Active Efflux and Diffusion Are Involved in Transport of Pseudomonas aeruginosa Cell-to-Cell Signals

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Journal of Bacteriology, February 1999, p. 1203-1210, Vol. 181, No. 4
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Active Efflux and Diffusion Are Involved in Transport of Pseudomonas aeruginosa Cell-to-Cell Signals

James P. Pearson, Christian Van Delden, and Barbara H. Iglewski^*

Department of Microbiology and Immunology, University of Rochester, Rochester, New York 14642

Received 16 October 1998/Accepted 2 December 1998

	ABSTRACT

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Many gram-negative bacteria communicate by N-acyl homoserine lactone signals called autoinducers (AIs). In Pseudomonas aeruginosa,cell-to-cell signaling controls expression of extracellular virulencefactors, the type II secretion apparatus, a stationary-phase sigmafactor ( $sigma$ ^s), and biofilm differentiation. The fact that a similar signal,N-(3-oxohexanoyl) homoserine lactone, freely diffuses throughVibrio fischeri and Escherichia coli cells has led to the assumptionthat all AIs are freely diffusible. In this work, transport ofthe two P. aeruginosa AIs, N-(3-oxododecanoyl) homoserine lactone(3OC₁₂-HSL) (formerly called PAI-1) and N-butyryl homoserine lactone(C₄-HSL) (formerly called PAI-2), was studied by using tritium-labeledsignals. When [³H]C₄-HSL was added to cell suspensions of P. aeruginosa, the cellularconcentration reached a steady state in less than 30 s and wasnearly equal to the external concentration, as expected for afreely diffusible compound. In contrast, [³H]3OC₁₂-HSL required about 5 min to reach a steady state, andthe cellular concentration was 3 times higher than the externallevel. Addition of inhibitors of the cytoplasmic membrane protongradient, such as azide, led to a strong increase in cellularaccumulation of [³H]3OC₁₂-HSL, suggesting the involvement of active efflux. A definedmutant lacking the mexA-mexB-oprM-encoded active-efflux pump accumulated[³H]3OC₁₂-HSL to levels similar to those in the azide-treated wild-typecells. Efflux experiments confirmed these observations. Our resultsshow that in contrast to the case for C₄-HSL, P. aeruginosa cellsare not freely permeable to 3OC₁₂-HSL. Instead, the mexA-mexB-oprM-encodedefflux pump is involved in active efflux of 3OC₁₂-HSL. Apparentlythe length and/or degree of substitution of the N-acyl side chaindetermines whether an AI is freely diffusible or is subject toactive efflux by P. aeruginosa.

	INTRODUCTION

Top Abstract Introduction Materials and methods Results Discussion References

Pseudomonas aeruginosa remains a leading cause of both nosocomial infections in immunocompromised patients and chronic infectionsin cystic fibrosis patients (reviewed in references 9 and 57).P. aeruginosa virulence depends on cell-associated factors, includingalginate and pili (5, 9), and secreted factors, includingtoxins, exotoxin A, and exoenzyme S (14, 28); proteases, elastase,alkaline protease, and LasA protease (13, 27, 47); and hemolysins,rhamnolipid, and phospholipase (25). Cell-to-cell signaling(quorum sensing) is required for expression of many P. aeruginosavirulence factors (see below) (6, 43).

Intrinsic resistance of P. aeruginosa to many antibiotics and disinfectants also causes clinical problems (49). The intrinsicresistance is due to low outer membrane permeability and to multidrugefflux pumps that reduce the cellular level of antibiotics (reviewedin references 11 and 30). Three known P. aeruginosa multidrugefflux pumps are encoded by the mexAB-oprM, mexCD-oprJ, and mexEF-oprNoperons, respectively (18, 45, 46). These pumps consistof a cytoplasmic membrane component of the resistance-nodulation-celldivision (RND) family (39) thought to function as a proton antiportexporter (i.e., MexB), an outer membrane component thought toform channels (i.e., OprM), and a membrane fusion protein thoughtto link MexB and OprM (reviewed in reference 29). BacterialRND pumps have also been shown to cause the efflux of many otherorganic compounds, including solvents and inhibitors (24, 29,50). However, no natural products of P. aeruginosa have yetbeen shown to be subject to efflux via RNDpumps.

