EspFu-Mediated Actin Assembly Enhances Enteropathogenic Escherichia coli Adherence and Activates Host Cell Inflammatory Signaling Pathways.

EPEC is among the leading causes of diarrheal disease worldwide. The colonization of the gut mucosa by EPEC results in actin pedestal formation at the site of bacterial attachment. These pedestals are referred to as attaching and effacing (AE) lesions. Here, we exploit the different molecular mechanisms used by EPEC to induce AE lesions on epithelial cells, showing that the effector EspFu is associated with increased bacterial attachment and enhanced epithelial colonization compared to the Tir-Nck pathway. Moreover, we also showed that actin pedestal formation can counterbalance the anti-inflammatory activity induced by EPEC, especially when driven by EspFu. Collectively, our findings provide new insights into virulence mechanisms employed by EPEC to colonize epithelial cells, as well as the host response to this enteric pathogen.

E nteric bacterial pathogens have evolved specialized infection strategies to manipulate host signaling pathways and facilitate the colonization of the gastrointestinal tract. Many of these pathogenic bacteria utilize the T3SS to translocate a repertoire of effector proteins into the host cell cytosol (1). These effectors, in a coordinated fashion, modulate several cellular processes, such as cytoskeletal dynamics, membrane trafficking, transcription, cell cycle progression, signal transduction, and ubiquitination (2).
Enteropathogenic Escherichia coli (EPEC) is one of the leading causes of diarrheal diseases worldwide, especially among children younger than 5 years of age (3,4). Similarly to other attaching-effacing (AE) pathogens (e.g., enterohemorrhagic E. coli [EHEC] and Citrobacter rodentium), EPEC employs effector proteins to remodel the host cytoskeleton, enabling its adherence to enterocytes and colonization of the intestinal epithelium. The cytoskeletal rearrangement promoted by EPEC culminates in AE lesions, which are characterized by the effacement of the microvilli, and the accumulation of polymerized actin beneath the attached bacteria, forming pedestal-like structures (5).
The majority of the genes required for AE lesion formation are contained within a pathogenicity island named the locus of enterocyte effacement (LEE) (6). The LEE region is organized into five major operons (LEE1 to LEE5), which encode the structural components of the T3SS (7), effector proteins (8), regulators, chaperones, the adhesin intimin (8), and its translocated receptor Tir (9). Tir is inserted into the eukaryotic membrane and phosphorylated by host cell tyrosine kinases at the C-terminal domain (at tyrosine Y 474 , yielding Tir Y-P ) after its interaction with intimin (10). Following phosphorylation, the mammalian protein Nck is recruited, where it activates the neural Wiskott-Aldrich syndrome protein (N-WASP), which in turn recruits the Arp2/3 complex, leading to a localized actin polymerization (11). In contrast, Tir from some EPEC and EHEC strains lacks the Y 474 and is not tyrosine phosphorylated (Tir S ). Instead of recruiting Nck, Tir S engages the non-LEE-encoded effector EspFu/TccP to promote pedestal formation (12,13). EspFu is also translocated to the host cell by the LEEencoded T3SS, where it bridges the interaction of Tir with the host IRSp53 and/or IRTKS proteins and N-WASP. A conserved Asn-Pro-Tyr motif (NPY) in Tir is a critical binding site for the I-BAR domain of IRSp53 and IRTKS (14), while the SH3 domain of these proteins directly binds to the C-terminal proline-rich region of EspFu (15). EspFu then interacts with the GTPase-binding domain (GBD) to activate N-WASP (12), recruiting the Arp2/3 complex and leading to actin polymerization. In addition, a subset of EPEC strains has the potential to induce actin polymerization by simultaneously utilizing the Tir-Nck and Tir-EspFu pathways (16)(17)(18)(19). However, it is unclear whether the ability to use converging pedestal formation pathways would confer a competitive advantage for these strains or whether host epithelial cells respond differently to these distinct actin polymerization pathways.
EPEC also encodes a vast repertoire of non-LEE-encoded effectors that are not directly involved with cytoskeleton remodeling but instead play an important role in the modulation of host inflammatory response during the course of infection (20)(21)(22)(23)(24)(25)(26)(27). These effectors are highly conserved among AE pathogens and are generally encoded by genomic islands, suggesting that the acquisition of these elements was necessary to attenuate the inflammatory response triggered by EPEC's interaction with the host cell. In fact, the attenuation of the inflammatory response triggered by AE pathogens is essential to establish a suitable niche for host colonization. For example, mutant strains of C. rodentium that are not able to suppress inflammation had lower murine intestinal colonization compared to wild-type strains (28). However, how this immunomodulation is impacted by the different actin polymerization mechanisms employed by EPEC to induce AE lesions is still poorly understood.
