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Journal of Bacteriology, March 2003, p. 1935-1941, Vol. 185, No. 6
0021-9193/03/$08.00+0     DOI: 10.1128/JB.185.6.1935-1941.2003
Copyright © 2003, American Society for Microbiology. All Rights Reserved.

Mutational Analysis of the Residue at Position 48 in the Salmonella enterica Serovar Typhimurium PhoQ Sensor Kinase

Sarah Sanowar, Alexandre Martel, and Hervé Le Moual^*

Department of Microbiology and Immunology, McGill University, Montréal, Québec, Canada H3A 2B4

Received 13 August 2002/ Accepted 22 November 2002

Top Abstract Introduction Materials and Methods Results Discussion Addendum References

 
The PhoP/PhoQ two-component regulatory system of Salmonella enterica serovar Typhimurium plays an essential role in controlling virulence by mediating the adaptation to Mg²⁺ depletion. The pho-24 allele of phoQ harbors a single amino acid substitution (T48I) in the periplasmic domain of the PhoQ histidine kinase sensor. This mutation has been shown to increase net phosphorylation of the PhoP response regulator. We analyzed the effect on signaling by PhoP/PhoQ of various amino acid substitutions at this position (PhoQ-T48X [X = A, S, V, I, or L]). Mutations T48V, T48I, and T48L were found to affect signaling by PhoP/PhoQ both in vivo and in vitro. Mutations PhoQ-T48V and PhoQ-T48I increased both the expression of the mgtA::lacZ transcriptional fusion and the net phosphorylation of PhoP, conferring to cells a PhoP constitutively active phenotype. In contrast, mutation PhoQ-T48L barely responded to changes in the concentration of external Mg²⁺, in vivo and in vitro, conferring to cells a PhoP constitutively inactive phenotype. By analyzing in vitro the individual catalytic activities of the PhoQ-T48X sensors, we found that the PhoP constitutively active phenotype observed for the PhoQ-T48V and PhoQ-T48I proteins is solely due to decreased phosphatase activity. In contrast, the PhoP constitutively inactive phenotype observed for the PhoQ-T48L mutant resulted from both decreased autokinase activity and increased phosphatase activity. Our data are consistent with a model in which the residue at position 48 of PhoQ contributes to a conformational switch between kinase- and phosphatase-dominant states.

Top Abstract Introduction Materials and Methods Results Discussion Addendum References

 
Two-component regulatory systems allow bacteria to adapt to a variety of environmental changes by modulating the expression of specific genes. The Salmonella enterica serovar Typhimurium PhoP/PhoQ two-component system plays an essential role in coordinating the expression of various virulence factors (9, 23). By modulating the expression of more than forty different genes, it controls adaptation to Mg²⁺-limiting environments, protein secretion by the type III secretion system located on Salmonella pathogenicity island 1, entry into epithelial cells, survival within macrophages, lipopolysaccharide modifications, and resistance to antimicrobial peptides (reviewed in references 8 and 12).

The PhoQ protein is a transmembrane histidine kinase sensor that is present in the inner membrane as a homodimer (Fig. 1). Each subunit consists of an N-terminal periplasmic ligand-recognition domain (residues 40 to 194) flanked by two transmembrane segments (TM1 and TM2) and a C-terminal cytoplasmic signaling domain (residues 215 to 487). The PhoQ protein has been shown to sense some external divalent cations such as Mg²⁺, Ca²⁺, and Mn²⁺ (10). It has been proposed that Mg²⁺ is the physiological signal controlling the PhoP/PhoQ system (11). Limiting concentrations of Mg²⁺ in the extracellular environment activate the cytoplasmic phosphorylation cascade by promoting the ATP-dependent autophosphorylation of PhoQ on an invariant His residue (His 277) (3, 26). Subsequently, the phosphoryl group is transferred from PhoQ to a highly conserved Asp residue (Asp 55) of the response regulator PhoP. DNA binding of phospho-PhoP promotes both transcription of PhoP-activated genes and repression of PhoP-repressed genes. In contrast, high concentrations of external Mg²⁺ stimulate the PhoQ phosphatase activity that dephosphorylates phospho-PhoP (3, 26). In turn, this represses transcription of PhoP-activated genes and derepresses PhoP-repressed genes. Thus, environmental Mg²⁺ controls the intracellular level of phospho-PhoP by coordinately regulating PhoQ autokinase and phosphatase activities (26).

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FIG. 1. Location of position 48 in the periplasmic domain of PhoQ. (A) Schematic representation of the PhoQ sensor kinase. The location of position 48 is shown by arrows. The cytoplasmic domain representation is based on the nuclear magnetic resonance structures of the E. coli EnvZ sensor kinase (7). It consists of a catalytic ATP-binding domain and a dimerization domain that contains the invariant histidine residue. (B) Partial alignment of the amino acid sequences of the S. enterica serovar Typhimurium PhoQ protein to homologues in E. coli, Klebsiella pneumoniae, Yersinia pestis, Providencia stuartii, Erwinia carotovora, P. aeruginosa, and X. fastidiosa. The arrow indicates position 48 (S. enterica serovar Typhimurium numbering). The bold line under the sequences indicates the N-terminal transmembrane segment (TM1), which has been predicted on the basis of a hydrophobicity plot.