Quorum sensing (or autoinduction) is the controlled expression of specific genes in response to extracellular chemical signalsproduced by the bacteria themselves (6). Typically cells emitan N-acyl homoserine lactone signal called an autoinducer (AI),which is usually synthesized by a LuxI-type AI synthase, intothe environment (6). At high cell densities, the AI reachesa threshold concentration and binds to a LuxR-type protein whichis then able to activate target genes (6). To date, luxR-luxI-typequorum-sensing systems and their N-acyl homoserine lactone AIshave been found in many different gram-negative bacteria (6).In P. aeruginosa the las (lasR-lasI) (7, 37) and rhl (rhlR-rhlI)(33, 34) quorum-sensing systems direct the synthesis of twodistinct AIs, N-(3-oxododecanoyl) homoserine lactone (3OC₁₂-HSL)(formerly called PAI-1) (40) and N-butyryl homoserine lactone(C₄-HSL) (formerly called PAI-2) (41, 59), respectively. LasRand 3OC₁₂-HSL activate expression of several genes, includinglasI itself (54), lasB (encoding elastase) (37), lasA (encodingLasA protease) (8), both xcp operons (xcpPQ and xcpR-Z, encodingthe type II secretion apparatus [3]), and rhlR (20, 44).Recently, the las quorum-sensing system was shown to be involvedin P. aeruginosa biofilm differentiation (4). C₄-HSL and RhlRalso activate expression of numerous genes, including rhlI itself(20), the rhamnolipid biosynthesis operon rhlAB (32, 42),lasB (1, 41, 42), and rpoS (encoding the stationary-phasesigma factor $sigma$ ^s) (20).

Although many different N-acyl homoserine lactone AIs have been isolated from various gram-negative bacteria, to date, alldifferences are in the N-acyl side chain length (from C₄ to C₁₄)or degree of substitution (either 3-oxo, 3-hydroxy, saturated,or unsaturated) (6, 26, 48, 55). All AIs have been assumedto be freely diffusible in bacterial cells. This assumption isbased on the fact that a radiolabeled Vibrio fischeri AI, N-3-oxo-hexanoylhomoserine lactone ([³H]3OC₆-HSL), was shown to freely diffuse into and out of V. fischeriand Escherichia coli cells (15, 42). Here, we studied theuptake and efflux of 3OC₁₂-HSL and C₄-HSL by P. aeruginosa cells.Our results indicate that [³H]C₄-HSL freely diffuses into and out of P. aeruginosa cells.In contrast, cellular concentrations of [³H]3OC₁₂-HSL are higher than external levels. Our results showthat the increased cellular level of [³H]3OC₁₂-HSL is not due to association with LasR or RhlR and suggestthat it is not due to active (inward) transport. We propose thatthe high cellular level of 3OC₁₂-HSL is probably due to partitioninginto the cell membranes. By use of P. aeruginosa $Delta$ (mexAB-oprM)mutant cells or poisoned wild-type cells, we also show that 3OC₁₂-HSLis subject to active efflux by the MexAB-OprMpump.

	MATERIALS AND METHODS

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Bacterial strains, plasmids, and culture conditions. The strains and plasmids used are shown in Table 1. Bacteria were grown at 37°C. When needed for plasmid maintenance, ampicillin(100 µg/ml) was included in cultures of E. coli and carbenicillin(200 µg/ml) was included in P. aeruginosa cultures. For $beta$ -galactosidasedeterminations, P. aeruginosa and E. coli were grown with shakingin PTSB medium (35) and supplemented A medium (40), respectively.Otherwise, P. aeruginosa cultures were grown with shaking in M9medium (52) containing 0.2% glucose and 1 mM MgSO₄. Overnightcultures were centrifuged (10,000 × g for 10 min at 20°C), andcell pellets were washed in fresh M9 medium and resuspended inM9 medium to an optical density at 660 nm of 0.075. These cultureswere then grown to mid-logarithmic growth phase (optical densityat 660 nm of 0.7). This corresponded to 1.3 × 10⁹ CFU/ml.

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TABLE 1. Bacterial strains and plasmids used

Preparation of cell suspensions. Cells were washed in KG buffer (10 mM potassium phosphate [pH 7.0], 0.03% glycerol) and resuspended in KG buffer to a celldensity of 8 × 10¹⁰ CFU/ml.

Chemicals. The syntheses of unlabeled 3OC₁₂-HSL, [³H]3OC₁₂-HSL (specific activity, 229 Ci/mmol), unlabeled C₄-HSL, and [³H]C₄-HSL (specific activity, 29.4 Ci/mmol) have been describedpreviously (38, 41, 42). [³H]3OC₁₂-HSL and [³H]C₄-HSL are labeled with tritium on the respective acyl sidechains (38, 42). Antibiotics and all other chemicals, includingthe three radioactive compounds [¹⁴C]ethylene glycol (specific activity, 1.5 mCi/mmol), [¹⁴C]dextran (specific activity, 1.25 mCi/g; average molecular weightof 70,000), and [¹⁴C]leucine (specific activity, 0.27 Ci/mmol), were purchased fromSigma Chemical Co., St. Louis,Mo.

