Bacterial strains, plasmids and growth conditions

Bacterial strains and plasmids can be viewed in Table S1. We consistently used Y. pseudotuberculosis YPIII/pIB102 (serotype III) as the parental strain. pIB102 is a virulence plasmid encoding for the Ysc-Yop T3SS and is a variant of cryptic pIB1. It differs only by a kanamycin resistance cartridge inserted into the yadA gene, which does not reduce the pathogenicity of YPIII/pIB102 in mouse models [27]. The strain also harbors an internal duplication within phoP located on the chromosome. This is predicted to generate an inactive truncated variant of the PhoP response regulator that impairs bacteria growth and survival inside macrophages [28]. Bacteria were normally cultivated in Luria-Bertani (LB) agar or broth at either 26°C (Y. pseudotuberculosis) or 37°C (E. coli) with aeration. When examining transcription and translation from rovA and inv, bacteria were grown at both 26°C and 37°C in LB broth to late stationary phase. These conditions were selected on the basis that reports from other laboratories have clearly established the peak rovA and inv expression occurs in bacteria grown at low temperature to stationary phase [22], [24]. Where required, antibiotics were added at the final concentrations of carbenicillin (Cb; 100 µg per ml), kanamycin (Km; 50 µg per ml), Trimethoprim (Tp; 10 µg per ml) and chloramphenicol (Cm; 25 µg per ml).

Mutant construction

To construct individual in-frame deletions, site-directed amino acid substitutions and nucleotide ‘shuffle’ mutations, we applied the standard overlap PCR technique using the relevant primer combinations listed in Table S2. To facilitate the sequencing process (performed by MWG Biotech AG, Ebersberg, Germany), all amplified fragments were initially cloned into pCR®4-TOPO TA (Invitrogen AB, Stockholm, Sweden). Confirmed fragments were then lifted into the mutagenesis vector, pDM4. These mutagenesis constructs were then conjugated by E. coli S17-1λpir into Y. pseudotuberculosis. Mutated alleles were initially introduced into the recipient genome by a single cross-over event. A second single cross-over event followed to secure the complete allelic exchange, which was initially screened for on the basis of sacB-dependent sucrose sensitivity [19], [29]. The presence of the mutated allele in the Y. pseudotuberculosis genome was then confirmed by diagnostic PCR and sequence analysis of the amplified regions flanking the mutation.

Western blotting

Protein derived from lysates of the bacterial pellet was fractionated by 12% (for invasin) or 15% (for RovA) SDS-PAGE. Protein was then transferred to Schleicher and Schuell Protran® nitrocellulose (GE Healthcare) using a Hoefer semi-dry transfer assembly. Proteins of interest were bound with specific rabbit polyclonal antibodies that were a gift from Petra Dersch (anti-RovA), Hans Wolf-Watz (anti-invasin), Thomas Silhavy (anti-MBP-CpxR) or Shu-ichi Nakayama (anti-CpxR). These were then detected with an anti-rabbit monoclonal antibody conjugated with horse radish peroxidase (GE Healthcare) and a homemade chemiluminescent solution.

nlpE cloning and expression

The primer combination for PCR amplification of Y. pseudotuberculosis nlpE is listed in Table S2. The DNA fragment was cloned into pBAD18 [30] using EcoRI/XbaI restriction to generate pJF027. This placed nlpE expression under arabinose control. The nlpE allele from E. coli cloned under arabinose control in pBAD18 (termed pND18) was a gift from Thomas Silhavy. These two constructs along with the vector control were electroporated into Yersinia. To induce nlpE expression, overnight bacterial cultures were used to seed fresh growth medium supplemented with 0.2% (w/v) L-arabinose and appropriate antibiotic selection.

Cloning, expression and purification of CpxR variants

Alleles encoding CpxR wild type and the CpxR_D51A and CpxR_M199A variants were amplified with gene specific primers (Table S2) using template DNA derived from parental Y. pseudotuberculosis or the respective mutants and cloned with NdeI and XhoI in front of the IPTG inducible promoter of pET22b(+). These expression plasmids were maintained in E. coli BL21(DE3) plysS allowing for the IPTG-inducible expression of individual CpxR variants fused to a C-terminal His₍₆₎ tag. Recombinant protein was purified as previously described [20].

Electrophoretic mobility shift assay (EMSA)

³²P end-labeled forward primers listed in Table S2 were used for the PCR amplification of the promoter regions of cpxR/P, rovA, ppiA, ail, ail-like, inv, psaA and psaE. The amplified DNA fragments were purified by agarose gel electrophoresis. Purified CpxR was mixed with the DNA fragments (∼2 to 5 nM) in a 20 µL reaction volume containing 20 mM Tris-HCl pH 7.0, 30 mM Acetyl phosphate, 125 mM KCl, 10 mM MgCl₂, 1 mM EDTA, 1 mM dithiothreitol, 0.25 mg per ml BSA and 5 µg per ml sonicated salmon sperm DNA. BSA corresponding to the highest CpxR concentration (1.5 µM) was used as a negative control, and about 7 fold excess of unlabeled PCR amplified DNA was used in a competition reaction. After incubation at 30°C for 1 h and addition of the DNA dye solution (40% glycerol, 0.05% bromophenol blue, 0.05% xylene cyanol), the mixture was loaded directly onto a pre-run 5% polyacrylamide gel. Gel electrophoresis was performed in 1× TBE at 100 V for 2 h at 4°C. After gel drying, signals were detected by autoradiography with a Storm 860 PhosphorImager (Molecular Dynamics).