The pho-24 allele of phoQ that was isolated after diethyl sulfate mutagenesis of S. enterica serovar Typhimurium strain LT2 resulted in constitutive expression of phoN, a PhoP-activated gene that encodes a periplasmic acid phosphatase (19). Like Salmonella phoP- or phoQ-defective strains, those strains harboring the pho-24 allele are attenuated for virulence in mice (13, 23, 24). The pho-24 allele confers a PhoP-constitutive phenotype (PhoP^c) to cells that is characterized by the constitutive expression and repression of PhoP-activated genes and PhoP-repressed genes, respectively (24). This altered pattern of gene expression results in pleiotropic effects that include decreased invasion of epithelial cells (2, 27) and defects in stimulating macropinocytosis and spacious phagosome formation in macrophages (1). It has subsequently been shown that a change of Thr to Ile at position 48 of the PhoQ protein was responsible for the phenotypes associated with the pho-24 allele (10, 14). Salmonella strains harboring the pho-24 allele of phoQ have been used in various studies to establish the involvement of the PhoP/PhoQ system in lipid A modifications (15), in resistance against host antimicrobial peptides (16, 25), and in resistance to bile (29). In addition, these strains have been used as carriers for heterologous antigens in live oral vaccines (17). Although the pho-24 mutation has been shown to increase net phosphorylation of PhoP (14), the mechanism by which this mutation affects signaling by the PhoP/PhoQ system remains unknown.

Our study assesses the molecular mechanism by which a mutation at position 48 in the PhoQ periplasmic domain affects catalytic activities in the cytoplasmic signaling domain. We generated mutants of the phoQ gene with amino acid substitutions at position 48 and analyzed the catalytic activities of the encoded proteins both in vivo and in vitro.

Top Abstract Introduction Materials and Methods Results Discussion Addendum References

 
Bacterial strains and growth conditions. Escherichia coli strain XL-1 Blue (Stratagene) was used for all DNA manipulations. E. coli strain BL21(DE3)/pLysE (Novagen) was used for protein expression. E. coli strain MG1607 [F^- (argF-lac)U169 araD139 rpsL150 ptsF25 fibB5301 rbsR deoC relA1 mgtA::placMu55 phoQ608::Tn10dCam], which was kindly provided by R. Utsumi, Kinki University, Japan (18), was used for ß-galactosidase analyses. Bacterial cultures were grown at 37°C with aeration in Luria-Bertani (LB) broth containing the appropriate antibiotics (100 µg of ampicillin per ml and 30 µg of chloramphenicol per ml).

Plasmids and DNA manipulations. Plasmid pET-Q, containing the S. enterica serovar Typhimurium phoQ gene under the control of the T7 promoter (26), was used to generate the series of mutants at position 48 (pET-Q-T48X). Site-directed mutagenesis was performed according to the method of Deng and Nickoloff (6). The native Thr residue at position 48 was replaced by a Ser residue by using primer Q-T48S (5'-AGTTTTGATAAAACCAGCTTTCGTTTGC-3'), by an Ala residue by using primer Q-T48A (5'-GTTTTGATAAAACCGCCTTTCGTTTGCTG-3'), by an Ile residue by using primer Q-T48I (5'-AGTTTTGATAAAACCATCTTTCGTTTGC-3'), by a Val residue by using primer Q-T48V (5'-GTTTTGATAAAACCGTCTTTCGTTTGCTG-3'), and by a Leu residue by using primer Q-T48L (5'-GTTTTGATAAAACCCTCTTTCGTTTGCTG-3'). Plasmid pET-P_His encoded the S. enterica serovar Typhimurium PhoP protein fused to a C-terminal His tag (PhoP_His) (26).

To carry out ß-galactosidase analyses, we constructed the plasmid pPRO-Q_His, in which the S. enterica serovar Typhimurium phoQ gene fused to a C-terminal His tag is overexpressed under the control of the tac promoter. This medium-copy-number plasmid harboring the p15A origin of replication was derived from pPROLar.A122 (Clontech) by inserting the lacI^q coding sequence and replacing the kanamycin resistance gene with the ampR gene. The pPRO-Q_His-T48X series of plasmids was constructed by subcloning the various 732-bp KpnI-MluI fragments from the pET-Q-T48X plasmids into pPRO-Q_His that had been digested with the same enzymes.

ß-Galactosidase assays. E. coli MG1607 cells transformed with the pPRO-Q_His-T48X series of plasmids were grown overnight at 37°C in LB broth supplemented with 0.1% glucose. Cultures were diluted 1:100 in LB broth supplemented with 0.1% glucose in the presence or absence of 10 mM MgCl₂. Cultures were grown to an optical density at 600 nm (OD₆₀₀) of 0.8 before induction with 1 mM isopropyl-ß-D-thiogalactopyranoside (IPTG) for 2 h. Cell lysates were prepared using reporter lysis buffer (Promega). ß-Galactosidase activity was measured, using ONPG (o-nitrophenyl-ß-D-galactopyranoside) as a substrate, as previously described (22). Expression levels of the PhoQ_His-T48X mutants were monitored by Western blotting. Proteins were separated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and transferred onto nitrocellulose membranes. His-tagged proteins were detected by using His•Tag monoclonal antibody (Novagen) and His•Tag AP LumiBlot reagents (Novagen) as recommended by the manufacturer.