Determination of cellular AI concentrations. The measurement of AI concentration was based on previously described techniques (15) with the following modifications.A 250-µl volume of cell suspension (2 × 10¹⁰ cells) was mixed with 50 µl of KG buffer containing the compoundof interest (unless otherwise specified, the concentrations wereas follows: [³H]3OC₁₂-HSL or [³H]C₄-HSL, 60 nM; [¹⁴C]leucine, 2.0 µM; [¹⁴C]ethylene glycol, 720 µM; or [¹⁴C]dextran, 1.7 µg/µl). Assay mixtures were incubated for 5 min(20 to 22°C) unless otherwise specified, and then duplicate 140-µlaliquots were centrifuged through 75 µl of Nyosil M25 siliconefluid (Nye Lubricants, New Bedford, Mass.) into 25 µl of aqueous2% trichloroacetic acid-10% glycerol and radioactivity was countedas described previously (15). One percent of the input [³H]3OC₁₂-HSL radioactivity entered the silicone fluid regardlessof whether cells were present, and this was corrected for in subsequentcalculations. No radioactivity was detected in the silicone fluidfor the other radioactivecompounds.

Cell volumes were calculated by a modification of a previously described method (51). We substituted P. aeruginosa PAO1and its derivatives for E. coli. We measured accumulation of thefreely permeative [¹⁴C]ethylene glycol in place of the [³H]-labeled AIs. Trapped extracellular fluid was measured by usingthe impermeative [¹⁴C]dextran.

[¹⁴C]leucine accumulation was also assayed by using the above-described technique. Prior to addition of the radiolabeled compounds,cells were pretreated for 30 min with chloramphenicol (final concentrationof 5 mM) to inhibit protein synthesis. Accumulation of both ³H-AIs was unaffected by pretreating the cells with chloramphenicol.Thus, chloramphenicol was not included in further experimentswith ³H-AIs.

Where indicated, either sodium azide (30 mM) or carbonyl cyanide m-chlorophenylhydrazone (CCCP) (250 µM) was added to de-energizecells as described previously (16, 22).

Efflux assay. Efflux of AI from cells was measured by comparing the cellular AI level with that remaining associated with the cells afterremoval of the external AI and then suspending the cells in alarge excess of AI-free buffer as described previously (15).Incubation times were 20 and 5 min for cells with [³H]3OC₁₂-HSL or [³H]C₄-HSL, respectively, to reach steady-state levels. Duplicate140-µl samples were transferred to 1.5-ml tubes and centrifugedfor 1 min at 13,000 × g (20 to 22°C). Cells from one of the sampleswere suspended in 1.4 ml of KG buffer and centrifuged for 2 minas before. AI levels remaining with the cells after washing wascompared with those remaining with cells that were not washed.Where indicated, sodium azide or CCCP was included in the washbuffer at the same concentrations as described above. Trappedextracellular fluid was corrected for by using [¹⁴C]dextran in place of the ³H-labeledAIs.

AI bioassays. E. coli MG4 $lambda$ I₁4(pPCS1) was used to measure 3OC₁₂-HSL as described previously (54). P. aeruginosa PAO-JP2(pECP61.5) was usedto measure C₄-HSL as described previously (42).

HPLC analysis of cellular AIs. Analysis of cellular AIs was based on a previously described technique (15). Briefly, cells were incubated with [³H]3OC₁₂-HSL or [³H]C₄-HSL as described above and centrifuged (13,000 × g for 1min at 20 to 22°C). Cell pellets were suspended in 20 µl of KGbuffer and extracted twice in 0.2 ml of ethyl acetate, and then20 nmol of unlabeled 3OC₁₂-HSL or 24 nmol of unlabeled C₄-HSLwas added as a carrier to 0.15 ml of the respective [³H]3OC₁₂-HSL or [³H]C₄-HSL extract. Each mixture was then evaporated under N₂ gas,and the material was dissolved in 10% (vol/vol) acetonitrile inwater and subjected to reverse-phase high-performance liquid chromatography(HPLC) (C₁₈ column, 0.46 by 25 cm). The HPLC flow rate was 1 ml/min,and elution conditions are indicated in Fig. 1.

