Genetic Analysis of Functions Involved in Adhesion of Pseudomonas putida to Seeds

doi:10.1128/JB.182.9.2363-2369.2000

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Journal of Bacteriology, May 2000, p. 2363-2369, Vol. 182, No. 9
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Genetic Analysis of Functions Involved in Adhesion of Pseudomonas putida to Seeds

Manuel Espinosa-Urgel,^* Amparo Salido, and Juan-Luis Ramos

Department of Plant Biochemistry and Molecular and Cellular Biology, Estación Experimental del Zaidín, Consejo Superior de Investigaciones Científicas, E-18008 Granada, Spain

Received 23 September 1999/Accepted 6 January 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Many agricultural uses of bacteria require the establishment of efficient bacterial populations in the rhizosphere, for whichcolonization of plant seeds often constitutes a critical firststep. Pseudomonas putida KT2440 is a strain that colonizes therhizosphere of a number of agronomically important plants at highpopulation densities. To identify the functions involved in initialseed colonization by P. putida KT2440, we subjected this strainto transposon mutagenesis and screened for mutants defective inattachment to corn seeds. Eight different mutants were isolatedand characterized. While all of them showed reduced attachmentto seeds, only two had strong defects in their adhesion to abioticsurfaces (glass and different plastics). Sequences of the lociaffected in all eight mutants were obtained. None of the isolatedgenes had previously been described in P. putida, although fourof them showed clear similarities with genes of known functionsin other organisms. They corresponded to putative surface andmembrane proteins, including a calcium-binding protein, a hemolysin,a peptide transporter, and a potential multidrug efflux pump.One other showed limited similarities with surface proteins, whilethe remaining three presented no obvious similarities with knowngenes, indicating that this study has disclosed novelfunctions.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Soil bacteria belonging to the species Pseudomonas fluorescens and Pseudomonas putida show metabolic versatility and a varietyof characteristics that makes them attractive for environmentaland agricultural uses (26). They can colonize the surface ofplant roots and the surrounding soil regions (rhizosphere) ina mutualistic association in which the bacteria obtain nutrientsfrom root exudates. In turn, some bacterial strains can promoteplant growth and have biocontrol potential against certain pathogens(39). Also, some P. putida strains have the ability to degradetoxic organic compounds, which are frequently present as contaminantsin the environment (26). P. putida KT2440, a derivative of thesoil isolate mt-2 which has been widely studied in relation tobiodegradation processes (17, 21, 28), can also colonizethe rhizosphere of agronomically relevant plants at high populationdensities, making it a suitable candidate for its use in rhizoremediation(20).

Agricultural uses of microorganisms often involve coating seeds with bacterial suspensions. Adhesion to the seed appears asa key element, since it determines the subsequent colonizationof the root system. Establishment of the bacterial populationin the root and colonization of the rhizosphere are essentialfor biocontrol efficiency (8). These latter events, root colonizationand survival in the rhizosphere, as well as responses to rootexudates, are being extensively studied at the molecular level(5, 25, 30, 32, 33), but very little is known regardingthe elements that are important for bacterial colonization ofseeds. Results obtained by DeFlaun and coworkers have shown thatsome P. fluorescens mutants defective in attachment to soil particlesare also defective in attachment to seeds (10, 11). Also,mutants of P. putida deficient in lipopolysaccharide have a limitedcapacity to attach to seeds and are impaired in root colonization(27). However, an exhaustive study of the functions specificallyinvolved in the adhesion of Pseudomonas cells to plant seeds hadnot been carried out. In this paper we report the isolation andthe phenotypic and molecular characterization of mutants of P.putida KT2440 deficient in adhesion to cornseeds.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains, plasmids, and culture conditions. P. putida KT2440 (17) was routinely used except for the mixed attachment experiments, for which KT2442, an otherwise isogenicrifampin-resistant derivative of KT2440 (17), was used. Escherichiacoli strains and plasmids used for transposon mutagenesis (SM10- $lambda$ pirharboring pUT-Km; HB101 harboring RK600) have been previouslydescribed (12). Plasmid pDLDLUX contains the luxABE genes ofVibrio fischeri cloned in a shuttle vector, under the controlof the P. putida dld (encoding D-lactate dehydrogenase) promoter(L. Molina, C. Ramos, and J. L. Ramos, unpublisheddata).

E. coli strains were grown at 37°C in Luria-Bertani (LB) medium (29). P. putida strains were grown at 30°C either in LBor in minimal medium (basal M9 medium [29] supplemented withFe-citrate, MgSO₄, and trace metals [1]) and with benzoate(15 mM) or glucose (0.4%, wt/vol) as a carbon source. Growth ratesand doubling times were analyzed on 20-ml cultures growing at30°C in 100-ml flasks with orbital shaking, measuring the opticaldensity at 600 nm at regularintervals.