Preparation of membranes enriched in the various PhoQ-T48X proteins. E. coli BL21(DE3)/pLysE cells, transformed with the pET-Q-T48X series of plasmids, were grown at 37°C in LB broth supplemented with appropriate antibiotics. Transcription of the phoQ gene was induced at an OD of 0.8 by adding 0.5 mM IPTG. After 4 h of induction, cells were harvested by centrifugation and membranes were prepared as described previously (20). Using the standard procedure of the Bio-Rad protein assay in the presence of 0.1% SDS, the total amount of protein in membranes was measured by the Bradford method. Expression of the various PhoQ-T48X proteins was visualized on an SDS-12.5% PAGE gel. After the Coomassie blue-stained gels were scanned, the percentage corresponding to the overproduced PhoQ-T48X proteins in membranes was estimated.

Expression and purification of PhoP_His. E. coli BL21(DE3)/pLysE cells transformed with the pET-P_His plasmid were grown at 22°C in LB broth supplemented with appropriate antibiotics. Cultures were induced overnight with 1 mM IPTG at an OD of 0.8, and cells were harvested by centrifugation, resuspended in loading buffer consisting of 20 mM Tris-HCl (pH 7.9), 500 mM NaCl, 50 mM imidazole, and 1 mM phenylmethylsulfonyl fluoride, and sonicated at 4°C. Cell debris was removed by centrifugation, and the supernatant was loaded onto a 1-ml HiTrap chelating column (Amersham Biosciences). The column was extensively washed with loading buffer and eluted using a 0 to 600 mM imidazole gradient in loading buffer. Fractions containing PhoP_His were pooled and dialyzed extensively against 20 mM Tris-HCl (pH 7.5)-50 mM NaCl-10% glycerol. The concentration of purified PhoP_His was measured using the Bio-Rad protein assay.

In vitro reconstitution of the PhoP/PhoQ signaling cascade. The net phosphorylation of PhoP was measured by incubating membranes containing the PhoQ-T48X proteins (approximately 1.5 µM PhoQ-T48X) with a sixfold molar excess of PhoP_His in a 15-µl volume of phosphorylation buffer (50 mM Tris-HCl [pH 7.5], 200 mM KCl, 0.1 mM EDTA, 5% glycerol) supplemented with 5 mM MgCl₂. Reactions were initiated by the addition of 0.1 mM [-³²P]ATP (10 Ci/mmol), incubated for 20 min at 22°C to reach an apparent steady state, and stopped by addition of 4x Laemmli SDS sample buffer (250 mM Tris-HCl [pH 6.8], 8% SDS, 40% glycerol, 0.02% bromophenol blue, 4% ß-mercaptoethanol). Reaction products were heated at 37°C for 3 min and applied to SDS-10% PAGE gels. Gels were dried and exposed to a PhosphorImager (Molecular Dynamics). Using Image Quant software (Molecular Dynamics), phosphorylated proteins were quantified by image analysis.

In vitro autophosphorylation assays. Membranes containing the PhoQ-T48X proteins (approximately 1.5 µM PhoQ-T48X) were autophosphorylated with 0.1 mM [-³²P]ATP (10 Ci/mmol) in a 15-µl volume of phosphorylation buffer supplemented with 0.1 mM MgCl₂ (26). The phosphorylation reactions were continued at 22°C for various times before being stopped by addition of 4x Laemmli SDS sample buffer. Reaction products were analyzed by SDS-PAGE as described above.

In vitro phosphatase assays. Purified PhoP_His was phosphorylated with membranes containing the overexpressed PhoQ-T48V protein in a 75-µl volume of phosphorylation buffer supplemented with 5 mM MgCl₂ and 0.1 mM [-³²P]ATP (10 Ci/mmol). After 20 min of incubation at 22°C, the reaction mixture was centrifuged at 16,000 x g for 10 min at 4°C to pellet membranes. The supernatant was loaded on a Micro Bio-Spin chromatography column (Bio-Rad) to remove unincorporated ATP, generated ADP, and MgCl₂. The flowthrough containing phospho-PhoP_His was immediately used for the phosphatase assay. Phospho-PhoP_His (15 µM) was mixed with membranes containing the PhoQ-T48X proteins (approximately 1.5 µM PhoQ-T48X) in a 15-µl volume of phosphorylation buffer supplemented with 10 mM MgCl₂. At various time points, reactions were stopped by the addition of 4x Laemmli SDS sample buffer. Phosphorylated products were analyzed as described above.

Top Abstract Introduction Materials and Methods Results Discussion Addendum References

 
Isolation of the PhoQ-T48X mutations. The residue at position 48 is located at the N terminus of the periplasmic domain of PhoQ, in close proximity to the first transmembrane segment (TM1) (Fig. 1A). Secondary structure predictions of the PhoQ periplasmic domain suggested that the Thr at position 48 is part of an -helix that is probably continuous with the postulated -helical TM1 (21). Although the Thr residue at position 48 is conserved in many PhoQ homologues, other amino acid residues (Ser, Ile, or Leu) are present at this position in the most distantly related PhoQ homologues (Fig. 1B). To understand the molecular mechanism by which the mutation T48I (the pho-24 allele of phoQ) affects the PhoQ catalytic activities, we used site-directed mutagenesis (6) to replace the native Thr residue with Ala, Ser, Val, Ile, and Leu residues. The rationale in mutating the Thr at position 48 of PhoQ is based on the polarity, size, and hydrophobicity of the side chains.