	RESULTS

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Cellular concentrations of P. aeruginosa AIs. In order to study AI uptake in P. aeruginosa, [³H]3OC₁₂-HSL or [³H]C₄-HSL was incubated with suspensions of wild-type cells (strainPAO1). After separation of the cells from the extracellular fluidby centrifugation through a layer of silicone fluid, radiolabeledAI was found to be associated with the cells. In order to calculatethe internal concentration of each AI and compare it with externalconcentrations, cellular AI is assumed to be unmodified. A structurallysimilar AI molecule, [³H]3OC₆-HSL, was reported to be unmodified in V. fischeri cells(15). To verify this assumption, P. aeruginosa PAO1 cells thathad been loaded with either [³H]3OC₁₂-HSL or [³H]C₄-HSL were extracted with ethyl acetate as described in Materialsand Methods. For [³H]C₄-HSL-loaded cells, 100% of the radioactivity was recoveredfrom the cells that had been loaded with this AI. In the caseof [³H]3OC₁₂-HSL, 75.2 ± 2.3% (average ± standard deviation [SD]; n= 3 independent experiments) of the radioactivity was recoveredfrom cells. In both cases, when the extracted radioactivity wasanalyzed by HPLC, >90% of the radioactivity applied to the HPLCcolumn eluted at the same point as the [³H]3OC₁₂-HSL and [³H]C₄-HSL standards, respectively (Fig. 1). For C₄-HSL these resultssupport the assumption that cellular radiolabel was in the formof unmodified [³H]C₄-HSL. For [³H]3OC₁₂-HSL, nearly all of the radiolabel extracted from cellswas unmodified [³H]3OC₁₂-HSL (Fig. 1), but 25% of the [³H]3OC₁₂-HSL remained associated with the cells. It is possiblethat this fraction of the total [³H]3OC₁₂-HSL accumulated by strain PAO1 may be chemically modified(such as by lactone ring hydrolysis or deacylation of the sidechain) by the cells. Chemical modification of [³H]3OC₁₂-HSL by the cells seems unlikely, because other AIs withstructurally similar lactone rings and shorter acyl side chains,i.e., [³H]C₄-HSL and [³H]3OC₆-HSL, are not modified by P. aeruginosa (Fig. 1) or V. fischeri(15), respectively. It is, however, more likely that the 25%of [³H]3OC₁₂-HSL remaining with cells may be unmodified yet is stronglyassociated with the cells (i.e., partitioned into the membranes)and could not be liberated by our method of extraction.

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FIG. 1. HPLC analysis of tritium-labeled material extracted from P. aeruginosa PAO1 that had been loaded with [³H]3OC₁₂-HSL (A) or with [³H]C₄-HSL (B) compared with [³H]3OC₁₂-HSL and [³H]C₄-HSL, respectively. Symbols: , material extracted from cells; $triangle$ , ³H-AI;

, percent (volume/volume) acetonitrile in water.

P. aeruginosa PAO1 incubated with [³H]C₄-HSL yielded a cellular/extracellular concentration ratio of 0.92, which is close tothe ratio of 0.96 obtained with the freely permeative [¹⁴C]ethylene glycol (Table 2). In contrast, the cellular [³H]3OC₁₂-HSL concentration was 3.35-fold higher than the externalconcentration (Table 2). The fact that 3OC₁₂-HSL appeared tobe concentrated by cells opened the possibility that active (inward)transport could be involved.

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TABLE 2. P. aeruginosa PAO1 cellular and external AI concentrations

To address whether the silicone fluid centrifugation technique would be able to distinguish between the active and passivetransport, the time course of P. aeruginosa uptake of [¹⁴C]leucine, which is known to be actively transported inward byP. aeruginosa (12), was measured (Fig. 2A). After 5 min of incubationin the presence of [¹⁴C]leucine, the cellular [¹⁴C]leucine concentration was greater than 20-fold higher than theexternal concentration (Fig. 2A), as previously reported (12).To demonstrate inhibition of active (inward) transport, cellswere preincubated with sodium azide, which has been shown to blockthe active transport of leucine in P. aeruginosa (12, 16).As expected, the [¹⁴C]leucine level in cells pretreated with sodium azide reachedonly approximately twice the external level (Fig. 2A). These experimentsdemonstrated that the silicone fluid centrifugation techniquewould be able to detect active (inward) transport systems.

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FIG. 2. Accumulation of radiolabeled compounds by P. aeruginosa. (A) [¹⁴C]leucine accumulation in strain PAO1 treated with chloramphenicol (5 mM); (B) accumulation of [³H]3OC₁₂-HSL (circles) and [³H]C₄-HSL (triangles) in strain PAO1; (C) accumulation of [³H]3OC₁₂-HSL (circles) and [³H]C₄-HSL (triangles) in mexAB-orpM mutant strain PAO200. Closed symbols, non-azide-treated cells; open symbols, cells treated with sodium azide (30 mM). Accumulation of each compound was determined as described in Materials and Methods. Data are the averages (± SDs) of results from two to five independent experiments.

We then measured the time courses of [³H]3OC₁₂-HSL and [³H]C₄-HSL accumulation in strain PAO1 under the same conditions (Fig.2B). In less than 30 s, the cellular concentration of [³H]C₄-HSL reached a steady-state level that was approximately equalto the external concentration (Fig. 2B). The same results wereobtained with the freely diffusible compound [¹⁴C]ethylene glycol (data not shown). P. aeruginosa cells seem tobe freely permeable to C₄-HSL, as V. fischeri cells are to 3OC₆-HSL(15). In contrast, [³H]3OC₁₂-HSL required about 5 min to reach a steady-state level,with a cellular-to-extracellular ratio of nearly 3 (Fig. 2B),suggesting that 3OC₁₂-HSL transport was more complex than simplediffusion.