In this study, we investigated the different molecular mechanisms used by EPEC to induce AE lesions on epithelial cells, showing that the effector EspFu is associated with increased bacterial attachment and enhanced epithelial colonization compared to the Tir-Nck pathway. Moreover, we also show that actin pedestal formation can counter-balance the anti-inflammatory activity induced by EPEC, especially when driven by EspFu.

RESULTS
The effector repertoire of EPEC BA320 strain. Usually, EHEC strains employ the Tir S -EspFu pathway (12,13) and EPEC strains use the Tir-Nck pathway (11) to form AE lesions. BA320 is an EPEC O55:H7 strain that was isolated from the stool of a child with acute diarrhea in 2003 during an epidemiological study focused on the etiology of acute diarrhea in children under 5 years old carried out in Salvador, Brazil (29). The BA320 strain was previously reported to have the potential to induce actin polymerization in cultured epithelial cells in vitro (30). Importantly, EPEC O55:H7 gave rise to EHEC O157:H7 (31).
We sequenced the genome of BA320 to better elucidate the molecular mechanisms employed by this strain to induce AE lesions, focusing on its effector repertoire. The draft genome of strain BA320 is 5,360,779 bp in size with 50.39% GϩC content, and it contains 5,281 coding sequences, 7 rRNA (rrn) operons, and 87 tRNA genes. A single 65-kb plasmid was detected, which does not correspond to the EPEC adherence factor (EAF) virulence plasmid. Also, the operons encoding the bundle-forming pilus (32) and Per regulators (33) were not found, corroborating previous studies that classified BA320 as an atypical EPEC strain (30,34).
The LEE pathogenicity island of BA320 is 34,166 bp long showing 99 and 91% nucleotide identities with the LEE regions of prototype strains EDL933 (EHEC O157:H7) and E2348/69 (EPEC O127:H6), respectively (Fig. 1A). Multiple sequence alignment showed higher nucleotide diversity between the LEE4 and LEE5 operons from BA320 and E2348/69, while the LEE1-3 operons shared higher similarity. Six effector-encoding genes (espG, espZ, espH, map, tir, and espF) are present in the LEE of BA320, of which Tir is the only one absolutely required for AE lesion formation on epithelial cells (35). Analysis of the Tir BA320 sequence identified the NPY motif implicated in the EspFumediated actin polymerization pathway in EHEC O157:H7, while the tyrosine residue Y474, required for Nck-dependent actin polymerization in EPEC O127:H6, was absent (Fig. 1B).
EspFu promotes actin remodeling and bacterial attachment to epithelial cells. BA320 induces actin polymerization on epithelial cells in vitro in a Nck-independent manner (30). Congruently, the genome analyses indicated that an EspFu-mediated signaling pathway would be the most likely molecular mechanism employed by BA320 to induce actin polymerization. In silico analysis showed that the espFu gene is located within a prophage, which shares low similarity to the CP-933U and Sp14 prophages from strains EDL933 and Sakai, respectively (see Fig. S1A in the supplemental material). The espFu gene of BA320 is 732 bp long and encodes a protein containing four almost identical 47-amino-acid proline-rich repeats (PRRs) with high similarity to EspFu from EHEC O157:H7 (strain EDL933) and EPEC O119:H6 (strain ICC199) (Fig. S1B).
While the wild-type BA320 strain (WT) is able to induce robust actin polymerization in vitro, the deletion of espFu resulted in the loss of this phenotype ( Fig. 2A), which was restored by an EspFu-producing plasmid (KOϩpEspFu), but not with an empty vector (KOϩvector). These findings were consistent with scanning electron microscopy (SEM) analysis showing the presence of actin pedestals on the surface of HeLa cells infected with WT and KOϩpEspFU but not with espFu-negative strains (Fig. 2B). Moreover, EspFu-producing strains were significantly more adherent than KO and KOϩvector ( Fig. 2C). These data indicate that EspFu plays an essential role in AE lesion formation and increases bacterial attachment to epithelial cells.
