Pseudomonas aeruginosa readily binds to stainless steel and other abiotic surfaces, causing major problems in both the medical and food industries. In this study, we show that P. aeruginosa binds to abiotic surfaces in a concentration-dependent, saturable manner during the initial stages of biofilm formation. P. aeruginosa type IV pili mediate binding to stainless steel as a pilus-deficient strain does not bind to steel, purified type IV pili bound in a concentration-dependent, saturable manner, and purified pili competitively inhibited whole cell binding. PAK pili can also bind polystyrene and polyvinylchloride in a concentration-dependant and saturable manner. As an antibody specific for the C-terminal pilin receptor binding domain inhibited adherence to abiotic surfaces, the role of the C-terminal receptor binding domain in mediating binding to steel surfaces was examined. A synthetic peptide of the PAK pilin epithelial cell receptor binding domain [PAK(128–144)ox] bound directly to steel with high affinity. The interaction of pili with steel was specifically inhibited by this peptide with an apparent Ki of ∼0.2 nM and effectively inhibited the binding of viable homologous and heterologous P. aeruginosa strains to steel with an apparent Ki of ∼4 nM. A single point mutation (K130I) in the PAO receptor binding domain was observed to abolish binding to stainless steel while binding to human buccal epithelial cells was enhanced. Therefore, the C-terminal receptor binding domain appears to have evolved for binding a variety of surfaces.
Type IV pili are composed of a single pilin subunit, PilA, and are assembled into long polar surface appendages (Folkhard et al., 1981). This assembly process ensures that the receptor binding domain is only located at the tip of the pilus (Lee et al., 1994). The pilus-associated epithelial cell receptor binding domain is located within residues 128–144 of the C-terminal region of PilA, the pilin structural protein (Irvin et al., 1989). This terminal binding domain specifically recognizes GalNAc-β-D-(1,4)-Gal moieties of asialo-GM1 as a minimal receptor (Sheth et al., 1994). Adherence to this receptor is specific and can be inhibited by a synthetic C-terminal receptor binding domain, PAK(128–144)ox, or by synthetic GalNAc-β-D-(1,4)-Gal (Sheth et al., 1994; Wong et al., 1995; Schweizer et al., 1998).
In this study, we examine the initial event of P. aeruginosa biofilm formation on stainless steel, namely the binding of the organism to the surface. We demonstrate that type IV pili specifically mediate binding to stainless steel and that the interaction with steel involves the previously identified pilin C-terminal epithelial cell receptor binding domain (Irvin et al., 1989). This synthetic peptide receptor binding domain was observed to bind to steel with high affinity and prevent binding of a variety of P. aeruginosa strains to steel. In addition, the C-terminal receptor binding domain also mediated binding to other abiotic surfaces including polyvinylchloride and polystyrene. Therefore, the C-terminal receptor binding domain has evolved to retain a structure for binding a variety of surfaces including both biotic and abiotic surfaces.
Initial colonization of stainless steel is dependent upon type IV pili in P. aeruginosa
While the involvement of type IV pili in biofilm formation on abiotic surfaces has been well documented (O’Toole and Kolter, 1998; Klausen et al., 2003), the molecular basis for that involvement has not been firmly established. Therefore, we investigated the ability of P. aeruginosa wild-type strains PAK, PAO, K122-4 and KB7, which display considerable differences in their pilin sequences, to bind to stainless steel (Fig. 1A and B). P. aeruginosa pilins are characterized by a highly conserved N-terminal α-helix and a semi-conserved C-terminal disulphide loop region but display minimal sequence similarity through the bulk of the protein (Fig. 1A). However, structural studies indicate that P. aeruginosa pilins are strikingly similar (Fig. 1B) (Hazes et al., 2000; Craig et al., 2003; Audette et al., 2004). P. aeruginosa strains PAK, PAO, K122-4 and KB7 were observed to rapidly bind to stainless steel surfaces (Fig. 2A, D, G and J), in agreement with previous results (Stanley, 1983; VanHaecke et al., 1990). Strains PAO and PAK bound more