Interaction of the Antiactivator FleN with the Transcriptional Activator FleQ Regulates Flagellar Number in Pseudomonas aeruginosa

doi:10.1128/JB.183.22.6636-6644.2001

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Journal of Bacteriology, November 2001, p. 6636-6644, Vol. 183, No. 22
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.22.6636-6644.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Interaction of the Antiactivator FleN with the Transcriptional Activator FleQ Regulates Flagellar Number in Pseudomonas aeruginosa

Nandini Dasgupta and Reuben Ramphal^*

Department of Medicine/Infectious Diseases, University of Florida, Gainesville, Florida 32610

Received 30 April 2001/Accepted 30 August 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Flagellar number in Pseudomonas aeruginosa is controlled by FleN, a putative ATP/GTP binding protein. Disruption of fleN resultsin multiflagellation of the otherwise monoflagellate strains PAKand PAO1 and is associated with a chemotactic defect. We proposethat flagellar number is maintained by the antiactivator FleN,which downregulates flagellar genes by binding to their transcriptionalactivator, FleQ, an enhancer binding protein belonging to theNifA subfamily. In this report we demonstrate direct interactionof FleN and FleQ in the yeast two-hybrid system. Mutagenesis ofthe putative ATP/GTP binding motif in FleN^24KQ and truncation of FleN at either the N or C terminus abrogatesthis interaction. FleN does not inhibit the DNA binding abilityof FleQ in vitro, thus indicating that it probably utilizes anothermechanism(s) to serve as a FleQantiactivator.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Flagella play an important role in the pathogenesis of infections caused by Pseudomonas aeruginosa, Campylobacter jejuni,Helicobacter pylori, and Vibrio cholerae (16, 21). For effectivemotility, bacteria need to maintain the characteristic numberand placement of their flagella. Studies from our laboratory indicatethat in the monoflagellate P. aeruginosa, flagellar number isdetermined by FleN, a putative ATP/GTP binding protein (6).Disruption of fleN resulted in multiflagellation of P. aeruginosa,and overexpression of FleN from a strong plasmid promoter inhibitedflagellar assembly. Analysis of other bacterial genomes includingthose of Pseudomonas putida, V. cholerae, H. pylori, Bacillussubtilis, and Aquifex aeolicus revealed a fleN homolog in theirrespective fla loci (6). Quite possibly some of these FleNhomologs play a role in determining flagellar number in theirrespective species, as FleN does in P. aeruginosa. Except forthe B. subtilis homolog Orf298, none of the other homologs havebeen characterized. Disruption of orf298 did not influence motility,but the effect on flagellar number, if any, was not reported (12).

Many flagellar genes and operons of P. aeruginosa are regulated by FleQ, a multidomain $sigma$ ⁵⁴-dependent transcriptional activator that belongs to the NifA/NtrCenhancer binding protein (EBP) family (1, 2, 23). In afleN mutant, there is a positive correlation between multiflagellationand upregulation of FleQ-dependent flagellar promoters of variousstructural and regulatory genes involved in the synthesis of theflagellar motor and switch (FliM, FliN, and FliG), the basal body(FliE and FliF), the basal body rod (FlgB and FlgC), the hook(FlgD and FlgE), the cap (FliD), the filament (FliC), the regulatoryproteins (FleS and FleR) (6), and the export apparatus (FlhA)(S. K. Arora, unpublished). This led us to believe that FleN exertedan antagonistic effect on FleQ-dependent transcriptional activation.FleN does not display a predictable DNA binding subsequence, makingit unlikely that it is a DNA binding protein that could functionas a repressor of fleQ (6) or FleQ-dependent flagellar genes.Moreover, FleQ amounts in both the wild-type PAK and the fleNmutant PAK-N (N. Dasgupta, unpublished) were similar, thus indicatingthat FleN inhibited FleQ posttranslationally. Therefore, the inhibitionhad to be mediated either through direct FleN-FleQ protein-proteininteractions or indirectly through otherintermediates.

EBPs of the NifA/NtrC family consist of an amino-terminal domain, a conserved central domain that catalyzes nucleoside triphosphatehydrolysis and interacts with the $sigma$ ⁵⁴ RNA polymerase holozyme and a C-terminal domain containing ahelix-turn-helix (H-T-H) motif required for recognition of upstreamactivator sequences (UAS) (19). EBPs, such as NtrC of Escherichiacoli, that require activation by their cognate histidine kinase(NtrB) through a phosphorylation event at their N-terminal phosphoacceptordomain (DDDK) belong to two-component systems (5, 19). OtherEBPs, like NifA of Klebsiella and Azotobacter, lacking the N-terminalphosphoacceptor domain are constitutively active both in vivoand in vitro in the absence of their antiactivator (4). Underappropriate conditions, the NifA antiactivator NifL negativelymodulates NifA through direct protein-protein interactions (10,13, 14, 18, 25).

The absence of both the typical phosphoacceptor domain residues DDDK in FleQ (DDS⁵⁹M instead) and a histidine kinase gene in the same operon as fleQ(1) suggests that the activation and regulation of FleQ maynot involve the phosphorelay mechanism characteristic of two-componentsystems such as NtrB/NtrC. However, it cannot be overlooked thatSer-59 has the potential to serve as an alternative site for phosphorylationby a nonhistidine kinase (e.g., serine kinase), resulting in FleQactivation. The other alternative mechanism regulating FleQ couldinvolve an antiactivator functioning in a similar manner to thatof the NifA/NifLpair.