DNase 1 footprinting assay

The primers pE-rovAfor3, pE-ppiAfor, pcpxRb and pcpxRfor were radioactively labeled with ³²P using γ³²P-ATP (Perkin Elmer) and T4 polynucleotide kinase (Fermentas). The labeled pE-rovAfor3, pE-ppiAfor and pcpxRb were paired with unlabeled pE-rovArev3, pE-ppiArev and pcpxPb respectively and used to PCR amplify promoter regions of rovA (314 bp), ppiA (276 bp) and the divergent cpxR-cpxP (245 bp). For a control, the labeled pcpxRfor was paired with unlabeled pcpxRrev for the PCR amplification of an internal region of cpxR (389 bp). Subsequently, 1.5 nM of the amplified DNA fragments and 0, 50, 100, 200 and 400 nM acetyl∼P phosphorylated CpxR_wt::His₆ were mixed in a 40 µL reaction containing 25 mM Hepes (pH 8), 100 mM potassium glutamate, 0.5 mg/mL BSA. After incubation of the reaction mixture at room temperature for 10 minutes, 4 µl DNase 1 (0.0005 mg/mL; Sigma) was added and the reaction was left for 80 seconds at 37°C. The DNase 1 digestion was stopped by addition of phenol/chloroform and 200 µL DNase 1 STOP (0.4 M sodium acetate (pH 5), 2.5 mM EDTA, 10 ug/mL herring sperm DNA), and then the DNA was precipitated using ethanol. Samples were analyzed on a 7% denaturing polyacrylamide gel and visualized with a Storm 860 PhosphorImager (Molecular Dynamics).

Visualization of phosphorylated CpxR (CpxR∼P)

Purified CpxR variants labeled with acetyl∼P were mixed with 2× loading buffer (0.02% (w/v) Bromophenol blue, 20% (v/v) Glycerol). For analysis, samples were either fractionated on a SDS-12%-PAGE or a Manganese(II)-Phos-tag™ (33 µM) 12.5% acrylamide gel. Purified CpxR∼P was detected by the Pro-Q® Diamond phosphoprotein gel staining method as described by the manufacturer (Invitrogen). To confirm equal loading, subsequent detection of total protein present on the same gel was revealed by SYPRO® Ruby staining (Invitrogen). In both cases, fluorescent output was recorded using a Fluor-S™ MultiImager (BioRad) and band intensity quantified with Quantity One® quantitation software version 4.2.3 (BioRad). The presence of recombinant purified CpxR∼P or that which is produced endogenously and present in bacterial lysates was also assessed by coupling Manganese(II)-Phos-tag™ acrylamide gel fractionation to immunoblotting with monospecific polyclonal anti-CpxR antiserum. The Manganese(II)-Phos-tag™ approach is an affinity based system for the recognition and separation of anionic substrates, such as phosphorylated proteins, during polyacrylamide electrophoresis [31]. For example, characteristic separation patterns for phosphoprotein isoforms can be generated according to the number and or site of the phosphate group. As a result, it later proved to be routinely applicable to in vitro and in vivo visualization of TCRS response regulator aspartate phosphorylation [32]. Samples for this analysis were generated from pelleted bacteria vigorously resuspended in 1.2 M formic acid preceding a very brief incubation at room temperature. Prior to fractionation, lysates were solubilized by addition of 4× loading buffer (250 mM Tris-HCl pH 6.8, 8% SDS, 40% glycerol, 4% BME, and 0.08% Bromophenol Blue,) and neutralized by the addition of minuscule amounts of 5 M NaOH.

Biophysical analysis of intact and digested CpxR∼P

The reduction of CpxR∼P using sodium borohydride was performed as described previously [33], [34]. Before the reaction, CpxR∼P was desalted using C₁₈ micro columns and dried by vacuum centrifugation [35], [36]. Controls were performed using unphosphorylated CpxR under identical conditions.

Intact mass determination of CpxR and CpxR∼P utilized purified recombinant CpxR, and this CpxR phosphorylated with acetyl∼P. Duplicate samples of both phosphorylated and non-phosphorylated CpxR were then desalted on homemade C₁₈ columns [35], [36]. For analysis by ESI-MS, the proteins were dissolved in 50% (v/v) acetonitrile containing 0.5% (v/v) formic acid. ESI-MS spectra of intact CpxR and CpxR∼P were acquired by ESI-MS in the positive ion mode using a Q-Tof ultima mass spectrometer (Waters, Manchester, UK). Spectra were acquired off-line using nano spray capillaries (Q-tof) from Proxeon (Odense, Denmark) and deconvoluted using the MassLynx 4.0 software.

