- Research article
- Open Access
Molecular adaptation of a plant-bacterium outer membrane protease towards plague virulence factor Pla
© Haiko et al; licensee BioMed Central Ltd. 2011
Received: 7 October 2010
Accepted: 11 February 2011
Published: 11 February 2011
Omptins are a family of outer membrane proteases that have spread by horizontal gene transfer in Gram-negative bacteria that infect vertebrates or plants. Despite structural similarity, the molecular functions of omptins differ in a manner that reflects the life style of their host bacteria. To simulate the molecular adaptation of omptins, we applied site-specific mutagenesis to make Epo of the plant pathogenic Erwinia pyrifoliae exhibit virulence-associated functions of its close homolog, the plasminogen activator Pla of Yersinia pestis. We addressed three virulence-associated functions exhibited by Pla, i.e., proteolytic activation of plasminogen, proteolytic degradation of serine protease inhibitors, and invasion into human cells.
Pla and Epo expressed in Escherichia coli are both functional endopeptidases and cleave human serine protease inhibitors, but Epo failed to activate plasminogen and to mediate invasion into a human endothelial-like cell line. Swapping of ten amino acid residues at two surface loops of Pla and Epo introduced plasminogen activation capacity in Epo and inactivated the function in Pla. We also compared the structure of Pla and the modeled structure of Epo to analyze the structural variations that could rationalize the different proteolytic activities. Epo-expressing bacteria managed to invade human cells only after all extramembranous residues that differ between Pla and Epo and the first transmembrane β-strand had been changed.
We describe molecular adaptation of a protease from an environmental setting towards a virulence factor detrimental for humans. Our results stress the evolvability of bacterial β-barrel surface structures and the environment as a source of progenitor virulence molecules of human pathogens.
Analyses of genomic sequences of bacterial pathogens have given an unprecedented view into their biology and evolutionary processes [1, 2]. A conclusion from these studies is that highly similar genes, many of which are associated with bacterial virulence, are found across great phylogenetic distances and in different genetic elements, which is indicative of horizontal gene transfer. These families of virulence factors - including toxins, transport systems, adhesins, and antibiotic resistance factors - have evolved by adaptive radiation of a functional progenitor molecule to and within other strains and species to support survival in differing ecological niches . The adaptation, or "evolutionary fine-tuning" of virulence factors that results in increased fitness, can involve modification of catalytic efficiency or substrate specificity of an enzyme, or alteration of bacterial interactions with target cells . The mechanisms of horizontal gene transfer and the functional diversity of bacterial toxin families and protein transport systems have been documented [2–4] but adaptive molecular evolution of bacterial virulence factors remains less understood in terms of altered structure/function relationships.
Yersinia pestis is the causative agent of plague, a zoonotic disease transmitted to humans usually by the bite of an infected flea . The bacterium spreads from the intradermal infection site into lymph nodes, causing bubonic plague, and subsequently to blood and to lungs, leading to pneumonic plague. The abilities to disseminate in the host and to cause high bacteremia are central for the transmission of the bacterium by the flea vector which feeds on contaminated blood. Y. pestis has been responsible for three human pandemics, which are estimated to have resulted in deaths of ca. 200 million humans . As a bacterial species Y. pestis is young, and recent population genetic studies have shown that the bacterium diverged from its ancestral species, the gastrointestinal pathogen Yersinia pseudotuberculosis, only ca. 13 000 years ago [6, 7]. The genome of Y. pestis has evolved through gene decay, recombination, single nucleotide changes, genome rearrangements, and horizontal gene transfer by acquisition of two Y. pestis-specific plasmids, of which the plasmid pPCP1 (pPst/pPla) potentiates bacterial dissemination from the primary intradermal infection site into lymph nodes [8, 9]. The decisive virulence factor encoded by pPCP1 is the surface protease plasminogen activator Pla. Deletion of pla attenuates Y. pestis millionfold in subcutaneously infected mice, whereas no difference is seen in intravenously infected mice . Pla is specifically needed for establishment of bubonic plague [10, 11], and a critical role of Pla has been described in pneumonic plague where it enables localized growth of Y. pestis in the lungs .