EspFu-mediated actin assembly promotes more efficient bacterial attachment and pedestal formation than the Tir:Nck-dependent pathway in EPEC BA320. In addition to EspFu, EPEC strains can also induce actin polymerization through the Tir:Nck-dependent pathway or even using both signaling pathways (18,19). To compare the different actin assembly pathways employed by EPEC, we genetically manipulated strain BA320 by targeting the AE effectors Tir and EspFu, and two sets of isogenic strains were generated: (i) BA320 (WT) and ΔespFu (KO), and (ii) KOct1 and KOct2 (Fig. 3A). These strains differ by the presence (WT and KOct1) or absence (KO and KOct2) of espFu, as well as by the location and type of tir (i.e., chromosomal and nonphosphorylated in WT and KO; plasmid encoded and phosphorylated in KOct1 and KOct2). Specifically, BA320 represents the EspFu-mediated actin assembly; KOct2 and KOct1 strains can induce actin rearrangement via Tir-Nck or both EspFu/Tir-Nck pathways, respectively, while KO is a pedestal-deficient strain.
All these EPEC strains showed similar growth profiles (Fig. S1C) and T3SS functionality, as assessed by the secreted levels of EspB (Fig. S1D). Immunofluorescence assays showed that Tir was translocated to host cells and colocalized with pedestals formed by BA320, KOct1, and KOct2 strains (Fig. 3B). The KO translocated Tir but did not induce The NPY motif is conserved in all three strains (in bold). Phosphorylated tyrosine (Y474) in Tir E2348/69 and equivalent residues in Tir BA320 and Tir EDL933 are boxed with a solid line. (C) In silico detection of the non-LEE-encoded effectors of EPEC E2348/69, EPEC B171, and EHEC Sakai in the EPEC BA320 genome using TBLASTN. Each square indicates the presence (in gray) or absence (in white) of an effector-encoding gene. robust actin rearrangement. Anti-phosphotyrosine (PY) labeling revealed that Tir of both KOct1 and KOct2 strains were phosphorylated similarly to Tir from the EPEC prototype strain E2348/69 (Fig. 3C), while Tir of BA320 was not phosphorylated after translocation to the host cell, as expected. These strains were then considered suitable for comparisons of the different actin assembly pathways used by EPEC.
Subsequent analyses of the dynamics of AE lesion formation by these strains showed that infections with BA320 resulted in a higher number of cells with pedestals compared to KOct1-and KOct2-infected cells. No significant difference was observed between KOct1-and KOct2-infected cells ( Fig. 4A and B). Notably, EspFu-producing strains were significantly more adherent than their espFu isogenic mutants (BA320 versus KO and KOct1 versus KOct2), with BA320 having the highest levels of bacterial attachment (Fig. 4C). Live cell imaging also revealed a higher number of attached bacteria and pedestals formed by BA320 in comparison to KOct1 and KOct2 strains over the course of infection (Fig. 4D, see also Videos S1 to 3 in the supplemental material). Similarly, the infection of HeLa cells with a tir mutant complemented with a plasmid expressing Tir BA320 (pTir) resulted in a higher number of attached bacteria and cells with pedestals compared to its isogenic pair KOct1 (Fig. S2), indicating that the differences observed in the dynamics of AE lesion formation were more likely due to the mechanism of pedestal formation rather than the location and/or mode of expression of tir (i.e., chromosomal in BA320 and plasmid-encoded in KOct1 and KOct2). Collectively, these results indicate that both bacterial attachment and pedestal formation are more efficient in the presence of EspFu, especially in combination with Tir S , which is not tyrosine phosphorylated.
Actin pedestal formation induced by EPEC activates inflammation-related pathways on epithelial cells. Transcriptomic analysis has provided valuable insights on bacterial-host interactions, as well on the processes leading to disease, including several studies using pathogenic E. coli infections (36)(37)(38). To investigate how different actin assembly pathways affect transcription of host cells, we performed RNA-Seq analysis using total mRNA purified from HeLa monolayers infected with the WT and the engineered BA320 strains for 6 h. This time point was chosen because after 6 h of infection, the effectors have been delivered, and actin has been rearranged into pedestals. The transcriptomic profiles of cells infected with pedestal-forming strains (BA320, KOct1, and KOct2) were compared to that from cells infected with a pedestaldeficient strain (KO). Uninfected cells were used as a control. By applying statistical Bacterial Attachment and Inflammation Driven by EspFu ® cutoffs of a false discovery rate (FDR) of Յ0.01 and fold change (FC) cutoffs of Ϫ1 Ն log 2 FC Ն 1, we found that 44, 33, and 108 genes were differentially expressed in cells infected with BA320, KOct1, and KOct2, respectively (Fig. 5A). It is important to point out that these pairwise comparisons involve both isogenic (WT versus KO) and not isogenic strains (KOct1 versus KO and KOct2 versus KO). Remarkably, cells infected with EspFu-expressing strains showed a greater number of upregulated genes, while the transcriptome of cells infected with a strain that exclusively uses the Tir-Nck pathway had predominantly downregulated genes (Table S2).