Because active (inward) transport of [¹⁴C]leucine was strongly inhibited when cells were pretreated with sodium azide, the effectof this poison on ³H-AI accumulation was also studied, and the results were surprising.Cellular [³H]3OC₁₂-HSL concentrations rose to 10 times the extracellularconcentrations (Fig. 2B), but azide treatment had no effect onaccumulation of [³H]C₄-HSL (Fig. 2B). These results suggest that 3OC₁₂-HSL is notactively transported into P. aeruginosa as isleucine.

Azide and other agents, such as potassium cyanide and CCCP, that de-energize the bacterial cytoplasmic membrane potential(i.e., proton motive force [PMF]) are known to cause increasesin cellular accumulation of various substances, including certainantibiotics (i.e., tetracyclines, fluoroquinolones, and some $beta$ -lactams)(21, 29). The increased accumulation occurs because PMF-dependentmultidrug efflux pumps become inactivated in de-energized cells(29). Thus, these amphipathic antibiotics are no longer subjectto active efflux out of the cells, resulting in the higher cellularantibiotic levels (29). In P. aeruginosa the mexAB-oprM operonconstitutively expresses a PMF-dependent multidrug efflux pump(23, 46). To address whether the increased cellular [³H]3OC₁₂-HSL concentrations observed in azide-treated cells weredue to inhibition of this efflux pump, the [³H]3OC₁₂-HSL concentration in a defined P. aeruginosa $Delta$ (mexAB-oprM)mutant, strain PAO200 (53), was measured. This strain is derivedfrom wild-type strain PAO1 and carries an unmarked deletion ofthe entire mexAB-oprM operon (53). The time course of accumulationof [³H]3OC₁₂-HSL by strain PAO200 cells (Fig. 2C) resembled that byazide-treated strain PAO1 cells (Fig. 2B). The [³H]3OC₁₂-HSL concentration observed in strain PAO200 cells wasabout eightfold higher than the external concentration, as wehad observed for azide-treated PAO1 cells (Fig. 2B and C). Azidetreatment of strain PAO200 resulted in almost no change in thecellular concentration of [³H]3OC₁₂-HSL (Fig. 2C). These results suggested that the cellularlevel of [³H]3OC₁₂-HSL is influenced by the presence of the mexAB-oprM-encodedefflux pump and further suggested that the high level of [³H]3OC₁₂-HSL accumulated in azide-treated wild-type cells is dueto inactivation of this PMF-dependent efflux pump. In contrast,when [³H]C₄-HSL was added to strain PAO200 cells, the cellular-to-externalconcentration ratios were not significantly increased comparedto those in strain PAO1 cells, and these levels were unaffectedby poison (Fig. 2C). Therefore, C₄-HSL accumulation in P. aeruginosaappears to be independent of MexAB-OprM.

Efflux of AIs. To further investigate the role of the mexAB-oprM-encoded PMF-dependent efflux pump on [³H]3OC₁₂-HSL accumulation in P. aeruginosa, and to confirm thatcells are freely permeable to [³H]C₄-HSL, AI efflux was studied (Fig. 3). In theory, a freelydiffusible compound would be expected to completely escape whencells loaded with the compound are transferred into a large volumeof medium lacking the compound. Moreover, this free diffusionprocess would occur independently of the presence or absence ofan active-efflux system. When strains PAO1 and PAO200 ( $Delta$ mexAB-oprM)were loaded with [³H]C₄-HSL and transferred to AI-free buffer, cellular levels ofthis AI decreased 100 and 95%, respectively (Fig. 3A). When CCCP-treatedcells (strains PAO1 and PAO200, respectively) were loaded with[³H]C₄-HSL and then transferred to AI-free buffer, 100% of the radiolabelescaped from the cells (Fig. 3A). These results confirmed thatP. aeruginosa cells are freely permeable to [³H]C₄-HSL and that the mexAB-oprM-encoded efflux pump has no effecton efflux of this AI.

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FIG. 3. Efflux of [³H]C₄-HSL (A) and [³H]3OC₁₂-HSL (B) from P. aeruginosa PAO1 (wild type), PAO-JP3 (lasR rhlR), or PAO200 (mexABA-oprM). Open bars, radioactivity loaded in cells; closed bars, radioactivity remaining in cells after suspension in AI-free buffer. Cells were de-energized with CCCP (250 µM) as indicated. Data are the averages (± SDs) of results from two to four independent experiments.