Pla belongs to an outer membrane protease family of omptins that have been detected in several Gram-negative bacteria of different phylogenetic groups; these bacteria commonly infect animals or plants . The omptin genes have spread through horizontal gene transfer by different mechanisms, and at least 16 members are known to date [13–16]. As omptin sequences are over 50% identical, they very likely fold similarly to the two structurally resolved members of the family, OmpT of E. coli  and Pla of Y. pestis . Both OmpT and Pla form a 70-Å long β-barrel of elliptical cross-section with ten antiparallel transmembrane β-strands, five surface-exposed loops (L1-L5) and four short periplasmic turns (T1-T4). The catalytic residues and the acidic, substrate-binding pocket, as well as the lipopolysaccharide-binding site are conserved in omptins [13, 17, 19]. This is in accordance with the finding that the cleavage site preferences of omptin proteolysis, analyzed mostly with short peptide substrates, are very similar: omptins cleave after basic residues, preferably between two basic amino acids [20–23]. With larger substrates, however, omptins are functionally diverse, and their genes have undergone adaptive evolution to support the life style of the bacterial host [14, 15, 24]. Insertions and deletions that give slight variation in the molecular sizes of omptins are mostly located in the solvent-accessible surface structures L1-L5, and the differential substrate selectivities of individual omptin proteases appear to be dictated by these surface loops, as observed by loop swapping and omptin chimeras [16, 19, 25, 26].
During infection, Pla seems to increase virulence mainly by interfering with the human plasminogen/fibrinolytic system that is critical in cell migration across tissue barriers. Pla cleaves the circulating, abundant zymogen plasminogen by a single cut to active plasmin  and also degrades two natural inhibitors of the plasminogen system, the serpins α2-antiplasmin (α2AP) and plasminogen activator inhibitor 1 (PAI-1) [16, 19]. Altogether, these activities result in uncontrolled plasmin activity. Plasmin is a broad-substrate protease involved in a number of (patho)physiological processes, of which fibrinolysis and damage of extracellular matrices contribute to bacterial dissemination within the host [12, 27, 28]. Pla has also non-proteolytic functions: it mediates invasion of Y. pestis into human epithelial and endothelial cells by an unknown mechanism as well as into mouse monocytes by binding to CD205 [29–31]. The Epo omptin is a close homolog of Pla, exhibiting 77% sequence identity, and it is encoded on a plasmid of the plant pathogen Erwinia pyrifoliae that causes tissue-destructive infection in pear trees . The functions of Epo in plant pathogenesis have not been systematically studied, but serpinolytic activity in vitro was recently shown .
The claim of directed evolution and adaptive molecular evolution is that natural selection generates particularly evolvable enzymes in response to rapidly fluctuating selective conditions and that proteins that require fewest mutations to adapt to novel conditions are the most likely to survive environmental changes . Evolvability has been argued to be a function of robustness, i.e., the capacity of a protein to withstand sequence variations without disruption of its binding or catalytic properties [33, 34]. Mutational robustness is dependent on a protein's intramolecular interactions, and the omptin molecule fulfils the criteria of an evolvable protein as defined by O'Loughlin et al. ; the β-barrel is a sturdy membrane-embedded molecule with flexible surface loops that can tolerate deletions and insertions without compromising molecular stability [35, 36]. Manifestations of the robustness of omptins include their unhurt catalytic activity after autocatalytic cleavage at L4 and the proteolytic specificity of omptin loop chimeras, which together have indicated that the five loops offer a flexible scaffold for recognition of different substrates [16, 19, 25, 26].
Evolutional studies on bacterial virulence factors highlight the importance of environment as an immense reservoir of evolvable potential progenitors of virulence factors . Pla of Y. pestis and Epo of E. pyrifoliae belong to the same subfamily of omptins which also contains the omptins PgtE of Salmonella enterica, Kop of Klebsiella pneumoniae, and the omptin of Enterobacter [15, 16]. These bacterial species infect mammals or plants or both, and have encountered mutual horizontal gene transfer. In this study we used the existing knowledge of omptin structure and function as a starting point for substitutional analysis, and addressed two specific questions on molecular adaptation: how many substitutions are needed and at which locations in Epo to gain a proteolytic function (plasminogen activation) and a non-proteolytic function (invasiveness) expressed by Pla.