Effect of the PhoQ-T48X mutations on the expression of a PhoP-activated gene. To examine the effects of the PhoQ-T48X mutations on the entire PhoP/PhoQ signaling pathway in vivo, we measured the expression of mgtA (a PhoP-activated gene that encodes a Mg²⁺ transporter) by measuring the ß-galactosidase activity of the mgtA::lacZ transcriptional fusion (18). E. coli MG1607 cells (a phoQ-defective strain) (18) were transformed with the various pPRO-Q_His-T48X plasmids encoding the S. enterica serovar Typhimurium PhoQ mutated proteins. To quantify the expression of the PhoQ-T48X proteins by Western blotting, we used plasmids encoding the PhoQ protein fused to a C-terminal tag of 6 histidine residues (PhoQ_His-T48X). The catalytic activities of the PhoQ_His protein were essentially similar to those of the untagged PhoQ protein, as judged by both in vivo and in vitro assays (data not shown).

As found in previous studies (10, 28), ß-galactosidase activity of cells producing wild-type PhoQ_His was decreased by about 10-fold when LB broth was supplemented with 10 mM MgCl₂, indicating that expression of mgtA was repressed by high concentrations of Mg²⁺ (Fig. 2). Levels of ß-galactosidase activity observed for cells producing either PhoQ_His-T48S or PhoQ_His-T48A were essentially similar to those obtained for cells producing wild-type PhoQ_His, whether or not LB broth was supplemented with MgCl₂ (Fig. 2). In contrast, mutations T48V and T48I in the PhoQ_His protein increased the levels of ß-galactosidase activity by 5-fold in the absence of MgCl₂ and by 14- to 23-fold in the presence of 10 mM MgCl₂. Although the PhoQ_His-T48I and PhoQ_His-T48V mutants responded to high concentrations of external MgCl₂, levels of ß-galactosidase activity produced by these cells grown in the presence of 10 mM MgCl₂ were higher than the level of ß-galactosidase activity obtained with cells producing wild-type PhoQ_His grown in the absence of MgCl₂. Interestingly, cells that produced the PhoQ_His-T48L protein showed low levels of ß-galactosidase activity whether or not LB broth was supplemented with 10 mM MgCl₂ (Fig. 2). Similar results were obtained by measuring the ß-galactosidase activity of the mgrB::lacZ transcriptional fusion (18) (data not shown). These data indicated that mutations T48V, T48I, and T48L in the PhoQ_His protein affect the PhoP/PhoQ signaling cascade. As observed previously for mutation T48I (24), mutation T48V confers to cells a PhoP constitutively active phenotype. In contrast, mutation T48L appeared to barely respond to changes in the concentration of external MgCl₂, conferring to cells a PhoP constitutively inactive phenotype.

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FIG. 2. Regulation of the mgtA::lacZ transcriptional fusion by the PhoQ-T48X mutants. (A) E. coli MG1607 cells carrying the pPROQHis-T48X plasmids were grown in LB broth or LB broth supplemented with 10 mM MgCl2. ß-Galactosidase activities are expressed in Miller milliunits. Data are the means of triplicate values with standard deviations. WT, wild type; Ctl., control. (B) Western blot analysis of the expression level of the various PhoQ-T48X mutants.

In vitro global activity of the PhoP/PhoQ-T48X systems. The level of phospho-PhoP inside the cell depends on both the autokinase and phosphatase activities of PhoQ. To assess in vitro the global activity of the PhoP/PhoQ-T48X systems, we reconstituted functional signaling pathways and measured the resulting net phosphorylation of PhoP. The various membranes containing the PhoQ-T48X proteins were incubated with a sixfold molar excess of PhoP_His in the presence of 5 mM MgCl₂. Figure 3 shows the amounts of [³²P]phospho-PhoP_His resulting from the catalytic activities of the various PhoQ-T48X proteins after a 20-min incubation period. For membranes containing the PhoQ-T48A, T48S, and T48L mutants, levels of radiolabeled PhoP_His were similar to those obtained with wild-type PhoQ (Fig. 3). Sixfold and ninefold increases in radiolabeled PhoP_His were observed with membranes containing the PhoQ-T48I and PhoQ-T48V mutants, respectively (Fig. 3). These data, consistent with our in vivo data shown in Fig. 2, confirmed that a Val or Ile residue at position 48 increases the net phosphorylation of PhoP. They also indicated that the Thr-to-Leu substitution did not affect the net phosphorylation of PhoP under these experimental conditions.

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FIG. 3. In vitro global activity of the PhoP/PhoQ-T48X regulatory systems. Membranes containing the PhoQ-T48X proteins were incubated at 22°C with a sixfold molar excess of PhoPHis in the presence of [-32P]ATP and 5 mM MgCl2. After 20 min, reactions (15 µl) were stopped by the addition of Laemmli SDS sample buffer. Aliquots were subjected to SDS-PAGE. The amount of 32P associated with the PhoPHis protein was quantitated with a PhosphorImager. Data are the means of triplicate values with standard deviations. WT, wild type.