Peptides of CpxR and CpxR-P were prepared using trypsin and pepsin. Protein was desalted using C₁₈ micro columns and dried by vacuum centrifugation [35], [36]. In-solution digestion using trypsin was performed for 40 min at 37°C in 10 µl of fresh 50% ammonium bicarbonate containing 10 ng/µl of sequencing grade trypsin (Promega Biotech AB, Nacka, Sweden). In-solution digestion using pepsin (pepsin from porcine gastric mucosa, Sigma Life Sciences) was performed for 40 min at 37°C in 20 µl of 5% (v/v) formic acid containing 20 ng/µl of pepsin. As an alternative protocol, in-solution digestion using pepsin was performed for 10 min at 37°C in 20 µl of 5% (v/v) formic acid containing 100 ng/µl of pepsin. The generated peptides were then purified using C18 micro-columns [35], [36] loaded with Poros R3 C₁₈ material (Applied Biosystems, Stockholm, Sweden) and dried by vacuum centrifugation. In addition, enrichment and purification of phosphorylated peptides was performed by affinity chromatography on titanium dioxides as described [37], [38], [39].

MALDI-MS of peptides were acquired using a Voyager DE-STR mass spectrometer (AB SIEX. Stockholm, Sweden) in the reflector mode and 2,5 dihydroxybenzoic acid (DHB) solution containing 0.5% (v/v) phosphoric acid as a matrix (2,5 dihydroxybenzoic acid solution G2039A) from Agilent Technologies, Dalco Chromtech AB, Sollentuna, Sweden. LC-MS/MS combined with ESI-TRAP and ETD-TRAP was performed using a HCT ultra ETD II mass spectrometer from Bruker linked to Easy nano LC from Proxeon. Spectra were acquired using the enhanced scanning mode covering a mass range from m/z 200 to m/z 1300.

Analysis of gene transcription by Reverse Transcription (RT)-PCR

Protocols detailing the isolation of total RNA, the reverse transcription of mRNA into cDNA and its use as template for subsequent PCR amplification with the gene specific primers listed in Table S2 are described in detail elsewhere [19], [20].

Phosphorylation of the CpxR residue Asp₅₁ by acetyl∼P

Phosphorylation of response regulators is thought to stimulate structural changes leading to formation of functional dimers – a prerequisite for efficient binding to target DNA. Thus, to determine if CpxR∼P truly mediates repression of Yersinia virulence, we first wanted to characterize CpxR phosphorylation in vitro using a high energy phosphate donor, acetyl∼P. We initially determined the minimal concentration of acetyl∼P needed to sufficiently in vitro phosphorylate CpxR. Purified CpxR_wt::His₆ was incubated with increasing concentrations of acetyl∼P. Aliquots were then fractionated on Manganese(II)-Phos-tag™ 12.5% acrylamide gels to monitor the extent of CpxR∼P. As little as 6.25 mM acetyl∼P was sufficient to phosphorylate the majority of CpxR (Figure 1). Moreover, the maximal achievable amount of CpxR∼P was reached in the presence of 25 mM acetyl∼P (Figure 1). Hence, in vitro phosphorylation of CpxR by acetyl∼P is a robust method for generating a high proportion of CpxR∼P molecules.

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Figure 1. In vitro phosphorylation of CpxR by acetyl∼P.

Wild type CpxR (CpxR_wt::His₆) was purified by metal affinity chromatography. Purified protein (1.25 µM) was incubated in sequentially increasing concentrations of acetyl∼P (AP). Samples were fractionated on a Manganese(II)-Phos-tag™ 12.5% acrylamide gel and then visualized by the SYPRO® Ruby staining method. Lanes: a, no addition of AP; b, 6.25 mM AP; c, 12.5 mM AP; d, 25 mM AP; e, 50 mM AP; f, 100 mM AP. Phosphorylated CpxR is indicated by a double asterisk and unphosphorylated CpxR by a single asterisk.

https://doi.org/10.1371/journal.pone.0023314.g001

On the basis of homology to the OmpR/PhoB response regulator family, the conserved aspartate at position 51 (Asp₅₁) is the predicted phosphorylation site of CpxR [9]. We therefore established a cpxR mutation in which Asp₅₁ was replaced with alanine. As a control, another mutant was constructed in which methionine at position 199 (Met₁₉₉) was replaced with alanine. Based on the helix-turn-helix DNA-binding motif prediction algorithm of Dodd and Egan [40], this substitution is predicted to disrupt a helix-turn-helix motif needed for DNA binding – a characteristic of the OmpR/PhoB family [41] (data not shown). C-terminal His₆-tagged fusions of CpxR_wt and the two CpxR_D51A and CpxR_M199A variants were then purified by affinity chromatography from E. coli. Acetyl∼P was used to investigate which of these purified proteins could still be phosphorylated. The Manganese(II)-Phos-tag™ acrylamide system was used to visualize phosphorylated protein. Only CpxR_wt::His₆ and CpxR_M199A::His₆ were deemed to be phosphorylated in vitro by acetyl∼P (Figure 2B). Given that CpxR_D51A::His₆ exhibited altered mobility in the Manganese(II)-Phos-tag™ acrylamide gel, we also confirmed the absence of phosphorylation using conventional SDS-12%-PAGE followed by visualization with the independent Pro-Q® Diamond phosphoprotein stain (Figure 2B). As expected therefore, Asp₅₁ appears to be a genuine site of CpxR phosphorylation.

