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The Pseudomonas aeruginosa Universal Stress Protein PA4352 Is Essential for Surviving Anaerobic Energy Stress

Institute of Microbiology, Technical University Braunschweig, Spielmannstr. 7, D-38106 Braunschweig, Germany,¹ Department of Cell Biology, German Research Centre for Biotechnology, Mascheroder Weg 1, D-38124 Braunschweig, Germany²

Received 2 March 2006/ Accepted 28 June 2006

	ABSTRACT

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During infection of the cystic fibrosis (CF) lung, Pseudomonas aeruginosa microcolonies are embedded in the anaerobic CF mucus. This anaerobic environment seems to contribute to the formation of more robust P. aeruginosa biofilms and to an increased antibiotic tolerance and therefore promotes persistent infection. This study characterizes the P. aeruginosa protein PA4352, which is important for survival under anaerobic energy stress conditions. PA4352 belongs to the universal stress protein (Usp) superfamily and harbors two Usp domains in tandem. In Escherichia coli, Usp-type stress proteins are involved in survival during aerobic growth arrest and under various other stresses. A P. aeruginosa PA4352 knockout mutant was tested for survival under several stress conditions. We found a decrease in viability of this mutant compared to the P. aeruginosa wild type during anaerobic energy starvation caused by the missing electron acceptors oxygen and nitrate. Consistent with this phenotype under anaerobic conditions, the PA4352 knockout mutant was also highly sensitive to carbonyl cyanide m-chlorophenylhydrazone, the chemical uncoupler of the electron transport chain. Primer extension experiments identified two promoters upstream of the PA4352 gene. One promoter is activated in response to oxygen limitation by the oxygen-sensing regulatory protein Anr. The center of a putative Anr binding site was identified 41.5 bp upstream of the transcriptional start site. The second promoter is active only in the stationary phase, however, independently of RpoS, RelA, or quorum sensing. This is the second P. aeruginosa Usp-type stress protein that we have identified as important for survival under anaerobic conditions, which resembles the environment during persistent infection.

	INTRODUCTION

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Pseudomonas aeruginosa is an adaptable opportunistic pathogen that causes a variety of nosocomial infections and burn-related sepsis and is also the dominant pathogen during infection of the cystic fibrosis (CF) lung (25, 27, 39). During infection, biofilm-like growth protects P. aeruginosa from the host immune response and the actions of antibiotics (11, 20, 37). Another factor important for persistent infection of the cystic fibrosis lung was identified by Worlitzsch et al. (45), who showed that the biofilm-like microcolonies of P. aeruginosa are embedded in oxygen-limited mucus. This oxygen-limited environment promotes the formation of more robust biofilms (45, 47). Particularly, the combination of oxygen restriction and biofilm growth seems to increase antibiotic tolerance and therefore promotes persistent infection by P. aeruginosa (9, 16, 20, 47).

Although anaerobic conditions are important for persistent infection, P. aeruginosa has only limited capabilities to grow and survive anaerobically. Anaerobic growth is sustained by denitrification (33, 49), which requires nitrate or nitrite. Both substrates were detected in small amounts (50 to 350 µM) in CF lung mucus and in airway surface liquid (19, 24, 45). In the absence of nitrate and nitrite, P. aeruginosa survives anaerobiosis by arginine fermentation, which allows moderate anaerobic growth (40). We recently identified a pyruvate fermentation pathway that allows anaerobic survival but does not sustain anaerobic growth (15). In the absence of pyruvate, arginine, or nitrate/nitrite, P. aeruginosa rapidly faces energy starvation in an anaerobic environment, and cell numbers decrease dramatically (7, 15). A proteome analysis of P. aeruginosa cells during pyruvate fermentation identified PA3309, a protein containing a universal stress protein (Usp) signature domain. This Usp-type protein was shown to be essential for survival during pyruvate fermentation (36) and was reported to be present in anaerobic biofilms (47). Moreover, we found the promoter of the corresponding gene to be induced in deeper layers of a biofilm. A proteome analysis of P. aeruginosa under pyruvate fermentation revealed 22-fold-increased production of a second Usp-type stress protein, PA4352 (36). In contrast to the PA3309 mutant, deletion of the PA4352 gene did not reduce survival during pyruvate fermentation. According to the Pfam database, the Usp signature is present in more than 1,000 proteins (4) from organisms of all domains of life (26). In Escherichia coli, Usp-type stress proteins are important for surviving various stress conditions and aerobic stationary phase (18, 26). However, their exact biological functions remain unclear, although more data have emerged from E. coli showing the physiological roles of the Usp proteins in iron metabolism, oxidative stress, adhesion, and motility (30).

In this study, we focused on the anaerobically induced Usp-type protein PA4352. This protein exhibits two Usp domains in tandem. We investigated the regulation of the PA4352 gene and the potential function of its product during starvation for energy, and thus its role in promoting survival in an anaerobic environment during persistent infection.