Substrate selectivity of Pla and Epo towards virulence-associated human proteins
Construction of Pla-Epo hybrid proteins
Bacterial strains and plasmids used in this study
Bacterial strain or plasmid construct
Escherichia coli XL1 Blue MRF'
Δ(mcrA) 183 Δ(mcrCB-hsdSMR-mrr) 173 endA1 supe44 thi-1 recA1 gyrA96 relA1 lac [F' proAB lacI q ZΔ M15 Tn 10 (tet)]
Expression vector, trc promoter, lacO operator, lacI, bla
pla in pSE380
epo in pSE380
Pla with 5 aa from Epo: 161 KGVRV→NQRPG
Epo with 5 aa from Pla: 159 NQRPG→KGVRV
Pla with 10 aa from Epo: 161KGVRV→NQRPG, 262 KN→TI, 268 VSIG→ASLD
Epo with 10 aa from Pla: 159NQRPG→KGVRV, 260 TI→KN, 266 ASLD→VSIG
Pla with 17 aa from Epo: 35 ETG→SNA, 88 MNE→QNS, 155 YT→SV, 161KGVRV→NQRPG, 262KN→TI, 268VSIG→ASLD
Epo with 17 aa from Pla: 33 SNA→ETG, 86 QNS→MNE, 153 SV→YT, 159NQRPG→KGVRV, 260TI→KN, 266ASLD→VSIG
Epo with 31 aa from Pla: 33SNA→ETG, 86QNS→MNE, 153SV→YT, 159NQRPG→KGVRV, 260TI→KN, 266ASLD→VSIG, 26 KELV→HEML, 101 GTDVNY→ATNVNH, I257T, H79N, D92E, S210D, S167N, D219G, E249D, G22S
Epo with 42 aa from Pla + the signal sequence: N-terminus from Pla until aa 45; the rest similar to pMRK431
Epo with the N-terminus from Pla until aa 45
pMRK410 with the N-terminus from Pla until aa 45
pMRK417 with the N-terminus from Pla until aa 45
pMRK431 with β2 from Pla
pMRK431 with β4 from Pla
pMRK431 with β5 from Pla
pMRK431 with β8 & β9 from Pla
pMRK431 with β10 from Pla
Plasminogen activation by Pla-Epo hybrid proteins
The stepwise accumulation of substitutions onto the Epo molecule was continued onwards from pMRK417 to pMRK431, where all 31 residues that differ between Epo and Pla and that are located on the extracellular side of the outer membrane on the protein have been substituted towards Pla. These substitutions in Epo did not change the cumulative plasminogen activation or the fragmentation pattern of plasminogen (data not shown). We recently reported that the single substitution I259T at loop 5 differentiates Pla of the pandemic Y. pestis lineages (which have PlaT259) from the Pla isoform of the ancestral lineages (PlaI259). This substitution decreases Pla-mediated cleavage of plasmin light chain that contains the catalytic domain, and thus increases the stability of the formed plasmin . An increase in plasmin stability and formation of the plasmin light chain after the I259T substitution was also observed in the series of Pla-Epo hybrid proteins in the present study.
Molecular environment of the substituted sites in Pla structure and Epo model
N159, Q160, p158
H101, a143, g145, i166
S210, t212, d259
t257, V268, a274
The five residues of the first substitution site are the longest consecutive difference between Pla and Epo. In the Pla structure, V163 at L3 packs together with apolar residues P160 at L3 and M210 at L4 at the inside of the barrel, while the L3 residues N159, Q160, and R161 in Epo point towards the water phase (Figure 5). The distinct functional effect of pMRK405 substitutions could well reflect changes in size of the binding pocket and differences in the electrostatic properties of the substrate docking surface.
The incremental substitutions of pMRK410 occur in L5. K262 and N263 are located in the very tip of L5, and in the Pla structure, both residues are in contact with L4. Most intriguingly, N263 forms a hydrogen bond with Pla-specific D212 in L4. Such an interaction is not possible between the corresponding residues in Epo, S210 and I261. Moreover, K262 of Pla points towards E207 in β7. This glutamate, and the threonine and the tyrosine hydrogen-bonded to it are identical in Pla and Epo, but the polar triplet at the outside of the barrel gets extended and strengthened in Pla by K262 (L5) from one side and by R164 (L3) from the other (Figure 5). The corresponding Epo-residues T260 and P162 are decisively smaller, and do not reach to the L4 residues. pMRK410 construct also includes swapping of 268VSIG/266ASLD in L5. These residues lie in a small β-structure , supposedly in the aqueous phase above the lipopolysaccharide layer. The residues in both proteins form similar interactions with their neighbors in same loop, except the Epo-specific D269 that in the model hydrogen bonds to a backbone carbonyl in the β1-strand. The end of loop L5 and the beginning of L1 are rather irregular; both areas differ between Pla and Epo, and a side chain-backbone hydrogen bond would stabilize the loops relative to each other. In the Pla structure, L1 residues D33-R38 form a network of hydrogen bonds.