Overall, a total of 143 genes were differentially expressed in cells infected with pedestal-forming strains compared to KO infections. With a few exceptions, the magnitude of expression of these genes was considerably small (a fold change of Ͻ4) (Table S2). Then, we restricted our analysis to only 33 differentially expressed genes (DEGs) that were shared among isogenic and nonisogenic comparisons in order to identify genes potentially modulated in response to pedestal formation induced by EPEC (Fig. 5B). Interestingly, hierarchical clustering of these 33 genes showed a very similar expression pattern in cells infected with EspFu-expressing strains (WT and KOct1), indicating that this could constitute a common set of genes modulated in response to EspFu-mediated actin assembly pathways (Fig. 5C).
Among the genes commonly modulated in response to pedestal formation, many were involved with inflammatory and/or apoptotic processes, particularly those that encode proinflammatory cytokines (IL-1A, IL-6, and IL-8), chemokines (CXCL1 and CXCL2), antiapoptotic factors (BIRC3), and prostaglandins (PTGS2), as well as genes that limit the immune response (NFKBIA, NFKBIE, and TNIP3), among others (Fig. 6A). Some  (Continued on next page) Bacterial Attachment and Inflammation Driven by EspFu ® of these genes were preferentially regulated in response to the EspFu-mediated pedestal formation, such as C8orf4, IER3, IL1A, NFKBIA, NFKBIE, and PTGS2. Validation of the transcriptome data by quantitative real-time PCR showed that the relative expression levels of four tested genes (CXCL1, IL-6, IL-8, and NFKBIA) exhibited the same regulatory trends as compared with RNA-Seq data set, except for IL-8 in KOct2infected cells that did not show a significant change in comparison with cells infected with KO (Fig. 6B).
We then hypothesized that the stronger inflammatory response triggered by EspFuexpressing strains could be most likely due to the presence of a greater number of AE lesions and attached bacteria, leading to a higher exposure to surface antigens such as LPS, flagellin, and immunogenic components of the T3SS, which are known to activate the inflammatory response in infections by AE pathogens (39)(40)(41)(42). To test this, we analyzed the expression profile of some proinflammatory genes in conditions where the bacterial loads on the surface of cells were normalized. By increasing the multiplicity of infection (MOI) from 10 to 100, we observed that KO and KOct2 adhered at the  same levels than their isogenic pairs BA320 (Fig. S3C) and KOct1 (Fig. S3G), respectively. As expected, the enhanced bacterial attachment by KO strain did not result in a significant increase of the number of cells with pedestals ( Fig. S3A and B), whereas KOct2 formed pedestals more efficiently under these conditions ( Fig. S3E and F). However, cells infected with BA320 showed a higher expression level of CXCL1 and IL-8 genes than cells infected with a similar bacterial load of KO (Fig. S3D), suggesting that the upregulation of these proinflammatory genes was mostly due to the pedestal formation driven by EspFu. Similarly, the infection of cells with KOct1, that employs EspFu in addition to Tir:Nck-mediated actin polymerization pathway, resulted in a higher expression of these same genes compared to cells showing the same bacterial load of KOct2 (Fig. S3H). Taken together, these results suggest that the activation of proinflammatory genes could be more likely due to the presence of an EspFu-mediated actin assembly mechanism rather than the enhanced exposure to bacterial surface antigens such as LPS, flagellin, and T3SS.
We next used the Ingenuity Pathway Analysis (IPA) tool to investigate possible biological interactions between the DEGs and to identify functional networks (canonical signaling pathways and upstream regulators) associated with the different actin assembly pathways induced by EPEC. To maximize the expression data available to the IPA software, we loosened the inclusion criteria by applying filters of Ϫ0.5 Ն log 2 FC Ն  Figure 7A shows the 10 most significantly affected canonical pathways in each comparison, ranked according to the P value, as well as the activation status based on the Z-score. Notably, most of these pathways were related to infectious processes, inflammatory responses, and immunological diseases, reinforcing our hypothesis that AE lesions induced by EPEC could activate inflammatory responses in host epithelial cells. Some pathways were commonly regulated in response to all pedestalforming strains, notably TNFR2 signaling (Fig. S4A), whereas others, such as IL-6 signaling (Fig. S4B) and MIF-mediated regulation of innate immunity, were preferentially activated in response to EspFu-or Tir:Nck-dependent mechanisms, respectively. We did not observe any pathway related to actin cytoskeleton signaling among those that were most significantly affected, suggesting that the expression of actin-related genes was not changed at this time point (6 h of infection), when the pedestals are already formed. Although we have not tested this, we speculate that the actin cytoskeleton signaling can be affected in the early stages of the infection, when the actin polymerization is triggered.