	MATERIALS AND METHODS

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Bacterial strains and growth conditions. The bacterial strains and plasmids used in this study are shown in Table 1. For standard molecular biology protocols, E. coli and P. aeruginosa strains were grown in Luria-Bertani (LB) medium as described before (36).

Growth conditions to elucidate the phenotype of the PA4352 mutant.

Secondly, the breakdown of the PMF was achieved by limiting oxygen in the aerobic electron transport chain after prolonged incubation in the aerobic stationary phase. Therefore, cultures of P. aeruginosa were first grown in LB medium under aerobic conditions to the stationary phase, which was reached at an OD₅₇₈ of 7.0. After 15 h of incubation in the stationary phase, the cultures were transferred into hermetically sealed bottles to generate an anaerobic environment. Survival was determined by viable-cell counts during the following 33 h. To save the phenotype with the alternative electron acceptor nitrate, KNO₃ (75 mM) was added to the prior aerobic cultures.

Thirdly, we showed that sensitivity of the mutant was caused by a depolarization of the membrane. PMF was destroyed with the protonophor carbonyl cyanide m-chlorophenylhydrazone (CCCP) in the anaerobic stationary phase. To prevent death in the anaerobic stationary phase caused by nitrate limitation, additional KNO₃ (30 mM) was added after 7 h in the stationary phase, and 0.2 mM CCCP was added to cause depolarization of the membrane.

Viable-cell counts and control experiments. Viable-cell counts were performed by plating aliquots of the anaerobic cultures on LB agar plates. After 24 h, aerobic-incubation colonies were counted and cell numbers were determined. In control experiments, we incubated LB agar plates containing 50 mM nitrate anaerobically. Under these conditions, we also observed small colonies and significantly reduced viability of the mutant, as with aerobic plating. However, anaerobic plating resulted in a delayed decrease in viability compared to aerobic plating but also confirmed clear premature death of the PA4352 mutant strain (data not shown). We also verified a decrease in viability of the wild-type and mutant strains by fluorescence microscopic analysis of the samples after the cells were stained using the Live/Dead BacLight kit (Molecular Probes, Leiden, The Netherlands) following the instructions of the manufacturer, which confirmed the death of cells during the anaerobic stationary phase.

Construction and testing of the promoter-lacZ reporter gene fusions. Chromosomal promoter-lacZ reporter gene fusions were constructed using the mini-CTX-lacZ vector (6). A 465-bp PCR product, covering the region between 454 bp and 6 bp upstream of the translational start site of the PA4352 gene, was generated using primers oKS18 (5'-GGAATTCACGGACTACGCCGACGAACC-3') and oKS19 (5'-CGCGGATCCACCTCC ATTGGCAGAGC-3'). oKS18 contained an EcoRI restriction site at the 5' end (underlined), and oKS19 contained a restriction site for BamHI, also at its 5' end (underlined). The EcoRI- and BamHI-digested PCR product was cloned between the EcoRI and BamHI sites of mini-CTX-lacZ to generate pNB003. Transfer of pNB003 in P. aeruginosa was carried out by a diparental mating using E. coli S17-pir as the donor. The CTX integrase of pNB003 promoted integration of the vector into the attB site of the P. aeruginosa genome. The vector was transferred into the P. aeruginosa wild type, the anr mutant strain PAO6261, and the dnr mutant strain BB71 to generate the P. aeruginosa strains NB007, NB023, and NB086, respectively (Table 1). In these mutant strains, parts of the mini-CTX-lacZ vector containing the tetracycline resistance cassette were deleted using an FLP (flippase) recombinase encoded by the pFLP2 plasmid (22). ß-Galactosidase assays were performed as outlined before in detail (15, 34, 36). The activities obtained were reported in Miller units (28).

To test the activation of P_PA4352 under anaerobic conditions, cells were incubated aerobically in LB and were transferred to anaerobic flasks at an OD₅₇₈ of 0.7. Activities were determined before and 4 h after the culture was shifted to anaerobic conditions.

The ß-galactosidase activities of aerobically grown cultures were determined in the exponential growth phase (OD₅₇₈, 0.7) and in the late stationary phase (16 h after entry into stationary phase) in LB.

Mutation of the putative Anr binding site in the PA4352 promoter. The Anr binding site of the PA4352 promoter was mutated using the crossover-PCR technique (21) to generate the promoter P_PA4352ANR. The putative Anr binding site TTGATGTGCATCAA (the target of the mutation is underlined) 75.5 bp upstream of the translational start site was mutated to TTGATGTGCATACG using the primers oNB044 (5'-GAAGCATCCGCCGTATGCACATCAAC-3') and oNB045 (5'-CATACGGCGGATGCTT CGGACTGAAACA-3') (mutated bases of the Anr binding site are underlined). The mutated promoter was amplified with oKS18 and oKS19 and cloned into the mini-CTX-lacZ vector as described above to generate the plasmid pNB019. This plasmid was introduced in the P. aeruginosa wild type and the mutants PAO6261 (anr), PAO-MW20 (rpoS::aacC1), and KS35 (relA) (Table 1) to generate the strains NB071, NB072, NB073, and NB074, respectively.