Influence of Mg²⁺ on the in vitro global activity of the PhoP/PhoQ-T48L system. With the exception of the PhoQ-T48L protein, all the PhoQ-T48X sensors responded to changes in the concentrations of external MgCl₂ (Fig. 2). To further investigate the apparent inability of this mutated protein to respond to MgCl₂, we performed in vitro global assays at increasing concentrations of MgCl₂. As shown in Fig. 4, increasing the concentration of MgCl₂ from 1 to 10 mM decreased levels of radiolabeled PhoP_His by about 10-fold for wild-type PhoQ. In contrast, the PhoQ-T48L mutant only produced a twofold decrease in the level of radiolabeled PhoP_His (Fig. 4). These data indicated that the PhoQ-T48L sensor barely responds to the absence of Mg²⁺, suggesting that the Thr-to-Leu substitution locks the protein in a conformation that confers a PhoP constitutively inactive phenotype.

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FIG. 4. Influence of Mg2+ on the in vitro global activity of the PhoP/PhoQ or PhoP/PhoQ-T48L regulatory system. Membranes containing the PhoQ or PhoQ-T48L proteins were incubated at 22°C with a sixfold molar excess of PhoPHis in the presence of [-32P]ATP and increasing concentrations of MgCl2. After 20 min, reactions (15 µl) were stopped by the addition of Laemmli SDS sample buffer. Aliquots were subjected to SDS-PAGE. The amount of 32P associated with the PhoPHis protein was quantitated with a PhosphorImager. WT, wild type.

In vitro autokinase activity of the PhoQ-T48X sensors. We wished to determine which of the individual PhoQ catalytic activities (autokinase and phosphatase) were affected by the mutations at position 48. We measured the initial rates of autophosphorylation of the various PhoQ-T48X sensors present in membranes. Using similar amounts of the various PhoQ-T48X proteins as judged by SDS-PAGE, autophosphorylation assays were performed as described in Materials and Methods. The PhoQ-T48I and PhoQ-T48V mutants were autophosphorylated at rates that are almost identical to that obtained for wild-type PhoQ (Fig. 5). In contrast, the Thr-to-Leu substitution (PhoQ-T48L) decreased the rate of autophosphorylation by about threefold (Fig. 5). Both the PhoQ-T48S and PhoQ-T48A mutants were autophosphorylated at rates that are fivefold slower than that obtained for the wild-type protein (Fig. 5). These data showed that the rates of PhoQ autophosphorylation vary significantly according to the nature of the substituting amino acid at position 48.

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FIG. 5. Initial rates of autophosphorylation of the PhoQ-T48X proteins. Membranes containing wild-type (WT) PhoQ (), PhoQ-T48A (), PhoQ-T48S (), PhoQ-T48V (), PhoQ-T48I (•), or PhoQ-T48L () were incubated in the presence of [-32P]ATP and 0.1 mM mgCl2 for 2 min at 22°C. Reactions (15 µl) were stopped by the addition of Laemmli SDS sample buffer. Aliquots were subjected to SDS-PAGE. The amount of 32P associated with the PhoQ protein was quantitated with a PhosphorImager.

In vitro phosphatase activity of the PhoQ-T48X sensors. Substitutions at position 48 might affect not only PhoQ autokinase activity but also its phosphatase activity. Therefore, we compared the phosphatase activities of the various PhoQ-T48X sensors in vitro. Purified [³²P]phospho-PhoP_His was incubated with membranes containing the various PhoQ-T48X proteins. Aliquots were removed at different time points, and the time course of the reaction was monitored as shown in Fig. 6. A control reaction in which [³²P]phospho-PhoP_His was incubated with control membranes lacking PhoQ indicated that [³²P]phospho-PhoP_His was stable during the reaction period. The phosphatase activities of PhoQ-T48I and PhoQ-T48V were decreased compared to that of wild-type PhoQ (Fig. 6). In contrast, the PhoQ-T48L protein and, to a lesser extent, the PhoQ-T48A protein showed increased phosphatase activities compared to wild-type PhoQ (Fig. 6). The phosphatase activity of PhoQ-T48S was essentially similar to that of wild-type PhoQ (Fig. 6). These data indicated that PhoQ phosphatase activity is also significantly affected by the various substitutions at position 48. Thus, we conclude that both the autokinase and phosphatase activities of PhoQ might be affected by the mutations at position 48.

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FIG. 6. Dephosphorylation of phospho-PhoPHis by the PhoQ-T48X proteins. [32P]phospho-PhoPHis was prepared and purified as described in Materials and Methods. Purified [32P]phospho-PhoPHis was incubated with either control membranes lacking PhoQ (Ctl.) or membranes containing PhoQ-T48X proteins. At indicated time points, aliquots (15 µl) were removed and reactions were stopped by the addition of Laemmli SDS sample buffer. Aliquots were subjected to SDS-PAGE. The amount of 32P associated with the PhoP protein was determined with a PhosphorImager. WT, wild type.

Top Abstract Introduction Materials and Methods Results Discussion Addendum References

 
Previous studies have shown that a change of a Thr to Ile at position 48 of the PhoQ histidine kinase sensor (pho-24 allele of phoQ) results in a constitutively active PhoP/PhoQ regulatory system in S. enterica serovar Typhimurium (10, 14, 24). In our study, we examined the influence of various amino acid substitutions (Ala, Ser, Val, Ile, and Leu) at position 48 of PhoQ on signal transduction by PhoP/PhoQ. We identified three distinct classes of mutations, two of which altered expression of the mgtA::lacZ transcriptional fusion (Fig. 2).