significantly to stainless steel than either K122-4 or KB7 (Fig. 2A, D, G and J). P. aeruginosa strain MS591 (Starnbach and Lory, 1992), a fliC– non-flagellated mutant of PAK, was observed to bind at considerably reduced levels compared with the parental PAK strain (Fig. 2A and P). P. aeruginosa strain PAKNP, a non-piliated pilA deficient mutant of PAK (Saiman et al., 1990), did not bind to steel surfaces (Fig. 2M), suggesting that P. aeruginosa adherence to stainless steel may be mediated by type IV pili. To further investigate the initial colonization of stainless steel, the binding kinetics of PAK cells and pili to steel was examined in a quantitative manner employing viable biotinylated cells and purified biotinylated PAK pili. PAK cells (Figs 3A and 4) and purified PAK pili (Fig. 3B) were observed to bind to steel surfaces in a saturable, concentration-dependent manner while PAKNP biotinylated cells (Figs 3A and 4) did not bind appreciably to the steel surface. Biotinylation had no effect on the ability of the purified pili to bind stainless steel as identical binding kinetics were observed with native pili when anti-PAK pili antibodies were utilized to quantify binding (data not shown). Furthermore, addition of low concentrations of purified PAK pili competitively inhibited the binding of biotinylated PAK cells to steel (Fig. 3C). As the length of PAK pili is not known, the molarity of the pili cannot be determined (van Schaik et al., 2005).
We established that P. aeruginosa stained with acridine orange were readily visualized by epifluorescence microscopy following binding to stainless steel (Fig. 1D). P. aeruginosa cells were visualized as fluorescent orange rods bound to areas of the steel that fluoresced green either through non-specific interaction of the fluorochrome with grain boundary regions or due to non-specific interaction of the fluorochrome with organic material that interacted with the grain boundaries in the steel. Green fluorescent material primarily associated with grain boundaries in the steel was observed in both strains PAK and PAKNP (Fig. 1D and E). In confirmation of these results, Pseudomonas sp. has recently been shown to colonize preferentially with grain boundaries (Sreekumari et al., 2001).
Effect of flagella and type IV pili mutations on binding to steel
Previous studies using P. aeruginosa FilC– and PilB– strains have established the importance of flagella and type IV pili during the initiation and development of biofilms on abiotic surfaces in static cultures (O’Toole and Kolter, 1998). To confirm our qualitative microscopic examination, a quantitative analysis of adherence to steel was performed. The binding of PAK-BΩ (PilB– mutant), a strain that does not assemble pili but does express PilA (Koga et al., 1993), to steel was compromised relative to wild-type and equivalent to that observed for PAKNP and PAKMS591 (Fig. 4). ELISA evidence indicates that PAKMS591 has less surface-exposed pili than does the PAK wild-type strain (data not shown). Strain PAK-DΩ (pilD-mutant) which lacks the prepilin peptidase and therefore does not express surface-exposed PilA (Koga et al., 1993) or functional type IV pili, bound roughly equivalent to mutant strains (PAKNP, PAKMS591 and PAK-BΩ) (Fig. 4). Although the binding curves differ slightly between mutant strains, all pili-deficient strains (PAKNP, PAK-BΩ and PAK-DΩ), and PAKMS591, bound significantly less than wild-type (Fig. 4). These results indicate that any mutation which abolishes the production of functional pili also reduces the ability to bind stainless steel.
Antibody inhibition studies
Addition of rabbit polyclonal anti-PAK pili antibodies (Lee et al., 1989) but not rabbit pre-immune serum strongly inhibited the binding of biotinylated PAK cells and pili (Fig. 5) to steel in a dose-dependent manner. These data indicate that the type IV pili mediates binding. Murine monoclonal antibody PK99H, which recognizes PAK PilA residues 134–140 exposed at the tip of the pilus (Lee et al., 1994; Wong et al., 1992), significantly inhibited the binding of PAK cells and pili to steel (Fig. 5). The inhibition of PAK binding to stainless steel by PK99H suggests that the C-terminal disulphide loop region of pilin, which contains an epithelial cell binding domain, may also function in mediating attachment to steel surfaces.