A compound utilizing an efflux pump would escape more readily from cells containing an active-efflux system than from mutantslacking the system. As shown above, in both azide-poisoned strainPAO1 cells and mutant cells lacking the mexAB-oprM-encoded effluxpump (strain PAO200), the cellular accumulation of [³H]3OC₁₂-HSL was higher than that in nonpoisoned strain PAO1 cells(Fig. 2B and C). In efflux experiments, the level of [³H]3OC₁₂-HSL initially loaded in strain PAO200 [ $Delta$ (mexAB-oprM)]cells and in poisoned PAO1 cells was therefore higher than thelevel of [³H]3OC₁₂-HSL initially loaded in unwashed strain PAO1 cells (Fig.3B). When the external [³H]3OC₁₂-HSL was removed and cells were suspended in AI-free buffer,60% of the cellular radioactivity escaped from the wild-type cellsand 30% escaped from mutant cells (strain PAO200) that lackedthe efflux pump (Fig. 3B). This strongly suggested that P. aeruginosacells are not freely permeable to [³H]3OC₁₂-HSL and that the mexAB-oprM-encoded efflux pump facilitatesefflux of this AI. Furthermore, when de-energized (CCCP-treated)strain PAO1 or PAO200 cells were loaded with [³H]3OC₁₂-HSL and then transferred to AI-free buffer, very little[³H]3OC₁₂-HSL escaped from either strain (Fig. 3B).

Therefore, unlike the freely permeative [³H]C₄-HSL, which completely escaped from cells, 40% of cellular [³H]3OC₁₂-HSL remained after transfer of strain PAO1 cells to AI-freebuffer. To address the possibility that the remaining [³H]3OC₁₂-HSL was bound to the AI-dependent transcriptional activatorproteins encoded by lasR and rhlR, strain PAO-JP3, a defined lasRrhlR double mutant, was tested for [³H]3OC₁₂-HSL efflux (and for [³H]C₄-HSL efflux as a control). The results were nearly identicalto those for efflux in strain PAO1 cells (Fig. 3). Therefore,the remaining cellular [³H]3OC₁₂-HSL in strain PAO1 was not irreversibly bound to the LasRor RhlR protein. In a time course efflux experiment in which bothCCCP-treated and nontreated wild-type cells that had been loadedwith [³H]3OC₁₂-HSL were suspended in AI-free buffer, 40% of the [³H]3OC₁₂-HSL remained after 1 min with the nontreated cells and80% remained with the CCCP-treated cells, as before. By 60 min(the duration of this experiment), 25% of the [³H]3OC₁₂-HSL remained with the nontreated cells whereas 50% remainedwith the CCCP-treated cells (data not shown). The fact that someof the [³H]3OC₁₂-HSL was released by CCCP-treated cells may be due to diffusionthrough the cell membranes in an efflux pump-independent fashion.This explanation would also account for the minor release of [³H]3OC₁₂-HSL by strain PAO200 shown in Fig. 3.

To confirm that the effects seen in strain PAO200 were due to the absence of mexAB-oprM, autoinducer efflux was measured inPAO200 cells containing either pUCP21T, a vector control plasmid,or pPS952, a pUCP21T derivative carrying a wild-type mexAB-oprMoperon. When strain PAO200 contained pPS952, [³H]3OC₁₂-HSL accumulated in these cells to levels similar to thoseobserved in wild-type PAO1 cells (Fig. 4B and 3B), about fourfoldless than for PAO200 containing the vector control. This indicatedthat efflux of [³H]3OC₁₂-HSL was restored when strain PAO200 contained a functionalmexAB-oprM-encoded pump. This efflux was strongly inhibited whenstrain PAO200(pPS952) cells were de-energized (Fig. 4B). As acontrol, efflux of [³H]C₄-HSL from the mexAB-oprM mutant containing the mexA⁺ mexB⁺ oprM⁺ plasmid was also assayed. As expected, 98 to 100% of the [³H]C₄-HSL was transported from the cells regardless of whethercells were de-energized or contained a functional mexAB-oprM operon(Fig. 4A).

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FIG. 4. Efflux of [³H]C₄-HSL (A) and [³H]3OC₁₂-HSL (B) from P. aeruginosa PAO200 in the presence (labeled mexAB-oprM⁺ [pPS952]) or absence (labeled vector [pUCP21T]]) of mexAB-oprM. Open bars, radioactivity loaded in cells; closed bars, radioactivity remaining in cells after suspension in AI-free buffer. Cells were de-energized with sodium azide (30 mM) as indicated. Data are the averages (± SDs) of results from two independent experiments.