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Figure 2. Phosphorylation of the CpxR residue Asp₅₁.

Wild type (CpxR_wt::His₆) and defined variants with the amino acid substitutions Asp₅₁Ala (CpxR_D51A::His₆) and Met₁₉₉Ala (CpxR_M199A::His₆) were purified by metal affinity chromatography. Purified proteins (1.25 µM) were incubated in the presence of 50 mM acetyl∼P (AP) (+). In A, samples were fractionated by a Manganese(II)-Phos-tag™ 12.5% acrylamide gel and then stained by the SYPRO® Ruby staining method. In B, samples were separated in a conventional SDS 12% polyacrylamide gel. Phosphorylated protein (upper panel) was specifically detected by the Pro-Q® Diamond phosphoprotein gel stain technique, while total protein (lower panel) was visualized by the SYPRO® Ruby staining method. Phosphorylated CpxR is indicated by a double asterisk and unphosphorylated CpxR by a single asterisk. The reason for the enhanced mobility of CpxR_D51A::His₆ when fractionated by Manganese(II)-Phos-tag™ acrylamide (Panel A) is uncertain.

https://doi.org/10.1371/journal.pone.0023314.g002

It is possible that substitution at Asp₅₁ may cause an extreme allosteric effect that prevents CpxR phosphorylation at an alternative site. As phosphorylation on Asp residues is considered to be unstable, our initial approach had the goal to reduce phosphorylated Asp₅₁ of CpxR∼P using sodium borohydride to a stable homoserine [33], [34] and to confirm this conversion by mass spectrometry. However, the yield of this reaction was very low so the approach was not continued. Instead, in vitro phosphorylation of CpxR was confirmed by intact mass determinations using ESI-MS (Figure S1). These experiments showed that the major product of in vitro phosphorylation of CpxR carried only one phospho group (Table 1). This is consistent with the model that Asp₅₁ is the principal phosphorylation site of CpxR. In addition, the intact mass determination showed that CpxR∼P was sufficiently stable to be analyzed without converting Asp₅₁ to homoserine by sodium borohydride reduction.

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Table 1. Summary of mass determination of CpxR and CpxR∼P by ESI-MS.

https://doi.org/10.1371/journal.pone.0023314.t001

Phosphorylation-dependent binding of CpxR∼P to virulence gene promoters in vitro

Having established that CpxR∼P carries only one phospho group that is likely to be at Asp₅₁, we now wanted to gain insight into the role of CpxR∼P in virulence gene regulation in Yersinia. In a previous study, we noted that the expression of genes encoding the potential adhesins Ail (ail – YPTB2867) and Ail-like (YPTB2113), as well as the confirmed adhesins pH6 antigen (psaA) and invasin (inv), are all influenced by loss of CpxA [20]. We made use of the purified CpxR_wt and CpxR_D51A His₆-tagged variants derived from Yersinia CpxR and performed an EMSA to examine if CpxR∼P bound to radiolabeled PCR- amplified DNA control regions upstream of these Yersinia virulence genes. All regions of amplified target DNA included a minimum of ∼300 bp upstream and 40 bp downstream of the translational start codon. Our experiments were controlled by incorporating DNA encompassing the cpxR/cpxP divergent promoter and the ppiA promoter, both of which are known to bind CpxR∼P either from Y. pseudotuberculosis [20] or E. coli [12], [17], [42]. We also included the rovA gene encoding the transcriptional activator of invasin [22], [23], and the psaE gene, which encodes a regulator for pH6 antigen expression [43]. As anticipated from data obtained in our earlier study [20], in vitro phosphorylated CpxR_wt bound the promoters of inv and rovA, as well as those known CpxR∼P regulon members ppiA and cpxR/cpxP (Figure 3). Interestingly, at least two distinct migration shifts of rovA, ppiA and cpxR/cpxP template was observed when using different concentrations of CpxR∼P. This could suggest that these particular promoters contain multiple CpxR∼P binding sites of differential affinity so that several CpxR molecules bind cooperatively. This would be reminiscent of how CpxR∼P is thought to bind the promoter of csgD involved in curli biogenesis in E. coli [44]. Here, we also demonstrate for the first time a mobility shift of DNA specific to the promoter regions of psaA and psaE. Crucially, identical unlabeled (‘cold’) template DNA could compete for CpxR∼P binding. Although the degree of successful competition varied for each template, the addition of cold DNA did reduce the amount of radiolabeled (‘hot’) cpxR/P, ppiA, rovA, inv, psaA and psaE template DNA being retarded in migration during electrophoresis (Figure 3). Quite possibly the ail (YPTB2867) promoter also represents a target of CpxR∼P considering that the higher CpxR∼P concentration (1.5 µM) bound to all available free DNA resulting in the complete retardation of the hot template (the unbound signal at the bottom of the gel disappears). This is distinct from the reduced amount of ail-like (YPTB2113) promoter template shifted by equivalent amounts of CpxR∼P. In this case, significant signal representing free unbound ail-like hot template still exists at the bottom of the gel (Figure 3). In fact, this degree of ‘non-specific’ CpxR∼P binding was also observed in the negative control represented by an internal fragment of cpxR encompassing the nucleotides +32 through to +420 downstream of the translational start (Figure 3). Finally, binding by the non-phosphorylated CpxR_D51A variant was not observed in our assay conditions as evidenced by the absence of a migration shift for any hot DNA template (Figure 3). Taken together, this demonstrates that CpxR phosphorylation at position 51 is required for direct and efficient binding of CpxR∼P to the rovA, inv, psaA and psaE (and possibly also the ail) virulence gene promoters. On the other hand, modulation of expression of the Ail-like homologue (YPTB2113) by CpxR∼P is apparently not via direct binding, but must presumably involve at least one other unknown regulatory intermediate.