Construction of P. aeruginosa PA4352, rhlR::Tc^r, lasR::Gm^R, and dnr mutant strains. To obtain unmarked gene deletion mutants, we used the well-established strategies based on sacB counterselection and FLP recombinase excision (22). To construct the suicide vector pNB007, the BamHI-digested gentamicin resistance cassette of pPS858 was cloned between two PCR fragments of the PA4352 gene in the multiple cloning site of pEX18Ap. The two PCR fragments contained DNA homologous to the upstream and downstream areas of the PA4352 gene. A 596-bp fragment containing the upstream promoter region of the PA4352 gene was amplified using primer oNB01 (5'-CGAGCTCTACGGCGACTTCGTCAAGG-3'), containing a SacI restriction site at the 5' end, and oNB02 (5'-CGGGATCCAAGCGGATGCTTCGGACT-3'), containing a BamHI site (both underlined). The primers oNB03 (5'-CGCGGATCCCTTCCGCCGCGCGCTGA-3'), containing a BamHI site, and oNB04 (5'-CCCAAGCTTCCCTGGCGCCGCTGACC-3'), containing a HindIII site (both underlined), amplified 617 bp of the corresponding downstream region of PA4352. The suicide vector pNB007 was used to replace the PA4352 gene with a gentamicin cassette by sacB-based counterselection. The resulting mutant, NB011, was verified by Southern blot analysis. Finally, FLP recombinase encoded by the pFLP2 plasmid removed the FLP recombinase target-flanked gentamicin cassette to generate NB015. A dnr knockout mutant was constructed using the same strategy described above. The primer pairs for amplification of the upstream region were oBB50 (5'-CCCAAGCTTAGCGTCGCCTGCTGTTG-3'), containing a HindIII site, and oBB51 (5'CGGGATCCGCGCCGCCGCTTGATCG-3'), containing a BamHI site (both underlined). The primer pairs for amplification of the downstream region were oBB53 (5'-CGGGATCCAAGGCTCGCGATGATGA-3'), containing a BamHI site, and oBB55 (5'-CGAGCTCTGCAGGCGGAACTGAAC-3'), containing a SacI site (both underlined). The resulting suicide plasmid was named pBB25, and the dnr knockout mutant was named BB71.

The two quorum-sensing mutants rhlR::Tc^r (NB075) and lasR::Gm^r (NB076) were constructed as described previously (5), using NB071 as the parental strain.

Complementation of the PA4352 knockout mutant. To circumvent the use of antibiotics during the complementation experiments, the PA4352 gene was integrated chromosomally into the attB site using the vector mini-CTX2. We amplified a 1,674-bp PCR product covering 659 bp of the PA4352 promoter region, the PA4352 gene, and 138 bp downstream of PA4352 using primers oNB01 (5'-CGAGCTCTACGGCGACTTCGTCAAGG-3'), containing a SacI restriction site at the 5' end, and oNB22 (5'-CCCAAGCTTCGGCAGCGTGCATATCC-3'), containing a HindIII site (both underlined). The product was digested with SacI and HindIII and ligated into mini-CTX2 to generate pNB011.

This vector was transferred into P. aeruginosa NB015 to generate NB060 by diparental mating using E. coli S17-pir as the donor and integrated into the attB site of the genome as described above. As a control, the empty mini-CTX2 vector was integrated into the genome of wild-type PAO1 and NB015 to generate NB058 and NB059, respectively.

Proteomic analysis. Cultures for proteome analysis were incubated aerobically in LB medium at 37°C. After 15 h of incubation in the stationary phase, cells were harvested by mixing the cell culture with a double volume of ice-cold potassium phosphate buffer (0.1 M; pH 7.4) and centrifugation at 8,000 x g for 30 min at 4°C. The cells were washed twice with potassium phosphate buffer and were resuspended in 1 ml potassium phosphate buffer. Proteins were isolated form the whole-cell suspension by extraction with an equal volume of phenol and subsequent acetone precipitation (36). The precipitated proteins were solubilized in sample buffer consisting of 7 M urea, 2 M thiourea, 4% 3-[(3-cholamidopropyl)-dimethylammonio]-1-propanesulfonate (CHAPS), 50 mM dithiothreitol, and 2% ampholytes (Bio-Lyte; Bio-Rad, Munich, Germany). The protein concentration was determined in the sample buffer using the PlusOne 2D Quant kit (Amersham Biosciences, Freiburg, Germany). Two-dimensional (2D) gel electrophoresis was performed using 17-cm immobilized pH gradient (IPG) strips covering a pH range from 5 to 8 (IPG Ready Strips; Bio-Rad, Munich, Germany). The IPG strips were loaded with 500 µg of protein, and isoelectric focusing was conducted for a total of 110,000 V · h. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis was performed at a constant temperature of 20°C with 1 W per gel for approximately 20 h using 10% polyacrylamide gels (25.5 by 20.5 cm). All gels were stained with ruthenium(II)-Tris-bathophenanthroline disulfonate as described before (36). The gels were documented with an FX-Scanner (Bio-Rad, Munich, Germany). Identification of protein spots was performed at the Gesellschaft für Biotechnologische Forschung, using a Bruker Ultraflex matrix-assisted laser desorption ionization-time of flight mass spectrometer.