As disruption of fleN led to an upregulation of FleQ activity, the present study was undertaken to determine whether FleNwas the putative antiactivator of FleQ. If so, we then wishedto determine whether preventing FleQ from binding to DNA UAS wasone of the possible mechanisms FleN employed to function as anantiactivator. Our studies indicate that FleN is the FleQ antiactivator.The entire FleN molecule, including its predicted N-terminal nucleotidebinding motif, is essential for this interaction. In vitro, theinteraction of FleN with FleQ did not prevent the latter's DNAbindingability.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Strains, plasmids, and media. The bacterial strains, yeast strains, and plasmids used in this study are listed in Table 1. Bacteria were grown in Luria-Bertani(LB) broth (24) at 37°C with shaking at 250 rpm or on LB agarplates, unless stated otherwise. The appropriate antibiotics wereused to maintain the plasmids in P. aeruginosa at the followingconcentrations: 150 µg of carbenicillin/ml (300 µg/ml for plates)and 50 µg of tetracycline/ml (100 µg/ml for plates). In E. coli,the following concentrations were used: 200 µg of ampicillin/mland 25 µg of tetracycline/ml. Yeast extract-peptone-dextrose andSD media (3) were used to propagate the yeast strains at 30°C.

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TABLE 1. Strains, plasmids, and primers used in this study

PCR. PCR was performed in a DNA Thermal Cycler 480 (Perkin-Elmer Cetus, Norwalk, Conn.) using Pfu DNA polymerase (Stratagene, LaJolla, Calif.) in 100-µl reaction volumes. Briefly, the reactionconsisted of 100 ng of template DNA, 1.5 mM MgCl₂, 1× polymerasebuffer, 0.2 mM concentrations of deoxynucleoside triphosphates,0.5 µM each primer (Table 1) (custom synthesized at Gemini Biotech,Alachua, Fla.), 2% dimethyl sulfoxide, and 1 U of DNA polymerase.The PCR was subjected to a cycling profile with an initial denaturationof 10 min at 94°C followed by 35 cycles of the following: denaturationfor 1 min at 94°C, annealing for 1 min at 45°C, and extensionfor 1 min/kb at 72°C. The template DNA used for PCR was eitherpurified genomic DNA isolated using the cetyltrimethylammoniumbromide procedure or a plasmid preparation using the alkalinelysis method (6). The PCR products were electrophoresed on1% SeaPlaque GTG agarose gel (FMC Bioproducts, Rockland, Maine)and stained with ethidium bromide, and the desired bands wereelectroeluted for furtherapplications.

MATCHMAKER two-hybrid system. Sequences encoding the two functional domains of the GAL4 transcriptional activator are cloned into two different shuttleexpression vectors, pGBT9 and pGAD424, which are part of the MATCHMAKERI two-hybrid system (Clontech, Palo Alto, Calif.). fleQ was amplifiedas a 1.5-kb PCR product using primers fleQ5PRI and Q3Pbam (Table1), which contain engineered EcoRI and BamHI sites, respectively.The product was digested with EcoRI and BamHI and ligated intovectors pGBT9 and pGAD424 with similar cohesive ends, yieldingpGBTQ and pGADQ, respectively. Similarly, fleN was amplified asan 880-bp PCR product with primers fln5peco and flnbam (Table1) and cloned to yield pGBTN and pGADN,respectively.

To map the interacting domain of FleN, a series of C-terminal deletions in FleN was constructed by cloning PCR products generatedusing fln5peco as the 5' primer and a variable 3' primer containinga BamHI site. flnN1bam, flnN2bam, flnN3bam, flnN4bam, and flnN5bam(Table 1) served as the variable 3' primers in the constructionsof pGADN1, pGADN2, pGADN3, pGADN4, and pGADN5, respectively. AnN-terminal deletion construct, pGADN-C, was constructed by cloningthe PCR product of flnCeco and flnbam (Table 1). fliA and flgMwere cloned in pGBKT7, yielding pGBKT7-A and pGBKT7-M, respectively(Table 1).

An appropriate combination of these recombinant plasmids was cotransformed into the yeast strain Saccharomyces cerevisiaeY190 according to the MATCHMAKER protocol and tested for interactionbetween FleQ and FleN, FliA and FleN, or FlgM and FleN. Transformantscontaining pGBT-derived plasmids were selected on SD plates lackingtryptophan, and those containing pGAD-derived plasmids were selectedon SD plates lacking leucine. Cotransformants containing pGBT/pGBKT7-and pGAD-derived plasmids were selected on SD plates lacking tryptophanand leucine. For His⁺ selection, the cotransformants were streaked on SD plates devoidof tryptophan, leucine, and histidine and containing 50 mM 3-aminotriazole.

Site-directed mutagenesis. Primer pairs mutN1 and mutNcomp2 (Table 1) were used in the QuikChange site-directed mutagenesis kit (Stratagene) to generatepGADN^24KQ according to the protocol provided in the kit. Briefly, 20 ngof column-purified (plasmid mini kit; Qiagen, Valencia, Calif.)plasmid template (pGADN) was used in a 50-µl amplification reactionmixture containing 1 µl of deoxynucleoside triphosphates, 1 µlof Pfu polymerase, 1.25 µl of each primer, and 5 µl of reactionbuffer. It was subjected to a cycling profile of initial denaturationfor 30 s at 95°C followed by 13 cycles of denaturation (95°C for30 s), annealing (60°C for 1 min), and extension (68°C for 20min). The contents were then treated with DpnI to digest the originalplasmid template. One microliter of the postdigestion amplificationreaction was used to transform E. coli XL1 blue cells, and transformantswere selected on LB-ampicillin (100 µg/ml) plates. A clone withthe desired site-specific mutagenesis, confirmed by sequencingusing primer GADf (Table 1), was subsequently used for furthercharacterization.

Construction of other recombinant plasmids. In order to express FleQ, FleN, and FleN^24KQ in P. aeruginosa from the inducible tac promoter of the vector pMMB67EH, the fleQ-and fleN-containing inserts from pGBTQ, pGADN, and pGADN^24KQ were cloned into EcoRI-BamHI sites of the vector, yielding pMMBQ,pMMBN, and pMMBN^24KQ, respectively. Truncated versions of FleN lacking amino acids261 to 280 and 271 to 280 were similarly expressed by cloningout the inserts from pGADN4 and pGADN5 into pMMB67EH, generatingpMMBN4 and pMMBN5,respectively.