Serpinolytic activity of Pla-Epo hybrids
Turning Epo into an invasin
Results of the invasion assay
Average invasion percentage
Number of assays
Erwinia species and Y. pestis colonize different habitats and have a very different pathogenic potential for humans. Bacterial virulence is normally dependent on several factors, and presence of Pla, although it is an exceptionally multifunctional and powerful virulence factor [8, 10–12, 16, 19, 26–28, 30, 31] does not alone explain the devastating virulence of Y. pestis. Our study however gives an example of how a single, specific virulence factor of the plague bacterium might have structurally adapted to its present form. Our results do not give a direct roadmap to the Pla molecular structure but rather describe how easily the substrate specificity of an omptin can evolve and how functions that are pathogenic in a novel environment can be gained. The role of surface loops in Pla proteolysis has earlier been documented by loop swapping [16, 26], and our results extend these findings by a more detailed substitutional analysis and by also conferring invasiveness onto a close ortholog of Pla.
Serpins are important regulators of cellular proteolysis and share structural features, which include a similar, exposed reactive center loop that binds to and inhibits the catalytic center of target proteases . The omptins in the Pla subfamily all cleave specifically the reactive center loop of the PAI-1 . Here we found that Epo can cleave the serpin α2AP, which is a shared target of Pla and PgtE [19, 41]. These findings indicate that serpinolytic activity is a common function in the Pla subfamily of omptins and might give selection advantage for survival and spread of bacteria in their hosts by increasing proteolysis in tissues. In contrast, omptins of the OmpT subfamily, OmpT of E. coli and SopA of Shigella, do not cleave PAI-1, despite high sequence similarity, conserved fold and active site structure . It is interesting to note that the Pla-Epo hybrid proteins encoded in pMRK405, pMRK410, and pMRK417 were more efficient than Pla or Epo in PAI-1 degradation. Also, further substitution towards Pla, encoded in pMRK431 and pMRK431β1, led to hybrid proteins that exhibited an activity similar to that of Pla and Epo. Acquisition of novel substrate specificities by proteases often leads to broad-specificity variants by initially favoring mutations that increase the conformational flexibility and destabilize specialized active site structures. thus reducing specificity for the original targets . The observation that intermediate Pla-Epo hybrid proteins were more efficient in PAI-1 degradation is in line with the assumption that serpinolytic activity is a property of a progenitor omptin in this subfamily and that Pla and Epo have diverged from this progenitor to have novel functions. The structural explanation for the increased efficiency is however unknown. The activating cleavage in plasminogen occurs between the R-V bond, while in PAI-1 and probably also in α2AP the cleavage occurs between R-M in the reactive center loop. Specialization to plasminogen cleavage by Pla seems to correlate with several stabilizing interactions between the surface loops, formed by Pla-specific residues.
A molecular explanation for the altered plasminogen activation encoded by pMRK410 remains speculative without more specific molecular data about omptin-target complexes, and more generally, because the in vivo mobility of the surface structures of the omptin barrel. Still, the structural analysis presented here suggests a possible explanation. Most importantly, we see multiple loop-loop interactions involving Pla-specific residues. These would result in reduced loop flexibility and a better defined binding pocket, promoting productive substrate binding. Second, we see a binding pocket altered in size and hydrophobicity. The pMRKX05 (where X is either 1 or 4) substitutions 161 KGVRV/NQRPG occur at one long end of the elliptical barrel opening, and the 268VSIG/ASLD at the other. This seems to imply that the polypeptide substrates bind across the long axis of the omptin pore, and the pMRKX10 mutations change the docking surface. Altogether, the Pla structure seems to allow close approach by the substrate, and the active site to be well stabilized by interloop interactions. Assuming this is the reason for the observed differences in plasminogen cleavage versus serpinolysis, it means that plasminogen binding and cleavage require a "preformed", tighter binding pocket.