Preparation of RNA for primer extension. Protocols for RNA preparation were based on a modified hot-phenol method (1, 41). For preparations of RNA, appropriate aliquots of cultures (25 ml of a culture with an OD₅₇₈ of 0.7, 5 ml of a culture with an OD₅₇₈ of 2, and 2.5 ml of a culture with an OD₅₇₈ of 5.0) were added to 25 ml of an ice-cold solution containing 20 mM Tris-HCl (pH 7.5), 5 mM MgCl₂, and 20 mM NaN₃. The cells were harvested by centrifugation (10 min at 4,400 x g and 4°C). The cell pellets were immediately frozen in liquid N₂.

The pellets were resuspended in cell lysis solutions consisting of 125 µl 0.3 M sucrose and 0.01 M sodium acetate (pH 5.2) and 125 µl 2% (wt/vol) sodium dodecylsulfate and 0.01 M sodium acetate (pH 5.2). For complete cell lysis, the resuspended cells were incubated at 65°C for 1 min before the addition of prewarmed (65°C) acidic phenol. After incubation at 65°C for 3 min, samples were dropped into liquid N₂ and centrifuged (12,110 x g) for 10 min at room temperature. This procedure was repeated with the upper phase three times following an extraction with acidic phenol-chloroform-isoamyl alcohol (25:24:1 [vol/vol/vol]) and once with chloroform-isoamyl alcohol (24:1 [vol/vol]). After ethanol precipitation, the RNA pellet was resuspended in 180 µl of 20 mM phosphate buffer (pH 6.5), 1 mM EDTA and 20 µl of a solution containing 200 mM sodium acetate (pH 4.5), 100 mM MgCl₂, 100 mM NaCl, and 15 U of DNase I and was then incubated for 30 min at room temperature. Finally, the RNA was purified by phenol-chloroform extraction and ethanol precipitation. The resulting RNA pellet was dissolved in 30 µl of H₂O.

Identification of the PA4352 transcriptional start site. The transcriptional initiation site of PA4352 was determined in the aerobic and anaerobic stationary phases (3 h after entering stationary phase) and in the exponential growth phase of an anaerobic denitrifying culture (OD₅₇₈ = 0.7). Thirty micrograms of RNA was used for primer extension analysis of the PA4352 transcript. Reverse transcription was initiated from the -³²P end-labeled primer oNB21 (5'-AGGACAGGTCGGTCGCCACCAGGATTC-3') by a standard procedure (3). The sequencing reaction was performed with the same primer and plasmid pNB010 containing the PA4352 gene. The primer extension products and the sequencing reactions were analyzed in a 6% denaturing polyacrylamide gel in Tris-borate buffer. The dried gel was analyzed by using a K-Screen (Kodak) and a phosphorimager (FX-Scanner; Bio-Rad).

	RESULTS

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Phenotype of the PA4352 mutant. Recently, we found increased production of the hypothetical protein PA4352 in a proteome analysis of Pseudomonas aeruginosa during pyruvate fermentation (36). However, a P. aeruginosa PA4352 knockout mutant showed no reduced survival during pyruvate fermentation (36). According to the Pfam database, the PA4352 protein belongs to the Usp-type stress proteins and contains two Usp domains in tandem (4). Escherichia coli usp mutants show decreased viability in response to various stress conditions (18). To determine if the P. aeruginosa PA4352 mutant shared a similar phenotype, we tested its sensitivity to H₂O₂, heat shock at 53°C, UV light, and osmotic shock with 3 M NaCl and 10% ethanol. No increased sensitivity was detected for the PA4352 mutant (data not shown), in contrast to published data for the E. coli uspA, uspC, uspD, and uspE mutants, which showed decreased survival under the tested growth conditions (18). Investigations of the P. aeruginosa PA4352 mutant under anaerobic growth conditions revealed no growth phenotype compared to wild-type P. aeruginosa during exponential growth in LB supplemented with 50 mM KNO₃. However, when the PA4352 mutant reached the anaerobic stationary phase, we observed the following phenotypes after 9 and 15 h of incubation in the stationary phase. First, after 9 h of incubation in the anaerobic stationary phase, we noticed a remarkably smaller colony size of the PA4352 mutant than of the wild-type colonies, when cells were plated on LB agar plates and incubated aerobically for viable-cell counts (see Materials and Methods) (Fig. 1). However, the numbers of CFU of the wild type and mutant did not differ at this time. To test whether smaller colony size corresponded to reduced growth rates, we determined the growth curve of the mutants. Aliquots of the 9-h anaerobic stationary-phase cultures were taken to inoculate fresh LB cultures and to monitor aerobic growth. The growth curve of the PA4352 mutant showed an extended lag phase compared to that of the wild type, while the growth rate after recovery was comparable to that of wild-type cells (doubling times: PAO1, 34 min; PA4352, 36 min) (Fig. 2).