Synthetic peptide inhibition of binding to steel
Antibody inhibition assays suggested that the cellular receptor binding domain of the pilus may also mediate binding to stainless steel. Therefore, competitive binding assays were utilized to test the ability of the C-terminal receptor binding domain to inhibit adherence of P. aeruginosa to steel. Previous studies demonstrated that the native C-terminal receptor binding domain (PAK128–144ox) mediates binding to GalNAc-β-D-Gal containing glycoconjugates (Sheth et al., 1994). The PAK pilin receptor binding domain (PAK128–144ox) inhibited the binding of both PAK wild-type cells and PAK pili to steel surfaces with apparent Ki's of ∼4 nM and ∼0.2 nM respectively (Fig. 6A and C). PAK(128–144)ox also inhibited the binding of PAKMS591 (compare Fig. 2P with Fig. 2Q) but had no effect on the binding of PAKNP (compare Fig. 2M and N). The peptide PAK(134–140), which constitutes a portion of the receptor binding domain, and has been demonstrated to bind with low affinity to respiratory epithelial cells (Yu et al., 1996), did not inhibit binding of PAK wild-type cells or PAK pili to steel surfaces, even at the exceptionally high peptide concentration of 100 µg ml−1 (Fig. 6B and D), nor did it inhibit the binding of strains PAO, K122-4 or KB7, in contrast to peptide PAK(128–144)ox (Fig. 2). In addition, neither PAK(22–52), a peptide derived from the N-terminal α-helix (residues 1–58) which should be buried in the native pilus fibre, nor PAK(117–125), a peptide consisting of a portion of β-strands 3 and 4 which models of the pilus fibre suggest will be displayed on the fibre surface (Hazes et al., 2000) (see Table 1 for peptide sequences and Fig. 1B), had any effect, even at high concentrations, on the binding of PAK wild-type cells or PAK pili to steel surfaces (Fig. 6B and D), indicating that these regions do not participate in pilus-mediated binding.
Table 1. Synthetic peptides and peptide sequences employed or referred to in this study.
Peptides were synthesized by solid phase and are N-α-acetylated with a free carboxyl except for PAK(134–140) which was synthesized as the N-α-acetylated amide peptide due to its short length. Peptides with a formed disulphide bridge between cysteine 129 and 142 are identified by an ox.
To determine whether the ability to interact with steel surfaces was a general attribute of the C-terminal receptor binding domain or a specific property of the PAK receptor binding domain, the ability of the PAO receptor binding domain to inhibit binding was examined. The synthetic PAO receptor binding domain, PAO(128–144)ox was observed to inhibit pilus-mediated binding to stainless steel in a similar manner to the native PAK peptide (Fig. 6E). To further confirm the specific nature of the receptor binding domain's interaction with steel surfaces, two additional control peptides, a scrambled PAO receptor binding domain PAO(128-144)ox_Scrambled and a linear variant of that sequence where the two cysteine residues have been replaced by alanine residues to eliminate the disulphide bridge, PAO(128–144)C129A/C142A_Scrambled, were utilized to assess the relative importance of sequence versus amino acid composition. Neither scrambled sequence was able to inhibit binding of PAK wild-type cells or PAK pili to steel surfaces, even at very high peptide concentrations (Fig. 6B and D). As a further control, peptides obtained through the trypsinization of bovine serum albumin (BSA) were utilized to confirm that the inhibition of binding was sequence-specific and not a common property of peptides. No inhibition of adherence was observed for either PAK whole cells (data not shown) or PAK pili even at high peptide concentrations (Fig. 6G). A PAO receptor binding domain mutant, PAO(128–144)oxK130I which has high affinity for human buccal epithelial cells (BECs) (Fig. 7C) was unable to inhibit P. aeruginosa whole cells or pili adherence to steel (Fig. 6). To further determine whether the receptor binding domain inhibited binding to steel by a competitive mechanism or by interacting with P. aeruginosa cells or pili, the ability of PAK(128–144)ox to bind to stainless steel was determined using the monoclonal antibody PK99H as a probe of peptide binding to steel (PK99H has been demonstrated to bind to both PAK(128–144)ox and PAK(134–140) when these peptides are bound to a cell surface receptor) (Irvin et al., 1989; Yu et al., 1996). PAK(128–144)ox bound with high affinity to stainless steel while PAK(134–140) bound only marginally to the steel surface at very high concentrations (Fig. 7A and B).