NdeI- and BamHI-digested PCR products generated by using primer pairs flnnde-flnN1bam and flnCnde-flnbam (Table 1) were clonedinto pET15bVP, yielding pET-fleN $Delta$ C and pET-fleN $Delta$ N, respectively.pET-fleN^24KQ was similarly constructed by cloning the NdeI- and BamHI-digestedPCR product obtained from using primer pair flnnde-flnbam (Table1) and pGADN^24KQ as the template. pIH-fleN was constructed by cloning the EcoRI-BamHIfleN insert in pGADN into vector pIH1119. This would allow theexpression of FleN as a fusion protein with the maltose bindingprotein (MBP) in E. coli.

Transformation of E. coli DH5 $alpha$ and electroporation of P. aeruginosa were performed using a standard protocol (6).

$beta$ -Galactosidase assay. The $beta$ -galactosidase filter assay of yeast strains was performed as described in the MATCHMAKER two-hybrid system protocol.Briefly, cotransformants grown on SD plates were transferred andsmeared on a piece of filter paper with a toothpick, immersedin liquid nitrogen for 30 s, and thawed on another piece of filterpaper prewetted with Z buffer (15) containing X-Gal (5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside).The paper was incubated at 30°C until a blue color was detected.For the liquid culture assay using o-nitrophenyl- $beta$ -D-galactopyranosideas the substrate, the protocol from the yeast protocol handbook(Clontech) was followed. Briefly, overnight liquid cultures weregrown in the appropriate SD selection medium and subcultured thefollowing day in yeast extract-peptone-dextrose medium for 3 to4 h until an optical density at 600 nm (OD₆₀₀) of 0.8 to 1.0 wasreached. One-milliliter culture aliquots were harvested, and cellswere washed with Z buffer and resuspended in 0.2 ml of Z buffer.Aliquots (0.1 ml) were transferred to separate tubes and subjectedto 4 cycles of freeze-thawing in liquid nitrogen and a 37°C waterbath. Z buffer (0.7 ml) and o-nitrophenyl- $beta$ -D-galactopyranoside(0.16 ml at a concentration of 4 mg/ml) were added to each tube,and the mixtures were vortexed and incubated at 30°C until a yellowcolor developed. Sodium carbonate (0.4 ml at a concentration of1 M) was added to the reaction, the tubes were centrifuged for10 min at 12,000 rpm in a microcentrifuge (Biofuge; Heraeus),and the OD₄₂₀ of the supernatant was noted. The $beta$ -galactosidaseunits were then calculated based on Miller's formula (15).

P. aeruginosa strains (PAK, PAK-Q, PAK-R, PAK-N) cotransformed with pMMB67EH-derived (pMMBN, pMMBN4, pMMBN5, and pMMBN^24KQ) and pDN19lac $Omega$ -derived (plac $Omega$ A and pMSZ5) plasmids were selectedon LB plates containing both tetracycline and carbenicillin. The $beta$ -galactosidase activities (15) of the respective promoterswere determined in liquid cultures grown in LB medium with theappropriate antibiotics under inducing (1 mM isopropyl- $beta$ -D-thiogalactopyranoside[IPTG]) and noninducing conditions at 37°C.

Expression and purification of MBP-FleQ and MBP. To overexpress MBP-FleQ, E. coli DH5 $alpha$ containing pIH-fleQ was grown at 37°C with IPTG induction and MBP-FleQ purified usingaffinity chromatography as described in the product manual (NewEngland BioLabs, Beverly, Mass.). The eluted protein was dialyzedat 4°C against 10 mM Tris-Cl (pH 7.9), 5% glycerol, and 1 mM dithiothreitol(DTT) prior to use. In order to purify MBP, E. coli DH5 $alpha$ transformedwith pIH1119 was cultured and processed in a manner similar tothat used for MBP-FleQpurification.

Expression and purification of MBP-FleN. Unlike the overexpression of MBP-FleQ, overexpression of MBP-FleN from pIH-fleN in E. coli DH5 $alpha$ resulted in its accumulationas inclusion bodies. To purify MBP-FleN in a soluble form fromthe inclusion bodies, a protocol using the detergent NDSB 201(nondetergent sulfobetaines) was adopted (28). Briefly, thebacterial pellet from a 100-ml IPTG-induced culture expressingMBP-FleN was resuspended in 2 ml of 50 mM HEPES (pH 7.5), 0.5M NaCl, 1 mM phenylmethylsulfonyl fluoride, and 5 mM DTT containing0.35 mg of lysozyme/ml and incubated at 20°C for 30 min. TritonX-100 was then added to a 1% concentration, and the suspensionwas passed through a French pressure cell at 20,000 lb/in² to lyse the cells. The inclusion bodies were pelleted by centrifugingthe lysate at 30,000 × g for 30 min at 4°C. The pellet was washedtwice with phosphate-buffered saline containing 1% Triton X-100.The inclusion bodies were solubilized in 50 mM HEPES (pH 7.5),6 M guanidine hydrochloride, and 25 mM DTT to a protein concentrationof 1 mg/ml. In order to facilitate the correct folding of MBP-FleN,which would minimize precipitation, 1 ml of the protein solutionwas diluted quickly in 9 ml of cold folding buffer (50 mM HEPES[pH 7.5], 0.2 M NaCl, 1 mM DTT, 1 M NDSB 201) by vortexing. Someof the protein precipitated as the solution appeared turbid. After1 h of incubation on ice, the solution was centrifuged to removethe aggregated protein fraction from the soluble protein. Thesupernatant was dialyzed against 10 mM Tris-Cl (pH 7.9), 5% glycerol,and 1 mM DTT and concentrated by sprinkling Sephadex G-50 on thedialysis tubing. The insoluble nature of MBP-FleN when expressedin E. coli posed a major hurdle in obtaining soluble MBP-FleNat concentrations higher than 400 to 500 ng/µl. Our attempts topurify FleN as a His-tagged fusion protein culminated in unavoidableaggregation of the protein when eluted from the Ni²⁺ Sepharose column. Under denaturing conditions, the protein elutedfrom the column efficiently, but subsequent aggregation couldnot be prevented in step dialysis. His-FleN purified under denaturingconditions was used as an antigen to generate polyclonal antibodiesin a rabbit (Cocalico Biologicals, Reamstown, Pa.).