The prediction of transcription factors (upstream regulators) potentially related to the gene expression changes reported in our data were also performed using IPA tool. Figure 7B shows the 10 most significantly affected upstream regulators in each comparison based on the P and Z-score values. Notably, most of these regulators were predicted to be activated in infections with EspFu-expressing strains and inhibited in cells infected with KOct2 strain. HIF1A was predicted to be the most relevant affected upstream regulator in all infections (Fig. S5A). Genes encoding proinflammatory cytokines, such as IL-1B and tumor necrosis factor (TNF) (Fig. S5B), were also found among the most affected upstream regulators, mainly in response to EspFu-mediated actin assembly.
Predominance of an anti-inflammatory response in epithelial cells infected with a pedestal-deficient EPEC strain. Interestingly, many immune-related genes that were upregulated in our data set were actually strongly downregulated in cells infected with a pedestal-deficient strain (KO) (Fig. 5C and 8), suggesting that EPEC can also The significance score (negative log of the P value) is indicated by the bars on the x axis, and the solid vertical black lines represent a P value significance threshold of 0.05. The color scheme depicted is based on Z-scores: orange indicates predicted activation, blue indicates predicted inhibition, and gray indicates that certain canonical pathway or upstream regulator is predicted to have significant involvement but the activation state cannot be determined based on the gene expression data (undetermined directionality).
induce an anti-inflammatory effect in epithelial cells in the absence of a robust pedestal formation. Thus, EPEC strains that generate pedestals, especially through EspFu mechanisms, are able to reverse this effect, which explains the fact that infections with pedestal-forming strains (BA320, KOct1, and KOct2) did not significantly affected the expression of proinflammatory genes compared to uninfected HeLa cells (mock control) ( Fig. 5C and 8).
Collectively, our data demonstrate that genes and pathways involved in inflammation are activated in response to pedestal formation induced by EPEC, especially when mediated by EspFu. Moreover, we also show that EPEC can employ anti-inflammatory mechanisms, as evidenced by the significant downregulation of these proinflammatory genes in epithelial cells infected with a pedestal-deficient strain (Fig. 9).

DISCUSSION
The hallmark of EPEC pathogenesis is the ability to utilize effector proteins to manipulate host cellular processes, leading to intimate bacterial attachment and intestinal colonization (43). However, several facets of these effectors remain unexplored. A large number of EPEC strains, prominently from the O55:H7 serotype, carry the espFu gene (16,18), indicating that EspFu is important for the pathogenesis of this pathotype. This distribution of espFu is interesting, given that EHEC O157:H7, which relies on EspFu for pedestal formation (12), evolved from EPEC O55:H7 (31). Here, we show that in addition for the requirement of EspFu for bacterial attachment and Previous studies demonstrated that isogenic espFu mutants of EPEC (44) and EHEC (45) were less adherent and did not induce robust actin rearrangement on epithelial cells. The introduction of an EspFu-expressing plasmid into a nonadherent strain of EPEC resulted in adherence and pedestal formation on HeLa cells (30). EspFu also increased the adherence of EPEC O125:H6 to human intestinal biopsy specimens in vitro (46) and enhanced the intestinal colonization by EHEC in infant rabbits and gnotobiotic piglets (47). Therefore, it has been proposed that the EspFu-driven pedestal could facilitate actin-mediated movement through the epithelium, enabling transmission to neighboring cells, thus promoting bacterial expansion beyond the original sites of infection and improving epithelial colonization (48).
AE lesion formation is a dynamic process that requires the timely and coordinate expression of the bacterial virulence machinery (49). AE pathogens evolved complex mechanisms to trigger actin polymerization on host cells (50). Here, we show that EspFu-mediated actin polymerization promoted a higher bacterial attachment and pedestal formation in comparison to the Tir:Nck-dependent pathway (Fig. 3). This higher efficiency is probably due to the presence of multiple PRRs domains in EspFu, which allows this effector to bind to more N-WASP molecules than Nck, which has only three SH3 domains (51,52). Surprisingly, the combination of these two mechanisms (EspFu and Tir-phosphorylation) did not increase pedestal formation (Fig. 3 and Fig. S2), suggesting that EspFu-driven actin polymerization is more efficient in association with the nonphosphorylated form of Tir (Tir S ). Our results corroborate previous findings showing that EspFu-expressing EPEC can more efficiently colonize epithelial cells in the presence of Tir EHEC (nonphosphorylated) compared to Tir EPEC (phosphorylated) (48). In addition, one can speculate that the host proteins IRTKS and Nck can compete for binding to Tir due to the proximity of their binding motifs. Thus, Tir-IRTKS binding would be favored in the absence of tyrosine phosphorylation, leading to the recruitment of EspFu and triggering the downstream signaling required for actin polymerization.