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Figure 3. Phosphorylation-dependent binding of CpxR to DNA upstream of Yersinia virulence genes.

Mobility shift assays were performed with purified CpxR_wt::His₆, and the non-phosphorylated mutant CpxR_D51A::His₆. Target DNAs were radiolabeled PCR fragments harboring the regulatory regions of cpxR/cpxP, ppiA, rovA, inv, ail (YPBT2867), ail-like (YPBT2113), psaA and psaE. An internal fragment of the cpxR gene was used as a negative control. The approximate size of each amplified PCR fragment is given in parentheses. Where indicated, the purified CpxR-His tagged variants were incubated with ‘hot’ DNA templates at the concentrations of 0.75 and 1.5 µM. All reactions were performed in the presence of the phosphodonor acetyl∼P and binding specificity was aided by the constant presence of BSA and non-specific single stranded DNA. EMSAs were further controlled by a reaction containing 1.5 µM BSA instead of CpxR or competition reactions in which excess ‘cold’ DNA template competed with ‘hot’ DNA for available CpxR∼P. The electrophoretic mobility of the ‘hot’ DNA fragments in the absence of bound protein is highlighted by an arrow, while DNA-CpxR∼P complexes are signified with an asterisk (*). In some cases, the extent of mobility shifted DNA was dependent on the CpxR∼P concentration. Two asterisks (**) indicate residual non-specific background binding noise and are not believed to represent bona fide binding targets of CpxR∼P.

https://doi.org/10.1371/journal.pone.0023314.g003

Mapping the DNA binding site of CpxR∼P in the rovA promoter

RovA is a global regulator of Yersinia gene expression, being responsible for fine-tuning expression of a multitude of genes involved in general housekeeping, environmental survival and pathogenicity [24], [25], [26]. Levels of RovA need to be strictly controlled; dissecting these control mechanisms will therefore benefit our general understanding of how this pathogenic bacterium responds and adapts to its prevailing environment. In order to determine how CpxR∼P controls the levels of rovA transcription, we performed a nuclease protection (footprinting) analysis to map the DNA binding site of CpxR∼P in the rovA promoter. A protected sequence of the sense strand estimated to be 5′-gcgtgctaacgataatgacaaaaattgacaaatcta-3′ was identified within the P2 promoter region of rovA (Figure 4). We could also identify protected regions in the sense strand of ppiA promoter (5′-ttctgttacgtaaatatccgtaaatgggtgg-3′) and the divergent cpxR-cpxP promoter (5′-gtcagggcatgtaaagctga-3′) (Figure 4). As expected, a control sequence residing downstream of the cpxR start codon was not protected from DNase1 digestion. In E. coli, the consensus CpxR∼P DNA binding sequence is represented by 5′-GTAAA(N)_4–8GTAAA-3′ [4], [42]. We manually inspected these DNase1 protected sequences for consensus CpxR∼P DNA binding motifs. A poorly conserved putative CpxR∼P binding site may lie in the protected region derived from the rovA promoter, while more obviously conserved consensus CpxR∼P binding motifs were observed in the protected sequence upstream of ppiA and between cpxP/cpxR (Figure 4).

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Figure 4. Mapping the CpxR∼P DNA binding site upstream of rovA by nuclease protection (footprinting) analysis.

DNase I footprinting assays were performed to investigate the binding of CpxR∼P to a region within the rovA, ppiA and cpxR-cpxP promoters. These 314 base pair (bp), 276 bp and 245 bp fragments respectively, were labeled on the sense strand before being incubated with CpxR∼P at the following final concentrations: 50 nM, lane c; 100 nM, lane d; 200 nM, lane e; 400 nM, lane f. The absence of CpxR∼P in lanes a and b is indicated by ‘–’. Reactions were resolved by denaturing PAGE and analyzed with a Molecular Dynamics PhosphorImager. Labeled pBR322 DNA digested with MspI (New England Biolabs) was used as a size marker (lane a). An estimation of the protected sequence is given on the right hand side of the panels. Based upon the E. coli consensus sequence of 5′-GTAAA(N)_4–8GTAAA-3, a putative CpxR∼P consensus binding site is highlighted in a gray box. A labeled internal fragment (389 bp) within the cpxR open reading frame served as a non-protected control.