View larger version (77K): [in this window] [in a new window]   FIG. 1. Phenotype of the CFU obtained from viable plating of P. aeruginosa wild-type cells and the PA4352 mutant on LB agar plates after 9 hours of anaerobic stationary phase. Cultures of P. aeruginosa were incubated anaerobically in LB supplemented with 50 mM KNO3. After 9 hours of incubation in the stationary phase, aliquots from (A) wild-type P. aeruginosa containing the empty mini-CTX2 vector (NB058), (B) the PA4352 mutant containing the empty mini-CTX2 vector (NB059), and (C) the complemented PA4352 mutant containing pNB011 with the PA4352 gene (NB060) were taken, and 50 µl of a 10–5 dilution was plated on LB agar plates. The plates were incubated aerobically for 20 h at 37°C.

View larger version (8K): [in this window] [in a new window]   FIG. 2. Effect of the PA4352 knockout in P. aeruginosa on recovery from nitrate starvation in the anaerobic stationary phase. Cultures of P. aeruginosa were incubated anaerobically in LB supplemented with 50 mM KNO3 and allowed to pass 9 h of stationary phase before being diluted in fresh LB medium. The inoculum contained 4.2 x 108 to 6.1 x 108 viable cells per ml as determined by viable-cell counts and Live/Dead staining (see Materials and Methods). The diluted cultures were incubated aerobically at 37°C to generate the growth curves shown of the wild-type strain containing the empty mini-CTX2 (NB058) (open triangles), the PA4352 mutant containing the empty mini-CTX2 vector (NB059) (filled squares), and the complemented PA4352 mutant (NB060) containing pNB011 with the PA4352 gene (open squares). To rescue the phenotype of the PA4352 mutant, one culture of the PA4352 mutant was supplemented with additional KNO3 (30 mM) 5 hours prior to dilution (filled circles).

Secondly, extended incubation in the anaerobic stationary phase for up to 15 h led to premature death of the PA4352 mutant. Again, viable-cell numbers were determined after serial dilutions of the anaerobic stationary-phase cultures were plated on LB agar, and CFU were monitored after aerobic incubation. We observed a 77-fold decrease in viability of the PA4352 mutant, while wild-type cells and complemented mutant cells showed only a 1.5- to 2-fold loss of viability. Figure 3A shows the time-dependent reduction of viability in the stationary phase after 7, 11, 13, and 15 h.

View larger version (30K): [in this window] [in a new window]   FIG. 3. Premature death of the PA4352 mutant caused by restriction of the terminal electron acceptor nitrate (A), by restriction of oxygen (B), and by addition of CCCP in the anaerobic stationary phase (C). (A) Cultures of P. aeruginosa were incubated anaerobically in LB supplemented with 50 mM KNO3. The survival (%) of wild-type cells containing the empty mini-CTX2 vector (NB058) (gray bars), of the PA4352 mutant containing the empty mini-CTX2 vector (NB059) (black bars), and of the complemented PA4352 mutant (NB060) (white bars) was determined by viable-cell counts during the stationary phase. One culture of the PA4352 mutant was supplemented with additional KNO3 (30 mM) 7 hours after entry into the stationary phase (striped bars). (B) Cultures of P. aeruginosa were incubated aerobically in LB, and as a control, an additional culture of the PA4352 mutant was incubated in LB supplemented with KNO3 (50 mM). After reaching the stationary phase, the cultures were incubated for an additional 15 h under aerobic conditions. To initiate anaerobiosis, the cultures were transferred to hermetically sealed bottles. The control culture of the PA4352 mutant grown in LB with 50 mM KNO3 was supplemented with additional KNO3 (30 mM) immediately after the shift to anaerobiosis to prevent nitrate limitation (striped bars). The survival (%) of wild-type cells containing the empty mini-CTX2 vector (NB058) (gray bars), the PA4352 mutant containing the empty mini-CTX2 vector (NB059) (black bars), and the complemented PA4352 mutant (NB060) (white bars) was determined by viable-cell counts during the stationary phase. (C) CCCP sensitivity was examined in the anaerobic stationary phase. After 7 h of stationary phase, cultures of P. aeruginosa wild-type cells containing the empty mini-CTX2 vector (NB058) (gray bars), the PA4352 mutant containing the empty mini-CTX2 vector (NB059) (black bars), and the complemented PA4352 mutant (NB060) (white bars) were supplemented with an additional 30 mM KNO3 and challenged with CCCP (0.2 mM). One culture of the PA4352 mutant was supplemented with KNO3 without CCCP (striped bars). All experiments were repeated three times, and standard deviations are indicated.

