Bristol BS8 1TD,² United Kingdom

Received 13 May 1997/Returned for modification 19 June 1997/Accepted 20 November 1997

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

In the mouse model of Salmonella typhimurium infection, the specialized antigen-sampling intestinal M cells are the primaryroute of Salmonella invasion during the early stages of infection.Under certain experimental conditions, M-cell invasion is accompaniedby M-cell destruction and loss of adjacent regions of the follicle-associatedepithelium (FAE), although the conditions responsible for expressionof the cytotoxic phenotype in a proportion of previous studieshave not been defined. In the present study, we have demonstratedthat the cytotoxic effect exerted by wild-type S. typhimuriumon mouse Peyer's patch FAE is dependent on the inoculum composition.We have also demonstrated that the extent of FAE destruction correlateswith the extent of M-cell invasion. Bacteria inoculated in Luria-Bertani(LB) broth induce extensive FAE loss and exhibit efficient M-cellinvasion, whereas bacteria inoculated in phosphate-buffered salinefail to induce significant FAE disruption and invade M cells atsignificantly lower levels. Similarly, inoculation in LB significantlyenhances invasion of Madin-Darby canine kidney cells by wild-typeS. typhimurium. Mutants defective for expression of invA, a componentof Salmonella pathogenicity island 1 which is vital for efficientinvasion of cultured cells, fail to induce FAE destruction and,when inoculated in LB, are attenuated for M-cell invasion. Variationin inv gene expression is, therefore, one possible mechanism bywhich inoculate composition may regulate the virulence of wild-typeS. typhimurium. Our findings suggest that the composition of thegut luminal contents may be critical in determining the outcomeof naturally acquired Salmonella infections and that both vaccineformulation and dietary status of vaccine recipients may significantlyaffect the efficacy and safety of live Salmonella oral vaccinedelivery systems.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Salmonella species are an important group of pathogens which infect a wide range of hosts to cause a variety of disease syndromes.One feature common to all of these disease syndromes is that followingoral ingestion, the bacterium must penetrate the intestinal epithelialbarrier prior to the initiation of disease. The mechanisms bywhich Salmonella invade the intestinal epithelium are unclear,although in vitro studies have identified several genes whichare required to optimize S. typhimurium invasion of epithelialcells. Many of these genes are located in Salmonella pathogenicityisland 1 (SPI1), located at centisome 63 on the Salmonella typhimuriumchromosome. These genes encode a type III protein secretion systemtogether with several of its target proteins (for a review, seereference 16). In vitro studies have demonstrated that invasionof cultured cells by Salmonella species is modulated by a varietyof environmental and growth conditions, including oxygen tension,osmolarity, carbohydrate availability, and bacterial growth phase(13, 24, 27, 35-37). Environmental modulation of in vitroinvasion is achieved by the regulation of SPI1-encoded invasiongene expression via a complex array of transcription factors (1,2, 21, 25, 32) which are thought to ensure that invasiongene expression and consequently epithelial invasion by S. typhimuriumare maximal under conditions present in the gut lumen.

The primary sites of Salmonella invasion in the host intestine are the ileal Peyer's patches and possibly also the cecal lymphoidpatches (4). The follicle-associated epithelium (FAE) whichoverlies these gut-associated lymphoid tissues includes the specializedantigen-sampling M cells which are a major site of invasion bya diverse range of pathogens (14, 19, 28). Recent studiessuggest that M cells play a pivotal role in the pathogenesis ofS. typhimurium since, at least during the early stages of infection,these cells are the primary site of S. typhimurium invasion inthe mouse intestine (7, 22). The role of the SPI1-encodedgenes in M-cell invasion is unclear, although recently we havedemonstrated that strains carrying mutations in the inv genesof SPI1 are severely attenuated for invasion of cultured cellsbut retain the capacity to invade mouse M cells (8).

The interaction of S. typhimurium with intestinal M cells induces the formation of prominent membrane protrusions termed membraneruffles (7, 8, 22). In addition, under certain experimentalconditions, wild-type strains of S. typhimurium induce M-celldestruction and extensive sloughing of adjacent areas of FAE (3,10, 22, 31, 33). The factors regulating the cytotoxicityof S. typhimurium have not been identified, although it is notablethat previous studies have used markedly different experimentalprotocols (3, 7, 8, 10, 22, 31, 33).