https://doi.org/10.1371/journal.pone.0023314.g004

Based on the analysis of these ‘footprints’, we used sited-directed mutagenesis to shuffle the order of the nucleotides predicted to compose the CpxR∼P binding sites upstream of ppiA, cpxR (and cpxP) and rovA (Figure 5A). Since the CpxR∼P binding site upstream of rovA might overlap with the −35 box of the P2 promoter [45], we generated two scramble mutants in this region. The first was designated Mt 1, which included alteration of the −35 box sequence. In contrast, the second mutant (Mt 2) left the −35 box sequence intact. Significantly, an EMSA revealed a clear reduction in the retardation of PCR amplified fragments of the mutagenized DNA by CpxR∼P (Figure 5B; designated ‘Mt’). Collectively, these data indicate that the sequence 5′-ACAAA(N)₅ACAAA-3′ overlapping with the −35 box of the P2 promoter and roughly located 360 nucleotides upstream of the rovA ATG start codon contributes to CpxR∼P binding. In addition, the 5′-GTAAA(N)₅GTAAA-3′ sequences situated ∼80 and ∼55 nucleotides upstream of ppiA and cpxR respectively are also bona fide CpxR∼P binding sites.

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Figure 5. Site-directed mutagenesis of the CpxR∼P DNA binding site upstream of rovA.

(A) As identified by DNase 1 foot-printing (see Figure 4), the potential CpxR∼P binding site sequence and position is shown relative to each ATG start codon within the regulatory regions of rovA and ppiA and the divergent cpxR/cpxP promoter (designated as ‘Wt’). Site-directed mutagenesis was performed to ‘shuffle’ the nucleotide sequence of each potential CpxR∼P binding site (designated as ‘Mt’). Since the initial mutation in the rovA sequence (‘Mt 1’) would potentially disrupt RNA polymerase binding because of an altered −35 region within promoter P2, a second mutation (‘Mt 2’) was performed in which the −35 region was left untouched. (B) Mobility shift assays with purified CpxR_wt::His₆ as outlined in the legend to Figure 3 were performed on radiolabled amplified DNA from these mutated templates. Once again, the electrophoretic mobility of the ‘hot’ DNA fragments in the absence of bound protein is highlighted by an arrow, while DNA-CpxR∼P complexes are signified with a single asterisk (*).

https://doi.org/10.1371/journal.pone.0023314.g005

In vivo accumulation of CpxR∼P in the Yersinia cytoplasm reduces levels of RovA

We predict that binding of CpxR∼P to the rovA promoter restricts transcription. Therefore, elevating available CpxR∼P in the Yersinia cytoplasm in turn should reduce detectable RovA levels. To test this, we took advantage of work performed in E. coli, whereby phosphatase deficient CpxA_T253P encoded by the allelic variant designated cpxA101* generally lead to a constitutively active Cpx pathway [5], [14]. Although never directly tested, such a mutant should accumulate unusually high levels of CpxR∼P. To test this in Yersinia, we constructed an in cis cpxA101* mutation in Y. pseudotuberculosis. We then utilized the Manganese(II)-Phos-tag™ acrylamide gel system to measure in vivo levels of CpxR∼P. Formic acid-lysed bacteria grown in LB broth to early stationary phase (OD₆₀₀ in the range of 0.85 to 0.95) at 26°C were fractionated on a Manganese(II)-Phos-tag™ 12.5% acrylamide gel and blotted with affinity purified anti-CpxR antiserum. Impressively high levels of both CpxR and CpxR∼P was detected in the cytoplasm of the Yersinia mutant completely lacking the cpxA allele (Figure 6). These two CpxR isoforms were also present in the cpxA101* background, although not to the same extent. Moreover, it seems that the vast majority of detectable CpxR is actually phosphorylated in this cpxA101* background. At present, reasons for why different levels and ratios of the two CpxR isoforms accumulate in these independent cpxA mutants are not clear. In contrast, CpxR was generally undetectable in parental bacteria or the cpxR mutants encoding the non-phosphorylated CpxR_D51A or the CpxR_M199A variant predicted to possess a defective winged helix-turn-helix domain (Figure 6). Given the noted toxicity of elevated CpxR∼P levels [4], [19], [20], accumulation of cytoplasmic CpxR∼P in the ΔcpxA and cpxA101* mutants does correlate with an inferior rate of growth (Figure S2A).

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Figure 6. In vivo detection of phosphorylated and unphosphrylated CpxR.

The Manganese(II)-Phos-tag™ acrylamide gel system was used to measure in vivo levels of CpxR∼P. Bacteria were cultured at 26°C in LB broth to stationary phase. After harvesting by centrifugation, bacteria were lysed with formic acid and samples rapidly fractionated on a Manganese(II)-Phos-tag™ 12.5% acrylamide gel and blotted with affinity purified anti-CpxR antiserum. Strains: parent, YPIII/pIB102; ackA, pta null mutant, YPIII69/pIB102; cpxA null mutant, YPIII07/pIB102; cpxA, ackA, pta null mutant, YPIII49/pIB102; cpxA101* encoding CpxA_T253P, YPIII51/pIB102; cpxA101*, ackA, pta null mutant, YPIII74/pIB102; mutated cpxR encoding CpxR_D51A, YPIII52/pIB102; mutated cpxR encoding CpxR_M199A, YPIII46/pIB102; cpxR null mutant, YPIII08/pIB102. The single asterisk (*) reflects non-phosphorylated CpxR, while the double asterisk (**) indicates phosphorylated CpxR accumulated in the Yersinia cytoplasm.