Nitrate limitation causes premature death of the PA4352 mutant.

Restriction of oxygen initiates premature death of the PA4352 mutant. P. aeruginosa also faces energy stress when aerobically grown cells enter an anaerobic environment. To analyze the effect of oxygen limitation, we performed a shift experiment. Wild-type cells (NB058), the PA4352 mutant (NB059) containing the empty mini-CTX2 vector, and the complemented PA4352 mutant (NB060) harboring the PA4352 gene cloned into mini-CTX2 (pNB011) were grown aerobically in LB to stationary phase. After 15 h of incubation in the aerobic stationary phase, the cultures were shifted to anaerobic conditions by transfer into hermetically sealed bottles. The viability of the PA4352 mutant declined 220-fold within 33 h of anaerobiosis, while the wild type and complemented mutant showed only a 4- and a 3.5-fold loss of viability, respectively (Fig. 3B). This experiment confirmed the role of PA4352 in surviving energy stress even after a shift from aerobic to anaerobic conditions.

Sensitivity of the PA4352 mutant to CCCP in the anaerobic stationary phase. To initiate energy starvation by depolarization of the membrane, we added CCCP to different strains in the anaerobic stationary phase. Wild-type cells (NB058), the PA4352 mutant (NB059) containing the empty mini-CTX2 vector, and the complemented PA4352 mutant (NB060) harboring the PA4352 gene cloned into mini-CTX2 (pNB011) were incubated anaerobically in LB supplemented with 50 mM KNO₃. After 7 h of incubation in the anaerobic stationary phase, the cultures were supplemented with additional KNO₃ (30 mM) to prevent premature death caused by nitrate limitation. At the same time, we initiated depolarization of the membrane by adding CCCP (0.2 mM). The numbers of CFU were determined at different time points during the incubation with CCCP, and survival was calculated as a percentage (Fig. 3C). After 9 h of incubation with CCCP, we observed a dramatic 1,110-fold decrease in viability for the PA4352 mutant, whereas only an 8-fold loss of viability was observed for the wild type. Complementation with pNB011 harboring PA4352 did not fully restore the phenotype but still reduced the 1,110-fold decline to a 32-fold decrease in viability.

Two promoters control expression of the PA4352 gene. The phenotypic characterization indicated induction of the PA4352 gene in response to oxygen limitation and in the stationary phase. To identify the transcriptional start point of P_PA4352, we performed primer extension analysis. Total cellular RNA was extracted from anaerobically grown P. aeruginosa wild-type cells in the exponential and early stationary phases. Additionally, we extracted the RNAs of wild-type cells and the anr mutant grown aerobically to early stationary phase (Fig. 4). The Anr protein is the global oxygen-sensing regulator of anaerobic metabolism in P. aeruginosa (35, 48) and was selected because of the presence of a putative Anr binding site in the upstream region of PA4352 (see below). We identified two transcriptional start sites in front of the PA4352 coding region. The first transcriptional start site was localized 33 bp upstream of the predicted start codon and was designated P1_PA4352. The second transcriptional start site was designated P2_PA4352 and was located 64 bp upstream of P1_PA4352.

View larger version (42K): [in this window] [in a new window]   FIG. 4. Primer extension analysis of PA4352 transcription, which identified the positions of P1PA4352 (A) and P2PA4352 (B). Total cellular RNA was extracted from aerobically grown cultures of the P. aeruginosa anr mutant (lanes 1) and wild-type cells (lanes 2) harvested in the early stationary phase and also wild-type cells cultivated under anaerobic conditions in the early stationary phase (lanes 3) and during exponential growth (OD578, 0.7) (lanes 4) in LB supplemented with 50 mM KNO3. Thirty micrograms of each prepared RNA was applied to primer extension analysis, using the primer oNB021, shown in panel C. The primer extension products were separated on a 6% urea-acrylamide gel, together with a sequencing ladder generated with oNB021. The complementary sequence of the transcription initiation start site is represented, and the 5' ends of the PA4352 transcripts are indicated by arrows. (C) Nucleotide sequence of the upstream and downstream regions flanking the transcriptional start sites of PA4352. The Anr binding site is boxed. The first few N-terminal amino acids of the PA4352 protein are shown in one-letter code. The position of the oligonucleotide (oNB021) used for primer extension is underlined.