The aim of this study was to test the hypothesis that the phenomenon of M-cell cytotoxicity is dependent on the compositionof the S. typhimurium inoculate. In addition, we have investigatedthe role of the inv genetic locus in Salmonella-induced cytotoxicity.Our results demonstrate that inoculate composition determinesthe extent of both M-cell invasion and the capacity to induceepithelial disruption. While S. typhimurium invades M cells byboth inv-dependent and inv-independent mechanisms, mutants defectivefor invA are unable to cause epithelial disruption and, underconditions which promote invasion and FAE destruction by the wildtype, are attenuated for M-cell invasion. These findings suggestthat variation in expression of SPI1-encoded invasion genes isone possible mechanism by which inoculate composition may regulateM-cell invasion and FAE destruction by wild-type S. typhimurium.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Bacterial strains and culture. Wild-type S. typhimurium strains IR715 and SR11 and mutant strain SB111 (an isogenic nonpolar invA mutant of SR11 [30])were prepared as previously described (7, 8). Briefly, asingle colony grown on Luria-Bertani (LB) agar was inoculatedinto 2 ml of LB broth and incubated with agitation at 37°C for7 h. From this starter culture, 10³ bacteria were inoculated into 5 ml of LB broth (in a 6-ml vial)and grown as a static culture overnight (16 h) at 37°C. Alternatively,to obtain stationary-phase bacteria grown under nutrient-limitingconditions, 10³ bacteria were inoculated into 5 ml of LB broth in a 30-ml vialand shaken vigorously overnight at 37°C. To determine the effectof inoculum composition, the bacteria were then pelleted and resuspendedthree times in either the original LB growth broth, phosphate-bufferedsaline, pH 7.4 (PBS), or PBS supplemented with 0.14 M mannitol,5 g of yeast extract per liter, or 10 g of tryptone per liter.In the remaining studies, bacteria were used directly in the LBgrowth broth, without pelleting and resuspension.

Mouse gut loop studies. Ligated jejunal/ileal Peyer's patch-containing gut segments were created in anesthetized adult female BALB/c mice as describedpreviously (7, 8) and infected with the bacterial (3 × 10⁹ bacteria/ml) or control preparations. After an appropriate incubationperiod, the mice were culled by cervical dislocation and the gutloops were rapidly removed. Harvested tissues were pinned flat,mucosal surface uppermost, on cork boards, rinsed thoroughly inPBS, and fixed in either 2% glutaraldehyde (in 100 mM sodium phosphatebuffer, pH 7.3) at 4°C or methanol ( $-$ 20°C) for at least 2 h. Tofacilitate subsequent examination of the FAE, villi were thenmicrodissected away from the domes.

Glutaraldehyde-fixed tissues which had been infected, unless otherwise stated, for 60 min were processed for scanning electronmicroscopy (SEM) as described previously (6) and examined witha Cambridge S240 SEM. All tissues were examined blind, and theextent of FAE destruction on each dome was assigned a score of0 to 4, where 0 denotes negligible damage (loss of <20 singlecells or <4 small cell clusters), 1 denotes low levels of damage(loss of $>=$ 20 single cells or $>=$ 4 but <10 small cell clusters),2 denotes moderate damage (loss of $>=$ 10 small cell clusters or $>=$ 5 large cell clusters), 3 denotes extensive damage (loss of $>=$ 1/6FAE), and 4 denotes very extensive damage (loss of $>=$ 1/2 FAE),small and large cell clusters being defined as areas equivalentto >4 but <10 cells and $>=$ 10 cells, respectively.

Methanol-fixed tissues infected for 15 min were processed for immunocytochemical localization of bacteria by staining withanti-Salmonella antibodies and fluorescein isothiocyanate (FITC)-conjugatedsecondary antibodies (7). M cells were localized by immersionfor 60 min in tetramethylrhodamine isothiocyanate (TRITC)-conjugatedUlex europaeus agglutinin 1 (UEA1; 67 µg/ml; Vector Laboratories,Peterborough, United Kingdom), a marker of mouse Peyer's patchM cells (6). The stained tissues were mounted in Vectashieldmounting medium (Vector Laboratories) and examined with a Bio-RadMRC-600 confocal laser scanning microscope (CLSM) equipped witha krypton-argon mixed-gas laser. S. typhimurium association withthe FAE was quantified by analyzing the z series of confocal opticalsections of randomly selected areas of FAE from four discretepredetermined peripheral regions of infected Peyer's patch domes.M-cell-associated bacteria were classified as adhered or invaded,invaded bacteria being defined as those at least 2 µm below thestrongly UEA1-stained M-cell surface. Areas where the FAE wasobscured (e.g., by mucus) were excluded from analysis.