The protein sites identified in this study enable the omptin to initiate activating cleavage of plasminogen but further substitutions are needed to stabilize plasmin. Swapping of loops between Pla and PgtE of S. enterica has revealed that L5 and the N-terminal region including L1 are crucial for the gelatinase activity by PgtE . The same regions and in addition L3 seem to be important in the activation of pro-matrix metalloproteinase 9 by PgtE . A residue deserving special attention is T259 of Pla, which is situated in L5 and faces into the barrel opening next to F215. We recently described that a single substitution at this site, T259I that is typical for ancestral Y. pestis lineages, increases the cleavage of the light chain of plasmin, thus decreasing the stability of the formed plasmin . The conservation of this mutation in pandemic isolates indicates that pla, after being acquired by Y. pestis, has evolved through a single nucleotide change to better support plasmin formation. The pPCP1 plasmid also encodes pesticin and pesticin immunity protein and is evolutionary related to colicin plasmids, in particular pColE1. It is possible that the pPCP1 plasmid has evolved through fusion of a pla progenitor gene and a ColE1-like plasmid.
The omptins autoprocess themselves at different protein sites . Formation of β-Pla-like peptide by Epo hybrid proteins was detected by E. coli expressing pMRK431 that encodes the substitution of all 31 differences between Pla and Epo at their surface-exposed parts. This indicates that autoprocessing is dependent on surface loops. Unexpectedly, these substitutions only slightly improved the invasiveness of recombinant E. coli. This indicates that the proteolysis and the invasiveness involve different regions of the omptin molecule and that the invasiveness, which among omptins has been detected only with Pla , is a more complex function than the proteolytic specificity. The plasmid pMRK431β1, constructed from pMRK431 to also encode the amino terminal residues 1-45 containing the β1-strand, induced similar level of invasiveness as seen with E. coli pMRK1. However, Pla amino terminus alone in Epo did not convert Epo to an invasin. At present we do not have an explanation for the requirement of transmembrane regions to induce invasion by Epo. Our hypothesis was that this might indicate TonB-dependency in invasion. TonB functions in energy coupling between the cytoplasmic and the outer membrane and is important in transport functions across the bacterial cell wall . The Pla and Epo sequences contain a homolog to the TonB box  at the amino terminus (11DSFTVAA in Pla and 9DSISVAT in Epo). A role for TonB in Pla-mediated invasion however seems unlikely, as expression of Pla or Epo in a tonB-deletion of E. coli XL1 mutant did not alter their invasiveness (T. Lehti and J. Haiko, unpublished). One possibility is that invasion requires membrane fusion which could differ between Epo and Pla, as outer membrane β-barrels are known to vary in their incorporation into different lipid micelles . It is also possible that changes in membrane-embedded residues have subtle effects on the orientation and activity of surface residues that make contact with the target cell. Finally, as a molecular event invasion is complex and may require several steps (adhesion, membrane fusion, host cell responses) that involve more than one omptin protein region. This is in line with the finding that extensive substitution was required to induce invasiveness into Epo.
Bacterial strains and plasmids
Bacterial strains and plasmids are listed in Table 1. pla and epo were available from previous work [19, 26]. Derivatives of pla and epo were cloned by recombinant two-step PCR as described earlier [19, 25] and expressed in the inducible pSE380 vector in E. coli XL1-Blue MRF as described earlier [19, 37]. The nucleotide sequences were confirmed by sequencing. The recombinant E. coli strains were cultivated overnight at 37°C in Luria broth (10 ml) supplemented with glucose (0.2% wt/vol), ampicillin (100 μg/ml), and tetracycline (12.5 μg/ml). For protein expression, the culture was pelleted, suspended in 150 μl of phosphate- buffered saline (PBS, pH 7.1), and plated on Luria plates containing 5 μM isopropyl-β-D-thiogalactopyranoside (IPTG) and antibiotics as described above. For the assays, bacteria were collected in PBS, pelleted, and adjusted to an optical density at 600 nm of 1.2 (corresponding to ca. 109 cells/ml) or 2.0 (2 × 109 cells/ml).
Human Glu-plasminogen (4 μg; American Diagnostica), was mixed with 8 × 107 bacteria in PBS in a total volume of 174 μl in microtiter plate (Nunc) wells, and 30 μl of the chromogenic plasmin substrate Val-Leu-Lys-p-nitroaniline dihydrochloride (S-2251, 2.5 mg/ml; Chromogenix) was added. Plasmin formation at 37°C was measured in a microtiter plate reader at 405 nm.