View larger version (12K): [in this window] [in a new window]   FIG. 5. (A) Induction of the PPA4352-lacZ fusion during anaerobiosis in P. aeruginosa wild type (black bars), the anr mutant (white bars), and the mutated promoter PPA4352ANR-lacZ in wild-type cells (gray bars). The strains were grown at 37°C in LB to an OD578 of 0.7 (time zero) and transferred to hermetically sealed bottles for a 4-hour incubation (time 4). ß-Galactosidase activities were determined at the indicated time points. (B) Expression patterns of PPA4352-lacZ in P. aeruginosa wild-type cells (black bars) and the anr mutant (white bars) and the PPA4352ANR-lacZ fusion containing a mutated Anr recognition site in wild-type cells (gray bars). The cells were grown aerobically in LB at 37°C. ß-Galactosidase activities were determined in exponential and late stationary phases (see Materials and Methods). All experiments were repeated three times, and standard deviations are indicated.

The P2_PA4352 promoter is active in the stationary phase. Primer extension experiments clearly showed that P2_PA4352 is active in wild-type cells in the stationary phase under aerobic and anaerobic conditions but not during anaerobic exponential growth (Fig. 4B). The P2_PA4352 transcript was also found in the anr mutant in the aerobic stationary phase (Fig. 4B). However, since only a faint P2_PA4352 transcript was detected, we used 2D gel electrophoresis to investigate if P2_PA4352 contributes to protein biosynthesis in the stationary phase. Wild-type cells, the anr mutant, and the PA4352 knockout mutant were grown aerobically in LB. Cells were harvested in the late stationary phase, and proteins were extracted for 2D gel electrophoresis. A protein spot corresponding to the PA4352 protein was identified by matrix-assisted laser desorption ionization-time of flight mass spectrometry in wild-type cells and the anr mutant strain (Fig. 6A to C). Since no Anr-dependent P1_PA4352 transcript was detected by primer extension experiments in the anr mutant strain, this protein is translated from the P2_PA4352 promoter alone. As expected, no PA4352 protein could be detected in the PA4352 mutant (Fig. 6D). Therefore, P2_PA4352 enables synthesis of the PA4352 protein in the stationary phase, independently of Anr.

View larger version (76K): [in this window] [in a new window]   FIG. 6. (A) Image of a 2D polyacrylamide gel showing the protein pattern of the P. aeruginosa wild type. Cells were grown to the stationary phase aerobically in LB and harvested for protein extraction after 15 h in the stationary phase. 2D gel electrophoresis was performed by using IPG strips covering a pH range from 5 to 8 (IPG Ready Strips; Bio-Rad, Munich, Germany). The ellipse marks the position of the PA4352 protein spot, and the boxed area indicates the enlarged zone shown in Fig. 6B to D. (B to D) Enlarged areas of 2D gel images indicating the positions of PA4352 in the P. aeruginosa wild type (B), the anr mutant (C), and the PA4352 mutant (D). The positions of the PA4352 protein spots are marked by ellipses.

View this table: [in this window] [in a new window]   TABLE 2. Induction of PPA4352ANR-lacZ in wild-type P. aeruginosa and various mutant strainsa

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

 
During our investigation of Pseudomonas aeruginosa anaerobic long-term survival, we identified increased production of two proteins containing Usp domains: PA3309 and PA4352 (36). Recently, we reported the regulation of the PA3309 gene and its gene product during long-term survival via pyruvate fermentation (36). While PA3309 is essential for survival during pyruvate fermentation, PA4352 is not. In order to elucidate the biological function of PA4352, we screened for mutant phenotypes of a PA4352 mutant strain and studied the regulation of the PA4352 promoter.

Primer extension analysis revealed two transcriptional start sites of PA4352, P1_PA4352 and P2_PA4352. We showed that P1_PA4352 is a typical Anr-dependent promoter. Anaerobic induction was shown to be independent of Dnr. Anr of P. aeruginosa is a homolog of the E. coli redox regulator Fnr and detects oxygen (35, 48). In the absence of oxygen, the Anr regulator activates transcription from Anr-dependent promoters by binding to a specific binding site termed the Anr box. The center of an Anr binding site of P1_PA4352 was located at position –41.5 bp with respect to the transcriptional start point, which is the reported optimal distance (17). Moreover, the Anr box is highly conserved and displays a perfect palindrome, TTGAT-XXXX-ATCAA. Mutation of this Anr box abolished promoter activity under anaerobic conditions, as shown by the promoter-lacZ fusions (Fig. 5A). Primer extension experiments confirmed that P1_PA4352 was active under anaerobic conditions but also showed promoter activity in the aerobic stationary phase. Stationary-phase induction of P1_PA4352 depends on Anr, since it is abolished in an anr mutant strain. Oxygen limitation in the stationary phase of aerobically shaken cultures was already shown by Cooper et al. (10), using an O₂ microelectrode, and could be explained by the high respiration level of high cell densities (10¹⁰ CFU/ml) in the stationary phase. The second promoter of PA4352, P2_PA4352, was induced only in the stationary phase under anaerobic and aerobic conditions and was also active in the anr mutant, showing an Anr-independent induction. Primer extension did not detect a transcript of P2_PA4352 in the exponential growth phase. Genes encoding Usp-type stress proteins in E. coli are induced in the stationary phase by guanosine 3'-diphosphate 5'-diphosphate, and this induction is abolished in a relA/spoT double mutant (26). In P. aeruginosa, stringent response was shown to depend strictly on the RelA protein (14, 38). Our lacZ reporter gene experiments showed that stationary-phase induction of P2_PA4352 does not depend on stringent response (RelA), the stationary-phase sigma factor RpoS, or quorum sensing (LasR and RhlR). Therefore, the regulatory system inducing P2_PA4352 in the stationary phase remains unknown. Stationary-phase induction was also observed for PA3309, the first Usp-type stress protein we identified in P. aeruginosa, but the regulation has not been elucidated (36). The identification of the regulator activating transcription in the stationary phase is currently our research focus.

