Role of NleH, a Type III Secreted Effector from Attaching and Effacing Pathogens, in Colonization of the Bovine, Ovine, and Murine Gut

ABSTRACT The human pathogen enterohemorrhagic Escherichia coli (EHEC) O157:H7 colonizes human and animal gut via formation of attaching and effacing lesions. EHEC strains use a type III secretion system to translocate a battery of effector proteins into the mammalian host cell, which subvert diverse signal transduction pathways implicated in actin dynamics, phagocytosis, and innate immunity. The genomes of sequenced EHEC O157:H7 strains contain two copies of the effector protein gene nleH, which share 49% sequence similarity with the gene for the Shigella effector OspG, recently implicated in inhibition of migration of the transcriptional regulator NF-κB to the nucleus. In this study we investigated the role of NleH during EHEC O157:H7 infection of calves and lambs. We found that while EHEC ΔnleH colonized the bovine gut more efficiently than the wild-type strain, in lambs the wild-type strain exhibited a competitive advantage over the mutant during mixed infection. Using the mouse pathogen Citrobacter rodentium, which shares many virulence factors with EHEC O157:H7, including NleH, we observed that the wild-type strain exhibited a competitive advantage over the mutant during mixed infection. We found no measurable differences in T-cell infiltration or hyperplasia in colons of mice inoculated with the wild-type or the nleH mutant strain. Using NF-κB reporter mice carrying a transgene containing a luciferase reporter driven by three NF-κB response elements, we found that NleH causes an increase in NF-κB activity in the colonic mucosa. Consistent with this, we found that the nleH mutant triggered a significantly lower tumor necrosis factor alpha response than the wild-type strain.

The human diarrheal pathogens enteropathogenic Escherichia coli (EPEC) and enterohemorrhagic E. coli (EHEC) (31) and the murine pathogen Citrobacter rodentium (reviewed in reference 28) colonize the host gastrointestinal tract via attaching and effacing (A/E) lesions, which are characterized by intimate adhesion to intestinal epithelia and localized effacement of brush border microvilli (21). EPEC was the first type of E. coli to be associated with human disease and is a major cause of infantile diarrhea in developing countries (reviewed in reference 2), while EHEC (O157 and non-O157 strains) is prevalent in developed countries and causes a wide spectrum of illnesses ranging from mild diarrhea to severe diseases such as hemorrhagic colitis and hemolytic uremic syndrome mediated by Shiga toxins (31).
EPEC, EHEC, and C. rodentium harbor the locus of enterocyte effacement (LEE) pathogenicity island, which is necessary for A/E lesion formation in vivo (26). The LEE encodes several gene regulators, the outer membrane adhesin intimin (18), the structural components of a type III secretion system (T3SS) (17), chaperones, and translocator and several effector proteins, including Tir (19), Map, EspG, EspF, and EspH (reviewed in reference 12), that are injected into enterocytes via the T3SS and differentially modulate cellular actin dynamics in vitro.
EHEC infection in humans frequently results from direct or indirect contact with ruminant feces; however, the molecular mechanisms underlying colonization of reservoir hosts are ill defined. The LEE-carried genes required for A/E lesion formation (e.g., those for Tir and intimin) play pivotal roles in colonization of such hosts by EHEC O157:H7 (4,7,37), and structural components of the T3SS were found by signaturetagged mutagenesis to be required for colonization of calves by EHEC O157:H7 and O26:HϪ (9,36). In addition to Tir, EspK has been shown to influence colonization of the bovine intestine (38), while Map (9), TccP/EspF U (37), and NleD (25) had no measurable effect. The roles of other T3SS effectors in colonization of ruminants are not known.