https://doi.org/10.1371/journal.pone.0023314.g006

In the absence of CpxA phosphatase activity, CpxR∼P may generate via non-specific low molecular weight phosphodonors such as acetyl∼P [5], [15], [16], [17]. Acetyl∼P is derived from the phosphotransacetylase (Pta) – acetate kinase (AckA) pathway [46]. Therefore, to investigate if this phosphodonor contributes to accumulated CpxR∼P in the ΔcpxA null mutant and the gain-of-function cpxA101* mutant producing CpxA_T253P, a full length ΔackA, pta null mutation was introduced into these bacteria. Since mutants lacking both ackA and pta genes should be incapable of synthesizing acetyl∼P [47], this second-site mutation should therefore reverse the build-up of CpxR∼P exhibited by the ΔcpxA and cpxA101* mutants. Indeed, CpxR∼P no longer accumulated in the ΔcpxA and cpxA101* mutants also lacking the ability to synthesize acetyl∼P (Figure 6), which to some extent suppressed the inferior growth rate of the single ΔcpxA and cpxA101* mutants (Figure S2A). The singular ΔackA, pta null mutant was also modestly growth restricted consistent with reports in E. coli (Figure S2A) [18], [48], [49]. However, it did not accumulate either non-phosphorylated or phosphorylated CpxR, being equivalent to parental bacteria where CpxR also remained below the level of detection in our assay (Figure 6). Hence, the Cpx pathway of Yersinia is subject to feedback inhibition that tightly restricts available CpxR∼P levels. However, in the absence of CpxA phosphatase activity, CpxR∼P readily accumulates by virtue of sensor kinase activity and/or small molecular weight phosphodonors associated with central metabolism.

Having established Yersinia mutants in which the in vivo levels of CpxR∼P were characterized, we used these to address whether elevated CpxR∼P levels restrict production of the RovA global regulator. RovA production from stationary phase bacteria grown in LB broth was analyzed by western blotting. Elevated levels of CpxR∼P accumulated in the ΔcpxA and cpxA101* mutants dramatically restricted RovA production (Figure 7). However, production to parental levels was restored in both mutants by the introduction of a second-site deletion of the ackA and pta genes (Figure 7). We also analyzed invasin, whose production is under RovA positive control. Not surprisingly therefore, invasin levels mirrored the pattern of RovA production in all strain backgrounds. Removal of the ackA and pta genes from parental Yersinia did not affect RovA or invasin production (Figure 7). We therefore conclude that cytoplasmic CpxR∼P accumulation is an important mediator of Yersinia virulence factor expression. The data also suggests that Yersinia low molecular weight metabolic intermediates, such as acetyl∼P, have the capacity to transfer high-energy phospho-groups to CpxR, and perhaps even other TCRS response regulators. Thus, this could be a way for Yersinia to effectively fine-tune global gene expression depending upon the prevailing environmental conditions such as nutrient supply.

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Figure 7. Cpx pathway activation influences the production of the RovA global regulator.

RovA and invasin production was determined from protein isolated from early stationary phase bacteria grown in LB broth at either 26°C or 37°C. Protein was separated on a 12% SDS-PAGE and then identified by immunoblot analysis using polyclonal rabbit antiserum raised against RovA or invasin. Strains: parent, YPIII/pIB102; ΔackA, pta null mutant, YPIII69/pIB102; ΔcpxA null mutant, YPIII07/pIB102; ΔcpxA, ΔackA, pta null mutant, YPIII49/pIB102; cpxA101* encoding CpxA_T253P, YPIII51/pIB102; cpxA101*, ΔackA, pta null mutant, YPIII74/pIB102. Molecular weights shown in parentheses are deduced from primary sequence. The single asterisk (*) reflects typical invasin degradation products, while two asterisks (**) indicates a non-specific protein band recognized by the anti-RovA antisera that also serves as a convenient loading control.

https://doi.org/10.1371/journal.pone.0023314.g007

Elevated levels of the NlpE lipoprotein reduce invasin and RovA levels

Examination of the Cpx response in the absence of a functioning CpxA protein is artificial. We therefore wanted to examine the repressive effect of CpxR∼P on RovA production following activation of the Cpx response in which the signal transduction cascade is still intact. Simulating natural Cpx TCRS responsiveness has been achieved by the over-production of the E. coli NlpE (NlpE_E.c) lipoprotein [50], [51]. We therefore transformed parent and CpxR defective Yersinia with pBAD18 derivatives encoding E. coli nlpE (termed pND18) or Y. pseudotuberculosis nlpE (NlpE_Y.p – pJF027) under the control of an arabinose inducible promoter. Since NlpE_Y.p shares less than 50% identity at the amino acid level with NlpE_E.c (Figure 8A), we considered that native NlpE could possibly be a better inducer of Cpx pathway activation in Yersinia. Bacteria were grown in the presence or absence of arabinose, and production of RovA and invasin was examined. Over-production of either NlpE_E.c or NlpE_Y.p in parental Yersinia caused a reduction in RovA and invasin production that was dependent on functional CpxR, because neither lipoprotein caused this decrease in the ΔcpxR null mutant (Figure 8B). Interestingly, NlpE_Y.p appeared to restrict RovA and invasin production to a greater degree. These data reinforce how Cpx pathway activation and the presence of CpxR∼P can restrict virulence factor production in Y. pseudotuberculosis.