The first class of mutations is represented by the mutations T48A and T48S. These mutations did not significantly alter the Mg²⁺-regulated expression of the mgtA::lacZ transcriptional fusion (Fig. 2). In vitro reconstitution of the PhoP/PhoQ-T48X systems showed that these mutations did not have an effect on the net autophosphorylation of PhoP (Fig. 3). However, analysis of the individual PhoQ catalytic activities showed that both mutations affected autokinase activity and, to a lesser extent, phosphatase activity (Fig. 5 and 6). Therefore, we conclude that in spite of differences in the individual activities, the balance between autokinase and phosphatase activity remained essentially unchanged for PhoQ-T48A and PhoQ-T48S. Interestingly, the side chains of Ala and Ser are smaller than that of the native Thr. Accordingly, we propose that small side chains or loss of the hydroxyl group at position 48 does not cause major structural alterations leading to important changes in the global activity.

The second class of mutations is represented by the mutations T48V and T48I (pho-24 allele of phoQ). Both mutations increased expression of the mgtA::lacZ transcriptional fusion and conferred a PhoP constitutively active phenotype (Fig. 2) (24). Both mutated proteins responded to increasing concentrations of Mg²⁺, albeit to a lesser extent than wild-type PhoQ (Fig. 2) (10). The increased net phosphorylation of PhoP observed for mutant T48V was essentially similar to that observed previously for the mutation T48I (Fig. 3) (14). By analyzing in vitro the individual autokinase and phosphatase activities, we found that PhoQ-T48V and PhoQ-T48I have decreased phosphatase activity whereas the rates of autophosphorylation were identical to that of wild-type PhoQ (Fig. 5 and 6). Thus, the PhoP constitutively active phenotype observed for the PhoP/PhoQ-T48V and PhoP/PhoQ-T48I systems is solely due to decreased phosphatase activity of PhoQ. For these mutated PhoQ sensors, the balance between autokinase and phosphatase activity shifted toward a kinase-dominant state. It is noteworthy that both Val and Ile are hydrophobic ß-branched residues, whereas the native Thr is a polar ß-branched residue. Importantly, only hydrophobic residues that were ß branched but not branched conferred a PhoP constitutively active phenotype. These observations suggest that the hydrophobicity as well as the shape of the residue at position 48 might be critical for PhoQ transmembrane signaling.

The third class of mutations is represented by the mutation T48L, which confers a PhoP constitutively inactive phenotype. For this mutation, expression of the mgtA::lacZ transcriptional fusion was repressed irrespective of the presence or absence of Mg²⁺ (Fig. 2). When compared to wild-type PhoQ, limiting concentrations of Mg²⁺ had minimal effect on the net phosphorylation of PhoP measured in vitro (Fig. 4). We found that this phenotype resulted from both a decreased autokinase activity and an increased phosphatase activity (Fig. 5 and 6). Thus, the PhoQ-T48L sensor is in a phosphatase-dominant state irrespective of the presence or absence of Mg²⁺. Leu is a hydrophobic residue that is isomeric to Ile but is branched. Thus, the longer side chain length of the Leu residue at position 48 might provide a steric hindrance that is responsible for the PhoP constitutively inactive phenotype observed for the PhoP/PhoQ-T48L system. This substantiates our hypothesis that both the shape and the hydrophobicity of residue 48 are critical for PhoQ transmembrane signaling.

The residue at position 48 of PhoQ might influence signal transduction by directly affecting Mg²⁺ binding or by interfering with the Mg²⁺-induced conformational signal that is transmitted through the membrane bilayer. The direct involvement of residue 48 in Mg²⁺ recognition is most unlikely, because the response to increasing concentrations of external Mg²⁺ was essentially similar for four of the five mutated PhoQ proteins analyzed (Fig. 2). It appears more likely that residue 48 is an important structural determinant for transmitting the Mg²⁺-induced transmembrane signal. Our data support our hypothesis that the side chain of residue 48 is involved in the conformational changes responsible for the switch between the kinase-dominant state and the phosphatase-dominant state.

Residue 48 of PhoQ is located at the N terminus of the periplasmic domain in close proximity to the cytoplasmic membrane (Fig. 1A). In closely related PhoQ homologues, like the PhoQ proteins of other enterobacteria, the Thr residue at position 48 is strictly conserved (Fig. 1B). In the Pseudomonas aeruginosa and Xylella fastidiosa PhoQ homologues, the residue 48 consists of an Ile and a Leu, respectively (Fig. 1B). Our results show that these mutations affect signaling of the Salmonella PhoQ protein. It is possible that in the three-dimensional structure of these proteins, compensating mutations counterbalance the presence of an Ile or a Leu at position 48. Alternatively, it is possible that the nature of the residue at position 48 modulates the level of expression of PhoP-regulated genes. Note that the environmental signal sensed by some of these PhoQ homologues may be different than Mg²⁺ (12). In other histidine kinase sensors, the corresponding region has been shown to be important for either transmembrane signaling or ligand recognition. The highly conserved I box that includes residues 41 to 53 of various EnvZ homologues has been shown to be involved in the signal transduction mechanism (30). The P box of the NarQ and NarX sensors that corresponds to a stretch of 17 conserved amino acids has been shown to be required for nitrate sensing and/or transmembrane signaling (4, 5, 31). Although the corresponding region in PhoQ homologues is not as highly conserved as the I box or the P box (Fig. 1B), the location of position 48 implies that this region is important for transmembrane signaling.