In vitro studies. The effect of inoculum composition on invasion of cultured epithelial cells by wild-type S. typhimurium was also examined.S. typhimurium IR715 was grown as described above and then pelletedand resuspended three times in fresh LB or PBS. After dilutionin LB or PBS to a concentration of approximately 10⁸/ml, the bacterial preparations were added to Madin-Darby caninekidney (MDCK) strain I cells cultured on permeable supports (Anocell;0.5 cm²; Nunc, Roskilde, Denmark) as described previously (20). After15 min of incubation at 37°C, the cell monolayers were washedsix times in PBS to remove nonadherent bacteria and transferredto PBS at 0°C to prevent further invasion. S. typhimurium adhesionand invasion was then quantified by differential immunocytochemicalstaining as described previously (20). Briefly, the monolayerswere incubated sequentially (at 0°C) with goat anti-Salmonellaantibodies and FITC-conjugated rabbit anti-goat immunoglobulinto label extracellular bacteria. After permeabilization in methanol,the monolayers were incubated with anti-Salmonella antibodiesand TRITC-conjugated rabbit anti-goat immunoglobulin at room temperatureto label extracellular and intracellular bacteria. Monolayerswere then examined with a Leica DM RBE epifluorescence microscope.Counts of adherent (FITC-labeled) and total (TRITC-labeled) bacteriaassociated with the monolayers were made in 10 randomly selectedfields (ca. 5,000 µm² per field) and used to calculate both the numbers of adheredand invaded bacteria per unit area.

Statistical analyses. The extent of FAE destruction (as defined by dome score values) induced by alternative inocula was initially analyzed by aKruskal-Wallis test, which revealed that FAE damage was significantlyaffected by the composition of the gut loop inoculum. Data obtainedfor pairs of alternative inocula were subsequently analyzed byDunn's multiple-comparison tests. Statistical analyses of S. typhimuriumassociation (adhesion and invasion, as defined by CLSM) with FAEcells in vivo and MDCK cells in vitro were performed by Mann-WhitneyU tests. For all statistical tests, P values of <0.05 were consideredsignificant; for direct comparisons of alternative inocula, thedata analyzed were obtained from experiments performed on thesame day and using the same batch of mice.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Effect of inoculum composition. (i) FAE destruction. SEM examination of tissues infected for 60 min with wild-type S. typhimurium strain IR715 resuspended in PBS revealed thepresence of M-cell-associated ruffles but little evidence of M-cellcytotoxicity or FAE loss (Fig. 1a and b). In contrast, S. typhimuriumresuspended in the original LB growth broth induced extensiveFAE damage (Fig. 1c to f) typically characterized by areas ofcell loss which were surrounded by cells denuded of microvilliand associated with the presence of invading bacteria (Fig. 1eand f). The areas of cell loss varied in size from single cells(presumably M cells) and small cell clusters to large areas ofFAE which were frequently scattered around the periphery of thedomes, a location which corresponds to the sites of maximum M-cellexpression (Fig. 1d). Very extensive areas of FAE representingover half of the dome surface were lost from a proportion (15%[16 of 109]) of infected domes (Fig. 1c).

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FIG. 1. SEM images of mouse Peyer's patch tissues infected for 60 min with wild-type S. typhimurium strain IR715 resuspended in PBS (a and b) or LB (c to f). (a and b) Bacteria in PBS fail to exert a cytotoxic effect. Shown are whole dome (a) and localized area of a dome surface (b), both with an intact FAE. M cells in panel b either display a normal microvillous morphology (M) or possess membrane ruffles (arrow). (c to f) Destruction of FAE by bacteria resuspended in LB. (c and d) Whole domes, with loss of extensive areas of FAE in panel c (arrows) and loss of localized, peripheral regions of FAE in panel d (arrows). (e) Localized region of FAE showing relatively unaffected areas interspersed by damaged regions (arrows). (f) High-power view of FAE, depicting an area of FAE loss (lower left), an intermediate zone of cells denuded of microvilli (arrows), and a relatively unaffected region (upper mid-right). Bacteria are visible in the damaged areas. Bars: a, c, and d, 100 µm; b and f, 10 µm; e, 20 µm.