C. rodentium is a natural mouse pathogen that, while causing colonic hyperplasia, shares many virulence factors with EPEC and EHEC (reviewed in reference 28). Following inoculation via the oral route, bacteria colonize the colon, typically peaking at day 9 before clearance at around day 17 (27). Recently we refined the C. rodentium mouse model by developing noninvasive real-time bioluminescence imaging (BLI) to monitor infection dynamics and tissue tropism in vivo (41). Using this method, we have shown that C. rodentium first targets the murine cecal patch and rectum before the infection spreads to the large intestine.
The genome sequences of EHEC O157:H7 strains EDL933 and Sakai, EPEC strain E2348/69, and C. rodentium strain ICC168 revealed that EHEC and EPEC contain two nleH alleles (34; A. Iguchi et al., unpublished data), while C. rodentium harbors only one nleH gene. NleH shares 49% sequence similarity with the Shigella flexneri T3SS serine/threonine kinase effector protein OspG, which prevents ubiquitination and subsequent degradation of phospho-IB␣ and downstream activation of the transcriptional factor NF-B, possibly via the phosphorylation of the E3 ubiquitin ligase SCF ␤-TrCP (Skp-Cullin-F box protein) complex (20). NF-B proteins are transcriptional factors that, when activated, control the transcription of a large number of genes, many of which are involved in the immune (inflammatory) response. The similarities between NleH and OspG prompted us to investigate its role in colonization and activation of the NF-B pathway in vivo.
The PCR product of the resistance cassette, flanked by approximately 50 bp of nleH, was digested with DpnI and the cassette electroporated into the recipient strains carrying pKD46, encoding the Red recombinase. Mutants were selected on selective LB plates with kanamycin or chloramphenicol. Recombinant clones were cured of pKD46 and the mutation confirmed by PCR using primers flanking nleH and primers within the antibiotic resistance gene. Growth curves have confirmed that the mutant and wild-type stains have identical growth rates in LB and minimal media. Mutations of the nleH1 and nleH2 genes created using the same method in EPEC strains were successfully complemented in trans during in vitro studies.
Oral inoculation of calves. All animal experiments were performed in accordance with the Animals (Scientific Procedures) Act 1986 and were approved by the local Ethical Review Committee. Groups of four 12-day-old Friesian bull calves were separately inoculated with approximately 10 10 CFU of wild-type 85-170 Nal r or 85-170 Nal r ⌬nleH1 ⌬nleH2 as described previously by Stevens et al. (33). The magnitude and duration of fecal excretion of the bacteria were followed daily for 14 days. Wild-type and mutant bacteria were enumerated by plating of triplicate serial dilutions of fresh feces collected by rectal palpation onto sorbitol-MacConkey agar supplemented with potassium tellurite (2.5 mg ml Ϫ1 ) (T-SMAC) containing 25 g ml Ϫ1 Nal (T-SMAC-Nal) and onto T-SMAC-Nal containing 50 g ml Ϫ1 kanamycin, respectively. Recovery of wild-type and mutant bacteria was confirmed by PCR from selected colonies using nleHflanking primers. The sensitivity of detection was 10 2 CFU/g. Fecal excretion data were statistically analyzed for the effect of mutation by means of an F test, with the data taken as repeated measurements and the animal as a covariant (Proc Mixed, Statistical Analysis System 1995; SAS Institute, Cary, NC). P values of Ͻ0.05 were considered significant.