The analyses of the transcriptional response of host epithelial cells to AE lesion formation ( Fig. 5 and 8) also demonstrates that many genes involved in immune processes (i.e., inflammation and apoptosis) were differentially expressed in cells in- fected with pedestal-forming EPEC strains, most prominently in response to EspFumediated actin polymerization. Activation of pathways and transcription factors associated with inflammation and apoptosis on epithelial cells required AE lesion formation ( Fig. 5 and 8). Although it is tempting to speculate that the stronger inflammatory response triggered by EspFu-expressing strains was most likely due to an enhanced bacterial association with the epithelium, our data suggest an additional mechanism by which EspFu-mediated actin polymerization can activate inflammation, since cells infected with similar bacterial loads responded differentially to the distinct actin polymerization mechanisms (Fig. S3). However, further studies are still need to better understand this mechanism.
Remarkably, EPEC can also suppress the inflammatory response, evidenced by the strong repression of proinflammatory genes in cells infected with a pedestal-deficient strain (espFu mutant) ( Fig. 5 and 8). Previous studies have demonstrated that NF-B activation is decreased during the course of infection by AE pathogens (53)(54)(55)(56) and that this anti-inflammatory activity depends on a functional T3SS (57). In agreement with this, our in silico analysis identified many effector-encoding genes in the BA320 genome that could be associated with immunomodulation, such as NleB, NleC, NleD, NleE, and NleH. Interestingly, this immunomodulatory activity was more efficiently counterbalanced by the inflammatory response induced by EspFu-mediated actin polymerization. Thus, an interesting future line of research will be to analyze the kinetics of expression and translocation of effectors involved with cytoskeleton rearrangement (such as Tir and EspFu) and immunomodulation during the infection by EPEC strains that employ different actin polymerization mechanisms.
One can speculate that some important observations of this study could be actually due to pairwise comparisons involving strains that are not isogenic (e.g., WT versus KOct1 and KOct2 versus KO). These strains differ regarding location and mode of expression of tir, which could affect the dynamics of infection and, as a consequence, the host response to this process. In fact, it has been shown that the relocation of tir to a plasmid can affect its function and only partially restore the phenotype conferred by this effector (58,59). However, we showed that the expression of Tir BA320 from a plasmid restored the ability of a tir deletion mutant to form actin pedestals to a level similar to that seen in cells infected with WT strain (Fig. 4 and Fig. S2). Thus, our data suggest that the differences observed in this study, including host response to pedestal formation, were more likely due to the different mechanisms of actin assembly triggered rather than the nonisogenic nature of the strains.
In summary, this study links actin-rearrangement through AE lesion formation with modulation of the host immune responses. It also highlights that different actinpolymerization-mediated pathways differentially impact this immunomodulation. The different distribution and combination of Tir and EspFu alleles in EPEC and EHEC pathotypes contributes to the plasticity of these enteric infections.

MATERIALS AND METHODS
Bacterial strains, plasmids, and growth conditions. The bacterial strains and plasmids utilized in this study are listed in Table S1 in the supplemental material. All strains were routinely grown in Luria-Bertani medium (LB) or low-glucose Dulbecco modified Eagle medium (DMEM) at 37°C. When adequate, media were supplemented with ampicillin (100 g/ml), kanamycin (50 g/ml), chloramphenicol (25 g/ml), or streptomycin (100 g/ml). Bacterial stocks were kept on LB supplemented with glycerol 20% (vol/vol) at -80°C.
Nonpolar mutants of espFu and tir in EPEC BA320 (serotype O55:H7) were constructed by using -Red recombination method (60). Briefly, PCR products were amplified from plasmids pKD3 and pKD4 with flanking regions matching espFu and tir, respectively, and were transformed into BA320 expressing the recombinases from plasmid pKD46. Colonies were selected from chloramphenicol or kanamycin LB plates, and the resistance cassette was resolved using flippase from temperature-sensitive plasmid pCP20, which was then cured through growth at 42°C. The nonpolar mutants were then confirmed by sequencing.