The dome score values obtained by SEM examination of 13 Peyer's patches from six mice infected with IR715 in LB and 12 Peyer'spatches from six mice infected with IR715 in PBS (mean dome scores= 2.2 and 0.7, respectively [Table 1]) were analyzed by Dunn'smultiple-comparison tests. These analyses revealed that inoculumcomposition significantly (P < 0.001) affects the capacity ofS. typhimurium to exert a cytotoxic effect on mouse Peyer's patchFAE following 60 min of incubation in gut loops. At this timepoint, bacteria in PBS induced minor damage to the FAE, as indicatedby the mean dome score values (0.7 for bacteria in PBS and 0.1for control PBS [Table 1]), although this damage was not statisticallysignificant (P > 0.05). In contrast, bacteria in LB induced extensiveFAE damage which was significantly greater (P < 0.001) than thatassociated with the control inoculum LB (mean dome scores = 2.2and 0.04, respectively [Table 1]). Time course studies revealedthat bacteria in LB fail to induce significant FAE destructionafter only 15 min of incubation in mouse gut loops (mean domescore = 0.2) but that damage is significant (P < 0.001) after30 min and becomes increasingly extensive after longer incubationperiods (mean dome scores = 1.9, 2.2, and 3.2 after 30, 60, and120 min of incubation, respectively). After 60 min of infectionin LB, bacteria grown to stationary phase under nutrient-limitingconditions induced FAE damage comparable to that induced by bacteriagrown under our standard protocol where bacteria were grown instatic, closed tubes (mean dome scores = 3.2 and 3.0, respectively).

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TABLE 1. Effects of inoculum composition and the invA gene on FAE destruction by S. typhimurium after 60 min of infection of mouse Peyer's patch gut loops

The induction of cytotoxicity by bacteria resuspended in the original LB growth broth was dependent on the simultaneous presenceof bacteria and LB broth and was independent of inoculum componentswhich had accumulated in the LB broth during prolonged bacterialgrowth, since FAE destruction was absent from tissues incubatedwith filtered bacterial growth broth (mean dome score = 0.1 [Table1]) and bacteria resuspended in fresh LB induced FAE destructioncomparable to that induced by bacteria resuspended in the originalLB growth broth (mean dome scores = 1.9 and 2.2, respectively).Salmonella-induced cytotoxicity was also independent of the pelletingand resuspension of bacteria during inoculum preparation, sinceIR715 prepared with or without three phases of pelleting and resuspensionin the original LB growth broth induced similar levels of FAEdamage (mean dome scores = 2.2 and 2.1, respectively).

To determine whether the relatively high osmolarity of LB (424 mosmol/liter) relative to that of PBS (292 mosmol/liter) mightbe solely responsible for the observed effect of inoculum compositionon Salmonella-induced cytotoxicity, bacteria were resuspendedin PBS supplemented with 0.14 M mannitol (440 mosmol/liter) andincubated for 60 min in mouse gut loops. SEM examination of infectedtissues revealed that raising the osmolarity of PBS failed toenhance Salmonella-induced FAE cell cytotoxicity (mean dome score= 0.8, compared to 0.7 for bacteria in unsupplemented PBS [Table1]). In contrast, supplementation of PBS with either yeast extractor tryptone at concentrations equivalent to those in LB was sufficientto increase Salmonella-induced FAE cell cytotoxicity (mean domescores = 2.8 and 2.7, respectively [Table 1]) to that observedfollowing bacterial inoculation in LB, whereas FAE damage wasabsent from control tissues incubated with PBS supplemented witheither yeast extract or tryptone (mean dome scores = 0, [Table1]).