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Figure 8. Inhibitory effect of NlpE overexpression.

(A) A ClustalW2 alignment colored by Boxshade (ver. 3.21) between NlpE_Y.p (NCBI annotation YPK_1090) from Y. pseudotuberculosis YPIII and NlpE_E.c (b0192) from E. coli K-12 strain MG1655. (B) Sampling and detection of invasin and RovA at stationary phase in LB broth at 26°C followed the procedure detailed in the legend to Figure 7. Additionally, NlpE_E.c (derived from E. coli) or NlpE_Y.p (Y. pseudotuberculosis) over-production was controlled by the presence (+) or absence (−) of 0.2% (w/v) L-arabinose. The pBAD18 empty expression vector served as a control. The strains used were: parent with empty vector, YPIII/pIB102, pBAD18; parent with NlpE_E.c, YPIII/pIB102, pND18; parent with NlpE_Y.p, YPIII/pIB102, pJF027; cpxR null mutant with empty vector, YPIII08/pIB102, pBAD18; cpxR null mutant with NlpE_E.c, YPIII08/pIB102, pND18; cpxR null mutant with NlpE_Y.p, YPIII08/pIB102, pJF027. Molecular weights shown in parentheses are deduced from primary sequence.

https://doi.org/10.1371/journal.pone.0023314.g008

CpxR∼P DNA binding is required for RovA repression in vivo

We have identified a CpxR∼P binding site in the regulatory regions of three genes of Yersinia; ppiA, cpxP/cpxR and rovA. We have also shown the accumulated CpxR∼P levels result in restricted RovA production. Therefore, we wondered whether RovA repression by CpxR∼P could be relieved by modulating the CpxR∼P binding site within the rovA promoter. The same rovA ‘shuffle’ mutations (Mt 1 and Mt 2) used to identify CpxR∼P binding in vitro (see Figure 5) were introduced in cis into the chromosome of the cpxA101* mutant of Y. pseudotuberculosis. This background was chosen because the Cpx pathway is constitutively active, CpxR∼P accumulation is relatively high and the integrity of the cpxRA transcriptional unit remains intact. Bacteria were grown to early-stationary phase and the extent of RovA production was examined by immunoblot. RovA levels were essentially undetectable in the cpxA101* mutant and this mutant also harboring rovA_{(Mt 1)} (Figure 9). Significantly however, RovA levels were restored in the cpxA101*, rovA_{(Mt 2)} double mutant indicating that the ‘Mt 2’ mutation made the rovA promoter non responsive to Cpx pathway activation. Similarly, RovA levels were also restored in the cpxA101*, cpxR/P_(Mt) double mutant (Figure 9). In this strain, cpxR transcription is not induced limiting the accumulation of CpxR∼P (data not shown). To confirm these data, we performed semi-quantitative RT-PCR analysis to gain some insight into rovA transcription levels. Compared to the single cpxA101* mutant, rovA transcription was elevated in both cpxA101*, rovA_{(Mt 2)} and cpxA101*, cpxR/P_(Mt) double mutants (Figure S3). Interestingly, rovA transcription in the cpxA101*, rovA_{(Mt 1)} mutant was still low, which explains the absence of RovA detection by western blotting (Figure 9). This indicates that the ‘Mt 1’ nucleotide shuffling within the putative −35 region (see Figure 5A) predictably affected RNA polymerase promoter recognition and transcriptional output from the ‘P2’ rovA promoter [45]. Collectively, these data therefore identify nucleotides upstream of rovA that are critical for the in vivo recognition by CpxR∼P and the subsequent repression of rovA transcription. Despite our EMSA results indicating multiple CpxR∼P binding sites, we believe that this sequence in the ‘P2’ rovA promoter is primarily responsible for governing CpxR∼P-dependent rovA regulatory control.

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Figure 9. RovA produced from a mutant allele lacking the upstream CpxR∼P DNA binding site is no longer restricted by Cpx pathway activation.

Y. pseudotuberculosis was grown until entry into early stationary phase at 26°C in LB broth. Bacterial cells were harvested and lysates prepared in loading buffer. Protein was separated on a 15% SDS-PAGE and then identified by immunoblot analysis using polyclonal rabbit antiserum raised against RovA. The molecular weight shown in parenthesis was deduced from primary sequence. The single asterisk (*) indicates a non-specific protein band recognized by the anti-RovA antisera. Strains: parent, YPIII/pIB102; cpxA101* encoding CpxA_T253P, YPIII51/pIB102; cpxR/cpxP_(Mt) (shuffle mutation of the CpxR∼P binding site identified in Figure 4) placed in the cpxA101* background, YPIII115/pIB102; rovA_{(Mt 1)} placed in cpxA101*, YPIII120/pIB102; rovA_{(Mt 2)} placed in cpxA101*, YPIII121/pIB102.

https://doi.org/10.1371/journal.pone.0023314.g009