As P. aeruginosa strains vary considerably in their ability to bind to steel surfaces (Fig. 2A, D, G and J), we sought to determine whether the PAK pilin receptor binding domain, PAK(128–144)ox, could inhibit the binding of other P. aeruginosa strains. Utilizing microscopy, we found that at very low concentrations (51 nM), PAK(128–144)ox substantially inhibits the binding of strains PAO, K122-4 and KB7 (compare Fig. 2D, G and J with Fig. 2E, H and K) while very high concentrations (100 µg ml−1) of PAK(134–140) have a minimal effect on binding to steel (compare Fig. 2A, D, G and J with Fig. 2C, F, I and L). The pilin receptor binding domain sequences of strains PAK, PAO, K122-4 and KB7 vary substantially (Fig. 1A and B, and Table 1), but all these receptor binding domains display a conserved antigenic epitope and compete for epithelial cell surface receptors (Sheth et al., 1995).
Binding to other abiotic surfaces
As type IV pili have been implicated in biofilm formation on polystyrene and polyvinylchloride surfaces, we sought to determine if the C-terminal receptor binding domain may function to mediate attachment to a variety of abiotic surfaces. PAK whole cells and pili were found to bind in a concentration-dependent and saturable manner to both polyvinylchloride and polystyrene plates (Fig. 8A–D). The murine monoclonal antibody PK99H significantly inhibited binding to both polyvinyl chloride and polystyrene surfaces (Fig. 8E and F). These data indicate that type IV pili mediate binding to these plastic surfaces which may be dependant on the C-terminal receptor binding domain.
We demonstrated that the initial binding of P. aeruginosa to stainless steel is concentration-dependent and exhibits classical saturation kinetics (Fig. 3). P. aeruginosa pili clearly play a major role in mediating whole cell binding to stainless steel as (i) pili-deficient strains are unable to adhere, (ii) pili bind to steel in a concentration-dependent, saturable manner, and (iii) pili competitively inhibit whole cell binding in a direct competition assay (Fig. 3).
Although Wozniak et al. (2003) demonstrated that alginate, the primary exopolysaccharide of P. aeruginosa, did not have a significant effect on the initial binding of Pseudomonas to abiotic surfaces, we have demonstrated that type IV pili are involved in the initial adherence. Therefore, while extracellular polysaccharide has long been proposed to play a major role in mature biofilms (Stoodley et al., 2002), type IV pili protein subunits may provide the initial attachment to abiotic surfaces (Figs 2 and 3). Evidence of an initial involvement of protein in biofilm formation on copper surfaces has been reported previously (Bremer and Geesey, 1991). Interestingly, a variety of proteins have the ability to mediate tight interactions with abiotic surfaces, including the Mytilus edulis foot proteins which are capable of mediating interactions with a variety of abiotic surfaces including metals and plastics (Suci and Geesey, 2001). A direct role for protein in mediating interactions with an abiotic surface, particularly a metal surface, is thus not without precedent.
While O’Toole and Kolter (1998) found that flagella play a significant role in biofilm formation, we found that P. aeruginosa lacking flagella yet expressing pili were able to bind to steel (Figs 2 and 4). In addition, any strain lacking the ability to assemble functional pili were unable to bind (Figs 2 and 4). The difference between our findings and those of O’Toole and Kolter (1998) may reflect the ability of bound cells to remain surface attached and differentiate into a microcolony, and subsequently a biofilm, as our data only report on events that occur within 1 h of a potential bacterial interaction with the surface.
To determine whether the C-terminal receptor binding domain of the pilus was responsible for adherence to stainless steel, as for immobilized BECs (Irvin et al., 1990; Schweizer et al., 1998), we employed monoclonal antibodies specific for residues in the C-terminal binding domain in a competitive inhibition assay. Monoclonal antibody PK99H recognizes residues 134–140 of PAK PilA (Wong et al., 1992), inhibits pilus-mediated binding to respiratory epithelial cells (Irvin et al., 1989), and confers protection from challenge with strain PAK in a mouse infection model (Sheth et al., 1995). PK99H inhibited pilus-mediated binding to stainless steel, indicating that the pili C-terminal receptor binding domain, residues 128–144 of PAK PilA, may specifically mediate the interaction with steel (Fig. 5).