When appropriate, antibiotics were added at the following concentrations (in micrograms per milliliter): chloramphenicol,30; kanamycin, 50; rifampin, 30; ampicillin, 100; and gentamicin,50. Chloramphenicol was routinely used for selection of KT2440or its derivatives, since this strain is naturally resistant tothisantibiotic.

Mutagenesis. Transposon mutagenesis with mini-Tn5-Km, a mini-Tn5 derivative carrying a kanamycin resistance marker (12), was performedby triparental mating. The recipient (P. putida KT2440), donor(E. coli SM10- $lambda$ pir harboring pUT-Km, the suicide vector carryingmini-Tn5-Km), and helper (E. coli HB101 with RK600) strains weregrown overnight in LB with the appropriate antibiotics. Afterincubation of the recipient at 42°C for 15 min, to temporarilyinactivate its restriction systems, 0.7 ml was mixed with 0.2ml of the donor and 0.1 ml of the helper. Cells were collectedby centrifugation, resuspended in 50 µl of fresh LB, and spottedon an LB plate. After overnight incubation at 30°C, cells werescraped off the plate and resuspended in 1 ml of LB, and serialdilutions were plated on selective minimal medium (M9 with benzoate,kanamycin, andchloramphenicol).

Seed attachment assays. Corn seeds were surface sterilized by washing twice for 15 min with 70% (vol/vol) ethanol and twice with 20% (vol/vol) bleach,followed by profuse rinsing with sterile deionized water. Priorto the attachment experiments, seeds were routinely hydrated for12 to 16 h. We have observed that this step increases bacterialadhesion to seeds. For the enrichment in adhesion-deficient mutants,25-ml syringes were filled with hydrated, surface-sterilized cornseeds. The bottom end of the syringes was closed, and differentdilutions of a pool of transposon mutants were added in 5 ml ofM9 basal medium. After their top ends were closed, the syringeswere incubated for 1 h with orbital agitation. The syringes werethen opened and washed with 5 ml of sterile M9 basal medium, andthe whole flowthrough (10 ml) was collected. Dilutions were platedin selective minimalmedium.

Qualitative adhesion assays were used as a fast method for the initial identification of putative attachment-deficient mutants.The assays were performed as follows. One microliter of overnightculture grown in LB was inoculated in 1 ml of M9 basal medium,and one seed was added to each bacterial suspension. After incubationfor 1 h at room temperature, seeds were removed, washed thoroughlywith deionized water, and introduced in tubes containing 1 mlof LB. Tubes were incubated at 30°C, and appearance of turbiditywas monitored over time, the rationale being that cells attachedto the seeds would start growing and dividing due to the presenceof fresh nutrients. Thus, a delay in the appearance of turbidityin a particular strain with respect to the wild type could reflectreduced bacterial attachment to theseeds.

For the quantitative assays, bacterial incubation with the seeds was done as described above except that the number of cellsinoculated was determined by plating serial dilutions on LB platesprior to addition of the seeds. After incubation, seeds were removed,washed, and transferred to tubes containing M9 basal medium. Thetubes were vortexed for 1 min to remove any bacteria that maynot have been tightly attached to the seed surface. Seeds werewashed again and disrupted by vortexing with 3-mm-diameter glassbeads in M9 basal medium (27). This procedure does not affectbacterial viability. To estimate the percentage of cells attachedto the seeds with respect to the number of inoculated cells, dilutionsof the resulting suspension were plated on selective medium. Eachassay was repeated at least threetimes.

Attachment of luminescent bacteria was detected as follows. Seeds incubated with the bacterial suspensions and washed as describedabove were placed on filter paper soaked with 0.01% (vol/vol)n-decyl aldehyde (Sigma). Seeds were then covered with plasticwrap, and luminescence was detected after overnight exposure ofautoradiographic film (Kodak X-Omat).

Motility and chemotaxis assays, antibiotic sensitivity, and microscopy. Motility was tested in 0.3% (wt/vol) agar plates, in LB or M9 with benzoate. Chemotaxis toward seeds was assayed with a proceduresimilar to that described by Van Bastelaere et al. (35), namely,100 µl of each overnight culture was mixed with a cooled (42°C)0.2% (wt/vol) water agar solution. The mixture was poured ontopetri dishes and allowed to solidify. Three seeds were then placedin different spots on the surface of each plate, and the plateswere incubated at 30°C. Positive chemotactic responses were observedafter 5 h as the appearance of concentric halos around theseeds.

Sensitivity to antibiotics was determined by measuring the inhibition halos on LB plates, with disks (bioMérieux) containingthe following amounts (micrograms) of the different antibiotics:ampicillin, 10; tetracycline, 30; carbenicillin, 100; piperacillin,100; streptomycin, 10; and gentamicin,10.

Bacterial morphology was visualized under phase contrast on a Zeiss Axioskop lightmicroscope.