SDS-polyacrylamide gel electrophoresis and Western analysis. Purified proteins were denatured by boiling in 2% sodium dodecyl sulfate (SDS)-1% $beta$ -mercaptoethanol-50 mM Tris-Cl (pH 7.5)(SSB). The samples were resolved on a 12.5% polyacrylamide gel,and the proteins were stained with Coomassie brilliant blue (24).For Western analysis (1), 3 µl of the bacterial lysate (cellpellet from 1.0 ml of bacterial culture resuspended and boiledin 100 µl of SSB) was electrophoresed on a 15% polyacrylamidegel and proteins were transferred to a polyvinylidene difluoridemembrane. The blot was developed using rabbit anti-FleN antibodyas the primary antibody and alkaline phosphatase-conjugated anti-rabbitimmunoglobulin G as the secondary antibody. Nitroblue tetrazoliumand BCIP (5-bromo-4-chloro-3-indolylphosphate) served as the substratesfor the colorreaction.

Gel retardation assay (GRA). The EcoRI-BamHI insert of plac $Omega$ A containing the FleQ-regulated flhA promoter was gel purified and end labeled with [ $alpha$ -³²P] dATP and the Klenow DNA polymerase (23). PAK-Q containingeither pMMB67EH or pMMBQ was grown in 10 ml of LB containing carbenicillinto an OD₆₀₀ of ~0.2, induced with 1 mM IPTG, and grown for another2 h. The culture was harvested, and the bacterial pellet was resuspendedin 1 ml of lysis buffer (50 mM Tris-Cl [pH 7.9], 1 mM EDTA, 1mM DTT, 1 mM phenylmethylsulfonyl fluoride) and passed througha French press at 20,000 lb/in². The lysate was cleared by centrifugation (12,000 rpm, BeckmanJA-20, 4°C, 30 min) and used in the binding reaction. The reactionmixture, consisting of 1 µl of deoxyinosine-deoxyctosine (2 µg/ul),0.5 µl of bovine serum albumin (10 mg/ml), 0.8 µl of magnesiumacetate (0.1 M), 1 µl of probe (500 to 700 cpm), and 1 µl of 1:5diluted PAK-Q lysate (vector control pMMB67EH or pMMBQ expressingFleQ), was incubated on ice for 30 min in a total volume of 10µl unless specifiedotherwise.

To determine the specificity of the binding of MBP-FleQ to the flhA probe, a cold flhA promoter fragment and herring spermDNA were included in the competition assay. Variable amounts ofthe purified proteins MBP, MBP-FleQ, and MBP-FleN or a combinationwere included in lieu of the lysate to study their respectiveeffect(s) on the mobility of the flhAprobe.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

FleN specifically inhibits FleQ-dependent transcriptional activation. It has been reported earlier (6) that the disruption of fleN leads to an upregulation of FleQ-dependent promoters. To ascertainwhether restoring and overexpressing FleN in the fleN mutant PAK-Nwould specifically downregulate the activity of FleQ-dependentpromoters, the flhA promoter (plac $Omega$ A) was chosen to representFleQ-dependent promoters and the PilR-dependent promoter of pilA(pMSZ5 [11]) was chosen to serve as a negative control in a $beta$ -galactosidase assay. plac $Omega$ A or pMSZ5 was cotransformed witheither pMMBN or pMMB67EH in PAK-N. The activities of the flhAand pilA promoters were measured in a $beta$ -galactosidase assay undernoninduced and induced (1 mM IPTG) expression of FleN from pMMBN.When compared to the activities of the vector control (pMMB67EH)under the same growth conditions, the uninduced leaky expressionof FleN from pMMBN downregulated the flhA promoter about 24-foldand induction (with 1 mM IPTG) of FleN from the tac promoter ofthe vector caused a further 4-fold reduction in the promoter activity.The pilA promoter and vector control (pDN19lac $Omega$ ) activities remainedessentially unaffected by FleN (Table 2). This suggested thatFleN specifically inhibited transcription of the FleQ-dependentflhA promoter in a dose-responsive manner. The same promoter exhibiteddownregulation in a FleR mutant background (PAK-R) when FleN expressionwas induced from pMMBN, whereas in a FleQ mutant background (PAK-Q),the flhA promoter showed poor baseline activity which remainedunaffected when FleN was induced from pMMBN. This is consistentwith the earlier observation that FleQ regulation of the flhApromoter is direct and not mediated in a cascade manner throughFleR (Arora, unpublished), the other response regulator in theP. aeruginosa fla locus. The observed upregulation of the flhApromoter in PAK-N when compared to PAK-R is in accordance withthe observed upregulation of FleQ dependent promoters in the fleNmutant.