To confirm that residues 128–144 were mediating the interaction between pili and steel, a variety of synthetic peptides were used in competitive inhibition assays. Strikingly, PAK(128–144)ox effectively inhibits the adherence of heterologous P. aeruginosa strains to stainless steel even at low concentrations (Fig. 2B, E, H and K), indicating that the ability to bind to steel through the C-terminal binding domain is conserved in all P. aeruginosa strains. The ability of the synthetic receptor binding domain, PAO(128–144)ox, to inhibit the binding of both PAK cells and pili to steel further supports our hypothesis that the C-terminal pilin receptor binding domain of the various pilins mediates binding to steel in addition to mediating binding to human respiratory epithelial cells.
Peptides with limited affinity for steel have been identified by phage display methodology and their affinity for steel has been correlated to their amino acid composition (Zuo et al., 2005). The interaction of the receptor binding domain with steel is not simply a function of the peptide amino acid composition as two scrambled sequences of the PAO receptor binding domain (one retaining the disulphide bridge and the other a linear variant where the two cysteine residues are replaced with alanine residues) failed to inhibit binding to steel (Fig. 6B and D). The PilA receptor binding domain binds to steel with high affinity in a sequence-specific manner, indicating that binding is likely dependent upon both the sequence and three dimensional structure of the peptide rather than upon the amino acid composition. The steel binding function is sequence-specific as PAO(128–144)oxK130I failed to inhibit binding to steel even though the affinity of this peptide for human BECs was enhanced (compare Fig. 6F with Fig. 7C). This observation suggests that the ability to bind to steel and human epithelial cells can be differentiated, indeed, the short synthetic peptide PAK(134–140) which has previously been demonstrated to have a low affinity for human BECs (Yu et al., 1996) did not inhibit binding to steel (Fig. 2). These results indicate that the two binding functions are readily differentiated by a single point mutation, suggesting that the molecular basis of the interaction with steel and epithelial cells is quite distinct, although both are dependent on the C-terminal receptor binding domain.
As type IV pili have also been implicated in biofilm formation on plastic surfaces, the ability of the PilA receptor binding domain to mediate adherence to two widely used plastics, polyvinylchloride and polystyrene, was examined. Direct binding assays demonstrate that PAK whole cells and pili adhere to plastics in a concentration-dependent and saturable manner (Fig. 8). As well, the monoclonal antibody PK99H was able to inhibit P. aeruginosa binding to both polyvinylchloride and polystyrene plates (Fig. 8). These data suggest that the C-terminal receptor binding domain is involved not only in adherence to stainless steel and BECs, but also to other abiotic substrates including plastics.
The PilA C-terminal receptor binding domain, displayed at the tip of the type IV pilus, mediates direct binding to both biotic and abiotic surfaces. Although the pilus is able to bind both substrates, the affinities differ by several orders of magnitude. However, as the single point mutation in the C-terminal receptor binding domain increased the affinity for BECs, it abolished the affinity for stainless steel. This supports our hypothesis that the receptor binding domain has retained sequence and structural elements required for adherence to a variety of surfaces. Therefore, we have determined that the C-terminal receptor binding domain is responsible for adherence to stainless steel and although the sequence varies widely between strains, attachment via this C-terminal receptor binding domain is a conserved function of the type IV pilus.