Biofilm formation assays. Formation of biofilms on abiotic surfaces was assessed essentially as described elsewhere (22). Cultures were grown overnightand inoculated (1:20 dilution) in 50 µl of LB or M9, supplementedwith either benzoate or glucose, in polystyrene microtiter dishes.After 4 h of incubation at 30°C, the wells were washed with deionizedwater, and 100 µl of a 1% (wt/vol) solution of crystal violetwas added to each well. Plates were incubated at room temperaturefor 15 min and washed thoroughly, and biofilm formation was quantified.For this purpose, the stain was solubilized by adding ethanol(200 µl twice) to each well. This solution was then transferredto an Eppendorf tube, and 600 µl of distilled water was added.Absorbance at 600 nm was then measured in a Perkin-Elmer Lambda20 spectrophotometer. Similar assays were performed on other surfaces,polypropylene (Eppendorf tubes), and borosilicate (glasstubes).

Analysis of proteins. A fast extraction method was used for preparation of surface proteins by heat treatment (19). One milliliter of each overnightculture was centrifuged, and cells were resuspended in 40 µl of0.9% (wt/vol) NaCl. After incubation for 15 min at 65°C and centrifugationat 3,000 × g for 5 min, supernatants were transferred to cleantubes and immediately frozen. Samples were boiled in the presenceof sodium dodecyl sulfate (SDS) and analyzed by SDS-polyacrylamidegel electrophoresis (SDS-PAGE) as described elsewhere (2).

DNA techniques. Preparation of plasmid and chromosomal DNA, digestion with restriction enzymes (Boehringer), electrophoresis, and Southernblotting were carried out using standard methods (2, 29).Hybridizations were done using the DIG DNA labeling and detectionkit (Boehringer) as instructed by the manufacturer. Electroporationof plasmid DNA into P. putida was done as described elsewhere(22).

DNA sequences from the transposon mutants were determined using arbitrary PCR (9) with Taq DNA polymerase (Pharmacia) ona Perkin-Elmer GeneAmp 9600. A first round of amplification wasdone by using the chromosomal DNA of the mutants as a template,with an arbitrary primer (ARB1; 5'-GGCACGCGTCGACTAGTACNNNNNNNNNNGATAT-3')and an internal primer of mini-Tn5, unique for the right end (TNEXT;5'-TGATGAATGTTCCGTTGCGCTGCC-3'). The first round was as follows:3 min at 95°C; 6 cycles of 30 min at 95°C, 30 min at 30°C, and1 min at 72°C; 30 cycles of 30 min at 95°C, 30 min at 50°C, and1 min 72°C; and an extension period of 7 min at 72°C. A secondround of amplification was done with 5 µl of the first-round reactionas the template as follows: 3 min at 95°C; 30 cycles of 30 minat 95°C, 30 min at 57°C, and 1 min at 72°C; and 7 min at 72°C.Primers used for the second round were those corresponding tothe conserved region of ARB1 (ARB2; 5'-GGCACGCGTCGACTAGTAC-3')and a second internal primer of mini-Tn5, closer to the end (TNINT;5'-GACCTGCAGGCATGCAAGCTCGGC-3').

Reaction mixtures were electrophoresed, and the most intense bands were isolated with a Qiagen gel extraction kit and sequenced.Sequencing was done on an ABI PRISM 310 automated sequencer, usingoligonucleotide TNINT as a primer. The ~40-bp distance betweenthis primer and the end of the mini-Tn5 provides an internal controlto ensure that the obtained sequence corresponds to the junctionbetween the transposon and thechromosome.

Sequences were analyzed and compared with the GenBank database by using BLAST programs (3). Preliminary sequence data forthe P. putida and P. aeruginosa genomes were obtained from TheInstitute for Genomic Research (www.tigr.org) and the PseudomonasGenome Project (www.pseudomonas.com),respectively.

Nucleotide sequence accession numbers. The sequences reported have been deposited in GenBank under accession no. AF182512 through AF182519.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Adhesion of P. putida KT2440 to corn seeds: roles of protein synthesis and surface proteins. To begin analyzing the functions involved in the attachment of KT2440 to corn seeds, we tested whether new synthesis of proteins,occurring in the presence of seeds, was required for attachment.Initially, quantitative analyses were performed as described inMaterials and Methods, incubating corn seeds with a suspensionof overnight grown cells diluted 1:1,000 in M9 basal medium. After1 h of incubation, the average number of attached bacteria was0.65% of the number of inoculated cells. To assess the role ofnewly synthesized proteins, tetracycline was added before incorporatingthe seeds to the bacterial suspension, in order to block translation.Addition of tetracycline had no effect on viability and did notaffect significantly the attachment of KT2440 to corn seeds. Thenumber of attached cells was approximately 89% with respect tothe control without tetracycline treatment, suggesting that mostof the functions required for efficient bacterial adhesion tothe seeds in the conditions of our experiments are already presentin the stationary-phase cultures of KT2440 after growth in richmedium.