Oral inoculation of lambs. Fifteen 6-week-old crossbred lambs were randomly divided into three equal groups, supplied with food and water ad libitum, and confirmed to be free of E. coli O157:H7 by enrichment and O157 immunomagnetic separation. All lambs were housed in biosecure containment level 2 accommodations. Each group was housed in a separate room with its own air handling. The animals were visited by experienced staff, who changed protective clothing between groups. Five lambs were each dosed orally with 10 9 CFU of either wild-type 85-170 Nal r or the isogenic ⌬nleH1 ⌬nleH2 mutant separately, or with wild-type 85-170 Nal r and the ⌬nleH1 ⌬nleH2 mutant together, suspended in 10 ml of 0.1 M phosphate-buffered saline (PBS) (pH 7.4). Approximately 24 h after oral inoculation and as required thereafter for up to 28 days, rectal fecal samples from each lamb were collected for direct plating onto SMAC supplemented with either 15 g of Nal/ml or 25 g of kanamycin/ml. Samples that were O157 negative on direct plating were enriched in buffered peptone water for 6 h at 37°C and then plated onto SMAC plates supplemented with the appropriate  antibiotic. Representative colonies were confirmed to be E. coli O157 by latex agglutination (Oxoid). For coinfection studies, the competitive index (CI) was calculated; it is defined as the ratio between the mutant and wild-type strains within the output (bacteria recovered from the host after infection) divided by their ratio within the input (initial inoculum). For this experiment, the input ratio was 1:1. The null hypothesis that CI ϭ 1 was tested by a two-sided t test. Murine models. Specific-pathogen-free female 6-to 8-week-old mice were used in this study. Wild-type inbred C57BL/6 and DBA-1 mice were purchased from Harlan UK Ltd. (Bicester, United Kingdom), while the transgenic lightproducing animal model DBA-1 NF-B-luc (Oslo) (P/N 119335) was purchased from Xenogen-Caliper Corp. (Alameda, CA). The transgenic light-producing animal model NF-B-RE-luc (Oslo)-Xen, commonly called NF-B-RE-luc (Oslo), carries a transgene containing three NF-B responsive-element (RE) sites from the immunoglobulin light-chain promoter and modified firefly luciferase cDNA. All animals were housed in individually HEPA-filtered cages with sterile bedding and free access to sterilized food and water. Independent experiments were performed at least twice (but only once for histology) using at least four mice per group.
Oral infection of mice, harvesting and collection of tissues, and bacterial stool counts. Mice were orally inoculated using a gavage needle with 200 l of overnight LB-grown bacterial suspension in PBS (ϳ5 ϫ 10 9 CFU). The number of viable bacteria used as the inoculum was determined by retrospective plating onto LB agar containing antibiotics. Stool samples were recovered aseptically at various time points after inoculation and the number of viable bacteria per gram of stool determined after homogenization at 0.1g ml Ϫ1 in PBS and plating onto LB agar containing the appropriate antibiotics. At selected time intervals postinfection, blood was collected by cardiac puncture and mice were sacrificed by cervical dislocation. Sections of distal colon were collected and snap frozen in liquid nitrogen before storage at Ϫ70°C prior to analysis. For coinfection studies, the CI was calculated as described previously by Mundy et al. (30). For this experiment, the input ratio of wild-type strain to mutant strain was approximately 1:2. The null hypothesis that CI ϭ 1 was tested by a nonparametric Wilcoxon two-tailed test using the GraphPad InStat software (GraphPad Software Inc., San Diego, CA).
In vivo BLI. Prior to imaging, the abdominal region of each mouse was depilated to minimize any potential signal impedance by melanin within pigmented skin and fur. Bioluminescence (photons s Ϫ1 cm Ϫ2 sr Ϫ1 ) from living infected animals was measured after gaseous anesthesia with isofluorane using the IVIS50 camera system (Xenogen-Caliper Corp., Alameda, CA). The sample shelf was set to position D (field of view, 15 cm). A photograph (reference image) was taken under low illumination prior to quantification of photons emitted from strain ICC180 at a binning of 4 over 1 to 10 min using the software program Living Image (Xenogen-Caliper Corp.) as an overlay on Igor (Wavemetrics, Seattle, WA). For anatomical localization, a pseudocolor image representing light intensity (from blue [least intense] to red [most intense]) was generated using the Living Image software and superimposed over the gray-scale reference image. Bioluminescence within specific regions of individual mice was also quantified using the region-of-interest tool in the Living Image software program (given as photons s Ϫ1 ). For expression of light from the NF-B reporter mice, 180 mg kg Ϫ1 D-luciferin (Gold Biotechnology, St. Louis, MO) dissolved in 250 l PBS (pH 7.8) was administered by intraperitoneal injection 5 min prior to imaging. As a positive control for luciferase gene expression from the NF-B-RE-luc (Oslo) mice, tumor necrosis factor alpha (TNF-␣) (2 g per mouse) was administered by intraperitoneal injection.