Bacterial strains, DNA and antibody sources
The P. aeruginosa strains used in this study were PAK, PAK 2Pfs (Bradley and Pitt, 1974), PAK-BΩ, a 2 kBΩ fragment containing a transcriptional terminator from pHP45 was inserted into the pilB gene, PAK-DΩ, the same transcriptional terminator was inserted into the pilD gene (Koga et al., 1993), PAKMS591, the gentamycin cassette from a pPC110 was inserted into the fliC gene (Starnbach and Lory, 1992), PAKNP the tetracycline cassette from pB322 was inserted into the pilA gene (Saiman et al., 1990), K122-4, a clinical isolate from a cystic fibrosis patient in Toronto which possesses both pili and flagella (Pasloske et al., 1988) and KB7, an isolate containing both pili and flagella (Wong et al., 1995). Several of these strains were generously provided by Dr Jessica Boyd (NRC Institute for Marine Biosciences, Halifax, Nova Scotia). The strain PAK 2Pfs, a multipiliated retraction-deficient strain, was used for the purification of pili only and not used in experimental conditions. The phenotypes of the P. aeruginosa strains with respect to expression of pili was experimentally verified by Western blotting with anti-PAK pilus-specific antisera and by direct ELISA with whole cells and heat inactivated whole cells (to determine the presence of surface-exposed pili), by the sensitivity to type IV pilus-specific phage, and by monitoring the twitching motility of the strains. P. aeruginosa was routinely grown at 37°C in Luria–Bertani broth (LB) or LB supplemented with 50 µg ml−1 tetracycline (Sigma) for PAKNP, 100 µg ml−1 of gentamycin for PAKMS591, or 50 µg ml−1 of streptomycin for strains PAK-BΩ and PAK-DΩ. The polyclonal antibodies generated against the PAK pili and associated pre-immune antisera used in this study have been reported previously (Paranchych et al., 1979).
Biotinylation of P. aeruginosa cells and purified pili
Biotinylation of bacteria was performed as previously described by Yu et al. (1996) with the following modifications. Harvested cells were suspended in 5 ml of phosphate buffered saline (PBS) (pH 6.8) with 75 µl of 20 mg ml−1 biotinamidocaproate N-α-hydroxysuccinimidyl ester dissolved in dimethylsulfoxide and incubated at 22°C with agitation (200 rpm) in a water bath shaker for 1 h. Cells were harvested by centrifugation (10 000 g for 10 min at 4°C) and washed four times before resuspension in 1.0 ml PBS, pH 6.8. Viable counts were performed before and after biotinylation. PAK pili were purified from PAK 2Pfs as described previously (Paranchych et al., 1979). The purity and integrity of the pili were assessed by 15% SDS-PAGE (Sambrook et al., 1989) and electron microscopy (Fig. 1C and F). The procedure used for the biotinylation of the purified pili has been previously described (Yu et al., 1996). The ability of the biotinylated pili to bind to asialo-GM1 and GM1 was determined as previously described (Lee et al., 1994) and the binding specificity for asialo-GM1 was confirmed to establish the functional binding activity of the pili following biotinylation.
Stainless steel binding assay
Grade 304 stainless steel 2B finish plates (20 gauge – 1 mm thick and 7.6 × 11.5 cm) were washed in 95% ethanol for 10 min, and rinsed with distilled water. Immediately before the binding studies, coupons were washed with 20 ml of acetone for 1 min with gentle agitation and rinsed with distilled water. Coupons were then assembled into a Schleicher and Schuell MinifoldTM System (Mandel Scientific). Biotinylated viable PAK cells or purified PAK pili (biotinylated or unbiotinylated) were added (100 µl per well in replicates of six) to the stainless steel manifold and incubated at 37°C for 1 h with gentle agitation. The manifold was subsequently washed five times with 250 µl per well Buffer A (PBS pH 7.4 containing 0.05% BSA). Binding was assessed using either streptavidin-horseradish peroxidase (HRP) or polyclonal PAK antibodies and secondary goat-anti-rabbit HRP (Bio-Rad). Substrate buffer (0.01 M sodium citrate buffer pH 4.2 containing 1 mM 2,2′-Azino-bis-(3-ethylbenzthiazoline-6-sulfonic acid) diammonium salt (ABTS) (Sigma) and 0.03% (v/v) hydrogen peroxide) was added (125 µl per well) and the manifolds were incubated at room temperature (RT) for 10 min with shaking at 150 rpm. The absorbance was determined at 405 nm using a Multiskan Plus version 2.01 plate reader following transfer of the reaction solution to 96 well flat-bottomed micro titer plates (Corning).