Outer membrane proteins have been shown to play an important role in the attachment to biotic and abiotic surfaces (15,22, 32). To determine the involvement of extracellular proteinsin the initial steps of seed colonization, adhesion assays wereperformed after incubation of the bacterial cultures in the presenceof 20 µg of proteinase K per ml. In this case, while viabilitywas unaffected, attachment was significantly reduced. The numberof attached cells was 20% of the number of cells attached in thecontrol without treatment. This result indicates that one or moresurface-located or secreted proteins are involved in the adhesionof bacterial cells to cornseeds.

Screening for mus derivatives of KT2440. To identify functions involved in the initial steps of seed colonization, we designed a screen to isolate mutants showingdeficiencies in adhesion to seeds, which we termed "mus" (mutantsunattached to seeds). The general procedure (outlined in Fig.1) is based on the column method described by DeFlaun and coworkers(10) to identify mutants of P. fluorescens unable to bind tosoil particles. KT2440 was mutagenized by random insertion ofmini-Tn5-Km (12). A pool of kanamycin-resistant mutants wasthen generated by collecting ~10,000 colonies, obtained aftermutagenesis, and plating in selective minimal medium (thus avoidingthe isolation of auxotrophs). Dilutions of this pool were incorporatedinto syringes filled with surface-sterilized corn seeds and thenincubated to enrich in attachment-deficient mutants describedin Materials and Methods. After incubation and collection of theflowthrough (i.e., cells that had not adhered to the seeds), dilutionswere plated in selective minimal medium. Four independent selectionexperiments were performed, in which 7 × 10³, 7 × 10⁴, 7 × 10⁵, and 2 × 10⁷ cells were inoculated into the columns; 300 of the colonies obtainedwere then tested individually for the ability to attach to seeds.For this second round of selection, each clone was grown overnight,and those with obvious growth defects were discarded. A qualitativeattachment assay was performed with the rest of the strains asdescribed in Materials and Methods. After incubation with eachbacterial suspension, washing, and subsequent incubation of theseeds at 30°C in tubes containing LB medium, appearance of turbiditywas monitored after 6 to 10 h. The clones presenting a delay inthe appearance of turbidity with respect to the wild type wereselected as being potentially defective in attachment and subjectedto a second round of a similar selection process. After theserounds of selection, 20 mutants were identified as putative musclones.

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FIG. 1. Summary of the screening strategy used to isolate mus derivatives of P. putida KT2440. Details are presented in the text.

Since we used a pool of colonies for the first selection step, it was possible that some of the mus clones obtained were identical.To eliminate these potential siblings, Southern hybridizationwas performed using pUT-Km as a probe on chromosomal DNA of the20 clones digested with BstEII, for which there is no site insidethe transposon. Only one band giving hybridization signals appearedin each case, indicating that a single copy of the transposonwas present in all the mutants (data not shown). When two or moreclones presented a band of the same size, only one of them wasselected, the rest being discarded as potential siblings (Table1), and some of them were confirmed later by arbitrary PCR andsequencing. Thus, eight clones were finally chosen for furtheranalysis.

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TABLE 1. Phenotypes of mus mutants

Phenotypic characterization of mus mutants. To begin the characterization of these eight mus mutants, we compared their growth rates to those of the parental strain indifferent culture media, to confirm that the delayed appearanceof turbidity observed in the qualitative attachment assays wasnot due to some metabolic defect affecting their growth. All ofthe mus clones showed doubling times similar to that of the wildtype in LB (55 ± 3 min) and in M9 minimal medium with either benzoate(95 ± 2 min) or glucose (99 ± 4 min) as a carbonsource.

Quantitative attachment assays were then performed as described above. Results are presented in Fig. 2A. Adhesion of all theselected mutants to corn seeds was significantly reduced withrespect to the wild type, ranging from 3.5 to 15 times fewer cellsrecovered from the disrupted seeds relative to the parental strain.To ensure that these reduced numbers were not simply due to themutants being unable to survive in basal M9 medium without a carbonsource during the period of incubation, the eight clones wereincubated in this medium for the same time but in the absenceof seeds. No significant loss of viability was observed in anycase (data not shown).

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FIG. 2. Adhesion of P. putida KT2440 (wild type [wt]) and mus mutants to corn seeds. (A) Quantitation of attachment of P. putida KT2440 and eight mus mutants to corn seeds. After 1 h of incubation with each bacterial suspension, seeds were washed and disrupted, and the number of attached cells was estimated as CFU after plating serial dilutions. Results are presented as percentage of attached cells with respect to the number of cells inoculated (average of at least three independent experiments). (B) Adhesion to corn seeds (left) of KT2440 and mus mutants harboring plasmid pDLDLUX, visualized by overnight exposure of film (right). (C) Adhesion of mus mutants (white bars) coinoculated with KT2442 (grey bar). Relative percentages of cells of each strain attached to the seeds (average of three independent assays) are shown.