Taken together, our data indicate that substitutions at position 48 of PhoQ affect the balance between autokinase and phosphatase activities. Our findings define the structural requirement at position 48 of PhoQ and suggest that this residue is critical for the transmission of the ligand-induced conformational signal through the membrane bilayer. Future studies will determine whether the conformational changes that involve residue 48 affect the dimeric interface of the protein or the structure of isolated subunits.

Top Abstract Introduction Materials and Methods Results Discussion Addendum References

 
After this paper was submitted, Regelmann et al. (A. G. Regelmann, J. A. Lesley, C. Mott, L. Stokes, and C. D. Waldburger, J. Bacteriol. 184:5468-5478, 2002) reported a similar study of the E. coli PhoQ sensor kinase. Although the PhoQ proteins of S. enterica serovar Typhimurium and E. coli are 86% identical and exhibit a Thr at position 48, the PhoQ-T48I mutants display opposite phenotypes.

 
We thank Ryutaro Utsumi for providing strain MG1607. We thank J. A. Kashul for editorial support.

This work was supported by grant MT-15551 from the Canadian Institutes for Health Research and by a fellowship to H.L.M. from Fonds de la Recherche en Santé du Québec (FRSQ). S.S. was the recipient of an F. C. Harrison Fellowship from the Department of Microbiology and Immunology, McGill University.

 
* Corresponding author. Mailing address: Lyman Duff Medical Building, McGill University, 3775 University St., Montréal, Québec, Canada H3A 2B4. Phone: (514) 398-6235. Fax: (514) 398-7052. E-mail: herve.le-moual{at}mcgill.ca.

Top Abstract Introduction Materials and Methods Results Discussion Addendum References

 