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TABLE 2. Assessment of the flhA promoter activity in the fleN, fleQ, and fleR mutant strains under induced expression of FleN from pMMBN

FleN and FleQ interact with one another in the yeast two-hybrid MATCHMAKER system. FleN does not downregulate transcription of fleQ (6), and the amount of FleQ in PAK, PAK-N, and PAK-N overexpressing FleNfrom pMMBN as detected by anti-FleQ antibody in Western analysisremained essentially comparable (Dasgupta, unpublished). Therefore,FleN-dependent inhibition of FleQ activity is possible eitherthrough the direct interactions of FleN with FleQ or through otherFleQ-dependent intermediates. To address the former possibility,we took advantage of the MATCHMAKER I two-hybrid system, whichutilizes two shuttle plasmids, pGBT9 and pGAD424 (see Materialsand Methods). pGBT9 was used for constructing a translationalfusion with either FleQ or FleN, yielding pGBTQ and pGBTN, respectively.Similarly, pGAD424 was used for constructing a translational fusionwith either FleQ or FleN, yielding pGADQ and pGADN, respectively.In the appropriate cotransformants, the direct interaction ofFleN and FleQ, if any, was phenotypically tested in a $beta$ -galactosidasefilter assay for LacZ activity and by growing the yeast on histidine-deficientmedia to examine the His⁺ phenotype. A positive $beta$ -galactosidase filter assay (blue colordevelopment) and a His⁺ phenotype were obtained with cotransformants of only pGBTN pluspGADQ and pGADN plus pGBTQ (Table 3). The combinations of pGBTNplus pGAD424, pGADN plus pGBT9, pGBTQ plus pGAD424, and pGADQplus pGBT9 were negative for both the assays. This indicated thatFleN and FleQ directly interacted with one another in the yeaststrain.

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TABLE 3. Assessment of yeast cotransformants with different combinations of plasmids for a positive $beta$ -galactosidase filter assay and His⁺ phenotype

To determine the specificity of the FleN-FleQ interaction, FliA, a sigma factor required for flagellin synthesis in P. aeruginosa(26), and FlgM, its antisigma factor (A. Frisk, J. Jyot, S.K. Arora, and R. Ramphal, submitted for publication), were substitutedfor FleQ. pGBKT7-A and pGBKT7-M carrying fliA and flgM (Frisket al., submitted), respectively, were introduced into Y190 harboringpGADN. The pGBKT7-M plus pGAD-A cotransformant served as a positivecontrol for the interaction between FlgM and FliA. The pGADN pluspGBKT7-A and pGADN plus pGBKT7-M cotransformants did not displaypositive $beta$ -galactosidase filter assays or the His⁺ phenotype (Table 3), indicating that FleN did not interact witheither FliA or FlgM. Thus, the FleN-FleQ interaction appears tobe specific. The $beta$ -galactosidase activities of the relevant cotransformants,quantitated using a liquid culture assay, are presented in Table3.

MBP-FleQ has the ability to bind to DNA enhancer elements in vitro. FleQ has a predicted H-T-H DNA binding motif at its C terminus. To activate transcription, an EBP like FleQ has to bind toDNA at the UAS. The antiactivator FleN could either be interferingwith this process or preventing FleQ from initiating open complexformation at the $sigma$ ⁵⁴ holoenzyme-occupiedpromoters.

To test the former, we first established the conditions for binding FleQ to flhA UAS in vitro and then assessed the effectsof FleN (if any) on it. We preferred using FleQ overexpressedfrom pMMBQ in the P. aeruginosa fleQ mutant PAK-Q, to ensure anyposttranslational modification(s) of FleQ that might enable DNAbinding. The promoter region of flhA (insert from plac $Omega$ A) wasend labeled (flhA probe) and examined in a GRA, using inducedculture lysates of PAK-Q harboring either pMMBQ or pMMB67EH. TheflhA probe exhibited a mobility shift with the FleQ-containinglysate of PAK-Q/pMMBQ but not with the vector control lysate ofPAK-Q/pMMB67EH (Fig. 1A). The protein binding to the flhA probeand generating the observed mobility shift was either FleQ orsome other protein that needed the FleQ activator for its synthesis.To address this, the GRA was repeated using affinity-purifiedMBP-FleQ and MBP proteins (Fig. 1B and 2), where FleQ was expressedas a fusion protein with MBP in E. coli. MBP-FleQ retarded theflhA promoter-containing fragment, whereas MBP alone did not generatea shift, confirming direct binding of MBP-FleQ to the flhA probe(Fig. 1B). The extent of retardation was directly proportionalto the amount of MBP-FleQ included in the assay. The ability ofthe cold flhA fragment to compete with the probe-FleQ complexand the inability of nonspecific DNA (herring sperm DNA) to competewith the same confirmed that the binding of MBP-FleQ to the flhAprobe was specific (Fig. 1C).

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FIG. 1. GRA with the flhA promoter probe. (A) Lysate from PAK-Q harboring either pMMB67EH (vector control, lane 2) or pMMBQ (expressing FleQ, lane 3). The free probe was electrophoresed in lane 1. (B) Purified MBP-FleQ and MBP proteins. Lane 1 depicts the free probe, and lanes 2 to 4 and lanes 5 to 7 contain 1.1, 2.2, and 4.4 µg of MBP-FleQ and MBP, respectively. +, present; $-$ , absent. (C) MBP-FleQ and cold flhA promoter or herring sperm DNA. Lanes 1 to 4 contain 5.6 µg of MBP-FleQ and cold flhA promoter fragment (lanes 2 and 3, 50 and 200 ng, respectively) or herring sperm DNA (lane 4, 1 µg). The arrow and arrowhead indicate the probe-FleQ complex and the free probe, respectively.

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FIG. 2. SDS-polyacrylamide gel electrophoresis profile of the purified preparations of MBP (~3 µg), MBP-FleQ (~5.6 µg), and MBP-FleN (~400 ng) following Coomassie blue staining. The molecular mass (in kDa) markers are shown.