A direct adhesion assay was performed to confirm the results obtained from the quantitative assays. For this purpose, KT2440and the eight mus strains were transformed with pDLDLUX, a plasmidharboring the bioluminescence genes luxABE under the control ofthe dld promoter, the expression of which is constitutive in P.putida (Molina et al., unpublished data). Attachment assays wereperformed with these luminescent strains as described in Materialsand Methods, and the results (Fig. 2B) were recorded by exposingautoradiographic film to the seeds after incubation with the bacterialsuspensions. In all cases, the seeds inoculated with the mus strainsshowed less luminescence than the seeds incubated with the parentalstrain, indicating a lower number of cells attached to the seeds.Although there is not an exact correlation between the data fromthe luminescence assay and the quantitative assay, this resultconfirms the attachment defects in all of the musmutants.

Adhesion of each mutant was also tested in coinoculations with KT2442, an otherwise isogenic rifampin-resistant derivativeof KT2440 (17). These assays were performed to determine whetherthe mutant cells were less competitive than the wild type in theiradhesion to seeds and whether the presence of the wild-type straincould restore the ability of some mutants to attach to corn seeds.Results are shown in Fig. 2C. In all cases, after coinoculationof seeds with KT2442 and the mutants (1:1 ratio), the number ofrifampin-resistant cells recovered was higher than the numberof kanamycin-resistant cells, indicating that the mutants havea competitive disadvantage in seed colonization (coincubationin the absence of seeds had no effect on viability of any of themutants). Yet, in two of the mixtures (with mus-9 and mus-24),the mutants constituted around 40% of the attached population,suggesting that the presence of the wild-type strain may partiallycomplement the defects of these mutants. In these two mutants,the percentage of cells attached doubled with respect to the percentageobtained in the individual assays (data notshown).

Motility and chemotaxis have been shown to play an important role in bacterial attachment to both biotic and abiotic surfaces(13, 23, 24, 36). Therefore, we tested the motility ofKT2440 and the eight mutants in 0.3% (wt/vol) agar plates, bothin LB and in M9 with benzoate. All of the strains were motileand indistinguishable in LB. However, when the assay was performedin M9 supplemented with benzoate, strains mus-5 and mus-13 presenteda delay in the formation of a motility halo, which was slightlybut consistently smaller than that of the remaining strains (Table1). We also performed a qualitative chemotaxis assay similarto that described by Van Bastelaere (35). KT2440 and the eightmutants were tested on 0.2% (wt/vol) agar plates for chemotaxistoward corn seeds, identified by the formation of concentric halosaround the seeds (see Materials and Methods). Differences weredetected only for mus-13 and mus-22, both of which showed a delayin the formation of chemotaxis halos (Table 1).

Colony and cell morphology were also monitored. Mutants mus-24 and mus-27 formed colonies slightly smaller than those formedby the rest of strains on LB plates; mutants mus-22 and mus-24presented altered morphology, cells being two to three times longerthan those of the parental strain (Table 1).

Attachment of mus mutants to abiotic surfaces. Mutants defective in biofilm formation on abiotic surfaces have been isolated and characterized in different bacterial species(22-24). We were interested in the possible correlation betweenattachment to biotic and to abiotic surfaces and whether the mutantsisolated in our screen showed a general adhesion deficiency orwere altered in functions specific for seed colonization. We thereforetested biofilm formation of KT2440 and the eight mus clones ondifferent abiotic surfaces. These experiments were performed essentiallyas described by O'Toole and Kolter (22) on polystyrene (microtiterdishes), polypropylene (Eppendorf tubes), and borosilicate (glasstubes) surfaces. Since biofilm formation can vary depending onthe growth medium, we also tested attachment to polystyrene ofcultures grown on LB and on M9 supplemented with either glucoseor benzoate. Biofilm formation was analyzed after 4 h of growthby staining with crystal violet. The amounts of attached cellswere quantified after solubilization of the stain and measurementof optical density at 600 nm. The results obtained in these assaysare shown in Fig. 3. Two mutants, mus-22 and mus-24, showed severedefects in biofilm formation in all the tested surfaces, independentlyof the growth medium. This result indicates that these cloneswere affected in general functions required for adhesion to bothbiotic and abiotic surfaces. The remaining mutants presented aslight reduction in biofilm formation in some of the growth conditionsor surfaces tested, but the differences with the parental strainwere generally not relevant. These results suggest that the interruptedgenes are more specifically involved in plant-bacterium interaction.

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FIG. 3. Biofilm formation on different abiotic surfaces, quantified by staining attached cells with crystal violet and measuring A₆₀₀ after solubilization of the stain with ethanol. Results are the average of four independent assays. wt, wild type.