Histopathology. Segments of the cecum and the terminal colon of each mouse were collected at 9 and 14 days postinoculation, rinsed of their content, and fixed in 10% buffered formalin for microscopic examination. Formalin-fixed tissues were then processed, paraffin embedded, sectioned at 5 m, and stained with hematoxylin and eosin (H&E) according to standard techniques. Sections were examined by light microscopy for the presence of intimately adhering bacteria on intestinal cells, as previously described (15). Crypt length was also evaluated, and the lengths of at least four well-oriented crypts were measured for each section. A nonparametric analysis of variance (ANOVA) with a posteriori comparisons was performed using commercially available GraphPad InStat v3.06 software (GraphPad Software Inc., San Diego, CA). P values of Յ0.05 were considered significant.
Immunohistochemistry. Snap-frozen colonic tissues, embedded in OCT mounting medium (VWR BDH, Lutterworth, United Kingdom), were sectioned using a cryostat to a thickness of 5 m. Sections were mounted on polysine slides (VWR BDH) and air dried overnight before fixing in acetone at room temperature for 20 min. After air drying for 1 h, sections were rehydrated in Trisbuffered saline (TBS) for 5 min and then incubated with antibodies against CD3, CD4, and CD8 (Serotec, Oxford, United Kingdom) at a dilution of 1:50 to 1:100 for 1 h. Sections were gently washed with TBS three times before addition of biotinylated anti-rat immunoglobulin G (Serotec) at a dilution of 1:200 with 4% (vol/vol) normal murine serum for blocking (Sera Laboratories International, Horsted Keynes, United Kingdom) for 30 min. After washing, a 1:200 dilution of 0.1% avidin-peroxidase (Sigma-Aldrich, Dorset, United Kingdom) was added and left for 30 min before further washing and treatment with diaminobenzadine substrate (Sigma-Aldrich) for 5 min. The reaction was stopped with excess TBS, and sections were counterstained with Mayer's hematoxylin (Sigma-Aldrich) for 30 s, dipped in acid alcohol, and washed in tap water for 5 min. Sections were dehydrated through an ethanol gradient of 70%, 90%, and 100% solutions (2 min each), followed by clearing in Histoclear (VWR BDH) and mounting in DPX (VWR BDH). A control slide using no primary antibody was also made to show endogenous peroxidase-containing cells. Stained cell populations were counted in five randomly selected fields per section, and data were expressed as the number of T cells per 250 m 2 of lamina propria.

RESULTS
The NleH T3SS effector homologues. NleH belongs to a family of T3SS effectors found in diverse enteric pathogens.
We employed BLASTp searches of the NCBI protein database using EPEC E2348/69 NleH1 as the query sequence. The Clustal W2 software (EMBL-EBI) was then used to create a phylogram of the different homologues (Fig. 1). Two major clusters were formed, one containing all the NleH effectors and the other containing closer homologues of OspG, including an OspG-like effector (90.8% identity to OspG of Shigella) from  EHEC O157:H7 strain EC4045. To determine the role of NleH proteins in vivo, we generated EHEC O157:H7 (strain 85-170) ⌬nleH1 ⌬nleH2 and C. rodentium (ICC169 and bioluminescent strain ICC180) ⌬nleH mutants. The EHEC O157:H7 ⌬nleH1 ⌬nleH2 double mutant is shed in greater numbers than the parental strain from orally challenged calves. To assess the role of NleH in intestinal colonization of calves by EHEC O157:H7, wild-type and mutant bacteria were separately inoculated into four 12-day-old Friesian bull calves. Both wild-type and mutant strains colonized the calves efficiently, and the mutant was excreted at lower levels than the wild type during the first 4 days. From day 7 the mutant was shed at higher levels than the wild-type strain, and the difference became statistically significant (P Ͻ 0.05) from day 10 onwards (Fig. 2). The course of the fecal excretion of the wild-type strain was consistent with previously observed patterns (10, 33, 37).