FleN does not inhibit FleQ binding to DNA. We next examined whether purified MBP-FleN inhibited the binding of purified MBP-FleQ to the flhA promoter fragment. If MBP-FleNcompeted with DNA to bind to MBP-FleQ, with increasing amountsof MBP-FleN there would be an accompanying increase in the availabilityof unbound probe. Alternatively, when interacting with MBP-FleQ,if MBP-FleN still allowed MBP-FleQ to bind to the probe, the probe-MBP-FleQ-MBP-FleNcomplex would be expected to be retarded in its mobility comparedto the probe-MBP-FleQ complex. MBP-FleN was incubated at roomtemperature either with or without MBP-FleQ in the binding reactionfor 30 min in a total volume of 25 µl (Fig. 3). MBP-FleN alonedid not bind to the flhA probe, ruling out the possibility ofFleN binding to DNA directly. The probe-protein complex in thereaction containing both MBP-FleQ and 4.2 µg of MBP-FleN (Fig.3, lane 5) displayed a slower mobility compared to the probe-MBP-FleQcomplex (Fig. 3, lane 2). One possible explanation for the observeddifference in mobility is the formation of a probe-MBP-FleQ-MBP-FleNtripartite complex which is larger than the probe-MBP-FleQ bipartitecomplex. The mobility of the probe-protein complex in the reactioncontaining both MBP-FleQ and MBP (Fig. 3, lane 6) was comparableto the probe-MBP-FleQ complex, indicating that FleN, not MBP,in MBP-FleN caused the difference in the mobility (Fig. 3, lane5). Inclusion of smaller amounts of MBP-FleN (800 ng) (Fig. 3,lane 4) did not exhibit a similar retardation, which was probablydue to the insufficient amount of FleN available to complex withFleQ. Based on the in vitro results presented here, it is apparentthat FleN does not inhibit FleQ from binding to DNA, thereby allowingthe FleN-FleQ interacting complex to bind to DNA. The possibilityof FleN modifying FleQ, and thereby influencing its transcriptionalactivator functions, cannot be ruled out at this stage.

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FIG. 3. Assessment of the influence of FleN on the FleQ-flhA promoter complex by GRA. The mobility profiles of the flhA probe alone (lane 1) and when incubated with either MBP-FleQ (5.1 µg, lane 2), MBP-FleN (4.2 µg, lane 3), MBP-FleQ (5.1 µg) plus MBP-FleN (800 ng) (lane 4), MBP-FleQ (5.1 µg) plus MBP-FleN (4.2 µg) (lane 5), or MBP-FleQ (5.1 µg) plus MBP (4.2 µg) (lane 6) are shown. C1 and C2 indicate the probe-MBP-FleQ and probe-MBP-FleQ-MBP-FleN complexes, respectively. The arrowhead indicates the mobility of the free probe in all of the lanes.

Conformation of FleN is central to its interaction with FleQ. The deduced amino acid sequence of FleN has 280 residues. In order to map the interacting domain of FleN, a series of FleNC-terminal deletion constructs, namely, pGADN1, pGADN2, pGADN3,pGADN4, and pGADN5, were tested in interaction studies with pGBTQ(GAL4BD-FleQ) (Fig. 4). As none of them exhibited a positive $beta$ -galactosidasefilter assay or His⁺ phenotype, we deduced that none of them interacted with FleQ.As pGADN5 (FleN containing amino acids 1 to 270), which containedthe smallest deletion (the last 10 amino acids), did not interact,it indicated that the interacting domain probably mapped in thatregion. To test this hypothesis, an N-terminally truncated construct(pGADN-C) with an intact C terminus (FleN containing amino acids107 to 280) was tested. The absence of an interaction (Fig. 4)disproved the hypothesis, suggesting that in the yeast two-hybridsystem, the overall conformation of FleN, rather than a domainstructure that could function in isolation, probably determinedits interaction with FleQ.

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FIG. 4. Two-hybrid assay to determine the interaction between mutated FleN constructs and FleQ. Symbols: +, positive $beta$ -galactosidase filter assay and His⁺ phenotype; $-$ , negative $beta$ -galactosidase filter assay and His phenotype.

FleN has a putative ATP/GTP binding motif at its N terminus (Fig. 4), referred to as the A consensus sequence or the P loop(17, 29). An appreciable proportion of proteins that bindto ATP or GTP share this glycine-rich conserved-sequence motif.It typically forms a flexible loop between a beta strand and analpha helix, which interacts with one of the phosphate groupsof the nucleotide. In FleN, this motif maps between a predictedbeta strand and alpha helix, indicating possible ATP/GTP binding.Mutagenesis of this motif in MinD (K $right-arrow$ Q), an ATPase involved inthe inhibition of cell division in E. coli, abrogated MinD activity(7). To examine the effects of a similar mutagenesis in FleNon its interaction with FleQ, pGADN^24KQ (AAG $right-arrow$ CAG) was generated and cotransformed with pGBTQ into theyeast strain Y190. Absence of a positive $beta$ -galactosidase filterassay and His⁺ phenotype indicated that the FleN^24KG fusion did not interact with the FleQ fusion (Fig. 4), thus indicatingthat the ATP/GTP binding motif of FleN was essential for interactingwith FleQ in vivo in yeast. We speculate that binding of ATP/GTPprobably facilitates the correct folding of FleN into a conformationthat promotes interaction withFleQ.