	DISCUSSION

Top Abstract Introduction Materials and methods Results Discussion References

This study shows that both C₄-HSL and 3OC₁₂-HSL diffuse into and out of P. aeruginosa. We found that the cellular concentrationof [³H]C₄-HSL quickly reached a steady state in wild-type P. aeruginosacells at a level that was nearly equal to the external level,suggesting a passive diffusion process. Thus, we have shown thatP. aeruginosa is freely permeable to C₄-HSL as both V. fischeriand E. coli are freely permeable to 3OC₆-HSL (15). In contrast,[³H]3OC₁₂-HSL required about 5 min to reach a steady-state cellularconcentration of nearly threefold the external level (Fig. 2B),indicating a more complex transport process. HPLC analysis indicatedthat P. aeruginosa did not modify the cellular [³H]C₄-HSL and did not modify 75% of the [³H]3OC₁₂-HSL that was loaded into the cells. The remaining 25%of the cellular [³H]3OC₁₂-HSL could have been chemically modified; however, it ismore likely that it is unmodified and partitioned into the cellmembranes. Most importantly, this 25% does not significantly influenceour conclusions about active efflux of [³H]3OC₁₂-HSL from P. aeruginosacells.

Thus, while 3OC₁₂-HSL freely diffuses into and out of P. aeruginosa, the cells accumulate more of this compound because ofpassive partitioning into membranes. Superimposed on these processes,3OC₁₂-HSL is subject to active efflux from P. aeruginosa via theMexAB-OprMpump.

[³H]3OC₁₂-HSL does not seem to be actively transported into P. aeruginosa. Indeed, accumulation of this AI was not inhibitedin de-energized cells but actually increased (Fig. 2B). De-energizationof the cytoplasmic membrane potential (i.e., PMF) by azide andother poisons such as CCCP results in a strong increase in theaccumulation of certain antibiotics by some gram-negative bacteria(21, 29). In P. aeruginosa these effects have been associatedwith inhibition of the PMF-dependent mexAB-oprM-encoded effluxpump (23, 46).

We have observed that a P. aeruginosa $Delta$ (mexAB-oprM) mutant accumulated about threefold more [³H]3OC₁₂-HSL than untreated wild-type cells. Because de-energizationof strain PAO200 cells had essentially no effect on the time courseof accumulation of [³H]3OC₁₂-HSL (Fig. 2C), these results strongly suggest that theMexAB-OprM efflux is the only PMF-dependent efflux pump involvedin regulation of cellular levels of 3OC₁₂-HSL under these conditions.However the P. aeruginosa mexCD-oprJ- and mexEF-oprN-encoded multidrugpumps may also be involved in efflux of 3OC₁₂-HSL under otherconditions where those operons would beexpressed.

From our efflux experiments we conclude that 3OC₁₂-HSL efflux depends on the presence of an active MexAB-OprM pump. Whilethis paper was being prepared, others also suggested that 3OC₁₂-HSLmay be exported by the mexAB-oprM-encoded pump (5a). Here, wefound that the percentage of [³H]3OC₁₂-HSL retained after resuspension in AI-free buffer washigher in de-energized wild-type cells and in mexAB-oprM mutantcells than in nontreated wild-type cells (Fig. 3B). The observationthat the remaining cellular 3OC₁₂-HSL slowly escaped even whenthe cells were de-energized suggests that a gradual release ofthis AI likely occurs in addition to active efflux of the majorityof cellular 3OC₁₂-HSL via the MexAB-OprM pump. One explanationfor the slow efflux of 3OC₁₂-HSL from the cells may be that 3OC₁₂-HSLpartitions into the cell membranes. The respective lengths ofthe acyl side chains of the two AIs are probably responsible forthe differences in accumulation observed between the relativelyhydrophobic 3OC₁₂-HSL and the more hydrophilic C₄-HSL. We proposethat 3OC₁₂-HSL transport by P. aeruginosa occurs by a mechanismsimilar to that of amphipathic antibiotics such as tetracycline,fluoroquinolones, and $beta$ -lactams. Nikaido has presented a modelin which those antibiotics diffuse and partition in gram-negativebacterial cell membranes and are subject to active efflux fromthe cells by PMF-dependent RND pumps (29). Recent results withan RND pump (AcrAB) of Salmonella typhimurium have extended thismodel and suggested that penicillins and cephalosporins containingmore-lipophilic side chains are more likely to partition intothe lipid bilayer of the cytoplasmic membrane (31). The modelsuggests that once these $beta$ -lactam antibiotics are partitionedinto the cytoplasmic membrane, they can then become substratesof the RND pump (31). Future studies will be required to elucidatethe likely mechanism(s) (i.e., membrane partitioning) apparentlyinvolved in 3OC₁₂-HSL accumulation, besides the role of the MexAB-OprMpump describedhere.

A natural substrate of MexAB-OprM. PMF-dependent RND pumps in P. aeruginosa are known to cause the efflux of various toxic substances, such as antibiotics (18,23, 45), fatty acid inhibitors (53), and organic solvents(24), out of cells. 3OC₁₂-HSL is the first example of a naturalproduct of P. aeruginosa that is subject to efflux by a PMF-dependentRND pump. Our results show that the other P. aeruginosa AI, C₄-HSL,is not a substrate of MexAB-OprM, which indicates specificityfor long-chain AIs. Based on the broad spectrum of compounds thatRND pumps are known to transport, other small amphipathic moleculesproduced by P. aeruginosa are likely to be subject to efflux bythese pumps aswell.