(ii) M-cell invasion. To determine whether S. typhimurium invasion of the FAE was also influenced by inoculate composition we examined tissues incubatedwith bacteria for only 15 min, since at this earlier time point,even bacteria suspended in LB failed to induce significant FAEcell damage, and quantification at later time points is of littlevalue since invasion is obscured by the onset of Salmonella-inducedcytotoxicity. Tissues dual stained to localize bacteria and Mcells were examined by CLSM; as previously described (7, 8),in all tissues examined, the vast majority of FAE-associated bacteriawere associated with the M cells. Our dual-staining techniquepermitted discrimination between M-cell-adherent and M-cell-invadedbacteria (Fig. 2), since the M-cell marker UEA1 strongly stainsthe apical surface of M cells (Fig. 2a), and consequently theposition of bacteria relative to the M-cell surface can be readilyidentified by examination of the z series of confocal opticalsections. Localization of M-cell-internalized bacteria was furtherassisted by very much weaker, diffuse UEA1 staining of the M-cellcytoplasm (Fig. 2c). Cumulated data from four Peyer's patchesinfected with IR715 in LB (total area FAE = 2.5 × 10⁵ µm²) and five Peyer's patches infected with IR715 in PBS (total areaFAE = 2.4 × 10⁵ µm²) revealed that S. typhimurium invasion of M cells was significantlygreater (P < 0.05) when inoculated in LB (3.45 ± 1.35 bacteriaper 1,000 µm²; mean ± standard error of the mean [SE]) than when inoculatedin PBS (0.07 ± 0.06 bacteria per 1,000 µm²; mean ± SE), demonstrating that invasion of M cells is enhancedby exposure to LB. Inoculate composition had a less dramatic effecton bacterial adhesion, although S. typhimurium adherence to Mcells was still significantly greater (P < 0.05) when inoculatedin LB (9.68 ± 1.07 bacteria per 1,000 µm²; mean ± SE) than when inoculated in PBS (1.14 ± 0.12 bacteriaper 1,000 µm²; mean ± SE). The observed increase in bacterial adherence (8-fold)associated with inoculation in LB may be a contributory factorto the increase in invasion (49-fold) but cannot be the sole factorinvolved.

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FIG. 2. CLSM images of mouse Peyer's patch FAE infected for 15 min with wild-type S. typhimurium strain IR715 suspended in LB and dually stained for M cells (a and c) and bacteria (b and d). (a and b) Surface views. Adhesion of three bacteria to the surface of an M-cell is accompanied by redistribution of M-cell surface UEA1 staining (a, arrow). (c and d) Images at 6-µm depth. A bacterium (d) has invaded an M cell (c, arrow); localization of bacteria within the M cell is facilitated by weak UEA1 staining of the M-cell cytoplasm. Bar = 5 µm.

(iii) Invasion of cultured epithelial cells. Following a 15-min infection with S. typhimurium IR715, invasion of MDCK cells was significantly greater (P < 0.0001) whenthe bacteria were inoculated in LB (2.14 ± 0.58 bacteria per 1,000µm²; mean ± SE; n = 12) than in PBS (0.14 ± 0.05 bacteria per 1,000µm²; mean ± SE; n = 12), demonstrating that inoculum compositionhas an effect in vitro similar to that observed in vivo. Inoculumcomposition had a much smaller effect on bacterial adhesion toMDCK cells, although adhesion was also significantly greater (P< 0.05) when bacteria were inoculated in LB (0.61 ± 0.12 bacteriaper 1,000 µm²; mean ± SE; n = 12) than in PBS (0.22 ± 0.06 bacteria per 1,000µm²; mean ± SE; n = 12). In common with the results obtained in vivo,the observed increase in bacterial adhesion (3-fold) can be onlya minor contributory factor in the observed increase in bacterialinvasion (15-fold) associated with inoculation in LB.

Effect of mutation in the invA gene. (i) FAE destruction. In common with IR715, infection of mouse gut loops for 60 min with the alternative wild-type strain SR11 suspended in PBSfailed to induce FAE destruction (8), whereas infection withSR11 suspended in LB resulted in extensive FAE destruction (Fig.3a and b) similar to that observed for IR715 (Fig. 1c to f). Incontrast, while infection with the invA mutant SB111 induced M-cellruffles, M-cell destruction and FAE loss were virtually absent(Fig. 3c and d) even after bacterial inoculation in LB. Statisticalanalyses of the dome score values obtained from 9 Peyer's patchesin three mice infected with SR11 and 15 Peyer's patches in sevenmice infected with SB111 (mean dome scores = 2.4 and 0.1, respectively[Table 1]) confirmed that, when bacteria are inoculated in LB,mutation in invA significantly (P < 0.001) attenuates Salmonella-inducedFAE cell cytotoxicity. The invA mutant SB111 failed to induceFAE damage beyond that associated with the control inoculum LB(mean dome scores = 0.1 and 0.04, respectively [Table 1]), incontrast to the wild-type strain SR11, which induced significantFAE damage (P < 0.001).

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FIG. 3. SEM images of mouse Peyer's patch tissues infected for 60 min with wild-type S. typhimurium strain SR11 (a and b) or its isogenic invA mutant SB111 (c and d), both suspended in LB. (a and b) Destruction of FAE by SR11. (a) Whole dome, showing peripheral regions of destruction (arrows); (b) localized region of FAE, depicting an area of FAE destruction (arrows) characterized by cell loss, microvillous denudation and the presence of associated bacteria, and a relatively unaffected area of FAE (upper region). (c and d) The invA mutant SB111 fails to exert a cytotoxic effect. Shown are whole dome (c) and localized area of a dome surface, both with an intact FAE. In panel d, the FAE is composed of enterocytes, a goblet cell (G), and M cells displaying a normal microvillous morphology (M) or surface membrane ruffles (arrows). Bars: a and c, 100 µm; b and d, 10 µm.