Molecular characterization of mus mutants. As indicated above, attachment of P. putida KT2440 to corn seeds appears to be strongly dependent on surface proteins, sincethe addition of proteinase K drastically reduces adhesion. Thus,it seemed reasonable that at least some of the mutants isolatedpresented defects in such proteins. To explore this possibility,surface proteins of KT2440 and the mus clones were analyzed bySDS-PAGE (Fig. 4). Several clones presented differences with respectto the parental strain, the most obvious being mus-20, mus-22,and mus-24. The latter two mutants showed similar results, withtwo bands of ~60 and ~29 kDa presenting clearly reduced intensitywith respect to the wild type. In mus-22 a third band, of ~40kDa, was missing. As for mus-20, two bands (~65 and ~45 kDa) ofstronger intensity with respect to KT2440 are apparent, whilea band of ~35 kDa shows reduced intensity. These results suggestthat the attachment defects of some of the mutants could be dueto alterations in their surface structures.

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FIG. 4. Surface proteins of KT2440 and mus strains. Surface proteins were analyzed by SDS-PAGE on a 12% polyacrylamide gel and staining with Coomassie brilliant blue. Bands showing less intensity in the mutants than in the parental strain (wild type [wt]) are marked with black arrows; bands with more intensity in the mutants than in KT2440 are indicated with white arrows. Positions of molecular weight markers are indicated in kilodaltons.

To determine the chromosomal locations of the transposon insertions and identify the gene disrupted in each case, arbitraryPCR (9) was performed with all mutants as described in Materialsand Methods. This technique allowed us to amplify fragments containing150 to 600 bp of DNA flanking the transposon insertion site. ThesePCR fragments were gel purified and sequenced. Sequences werecompared with the unfinished genome of P. putida KT2440. The insertionsites in four mutants (mus-13, mus-21, mus-24, and mus-27) couldbe unambiguously identified (Table 2). In these cases, sequencesof ~2 kb around the insertion point were then used for comparisonswith the databases using BLAST programs (3). For the remainingmutants, the sequences obtained from the PCR fragments were used.The results from these analyses are summarized in Table 2. Forthree loci, mus-9, mus-20 and mus-22, no significant match couldbe found with any sequences in the databases. In the case of mus-5,some similarity could be found with a putative adhesion factorof E. coli resembling the prn gene of Bordetella pertussis. Theproduct of this gene, pertactin, is a virulence factor involvedin bacterial adhesion to eukaryotic cells (37).

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TABLE 2. Molecular characterization of mus mutants

In the remaining four mutants analyzed, the insertion had taken place in genes with known homologues in other microorganisms.Of these, mus-24 showed similarities with various surface proteins,including hemolysins and other toxins, all of which present arepeated motif presumably involved in binding of calcium. Calcium-bindingproteins have been identified as important factors in root colonizationand nodulation by Rhizobium (16, 32). The gene showing thehighest similarity with mus-24 was expE1 of Sinorhizobium meliloti(6), which is in turn closely related to the nodulation factornodO of Rhizobium. Locus mus-27 showed similarities with hemolysinsof Serratia marcescens, Proteus, and the fish pathogen Edwardsiellatarda (18). As for mus-13, the locus where insertion had takenplace presented significant similarities with the E. coli cstAgene (coding for carbon starvation protein A [31]) and otherE. coli homologues of cstA which code for putative carbon starvationproteins. CstA is a membrane protein apparently involved in peptidetransport (31), whereas the functions of the other homologuesare not known. Also mus-21 shows similarity to membrane proteins,the products of the kefB and kefC genes of E. coli and Myxococcus,both of which are glutathione-regulated K⁺ efflux pumps (4).

It has been recently reported that a toxin-responsive efflux pump could be important for interaction of a fungal pathogenwith rice plants (34). Also, multidrug resistance has been associatedwith bacterial adhesion to eukaryotic cells (14). We thereforeconsidered the possibility of mus-21 being affected in a genecoding for a multidrug efflux pump. Sensitivity of KT2440 andmus-21 to various antibiotics was tested. In general, mus-21 wassignificantly more sensitive to all the $beta$ -lactam antibiotics tested(ampicillin, carbenicillin, and piperacillin) than the parentalstrain, while it did not show significant differences in resistanceto tetracycline, streptomycin, and gentamicin. These results suggestthat the gene affected in strain mus-21 could in fact code fora multidrug efflux pump involved in transport of $beta$ -lactamantibiotics.