To assess whether the overall conformation of FleN and its nucleotide binding motif were essential for the functioning ofFleN in the P. aeruginosa milieu, three FleN mutants with eitheran N-terminal truncation, a C-terminal truncation, or a mutatedATP binding motif were studied in PAK-N. From earlier studies(6), we were aware that the restoration of motility was sensitiveto the amounts of FleN. Excessive FleN was detrimental to flagellarbiogenesis. The expression of FleN (His-FleN) from the T7 promoterof pET-fleN without the T7 RNA polymerase in PAK-N restores motilityand restricts the number of flagella to a single polar flagellum.Therefore, the same vector background (pET15BVP) was chosen toinsert fleN regions present in pGADN1 (amino acids 1 to 106),pGADN-C (amino acids 107 to 280), and pGADN^24KQ as PCR products, yielding pET-fleN $Delta$ C (C terminus deleted), pET-fleN $Delta$ N(N terminus deleted), and pET-fleN^24KQ (nucleotide binding motif mutated), respectively. These plasmidswere electroporated into PAK-N and assessed for the ability tocomplement the fleN mutation. None of them restored motility (Fig.5A). To examine the stable expression of the FleN mutant proteinsfrom the plasmid, Western analysis using polyclonal anti-FleNantibodies was performed (Fig. 5B). The amount of expression ofFleN^24KQ from pET-fleN^24KQ was comparable to that of FleN from pET-fleN, denoting that FleN^24KQ was unable to complement the motility defect in the FleN mutantprobably due to its inability to functionally interact with FleQ.The expression of truncated FleN from pET-fleN $Delta$ C and pET-fleN $Delta$ Nwas not detectable under the same conditions. The same plasmidsdirected the detectable expression of the truncated FleN proteinswhen introduced into P. aeruginosa (PAO1/T7) and E. coli (BL21pLysS) strains carrying the T7 RNA polymerase gene (data not shown),indicating that the plasmid constructs used were correct. Thesedata suggest that the truncated FleN proteins FleN $Delta$ 107-280 andFleN $Delta$ 1-106 either are too poorly expressed in the absence of T7RNA polymerase in PAK-N to allow immunodetection or are unstable.

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FIG. 5. (A) Comparison of the motility phenotypes of PAK-N containing pET15bVP (a, vector control), pET-fleN (b, wild-type FleN), pET-fleN $Delta$ C (c, FleN containing amino acids 1 to 106), pET-fleN $Delta$ N (d, FleN containing amino acids 107 to 280), and pET-fleN^24KQ (e, FleN^24KQ). (B) Western analysis of wild-type PAK and PAK-N strains with anti-FleN polyclonal antibody (1:2,000). Lane 1, wild-type PAK; lane 2, PAK-N (pET15bVP); lane3, PAK-N (pET-fleN) and lane 4, PAK-N (pET-fleN^24KQ). The arrow indicates FleN in wild-type PAK (lane 1), and the arrowheads indicate His-FleN (lane 3) and His-FleN^24KQ (lane 4) expressed from the respective plasmids in PAK-N. The molecular mass (in kDa) markers are indicated.

Since the expression of the truncated FleN proteins from the pET constructs in PAK-N was not optimal for detection, in orderto allow assessment of the respective truncations in complementingthe fleN mutant based on the motility assay, we resorted to measuringthe activity of the FleQ-dependent flhA promoter, which is sensitiveto the levels of functional FleN. We tested the ability of thesmallest truncations in FleN (FleN $Delta$ 261-280 and FleN $Delta$ 271-280) andFleN^24KQ to inhibit FleQ-dependent transcriptional activation of the flhApromoter. pMMBN4, pMMBN5, and pMMBN^24KQ, expressing FleN $Delta$ 261-280, FleN $Delta$ 271-280, and FleN^24KQ, respectively, were introduced into PAK-N/plac $Omega$ A. The flhA promoteractivities of these strains were examined in a $beta$ -galactosidaseassay (Table 4). PAK-N cotransformed with plac $Omega$ A and pMMBN servedas the positive control for downregulation of the flhA promoterby FleN. There was no appreciable downregulation of the promoteractivity by either of the truncated FleN constructs (pMMBN4 andpMMBN5) or FleN^24KQ (pMMBN^24KQ), whereas the wild-type FleN-expressing construct of pMMBN downregulatedthe activity of the same promoter. The level of expression ofeach of the truncated FleN proteins (FleN $Delta$ 261-280 and FleN $Delta$ 271-280)and FleN^24KQ from the respective plasmids was comparable to that of wild-typeFleN from pMMBN (data not shown). Thus, the truncated FleN proteinsand FleN^24KQ tested here are not competent to inhibit FleQ dependent transcriptionalactivation. This incompetence could be attributed to their inabilitiesto interact with FleQ, as observed earlier in the yeast two-hybridsystem.

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TABLE 4. Comparison of wild-type and mutated FleN proteins in their ability to downregulate the flhA promoter (plac $Omega$ A) activity in a $beta$ -galactosidase reporter assay

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The general mechanism of activation for EBPs involves a modification in their N termini through phosphorylation at their phosphoacceptordomains (17). On the other hand, certain EBPs (activator), e.g.,NifA, in the $gamma$ subdivision of the Proteobacteria, which lack theN-terminal domain for modification, remain constitutively activeand are modulated through inhibition of their activities whenbound to another protein, e.g., the antiactivator NifL (4,9, 18). The absence of both a typical phosphoacceptor domainin FleQ and an accompanying sensor kinase gene favors the modulationof FleQ activity by an antiactivator rather than by phosphorylationand dephosphorylation. FleN appeared to be the ideal candidatefor an antiactivator of FleQ because the absence of FleN resultedin the upregulation of FleQ-dependent promoters (7) includingthe flhA promoter (this study), and the overexpression of FleNdownregulated the FleQ-dependent flhA promoter as observed inthis study (Table 2).

A positive assay for interaction between FleN and FleQ in the yeast two-hybrid system suggested direct protein-protein interactionsbetween FleN and FleQ in regulating the flagellar number of P.aeruginosa. In order to map the interacting domain of FleN, interactionstudies of yeast with six truncated constructs (FleN $Delta$ 107-280,FleN $Delta$ 191-280, FleN $Delta$ 251-280, FleN $Delta$ 261-280, FleN $Delta$ 271-280, and FleN $Delta$ 1-106)and one mutated construct (ATP/GTP binding motif, FleN^24KQ) of FleN were conducted. Inability of the truncated and the mutatedconstructs to interact with FleQ in the yeast two-hybrid system(Fig. 4) suggested that the interacting domain in FleN was notrestricted to the N or Cterminus.