For complementations, espFu and tir genes were amplified from BA320 and E2348/69 (EPEC O127:H6) genomic DNAs, respectively, using the primers described in Table S1, and then cloned into pACYC184 under the control of the Tet promoter.
Whole-genome sequencing, assembly, and annotation. A bacterial culture was grown at 37°C overnight and then centrifuged, and the pellet was used for DNA extraction. Total DNA was sequenced  (67), and only assembled plasmids that were also detected by PlasmidSeeker (version 1.0) (68) on total genome assembly were considered valid plasmid assemblies. Genome and plasmid annotations were carried out using Prokka (version 1.14.3) (69).
Growth curve. Overnight cultures in LB were diluted 1:1,000 in 3 ml of low-glucose DMEM on a 6-well plate and then statically grown for 6 h at 37°C under 5% CO 2 . Aliquots (10 l) were collected every 1.5 h, serially diluted in phosphate-buffered saline (PBS), and plated onto LB agar containing selective antibiotics for CFU enumeration. All strains were tested in triplicates, and at least two independent experiments were performed.
Western blotting for secreted proteins. Secreted proteins from cultures grown for 6 h in lowglucose DMEM at 37°C and 5% CO 2 were prepared as previously described (7). Portions (10 g) of bovine serum albumin (BSA) were added to secreted protein samples as a loading control. The proteins were separated by SDS-PAGE, transferred to polyvinylidene fluoride (polyvinylidene difluoride) membranes, probed with rabbit polyclonal anti-EspB serum, and visualized with enhanced chemiluminescence (Thermo Fisher) using the ChemiDoc touch imaging system (software 1.0.0.15) with Image Lab 5.2.1 software for image capture display.
Cell culture and bacterial infections. HeLa (human cervical adenocarcinoma) cells were maintained in high-glucose DMEM supplemented with 10% fetal bovine serum (FBS) and penicillin-streptomycinglutamine and grown at 37°C and 5% CO 2 . The Lifeact::GFP-expressing HeLa cell line was obtained with the Flip-In system (Invitrogen), according to the method of Gruber and Sperandio (49) and maintained in high-glucose DMEM supplemented with 10% FBS, penicillin-streptomycin-glutamine, and hygromycin (50 g/ml). Hygromycin was not added when cells were split before infection.
For infection assays, cells grown overnight to about 80% confluence at 37°C and 5% CO 2 were washed with PBS, kept in fresh low-glucose DMEM supplemented with 10% FBS, and then infected at an MOI of 10, unless otherwise stated, with overnight bacterial cultures statically grown in LB. Infections were allowed to proceed for 6 h at 37°C and 5% CO 2 , being the medium replaced after 3 h. Inoculum inputs were verified by plating onto LB plates containing selective antibiotics.
FAS assay. Fluorescent actin staining (FAS) assays were performed as described by Knutton et al. (79) to examine pedestal formation. HeLa cells were cultivated in 12-well plates with rounded glass coverslips. After 6 h of infection, the cells were washed with PBS, fixed with formaldehyde and permeabilized with 0.2% Triton X-100. The preparations were then treated with fluorescein isothiocyanate (FITC)-labeled phalloidin and 4=,6=-diamidino-2-phenylindole (DAPI) to visualize actin accumulation and bacteria/HeLa DNA, respectively. Slides were mounted with ProLong antifade (Molecular Probes) and visualized with a Zeiss LSM880 confocal laser scanning microscope. Pedestal formation was quantified by randomly imaging different fields of view while recording the number of cells showing actin accumulation foci. At least four fields were enumerated for each condition, with each field containing at least 20 cells. All strains were tested in triplicates and at least three independent experiments were performed.
Live-cell imaging. Lifeact::GFP-expressing HeLa cells were cultured in 35-mm glass-bottom dishes (MatTek) and then infected with mCherry-expressing bacteria (stained in red) at an MOI of 100. Infections were allowed to continue for 2 h at 37°C and 5% CO 2 ; the cells were then washed and visualized by live-cell imaging with an Olympus Fluoview Fv10i confocal laser scanning microscope. Images were taken every 6 min for 2 h.
Quantitative adherence assay. HeLa cells were seeded in 24-well plates, infected for 6 h as described above and then extensively washed with PBS to remove the nonadherent bacteria. Cells were lysed in PBS plus 1% Triton X-100 for 30 min with rocking at room temperature, and recovered bacteria were then serially diluted and plated onto LB plates containing selective antibiotics. Colonies were enumerated after overnight incubation at 37°C. All strains were tested in triplicates and at least three independent experiments were performed.