1
1. Alpuche-Aranda, C. M., E. L. Racoosin, J. A. Swanson, and S. I. Miller. 1994. Salmonella stimulate macrophage macropinocytosis and persist within spacious phagosomes. J. Exp. Med. 179:601-608.[Abstract/Free Full Text]
2
2. Behlau, I., and S. I. Miller. 1993. A PhoP-repressed gene promotes Salmonella typhimurium invasion of epithelial cells. J. Bacteriol. 175:4475-4484.[Abstract/Free Full Text]
3
3. Castelli, M. E., E. García Véscovi, and F. C. Soncini. 2000. The phosphatase activity is the target for Mg²⁺ regulation of the sensor protein PhoQ in Salmonella. J. Biol. Chem. 275:22948-22954.[Abstract/Free Full Text]
4
4. Cavicchioli, R., R. C. Chiang, L. V. Kalman, and R. P. Gunsalus. 1996. Role of the periplasmic domain of the Escherichia coli NarX sensor-transmitter protein in nitrate-dependent signal transduction and gene regulation. Mol. Microbiol. 21:901-911.[CrossRef][Medline]
5
5. Chiang, R. C., R. Cavicchioli, and R. P. Gunsalus. 1997. "Locked-on" and "locked-off" signal transduction mutations in the periplasmic domain of the Escherichia coli NarQ and NarX sensors affect nitrate- and nitrite-dependent regulation by NarL and NarP. Mol. Microbiol. 24:1049-1060.[CrossRef][Medline]
6
6. Deng, W. P., and J. A. Nickoloff. 1992. Site-directed mutagenesis of virtually any plasmid by eliminating a unique site. Anal. Biochem. 200:81-88.[CrossRef][Medline]
7
7. Dutta, R., L. Qin, and M. Inouye. 1999. Histidine kinases: diversity of domain organization. Mol. Microbiol. 34:633-640.[CrossRef][Medline]
8
8. Ernst, R. K., T. Guina, and S. I. Miller. 2001. Salmonella typhimurium outer membrane remodeling: role in resistance to host innate immunity. Microbes Infect. 3:1327-1334.[CrossRef][Medline]
9
9. Fields, P. I., E. A. Groisman, and F. Heffron. 1989. A Salmonella locus that controls resistance to microbicidal proteins from phagocytic cells. Science 243:1059-1062.[Abstract/Free Full Text]
10
10. García Véscovi, E., F. C. Soncini, and E. A. Groisman. 1996. Mg²⁺ as an extracellular signal: environmental regulation of Salmonella virulence. Cell 84:165-174.[CrossRef][Medline]
11
11. Groisman, E. A. 1998. The ins and outs of virulence gene expression: Mg²⁺ as a regulatory signal. BioEssays 20:96-101.[CrossRef][Medline]
12
12. Groisman, E. A. 2001. The pleiotropic two-component regulatory system PhoP-PhoQ. J. Bacteriol. 183:1835-1842.[Free Full Text]
13
13. Groisman, E. A., E. Chiao, C. J. Lipps, and F. Heffron. 1989. Salmonella typhimurium phoP virulence gene is a transcriptional regulator. Proc. Natl. Acad. Sci. USA 86:7077-7081.[Abstract/Free Full Text]
14
14. Gunn, J. S., E. L. Hohmann, and S. I. Miller. 1996. Transcriptional regulation of Salmonella virulence: a PhoQ periplasmic domain mutation results in increased net phosphotransfer to PhoP. J. Bacteriol. 178:6369-6373.[Abstract/Free Full Text]
15
15. Guo, L., K. B. Lim, J. S. Gunn, B. Bainbridge, R. P. Darveau, M. Hackett, and S. I. Miller. 1997. Regulation of lipid A modifications by Salmonella typhimurium virulence genes phoP-phoQ. Science 276:250-253.[Abstract/Free Full Text]
16
16. Guo, L., K. B. Lim, C. M. Poduje, M. Daniel, J. S. Gunn, M. Hackett, and S. I. Miller. 1998. Lipid A acylation and bacterial resistance against vertebrate antimicrobial peptides. Cell 95:189-198.[CrossRef][Medline]
17
17. Hopkins, S., J. P. Kraehenbuhl, F. Schodel, A. Potts, D. Peterson, P. de Grandi, and D. Nardelli-Haefliger. 1995. A recombinant Salmonella typhimurium vaccine induces local immunity by four different routes of immunization. Infect. Immun. 63:3279-3286.[Abstract]
18
18. Kato, A., H. Tanabe, and R. Utsumi. 1999. Molecular characterization of the PhoP-PhoQ two-component system in Escherichia coli K-12: identification of extracellular Mg²⁺-responsive promoters. J. Bacteriol. 181:5516-5520.[Abstract/Free Full Text]
19
19. Kier, L. D., R. M. Weppelman, and B. N. Ames. 1979. Regulation of nonspecific acid phosphatase in Salmonella: phoN and phoP genes. J. Bacteriol. 138:155-161.[Abstract/Free Full Text]
20
20. Le Moual, H., T. Quang, and D. E. Koshland, Jr. 1998. Conformational changes in the cytoplasmic domain of the Escherichia coli aspartate receptor upon adaptive methylation. Biochemistry 37:14852-14859.[CrossRef][Medline]
21
21. Lesley, J. A., and C. D. Waldburger. 2001. Comparison of the Pseudomonas aeruginosa and Escherichia coli PhoQ sensor domains. Evidence for distinct mechanisms of signal detection. J. Biol. Chem. 276:30827-30833.[Abstract/Free Full Text]
22
22. Miller, J. H. 1972. Experiments in molecular genetics. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
23
23. Miller, S. I., A. M. Kukral, and J. J. Mekalanos. 1989. A two-component regulatory system (phoP phoQ) controls Salmonella typhimurium virulence. Proc. Natl. Acad. Sci. USA 86:5054-5058.[Abstract/Free Full Text]
24
24. Miller, S. I., and J. J. Mekalanos. 1990. Constitutive expression of the phoP regulon attenuates Salmonella virulence and survival within macrophages. J. Bacteriol. 172:2485-2490.[Abstract/Free Full Text]
25
25. Miller, S. I., W. S. Pulkkinen, M. E. Selsted, and J. J. Mekalanos. 1990. Characterization of defensin resistance phenotypes associated with mutations in the phoP virulence regulon of Salmonella typhimurium. Infect. Immun. 58:3706-3710.[Abstract/Free Full Text]
26
26. Montagne, M., A. Martel, and H. Le Moual. 2001. Characterization of the catalytic activities of the PhoQ histidine protein kinase of Salmonella enterica serovar Typhimurium. J. Bacteriol. 183:1787-1791.[Abstract/Free Full Text]
27
27. Pegues, D. A., M. J. Hantman, I. Behlau, and S. I. Miller. 1995. PhoP/PhoQ transcriptional repression of Salmonella typhimurium invasion genes: evidence for a role in protein secretion. Mol. Microbiol. 17:169-181.[CrossRef][Medline]
28
28. Soncini, F. C., E. García Véscovi, F. Solomon, and E. A. Groisman. 1996. Molecular basis of the magnesium deprivation response in Salmonella typhimurium: identification of PhoP-regulated genes. J. Bacteriol. 178:5092-5099.[Abstract/Free Full Text]
29
29. Van Velkinburgh, J. C., and J. S. Gunn. 1999. PhoP-PhoQ-regulated loci are required for enhanced bile resistance in Salmonella spp. Infect. Immun. 67:1614-1622.[Abstract/Free Full Text]
30
30. Waukau, J., and S. Forst. 1999. Identification of a conserved N-terminal sequence involved in transmembrane signal transduction in EnvZ. J. Bacteriol. 181:5534-5538.[Abstract/Free Full Text]
31
31. Williams, S. B., and V. Stewart. 1997. Discrimination between structurally related ligands nitrate and nitrite controls autokinase activity of the NarX transmembrane signal transducer of Escherichia coli K-12. Mol. Microbiol. 26:911-925.[CrossRef][Medline]

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Journal of Bacteriology, March 2003, p. 1935-1941, Vol. 185, No. 6
0021-9193/03/$08.00+0     DOI: 10.1128/JB.185.6.1935-1941.2003
Copyright © 2003, American Society for Microbiology. All Rights Reserved.

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