In P. aeruginosa, three of the above described mutated FleN proteins (FleN $Delta$ 261-280, FleN $Delta$ 271-280, and FleN^24KQ), when tested in $beta$ -galactosidase assays (Table 4), failed todownregulate FleQ-dependent transcriptional activation (flhA promoter),whereas wild-type FleN succeeded. Thus, interaction of FleN andFleQ correlates with FleN-dependent inhibition of FleQ activity.It is likely that the conformation of FleN and its ability tobind to ATP/GTP are important for interacting with FleQ in vivo.This is unlike NifL, where the C-terminal domain is sufficientto interact with NifA and inhibit its activity (20). Recently,NifL of Azotobacter vinelandii was reported to be competent ininhibiting NifA via a concerted mechanism in which DNA binding,catalytic activity, and potential interaction with the RNA polymerasewere controlled by NifL in order to prevent transcriptional activationunder detrimental environmental conditions (4).

FleQ is predicted to bind to UAS of FleQ-dependent promoters by virtue of its C-terminal H-T-H motif. Purified MBP-FleQ expressedin E. coli was competent to bind to the flhA UAS in vitro, indicatingthat a posttranslational modification (e.g., phosphorylation)restricted to a P. aeruginosa host was not essential for enablingMBP-FleQ to bind to DNA. To function as an antiactivator of FleQ,FleN could either be inhibiting open complex formation at FleQ-dependentpromoters or preventing efficient DNA binding at UAS. Alternatively,it could be a concerted inhibition of both the processes leadingto a cumulative synergistic effect as seen in the NifA/NifL pair(4). We chose to examine the effect of FleN (if any) on theability of FleQ to bind to DNA utilizing the flhA promoter probeas a representative. Inclusion of MBP-FleN in a GRA binding reactionwith MBP-FleQ indicated that the presence of MBP-FleN apparentlydid not abrogate or reduce MBP-FleQ-DNA complex formation (Fig.3). It instead resulted in the formation of a larger complex presumablyconsisting of MBP-FleQ, MBP-FleN, and the flhA promoter probeowing to the interaction of FleN with FleQ. These results suggestthat FleN does not inhibit FleQ from binding to the DNA enhancerelements in vitro. The exact mechanism of FleN-imposed downregulationof FleQ through FleN-FleQ interaction remains to beuncovered.

As FleN is an antiactivator of FleQ, one would expect its expression to be regulated, rather than constitutive, to allow balancedsynthesis of the two proteins. Unlike the coordinated synthesisof NifA and NifL from one operon in Klebsiella pneumoniae (8,9), FleQ and FleN do not belong to the same operon in P. aeruginosa(1, 6, 27). Regulation of fleN transcription could serveas an alternative mechanism for achieving a balanced level ofFleN synthesis. As analysis of the immediate upstream sequencesof fleN did not reveal a putative promoter (6), we believefleN is part of the flhF fleN operon which may be cotranscribedfrom the promoter upstream of flhF (Arora, unpublished; Dasgupta,unpublished), a gene responsible for the polar placement of flagella(22). In P. aeruginosa, the flhF fleN promoter is positivelyregulated by RpoN ( $sigma$ ⁵⁴) and FleQ (Arora, unpublished), indicating that FleQ apparentlydrives the synthesis of its own antiactivator, FleN. This suggeststhat under physiological conditions, FleN and FleQ could be envisagedto utilize a feedback mechanism to regulate the activities ofone another and thereby control (i) flagellar number and (ii)the unnecessary continuing synthesis of early flagellar componentsin P. aeruginosa. The interaction of FleN with FleQ thus servesas a major regulatory checkpoint in controlling the synthesisof the flagellarcomponents.

	ACKNOWLEDGMENTS

We thank M. S. Swanson for providing the yeast strain and plasmids used in the yeast two-hybrid system and S. K. Arora forhelpful discussion during preparation of themanuscript.

This work was supported by NIH grant AI45014 to R.R.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Medicine/Infectious Diseases, P.O. Box 100277, JHMHC, University of Florida,Gainesville, FL 32610. Phone: (352) 392-2932. Fax: (352) 392-6481.E-mail: ramphr{at}medmac.ufl.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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Appl. Environ. Microbiol.	Infect. Immun.	Eukaryot. Cell
Mol. Cell. Biol.	J. Virol.	Microbiol. Mol. Biol. Rev.

1.	Arora, S. K., B. W. Ritchings, E. C. Almira, S. Lory, and R. Ramphal. 1997. A transcriptional activator, FleQ, regulates mucin adhesion and flagellar gene expression in Pseudomonas aeruginosa in a cascade manner. J. Bacteriol. 179:5574-5581[Abstract/Free Full Text].
2.	Arora, S. K., B. W. Ritchings, E. C. Almira, S. Lory, and R. Ramphal. 1998. The Pseudomonas aeruginosa flagellar cap protein, FliD, is responsible for mucin adhesion. Infect. Immun. 66:1000-1007[Abstract/Free Full Text].
3.	Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1995. Current protocols in molecular biology. John Wiley & Sons, Inc., New York, N.Y.
4.	Barrett, J., P. Ray, A. Sobczyk, R. Little, and R. Dixon. 2001. Concerted inhibition of the transcriptional activation functions of the enhancer-binding protein NIFA by the anti-activator NIFL. Mol. Microbiol. 39:480-494[CrossRef][Medline].
5.	Bourret, R. B., K. A. Borkovich, and M. I. Simon. 1991. Signal transduction pathways involving protein phosphorylation in prokaryotes. Annu. Rev. Biochem. 60:401-411[CrossRef][Medline].
6.	Dasgupta, N., S. K. Arora, and R. Ramphal. 2000. fleN, a gene that regulates flagellar number in Pseudomonas aeruginosa. J. Bacteriol. 182:357-364[Abstract/Free Full Text].
7.	de Boer, P. A. J., R. E. Crossley, A. R. Hand, and L. I. Rothfield. 1991. The MinD protein is a membrane ATPase required for the correct placement of the Escherichia coli division site. EMBO J. 10:4371-4380[Medline].
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