The sequences obtained from all the mutants were also compared with the genome of P. aeruginosa (Table 2), which is finishedbut not completely assembled. Only mus-13 and mus-21 showed obviousmatches with sequences from P. aeruginosa, with 86 and 82% identicalresidues at the nucleotide level, respectively. Relevant similaritywas also found for mus-9, but only in the last 50 nucleotidesof the sequenced fragment (90% identities). Completion of theassembly of the sequences of both the P. aeruginosa and P. putidagenomes will allow us to distinguish which of the genes identifiedhere are present in the two species and which are specific ofP. putida.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

To understand the functions and processes involved in bacterial colonization of plant seeds, we have developed a screen toisolate mutants of P. putida defective in adhesion to corn seeds.The first step of the screen, passing a pool of insertional mutantsthrough a seed column, was an efficient system to enrich in musderivatives of KT2440, although the possibility of having missedmutants defective in cell-to-cell interactions cannot be discardedas a potential disadvantage of this selection procedure. Thiscaveat notwithstanding, out of 300 clones obtained from four independentenrichment experiments, tested individually, 20 presented thedesired phenotype consistently. Several of these proved to bepossible siblings, based on Southern analysis, some confirmedby sequencing. Thus, eight different mutants were finally identified.All of them show clear defects in the ability to adhere to cornseeds, both by themselves and when inoculated with the parentalstrain. The fact that identical insertion mutants were isolatedin independent selection experiments validates the screen andmay give an idea of the most important functions required forthe attachment to seeds under the conditions used here. Extracellularproteins seem to play an important role in attachment, as suggestedby the decrease in adhesion when KT2440 is incubated with proteinaseK and by the fact that several of the mutants show alterationsin their patterns of surfaceproteins.

The eight mus clones have been further characterized, and the insertion sites have been sequenced. All correspond to genesthat have not been described before in P. putida. Three of themgave no significant match with sequences in the databases, indicatingthat they could code for novel functions related to seed colonization.Of the remaining five, an interesting finding is that two loci,mus-5 and mus-27, have similarities with genes of other organismscoding for factors involved in pathogenesis (pertactin and hemolysins).These factors are involved in the early steps of bacterial colonizationof host tissues. Another locus, mus-21, codes for a putative multidrugefflux pump. Such an efflux pump has been recently identifiedas a pathogenicity factor in Magnaporthe grisea, the fungus responsiblefor rice blast disease (34). The function of such transporterswould be to protect the microorganism against toxic compoundsproduced by the plant as a defense response. Finally, mus-24 showsa putative calcium-binding motif present in nodulation proteinsas well as in virulence factors and other surface proteins. Allof these data suggest that there are common mechanisms involvedin the early stages of colonization of host tissues by pathogenicand nonpathogenicmicroorganisms.

A noticeable result is the fact that the mutants identified in our screen were not affected in other functions previouslyknown to play a role in adhesion, such as flagella, pili, or otheraggregation factors (7, 13, 15, 24). Motility has beenshown to play an important role in the attachment of Pseudomonasand other bacteria to biotic and abiotic surfaces (23, 24,36). However, none of the mus clones were nonmotile, althoughtwo of them showed a slight defect in minimal medium. We alsoexpected to find mutants deficient in chemotaxis, another importantfactor in bacterial attachment (24, 36). Again, two mutantsshowed a slight defect but not a null phenotype. It could be thatin our experimental conditions the relative importance of thesefunctions was diminished. Incubating the bacteria in a columnfilled with seeds, with constant agitation, probably facilitatesadhesion without the need for cells to move toward the seeds.The situation may be different in natural settings, where thebacteria have to find the seeds. It is worth noticing, however,that mus-13 showed defects both in motility in minimal mediumand in chemotaxis. Transposon insertion in this clone had takenplace in a locus very similar to a family of E. coli genes includingcstA, the product of which seems to be involved in peptide transport(31). It is possible that peptides and amino acids, which arerelevant components of root exudates (25), act as chemoattractantstoward the seeds, being recognized and utilized as nutrients bythe bacterial cells. The fact that mus-13 shows a strong defectin seed attachment, and that siblings of this mutant (up to eight)were isolated in all four independent screens, suggests that thisgene plays a key role in seedcolonization.

We have also investigated whether mus clones were generally defective in adhesion, although none of the genes identified herecorrespond to previously identified genes involved in attachmentof Pseudomonas to abiotic surfaces (22). Two of the mutants,mus-22 and mus-24, appear to be severely affected in biofilm formationon abiotic surfaces; the rest do not show appreciable defects.Thus, two types of mutants seem to have been isolated, some withgeneral defects in adhesion to solid surfaces and others whichappear to be more specifically deficient in seed attachment. Ithas been proposed that bacterial biofilm formation proceeds throughdivergent pathways depending on whether the surface can be a sourceof nutrients or not (38). Our results may support that idea,although there are common elements involved in both, exemplifiedby mutants mus-22 and mus-24.

The results presented here give an overview of the important functions for seed colonization by P. putida. Although a moredetailed analysis of the identified genes and their specific roleswill be required, several conclusions can be drawn from this study.First, the isolation of genes of unknown function and with noobvious similarities with previously described genes indicatesthat we may be unraveling novel elements of the physiology andgenetics of Pseudomonas. Second, there seem to be somewhat divergentprocesses involved in bacterial adhesion to biotic and abioticsurfaces, with some aspects common to both. Finally, the similaritiesof several of the genes identified here with virulence factorsof pathogenic microorganisms suggest that initial colonizationof host tissues proceeds via similar or common pathways. Thus,as suggested by previous findings (15, 23), there seems tobe a thin line between pathogenesis and mutualistic associationof bacteria with eukaryoticorganisms.