A systematic screening for the phenotype of the PA4352 mutant revealed reduced survival in the anaerobic stationary phase, which was triggered by nitrate limitation. Addition of extra KNO₃ to PA4352 mutant cells in the stationary phase rescued the observed phenotype. After 9 h of anaerobic incubation, the restriction of nitrate as a terminal electron acceptor resulted first in delayed growth of the mutant after transfer to upshift conditions and, second, in premature death of the PA4352 mutant during extended (15-h) anaerobic incubation. We observed a 77-fold decrease in viability of the PA4352 mutant, whereas wild-type cells and the complemented mutant showed only a 1.5- and 2.0-fold decline, respectively. A similar phenotype was observed when cells were shifted from the aerobic stationary phase to anaerobic conditions. We observed a 220-fold loss in viability of the PA4352 mutant, while wild-type cells and the complemented mutant showed only a slight 4-fold decrease of viability after 33 h of anaerobiosis. Since we complemented the mutant with the PA4352 gene, we showed that the observed phenotype is restricted to the absence of the PA4352 gene. We confirmed the observation that PA4352 is involved in surviving energy stress in an independent experiment. The uncoupler of the electron transport chain, CCCP, was used to depolarize the membrane and to induce energy starvation under anaerobic conditions. Again, we observed a significant loss of viability of the PA4352 mutant compared to the wild type. This confirms that PA4352 is important for surviving anaerobic energy stress. Therefore, PA4352 might play an important role during persistent infection of the CF lung and could contribute to survival of P. aeruginosa cells inside microcolonies in anaerobic mucus plaques.

A comparison of the properties of P. aeruginosa PA4352 to those of the E. coli Usp-type stress proteins indicates different functions. None of the typical uspA mutant phenotypes, such as UV sensitivity or reduced survival in the aerobic stationary phase, were observed for the P. aeruginosa PA4352 mutant (data not shown). CCCP sensitivity was reported for UspG (named UP12 in reference 8), however, under aerobic conditions. No anaerobic phenotype has been described for the E. coli Usp-type stress proteins. Interestingly, Usp-type stress proteins are found to be induced in response to oxygen starvation in mycobacteria (31, 32). Mycobacteria face oxygen limitation during infection when incorporated into fibrous granulomas, which leads to a nonreplicative persistent state (42, 43). It will be interesting to see if Usp-type stress proteins contribute to anaerobic survival of bacteria and if Usp-type stress proteins are important for persistent infection in P. aeruginosa and other pathogens.

. . . .

	ACKNOWLEDGMENTS

 
We thank Dieter Jahn for continuous support and for critically reading the manuscript and Beatrice Benkert from our laboratory for the construction of the unmarked dnr mutant strain. We are indebted to H. P. Schweizer (University of Colorado) for providing the pEX18Ap, mini-CTX-lacZ, pFLP2, and mini-CTX2 plasmids; Dieter Haas (Université de Lausanne, Lausanne, Switzerland) for providing the P. aeruginosa anr mutant; and E. P. Greenberg (University of Iowa) for supplying the P. aeruginosa rpoS mutant. We thank Miguel Camara (University of Nottingham, United Kingdom) for providing the plasmids pSB219.9A and pSB224.10A for construction of the lasR and rhlR knockout mutants in P. aeruginosa.

The investigation was supported by funds from the Deutsche Forschungsgemeinschaft, the German Research Centre for Biotechnology, and the Fonds der Chemischen Industrie. K.S. was supported by the DFG-European Graduate College 653.

	FOOTNOTES

 
* Corresponding author. Mailing address: Institute of Microbiology, Technical University Braunschweig, Spielmannstr. 7D-38106, Braunschweig, Germany. Phone: 49 531 3915857. Fax: 49 531 3915854. E-mail: m.schobert{at}tu-bs.de.

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