(ii) M-cell invasion. CLSM analysis of dually stained FAE from seven Peyer's patches infected for 15 min with SR11 (total area FAE = 8.4 × 10⁵ µm²) and six Peyer's patches infected with SB111 (total area FAE= 5.5 × 10⁵ µm²) revealed that significantly more (P < 0.05) wild-type SR11 (1.73± 5.51 bacteria per 1,000 µm²; mean ± SE) than invA mutant SB111 (0.15 ± 0.07 bacteria per1,000 µm²; mean ± SE) bacteria invaded M cells demonstrating that underthese inoculum conditions, the invA mutation attenuates M-cellinvasion. The invA mutation also induced a small, but not statisticallysignificant, attenuation of M-cell adhesion (P = 0.0734), thelevel of M-cell adhesion by the parental wild-type strain SR11being 4.10 ± 0.97 bacteria per 1,000 µm² (mean ± SE) compared with 1.37 ± 0.42 bacteria per 1,000 µm² (mean ± SE) for the invA mutant SB111.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

We have demonstrated that the capacity of wild-type strains of S. typhimurium to induce M-cell damage and FAE disruption inthe mouse gut loop model of infection is dependent on the inoculumcomposition. This observation accounts for the divergent resultspreviously obtained following S. typhimurium infection of mousegut loops. After a 60-min infection period, extensive FAE destructionis induced by bacteria suspended in bacterial growth broth (22,31, 33) and is absent if the bacteria are suspended in PBS(7, 8, 10). The S. typhimurium-induced FAE damage observedby us in the present study and by others in previous studies (3,22, 31, 33) was similar to the Peyer's patch ulcerationsinduced by S. typhi in human typhoid fever (29), an observationwhich further validates the mouse model of S. typhimurium infectionas a model of human typhoid. Interestingly, there is some evidencethat S. typhi also induces M-cell destruction following incubationin mouse Peyer's patch gut loops (23), although it is unclearwhether this damage equates to the lesions associated with S.typhimurium infection (31).

Our results also demonstrate that in addition to regulating FAE destruction, inoculum composition determines the extent ofM (and MDCK) cell invasion by S. typhimurium. Efficient M-cellinvasion correlates with the induction of cytotoxicity, whichsuggests that M-cell invasion and Salmonella-induced cytotoxicityare closely related events. Daniels et al. (10) demonstratedthat bacteria in PBS induce extensive FAE destruction only afterprolonged incubation periods (180 min) in mouse gut loops. Togetherwith our data, this observation suggests that Salmonella-inducedcytotoxicity is delayed by bacterial inoculation in PBS as a consequenceof the observed decrease in bacterial invasion or, alternatively,that bacteria in PBS fail to express the destructive phenotypeand require growth conditions present within the tissues to stimulateexpression of the appropriate genes. Although we found no evidencein the present study that cytotoxicity and invasion are separatelyregulated, this possibility cannot be excluded, particularly sincerecent evidence suggests that M-cell destruction, but not invasion,is linked to expression of slyA (10).

We have demonstrated that M-cell invasion can proceed via both inv-dependent (this study) and inv-independent (reference 8and this study) routes. In our previous study using bacteria suspendedin PBS (8), the extents of invasion by wild-type and invA mutantstrains appeared to be similar, although the possibility thatthe invA mutation can cause a small attenuation in invasion couldnot be excluded since quantification was impractical due to variableand relatively low numbers of bacteria which invaded under theseinoculum conditions. In the present study, bacterial suspensionin LB increased invasion by wild-type bacteria, thereby facilitatingquantification, and we were able to demonstrate that under thesealternative inoculum conditions, inv-dependent invasion is moreefficient than inv-independent invasion. Since it is now clearthat when inoculated in LB, an intact invA gene is essential forefficient M-cell invasion, we must now qualify our previous observationthat mutation in SPI1 has no apparent effect on M-cell invasion(8) to include only those bacteria inoculated in PBS.