Degradation of α2-antiplasmin and plasminogen
Cleavage of human α2AP (0.8 μg; Calbiochem) was tested as detailed earlier [19, 41], by using 3 × 107 bacteria and the incubation for 2 h at 37°C. Plasminogen degradation with anti-human plasminogen antibody (American Diagnostica) was assessed by incubating 2.5 μg human Glu-plasminogen and 4 × 107 bacteria in PBS for 2 h shaking at 37°C. The cells were pelleted, and the supernatants were boiled with SDS-PAGE loading buffer. Samples (10 μl) were run in a 12% (wt/vol) SDS-PAGE gel and transferred onto a polyvinylidene difluoride membrane (GE Healthcare). The detection was done with polyclonal anti-human plasminogen antibody (1 mg/ml, diluted 1:1000), peroxidase-conjugated anti-rabbit IgG (1:2500; GE Healthcare), and enhanced chemiluminescence detection reagents (GE Healthcare) according to the manufacturer's instructions. The membrane was exposed to X-ray film (Agfa) for 15 s. In assays where plasminogen cleavage was detected with monoclonal anti-human plasminogen catalytic domain antibody (R&D Systems), the following modifications were made: Glu-plasminogen (3 μg) and 4.8 × 107 bacteria were incubated for 3 h. After incubation, supernatant samples of 15 μl were electrophoresed and detection was done with the monoclonal antibody (500 μg/ml, diluted 1:500) and peroxidase-conjugated anti-mouse IgG (GE Healthcare; 1:1000). The exposure time was 5 min.
Degradation of PAI-1/vitronectin complex
Recombinant active human PAI-1 (2.5 μg; American Diagnostica) and human plasma Vn (5 μg; Promega) were incubated for 1 h at 37°C in a volume of 5 μl to form a complex . Bacteria (20 μl, 4 × 107 cells) in PBS were incubated with the complex for 2 h at 37°C. The bacteria were pelleted, and the supernatants were run in a 12% (wt/vol) SDS-PAGE gel, and PAI-1 and Vn were detected by Western blotting with polyclonal anti-PAI-1 (1:5000, Calbiochem) or anti-Vn (1:1000, Calbiochem) antibodies, alkaline-phosphatase-conjugated anti-rabbit immunoglobulin G (Dako) and phosphatase substrate.
Detection of Pla-Epo hybrids with anti-Pla, anti-Epo, and anti-Pla loop sera
The cell envelope samples were made by sonicating bacteria (109 cells/ml) in PBS on ice with 2.5 mM ethylene diamine tetra-acetic acid (EDTA). The remaining cells were pelleted, and the supernatants were centrifuged further. The cell envelopes in the supernatants were pelleted and suspended in PBS and SDS-PAGE loading buffer. Whole-cell samples were made by boiling the bacteria (109 cells/ml) with SDS-PAGE loading buffer, and the samples were loaded into a 12% (wt/vol) SDS-PAGE gel, electrophoresed, and transferred onto a nitrocellulose membrane. The proteins were detected with a mixture of anti-His6-Pla antiserum, antipeptide sera against Pla loops 3 and 5 , and anti-His6-Epo antiserum (1:1000). The detection was done with alkaline-phosphatase-conjugated anti-rabbit immunoglobulin G (IgG; Dako) and phosphatase substrate.
Invasion into ECV304 cells
Endothelial-like ECV304 cell line was cultivated in Medium 199 (Gibco) supplemented with 10% fetal calf serum (Gibco) and 2 mM L-glutamine (Gibco) and grown at 37°C with 5% CO2 for 3-4 days. Bacterial invasion into ECV304 cells was studied using gentamicin protection assay . ECV304 cells were grown at 24-well plate (Nunc) for 3-4 days. The eukaryotic cells were washed with PBS and Medium 199 was added. Bacteria (105 cells) in Medium 199 were added, and the plate was centrifuged (128 × g, 10 min). The cells were incubated at 37°C with 5% CO2 for 2 h. The wells were washed with PBS, and the extracellular bacteria were killed with gentamicin (100 μg/ml). ECV304 cells were lysed with 0.2% Triton X-100, and the number of intracellular bacteria was determined by viable counting. The invasion percentages were calculated by comparing the amount of the bacteria incubated with the eukaryotic cells to the amount of intracellular bacteria.
Molecular modelling of protein structures
We thank Raili Lameranta and Janne Tynell for technical assistance and Enni Korhonen and Jaakko Lyytinen for help in statistical analysis. This work was financially supported by the European Union Network of Excellence EuroPathoGenomics program (grant number CEE LSHB-CT-2005-512061), Research Foundation of the University of Helsinki, Viikki Graduate School in Molecular Biosciences, Magnus Ehrnrooth Foundation, and the Academy of Finland (grant numbers 116507 and 130202).
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