Contribution of NleH1 and NleH2 to colonization of conventional 6-week-old-lambs. A 6-
week-old lamb model was next used to compare the persistence of an E. coli O157:H7 ⌬nleH1 ⌬nleH2 double mutant and the isogenic wild-type strain. The ability of the mutant to establish itself and persist in lambs was investigated by monitoring the viable counts recovered in fecal pellets collected per animal. When given as a single inoculum, the wild-type E. coli O157:H7 isolate produced the classical shedding pattern in lambs, as described previously (5,42), persisting in relatively high numbers during the early stages of infection and then declining by day 11 postinoculation (Fig. 3A). The ⌬nleH1 ⌬nleH2 mutant demonstrated a similar shedding pattern, except that positive fecal samples were noted only until day 12 postinoculation (Fig. 3A). When both isolates were administered in the same inoculum, the wild type persisted for 4 days longer than the ⌬nleH1 ⌬nleH2 mutant (data not shown). The mean CI was signifi- cantly less than 1 for all time points where it could be calculated except day 1 (Fig. 3B), demonstrating that the wild-type strain outcompeted the ⌬nleH1 ⌬nleH2 mutant in the ovine model. Contribution of NleH to colonization in the C. rodentium murine model. We followed the anatomical localization and pathogenic burden using BLI and viable counts in stools of mice infected with either wild-type or ⌬nleH C. rodentium. Using BLI, we observed that both the wild-type and mutant strains colonized the cecal patch and rectum by day 3 to 4 postinfection. After adaptation to the in vivo environment (day 6 to 7), the entire distal colon was then heavily infected. Clearance began by day 10, at which point light intensity decreased. By day 14 the gastrointestinal tract had mostly cleared the infection (Fig. 4). Viable counts of bacteria in stool mirrored the results obtained by BLI; no significant differences in viable bacterial counts of the wild-type and ⌬nleH mutant strains were seen (Fig. 5A). However, the ⌬nleH C. rodentium mutant was significantly out competed by the wild-type strain in a mixed infection (Fig. 5B).

NleH does not affect A/E lesion formation and T-cell infiltration in the C. rodentium murine model. The hallmarks of C. rodentium infection include induction of extensive colonic hyperplasia and influx of T cells into the colonic lamina propria.
Histological examination and measurement of crypt length did not reveal any differences between the parent and mutant strains (data not shown). Immunohistochemistry, performed to investigate the influx of CD3 ϩ , CD4 ϩ , and CD8 ϩ T cell subsets into the colonic lamina propria at 14 days postinoculation, revealed that although the ⌬nleH mutant-infected animals showed slightly fewer CD3-and CD4-positive T cells in the lamina propria, no significant differences were observed between animals infected with the mutant or wild-type C. rodentium strains (data not shown). Immunofluorescent staining with anti-O152 and SEM analysis at day 9 or day 14 postinoculation did not reveal any differences between the wild-type and ⌬nleH C. rodentium strains (Fig. 6).

NleH influences NF-B levels and expression of TNF-␣ in vivo.