In the present study, when inoculated in LB, the invA mutant was attenuated for M-cell invasion by ca. 12-fold, a figure whichis less than that observed for this and other invA mutants incultured cells (100- to 500-fold [8, 17]) but is consistentwith the observations that invA mutants exhibit increased 50%lethal dose values and decreased Peyer's patch colonization followingoral inoculation of mice but still readily kill infected animals(17). Assuming that M-cell invasion is the major route of intestinalinvasion by invA mutants (as indicated by our gut loop studies),the latter observation clearly demonstrates that the inv-independentroute of M-cell invasion is of clinical significance. Since wild-typebacteria in PBS exhibited levels of M-cell invasion similar tothose exhibited by the invA mutant, we propose that the low levelsof M-cell invasion associated with bacterial inoculation in PBSmay similarly be sufficient to cause disease. This observationmay be relevant to the real-life situation, since similarly lowlevels of bacterial invasion may occur in unhealthy individualswhose diet is largely restricted to fluids. Our observation thatinvasion by the inv-independent route is unaccompanied by FAEdestruction is consistent with the failure of other groups todetect FAE destruction by inv mutants (22, 33), although atthis stage it is unclear whether failure of inv mutants to induceFAE destruction is solely a result of insufficient bacterial invasion,or whether SPI1-encoded proteins have an additional role in thedestructive process. Some previous studies have failed to demonstrateM-cell invasion by SPI1 mutants (22, 33), a result which isinconsistent either with our observations (reference 8 andthis study) or the relatively modest increase in oral 50% lethaldose values associated with these mutations (17, 33). We suggestthat given the uneven distribution of FAE-associated bacteria(7, 19), the low levels of M-cell invasion exhibited by SPI1mutants which we have identified by CLSM examination of largeareas of FAE may be overlooked in studies which have used transmissionelectron microscopy to examine relatively small samples of M cells.

The mechanisms by which bacterial inoculation in LB enhances invasion and FAE destruction by wild-type S. typhimurium areunclear. It is unlikely that the observed phenomena are a consequenceof variations in media pH or oxygen tension, since LB and PBShave similar pH values and the bacterial inocula were preparedin identical fashions to eliminate variations in oxygen tension.Our experiments with high-osmolarity PBS also demonstrate thatthe effect of LB on S. typhimurium virulence is not solely a consequenceof medium osmolarity. In combination with the observation thataddition of either yeast extract or tryptone to PBS raises thelevels of Salmonella-induced FAE cell cytotoxicity to those associatedwith bacterial suspension in LB, these findings suggest that theobserved increase in S. typhimurium virulence associated withbacterial inoculation in LB may be a consequence of componentspresent in all these media. The possible effect of inoculate compositionon Salmonella virulence could be mediated nonspecifically by effectson bacterial growth phase or by more subtle effects on the physiologicalstatus of the bacteria, although during our experiments we attemptedto minimize the effects of variations in bacterial growth phaseby using bacteria derived from overnight cultures at high concentrationin the test inocula. In addition, we demonstrated that bacteriagrown to stationary phase under nutrient-limiting conditions stillreadily induce FAE destruction when inoculated in LB. These datasuggest that FAE invasion and destruction are regulated by oneor more components of LB which are not exhausted by growth tostationary phase. Addition of tryptone or yeast extract to PBShad effects on FAE destruction similar to those of bacterial inoculationin LB, suggesting that amino acid supply may be critical to thedestruction process. This proposal is consistent with the observationthat Salmonella invasion in vitro is reduced by prolonged inhibitionof bacterial protein synthesis, as is likely to occur in bacteriasuspended in PBS (26). It is possible that enhanced motilityof bacteria suspended in LB relative to those in PBS (unpublishedobservation) contributed to the increase in bacterial adhesionobserved both in vitro and in vivo following inoculation in LB,although other factors may also have affected bacterial adherence.It is clear, however, that variations in bacterial adherence werenot alone sufficient to account for the observed effects of inoculumcomposition on bacterial invasion, and additional factors musthave contributed to the effect of inoculum composition on S. typhimuriumvirulence.