	ACKNOWLEDGMENTS

We thank A. Hurtado for DNA sequencing and G. O'Toole for suggestions and helpful discussions. Preliminary sequence data wereobtained from The Institute for Genomic Research and the PseudomonasGenomeProject.

This work was supported by grant BIO4-CT97-2313 from the EuropeanUnion.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Plant Biochemistry and Molecular and Cellular Biology, Estación Experimentaldel Zaidín, Consejo Superior de Investigaciones Científicas,E-18008 Granada, Spain. Phone: 34-958-121011. Fax: 34-958-129600.E-mail: mespinos{at}eez.csic.es.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Abril, M. A., C. Michán, K. N. Timmis, and J. L. Ramos. 1989. Regulation and enzyme specificities of the TOL plasmid-encoded upper pathway for degradation of aromatic hydrocarbons and expansion of the substrate range of the pathway. J. Bacteriol. 171:6782-6790[Abstract/Free Full Text].
2.	Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1987. Current protocols in molecular biology. John Wiley & Sons, New York, N.Y.
3.	Altschul, S. F., T. L. Madden, A. A. Schäffer, J. Zhang, Z. Zhang, W. Miller, and D. J. Lipman. 1997. Gapped BLAST and PSI-BLAST: a new generation of protein database search programs. Nucleic Acids Res. 25:3389-3402[Abstract/Free Full Text].
4.	Bakker, E. P., I. R. Booth, U. Dinnbier, W. Epstein, and A. Gajewska. 1987. Evidence for multiple K⁺ export systems in Escherichia coli. J. Bacteriol. 169:3743-3749[Abstract/Free Full Text].
5.	Bayliss, C., E. Bent, D. E. Culham, S. MacLellan, A. J. Clarke, G. L. Brown, and J. M. Wood. 1997. Bacterial genetic loci implicated in the Pseudomonas putida GR12-2R3-canola mutualism: identification of an exudate-inducible sugar transporter. Can. J. Microbiol. 43:809-818[Medline].
6.	Becker, A., S. Ruberg, H. Kuster, A. A. Roxlau, M. Keller, T. Ivashina, H. P. Cheng, G. C. Walker, and A. Puhler. 1997. The 32-kilobase exp gene cluster of Rhizobium meliloti directing the biosynthesis of galactoglucan: genetic organization and properties of the encoded gene products. J. Bacteriol. 179:1375-1384[Abstract/Free Full Text].
7.	Buell, C. R., and A. J. Anderson. 1992. Genetic analysis of the aggA locus involved in agglutination and adherence of Pseudomonas putida, a beneficial fluorescent pseudomonad. Mol. Plant-Microbe Interact. 5:154-162[Medline].
8.	Bull, C. T., D. M. Weller, and L. S. Thomashow. 1991. Relationship between root colonization and suppression of Gaeumannomyces graminis var. tritici by Pseudomonas fluorescens strain 2-79. Phytopathology 81:954-959[CrossRef].
9.	Caetano-Annoles, G. 1993. Amplifying DNA with arbitrary oligonucleotide primers. PCR Methods Appl. 3:85-92[Medline].
10.	DeFlaun, M. F., A. S. Tanzer, A. L. McAteer, B. Marshall, and S. B. Levy. 1990. Development of an adhesion assay and characterization of an adhesion-deficient mutant of Pseudomonas fluorescens. Appl. Environ. Microbiol. 56:112-119[Abstract/Free Full Text].
11.	DeFlaun, M. F., B. Marshall, E.-P. Kulle, and S. B. Levy. 1994. Tn5 insertion mutants of Pseudomonas fluorescens defective in adhesion to soil and seeds. Appl. Environ. Microbiol. 60:2637-2642[Abstract/Free Full Text].
12.	de Lorenzo, V., M. Herrero, U. Jakubzik, and K. N. Timmis. 1990. Mini-Tn5 transposon derivatives for insertion mutagenesis, promoter probing, and chromosomal insertion of cloned DNA in gram-negative eubacteria. J. Bacteriol. 172:6568-6572[Abstract/Free Full Text].
13.	De Weger, L. A., C. I. M. Van der Vlugt, A. H. M. Wijfjes, P. A. H. M. Bakker, B. Schippers, and B. J. J. Lugtenberg. 1987. Flagella of a plant growth-stimulating Pseudomonas fluorescens strain are required for colonization of potato roots. J. Bacteriol. 169:2769-2773[Abstract/Free Full Text].
14.	Di Martino, P., D. Sirot, B. Joly, C. Rich, and A. Darfeuille-Michaud. 1997. Relationship between adhesion to intestinal Caco-2 cells and multidrug resistance in Klebsiella pneumoniae clinical isolates. J. Clin. Microbiol. 35:1499-1503[Abstract].
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