A recent study has shown that OspG inhibits degradation of IB and hence activation of NF-B and that a Shigella ospG mutant induces a stronger inflammatory response than the wild-type strain after inoculation of rabbit ileal loops (20). In order to determine if NleH influences activation of NF-B in vivo, we infected NF-B-RE-luc reporter mice with C. rodentium wild-type strain ICC169 or ICC169 ⌬nleH; mice inoculated with the commensal E. coli strain ICC299 (Table 1) or PBS were used as controls. The number of nleH mutant bacteria shed from this mouse strain was similar to that of the wild type (data not shown). No significant differences in whole-body (including chest, neck, abdomen, and rectum) luminescence counts were recorded by live imaging, at any time point, between PBS-gavaged animals and those gavaged with wild-type C. rodentium, the nleH mutant, or the commensal E. coli. On day 14 postchallenge, we recorded luminescence counts in different organs. While no significant difference in the luminescence counts was seen in the mesenteric lymph nodes, spleens, and ceca of the different mouse groups (Table 4), there was a significant (P ϭ 0.0024) 2.5-fold increase in the signal from the colon in mice infected with the wild-type C. rodentium compared to those inoculated with C. rodentium ⌬nleH, E. coli ICC299, or PBS ( Fig. 7A and B). This difference was similar to the three-to fourfold-increased luminescent signal seen after mice were inoculated with TNF-␣ as a positive control (data not shown).
As NF-B induces the transcription of many proinflammatory cytokines such as TNF-␣ and IFN-␥, we compared the levels of their transcripts in uninfected mice and mice infected with either wild-type or ⌬nleH mutant C. rodentium. RNA extracted from distal colons of mice was subjected to semiquantitative RT-PCR. Transcript levels were quantified as a ratio of TNF-␣ or IFN-␥ to ␤-actin. This revealed that the levels of TNF-␣ mRNA were significantly higher in tissues extracted from infected mice than in those from uninfected control mice. Mice infected with the wild-type C. rodentium had significantly higher TNF-␣ transcript levels than those infected with the ⌬nleH mutant (Fig. 8). The levels of IFN-␥ transcript were comparable in all mouse groups (data not shown).

DISCUSSION
Many gram-negative bacterial pathogens use T3SS effectors to modulate host cell signaling pathways. Effector proteins can trigger local (e.g., alteration in the cytoskeleton) or systemic (e.g., immune response) changes. Colonization of the mucosal surface requires temporal modulation of the host immune status. While downregulation of innate immunity might aid the pathogen to launch an infection and to reach a critical mass, activation of the immune system might assist the pathogen in its competition with the resident gut microflora. It is therefore not surprising that pathogenic bacteria are equipped with virulence factors which have antagonistic immune modulation activities. Indeed, in a recent report Lupp et al. demonstrated that C. rodentium population expansion in vivo is mediated by an inflammatory response that disrupts the endogenous intestinal microbiota (22). In contrast, using polarized culture models, Ruchaud-Sparagano et al. have shown that EPEC inactivates innate immune responses in vitro (32).
In this study we investigated the role of NleH in colonization, competitiveness, and activation of the NF-B pathway in vivo. EPEC O127:H6 E2348/69 and EHEC O157:H7 EDL933 and Sakai contain two, almost identical, copies of nleH, while C. rodentium harbors only a single nleH gene. The functional consequences of this gene duplication are not known. Interestingly, a recent shotgun sequencing of a number of EHEC O157:H7 isolates has shown that they contain, in addition to nleH, a gene whose product shares 90.8% sequence identity with OspG (NCBI BLASTp).
Investigation of the contribution of NleH toward colonization and competitiveness of EHEC O157:H7 in bovine and ovine hosts, which are important animal reservoirs of the pathogen, showed that the EHEC O157 ⌬nleH1 ⌬nleH2 double mutant was shed in greater numbers than the parental strain from orally challenged calves, significantly from day 10 postinoculation. The precise effect of deleting nleH on factors or regulatory mechanisms involved in EHEC O157:H7 colonization in bovine intestines remains to be investigated. In singleinfection studies with lambs, there was no statistical difference in shedding after oral inoculation with the same strains. However, CIs measured following oral inoculation of lambs with a mixture of wild-type EHEC O157:H7 and the ⌬nleH1 ⌬nleH2 double mutant revealed that the mutant was significantly outcompeted. The reasons for the different phenotypes observed in the bovine and ovine models are currently not known. However, these results show that effector proteins might have dissimilar or even opposite functions in different hosts.