It is possible that inoculum composition modifies S. typhimurium virulence by regulating the expression of Salmonella-encodedgenes which control invasion and bacterium-induced FAE destruction.This hypothesis is consistent with previous studies which havedemonstrated that in vitro expression of the SPI1-encoded invasiongenes (including inv) and, consequently, S. typhimurium invasionof epithelial cell lines are regulated by a variety of environmentaland growth conditions, including growth phase, oxygen tension,osmolarity, and pH, via a complex group of transcription factors(1, 2, 5, 18, 21, 25, 32). The complexity ofthis system is emphasized by the observation that invasion geneexpression is regulated in a coordinate manner and is dramaticallyrepressed if only a single factor is suboptimal (2). In thisstudy, we have demonstrated that the inv genetic locus is essentialboth for efficient M-cell invasion when bacteria are suspendedin LB and for Salmonella-induced FAE destruction. From these results,it is tempting to speculate that the observed increase in M-cellinvasion and FAE destruction by wild-type S. typhimurium associatedwith inoculation in LB may be a consequence of enhanced inv geneexpression in this medium. It is clear that further studies arerequired to identify the medium components responsible for theobserved effects of inoculum composition on Salmonella virulenceand to characterize the mechanisms involved.

Our finding that S. typhimurium invasion and cytotoxicity are regulated by inoculum composition suggests that experimentsdesigned to identify the genetic basis of Salmonella invasionand epithelial destruction must be interpreted with caution, sinceboth the inoculum composition and dietary intake of the experimentalanimals may affect the observed bacterial virulence. While ourstudies have so far been restricted to the mouse gut loop modelof infection, intragastric infection of mice with wild-type S.typhimurium similarly results in M cell destruction and FAE loss(3, 10), and it may therefore be hypothesized that inoculumcomposition and the nutritional state of the animal also influencethe outcome of orally acquired Salmonella infections. Since anyFAE loss is likely to result in extensive invasion by this andother gut luminal microorganisms, our observations suggest thatthe composition of the gut luminal contents (which is in turnaffected by the foodstuffs ingested) is crucial for determiningthe outcome of naturally acquired Salmonella infections. To furtherinvestigate the possible effects of dietary intake on the outcomeof Salmonella infection in the naturally infected host, futureexperiments should be based on conditions which more closely mimicthe natural situation (i.e., oral infection of bacteria in feedstuffsor water) and the effects of inoculum size, feedstuff composition,and gastric and intestinal environments on Salmonella virulencein both healthy and diseased individuals should be determined.Interestingly, in addition to the clinical syndromes which mayresult from the acute stages of S. typhimurium-induced M-celldestruction and FAE loss, it has been proposed that uncontrolledpenetration of microorganisms and nutritional macromolecules throughdamaged areas of intestinal epithelium may also result in chronicdisease syndromes due to the excessive stimulation of antigen-presentingcells and activation of potentially damaging inflammatory reactions(9, 11). These pathogenic mechanisms may account for theobservations that lymphoid follicle ulceration is an early featureof Crohn's disease (15, 34) and that M-cell degeneration ispresent in a proportion of patients suffering from spondylarthropathy(9). The possible role of M-cell destruction in these diseaseprocesses awaits further investigation.

In recent years there has been much interest in the use of attenuated Salmonella strains as carriers of heterologous antigensin oral vaccine delivery systems (reviewed in reference 12).Our observations that inoculum composition significantly affectsthe virulence of S. typhimurium have important implications forthe design of Salmonella-based vaccines, since they suggest thatvaccine formulation and intestinal contents of the vaccine recipientmay have significant effects on both vaccine efficacy and safety.Live Salmonella-based vaccines should clearly be designed suchthat intestinal epithelial invasion is sufficient to ensure effectiveimmunization but that bacterial invasion occurs in the absenceof significant damage to the FAE. Identification of the molecularmechanisms responsible for intestinal invasion and FAE destructionby Salmonella species must now be priority areas for research.

	ACKNOWLEDGMENTS

We thank A. J. Bäumler for providing S. typhimurium IR715 and J. E. Galán for providing strains SR11 and SB111. We alsothank T. A. Booth, Biomedical Electron Microscopy Unit, Universityof Newcastle upon Tyne, for assistance with scanning electronmicroscopy.

This work was supported by Wellcome Trust Veterinary Research Fellowship 041573/Z/94/Z awarded to M.A.C. Additional supportwas supplied by Royal Society equipment grant 17996 to M.A.J.The School of Medical Sciences Cell Imaging Facility, Universityof Bristol, is supported by Medical Research Council InfrastructureAward G4500006.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Physiological Sciences, Medical School, University of Newcastle uponTyne, Newcastle upon Tyne NE2 4HH, United Kingdom. Phone: 44 191222 7772. Fax: 44 191 222 6706. E-mail: Ann.Clark{at}newcastle.ac.uk.

Editor: P. J. Sansonetti

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