SEM. Infection assays were performed in 24-well plates with rounded glass coverslips for 6 h as described above and then processed according to the method of Knutton (80) to visualize the bacterial interaction with the cell surface. Briefly, preparations were fixed with a solution of 4% paraformaldehyde and 3% glutaraldehyde in 0.1 M sodium cacodylate buffer (pH 7.2), postfixed with 1% osmium tetroxide, and dehydrated with ethanol (60,70,80,90,95, and 100%). Samples were then subjected to critical point drying with carbon dioxide, mounted on stubs, and coated with a thin layer of gold prior to the visualization under scanning electron microscopy (SEM; QUANTA 250; FEI Company) operating at 12.5 kV and a working distance of 6.6 mm.
Immunofluorescence assay. HeLa cells were cultured in 24-well plates with rounded glass coverslips or 8-well Lab-Tek chamber slides and then infected for 6 h at 37°C and 5% CO 2 . After the infections, the cells were washed with PBS, fixed with formaldehyde, permeabilized with PBS plus 0.2% Triton X-100, and blocked with PBS plus 2% BSA. Samples were then probed with rabbit polyclonal anti-Tir (1:2,000) primary antibodies and Alexa Fluor 566-goat anti-rabbit (Molecular Probes) secondary antibody at a dilution of 1:1,000. Actin and DNA were stained with FITC-phalloidin (1:50) and DAPI (1:2,000), respectively. To detect the phosphorylation of Tir, the preparations were treated with monoclonal antiphosphotyrosine clone PY20 antibody conjugated with FITC (Thermo Fisher) at a dilution of 1:100, and DNA was stained with propidium iodide (1:1,000). Slides were mounted with ProLong antifade and visualized with a Zeiss LSM880 confocal laser scanning microscope.
RNA sequencing library preparation and data analysis. For transcriptomic analysis, HeLa cells were grown in 6-well plates and infected for 6 h at 37°C and 5% CO 2 . Following the incubation period, both infected and uninfected cells were washed with PBS, and total RNA was isolated from biological replicates with an RNeasy minikit (Qiagen) according to the manufacturer's instructions. RNA samples were treated with DNase I (Thermo Fisher) and repurified using RNeasy minikit columns.
A total of 10 g from each DNase-treated RNA sample was processed for sequencing. Briefly, RNA quality and integrity were analyzed on the Agilent 2100 BioAnalyzer (Agilent Technologies). Samples with an RNA Integrity Number (RIN) of Ͼ8 were subjected to an enrichment of polyadenylated RNA, which was used in the preparation of cDNA libraries with TruSeq RNA Sample Prep (Illumina), according to the manufacturer's instructions. cDNA was A-tailed, and indexed adapters were ligated. After adapter ligation, samples were PCR amplified and purified with AMPure XP beads and then validated again on the Agilent 2100 Bioanalyzer. Samples were quantified with the Qubit fluorometer before being normalized, pooled, and then sequenced on the Illumina NextSeq 500 with read configuration as 75-bp, single-end reads. Totals of 25 to 40 million reads were generated for each sample. Two biological replicates for each condition were tested.
Quantitative real-time PCR assays. For RNA-Seq validation, HeLa cells were infected, and RNA samples were isolated with TRIzol reagent (Thermo Fisher) according to the manufacturer's instructions. A total of 1 g of DNase-treated RNA was reverse transcribed to cDNA by using a SuperScript III kit (Thermo Fisher) with random primers. The diluted cDNAs were mixed with validated primers (Table S2) and SYBR green mix, and the reactions were then cycled in 384-well plates on the QuantStudio 6 Flex system (Applied Biosystems). Data were collected using QuantStudio real-time PCR software (Applied Biosystems). All data were normalized to the levels of the beta-2 microglobulin (B2M) gene and then analyzed using the comparative cycle threshold method (ΔΔC T ).
Statistical analysis. Statistical significance was determined by unpaired Student t test or one-way analysis of variance (ANOVA [for multiple comparisons]). A P value of Ͻ0.05 was considered significant.
Data availability. This whole-genome shotgun project has been deposited at DDBJ/ENA/GenBank under accession no. NZ_SGUH00000000. The RNA-Seq data can be accessed using accession no. GSE141446 at the NCBI GEO database.

ACKNOWLEDGMENTS
We thank Don Gammon and Emily Rex for their help with live-cell imaging experiments, the UT Southwestern Live-Cell Imaging Facility Core for the assistance with confocal microscopy, and the UT Southwestern McDermott Center Next Generation Sequencing (NGS) for the RNA-Seq analysis.
This study was supported by NIH grants AI0530167, AI05135, AI077613, and 572