In order to determine the contribution of NleH to infection with C. rodentium, we mutated nleH in the wild-type ICC169 and luminescent ICC180 strains. Deletion of nleH from C. rodentium had no significant effect on in vivo tissue tropism, bacterial burden, colonic hyperplasia, or infiltration of CD3 ϩ , CD4 ϩ , and CD8 ϩ cells to the lamina propria. A subtle phenotype was recently reported for C. rodentium ⌬nleH in single infection, as expansion of the mutant population in vivo lagged behind that of the wild-type population during early stages (6 days postchallenge), although at later stages (10 days) the mutant and wild type colonized at comparable levels (11). The reasons for the different results might be due to the mouse status (i.e., composition of the normal gut flora), preparation of the inocula, or bacterial strains. Importantly, we found that in a mixed infection the nleH mutant was significantly outcompeted by the wild-type strain, suggesting that expression of NleH increases the bacterial fitness in vivo. This could explain the need for conservation and multiplicity of the gene in EHEC and EPEC strains.
As we did not observe any difference in colonization and clearance dynamics, hyperplasia, and T-cell infiltration between the wild-type and ⌬nleH mutant strains, NleH appears to have a local rather than systemic role, possibly in displacing   the normal gut flora. Considering that both NleH (C. Hemrajani, unpublished data) and OspG (20) are protein kinases and share a high level of sequence identity, we investigated, using reporter mice, if NleH plays a role in activation of the NF-B pathway. Unexpectedly, we found lower activation of NF-B in the colon in mice infected with the C. rodentium ⌬nleH mutant than in those infected with the parental wild-type strain. Consistent with these results, we found lower colonic levels of TNF-␣ at 14 days postchallenge in mice infected with the ⌬nleH C. rodentium mutant than in those infected with the wild-type strain, while no difference was recorded for IFN-␥. These data suggest that NleH triggers local activation of NF-B, which in turn leads to a differential increase in the levels of proinflammatory cytokines. Collectively these results demonstrate that the role of NleH during infection is host specific. NleH, one of the core and conserved T3SS effectors in A/E pathogens, is likely to work with other effectors in optimizing the level of local gut inflammatory responses and the relationship with the endogenous gut flora for the benefit of the pathogen. FIG. 7. NF-B activation in organs of mice at 14 days postchallenge. Luminescence was measured in extracted organs. NF-B-RE-luc reporter mice were inoculated with wild-type (strain ICC169) or ⌬nleH C. rodentium. (A) Representative bioluminescence images captured using the IVIS50 camera system are shown (cecum [1], mesenteric lymph nodes [2], colon [3], spleen [4], and intestine [5]. Luminescence was quantified using the region-of-interest tool in the Living Image software (given as photons s Ϫ1 ). (B) Graph of luminescence in extracted colons shows a significant loss of NF-B activation in the absence of nleH. ‫,ءءء‬ P Ͻ 0.005.
FIG. 8. Semiquantitative TNF-␣ and ␤-actin RT-PCRs were performed on RNA isolated from colons of uninfected mice or mice orally challenged with wild-type or ⌬nleH C. rodentium. Median TNF-␣ levels (measured as a ratio of TNF-␣ to ␤-actin) in C. rodentium-infected mice were considered the basal level of activation by wild-type bacteria in each experiment and taken as 100%. All TNF-␣/␤-actin ratios were compared to this and expressed as a percentage of the median TNF-␣ level during wild-type infection. GeneTools (Syngene) was used for densitometric analysis. Two repetitions, each using four or five mice per group, were conducted and graphed. The one-way ANOVA Bonferroni multiple-comparison test was used to determine significance, as the three groups had normal distributions. ‫,ءءء‬ P Ͻ 0.001.