Cell-to-cell signaling and RND pumps. The discovery that 3OC₁₂-HSL is subject to efflux by an RND pump suggests that regulation of genes controlled by 3OC₁₂-HSLand LasR, such as those encoding elastase (lasB) or the type IIsecretion apparatus (xcp operons), is likely to be affected bythe presence of a MexAB-OprM pump and PMF. In theory, as PMF decreases,the efflux pump activity would also decrease, causing the cellularconcentration of 3OC₁₂-HSL to rise. The expected result wouldbe increased activation of las quorum-sensing target genes suchas those mentioned above. Interestingly, in the early 1980s othersobserved that in P. aeruginosa, extracellular protease productionincreased as the PMF decreased (58). Those findings, togetherwith the results presented here which demonstrate that 3OC₁₂-HSLconcentrations in P. aeruginosa cells are higher in de-energizedcells or those lacking the MexAB-OprM efflux pump, suggest thatthe timing of induction of genes controlled by LasR and 3OC₁₂-HSLmay be affected by PMF-dependent AI efflux. A higher cellular3OC₁₂-HSL concentration would be expected sooner during the growthof P. aeruginosa lacking a functional MexAB-OprM efflux pump,resulting in earlier expression of target genes. Indeed, P. aeruginosaquorum-sensing target genes are controlled by a hierarchy of inductionbased on the AI concentration (43, 54). Because of the rolesthat the las quorum-sensing system play in virulence and biofilmdifferentiation (4, 56), experiments with the mexAB-oprMmutant will need to examine if the timing of biofilm differentiationand virulence areaffected.

Because 3OC₁₂-HSL may be partitioned into the P. aeruginosa membranes by the same mechanism as other amphipathic compounds,future studies will need to examine the role of P. aeruginosamembranes in quorum sensing. Although others have shown that inV. fischeri the 3OC₆-HSL-dependent transcriptional activator ofthe lux genes, LuxR, is associated with the inner membrane (19),it is not known whether LasR associates with the P. aeruginosainnermembrane.

Components of quorum-sensing systems (a luxR-luxI homologue and/or an N-acyl homoserine lactone AI) and RND-type efflux systems(a mexA, mexB, or oprM homologue or all three) have been identifiedin numerous gram-negative bacteria. Agrobacterium tumefacianssynthesizes 3OC₈-HSL (60), Rhizobium leguminosarum is knownto produce 7,8-cis-3-hydroxy-C₁₄-HSL (10), Rhizobium melilotiproduces an AI of unknown structure (10) which comigrates inHPLC with 7,8-cis-C₁₄-HSL of Rhodobacter sphaeroides (48), andPseudomonas putida and Burkholderia cepacia also produce AI activitydetected in a 3OC₈-HSL assay (39a). Homologues of at least onecomponent of the P. aeruginosa MexAB-OprM system have been identifiedin all of these species except R. sphaeroides. In the plant symbiontsR. meliloti and R. leguminosarum, the respective mexAB-oprM homologuesmay be involved in efflux of nodulation signals (29, 39).In P. putida, the srpABC operon and ttgB, respectively, were shownto cause efflux of organic solvents (17, 50). In the humanpathogen B. cepacia, a mexAB-oprM homologue is involved in multipleantibiotic resistance (2), and in the plant pathogen A. tumefacians,ifeAB encode an isoflavanoid-inducible efflux pump that is involvedin colonization of plant roots (36). Thus, it is likely thatcell-to-cell communication systems in species other than P. aeruginosathat rely on N-acyl homoserine lactones containing long-chainAIs will also involve RNDpumps.

	ACKNOWLEDGMENTS

We thank H. P. Schweizer for providing the P. aeruginosa mexAB-oprM mutant PAO200 and plasmids. We also thank A. Kende forearlier collaboration on the synthesis of tritium-labeled 3OC₁₂-HSL,E. P. Greenberg for advice and the use of his centrifuge, andV. Clark for her advice and critical evaluation of thedata.

This work was supported in part by NIH grant AI33713 (to B.H.I.), NIH predoctoral training grant 5T32AI07362 (to J.P.P.),and Wilmot Foundation and Swiss Research Federation grants (toC.V.D.).

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology and Immunology, University of Rochester, Box 672, 601 ElmwoodAve., Rochester, NY 14642. Phone: (716) 275-3402. Fax: (716) 473-9573.E-mail: bigl{at}uhura.cc.rochester.edu.

Present address: Department of Microbiology, Protein Design Labs, Fremont, CA94555.

Present address: Department of Genetics and Microbiology, University of Geneva, 1211 Geneva 4,Switzerland.

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Abstract
Introduction
Materials and methods
Results
Discussion
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