Buccal epithelial cell assay
Buccal epithelial cell assay was completed as described by McEachran and Irvin (1985), with the following modifications. Corning 24 well tissue culture treated ELISA plates were incubated with 500 µl of a 1 µg ml−1 poly L-lysine solution at 75°C overnight before washing for 15 min with PBS three times. Gluteraldehyde (25%, 125 µl per well) was incubated for 1 h at 37°C. Wells were washed as previously stated. BECs, harvested from 10 healthy volunteers, were filtered through a fine (70 µl) nylon mesh (Spectrum) and added to the prepared ELISA plate for overnight fixation at 37°C. Binding studies were performed as noted above.
Antibody inhibition studies
Biotinylated viable PAK whole cells or biotinylated purified PAK pili were mixed with 50 µl of a 10−2 dilution of pilus-specific antibody (note that all antibodies were initially set to the same titer via an ELISA employing purified pili as an antigen) or pre-immune rabbit sera in PBS buffer, pH 7.4, with a vortex mixer and incubated for 1 h at 37°C. The cell or pili mixture was utilized for binding assays as previously described (Yu et al., 1996). Concentrations of biotinylated PAK cells or biotinylated PAK pili ranged from 0 to 3.0 × 1016 cfu ml−1 and 0 to 1.5 µg ml−1 respectively. The steel surface was washed five times with Buffer A, incubated with 100 µl of either a rabbit anti-IgG HRP, for the polyclonal antibody or mouse anti-IgG HRP for the monoclonal antibodies. After an 1 h incubation at 37°C, the steel surface was washed as described, and ABTS substrate solution (125 µl per well) was added for 15 min. The two pilus-specific antibodies used in this study, a polyclonal anti-PAK pili antibody (Lee et al., 1989) and monoclonal antibody PK99H (Doig et al., 1990), have been previously described. Rabbit pre-immune serum, which had previously been determined to be free of anti-P. aeruginosa antibodies by ELISA, was utilized as a control.
Peptide synthesis and competitive peptide inhibition assays
The peptides described in Table 1 were synthesized as the N-α-acetylated free carboxyl form, except for PAK(134–140) which was synthesized as the N-α-acetylated and C-terminal amide form, by solid-phase peptide synthesis and purified by reversed-phase high-performance liquid chromatography (HPLC) as previously reported (Wong et al., 1992; Wong et al., 1995). Peptides containing two cysteine residues were air-oxidized to generate the disulphide bridged form of the peptide with disulphide formation being experimentally confirmed (Campbell et al., 1995). Synthetic peptides PAK(128–144)ox, PAK(117–125), PAK(134–140), PAO(128–144)ox, PAK(128–144)oxK130I, PAO(128–144)ox_Scrambled and PAO(128–144)C129A/C142A_Scrambled were dissolved in Buffer A and incubated with either 1015 cfu ml−1 biotinylated viable PAKwt cells or 0.75 µg ml−1 of biotinylated purified PAK pili such that the final peptide concentration ranged from 51 nM to 51 µM. The samples were then utilized directly in a steel surface binding assay as described above.
Trypsinized BSA peptides
Bovine serum albumin (BSA) (Biotech grade Fisher) was dissolved in PBS pH 7.4, and heat denatured by boiling in a water bath for 1 h. Trypsin (50 µl of a 1 mg ml−1 solution) was then added to a 10 mg ml−1 heat denatured BSA solution and incubated at RT overnight with gentle agitation. Trypsin was heat inactivated via boiling water bath for 1 h before use in competitive peptide inhibition assays as listed above.
Direct binding of peptides to steel
To confirm that the pilin receptor binding domain was directly interacting with the steel surface rather than indirectly inhibiting cell or pilus binding to steel, direct binding of the synthetic receptor binding domain was assessed. The binding of the synthetic peptides to steel was determined by a modified immunoassay that has been previously described (Yu et al., 1996). Synthetic peptides PAK(128–144)ox and PAK(134–140) were prepared in Buffer A (0–51 µM). The peptides were then added directly to wells (100 µl per well in replicates of six) formed on the steel surface and incubated for 1 h at 37°C without agitation. Following five washes with Buffer A (250 µl per well), a 1:5000 dilution of PK99H was added to each well (100 µl per well) and incubated for 1 h, and washed as described. Secondary antibody Goat anti Rabbit IgG HRP (100 µl per well of a 1:3000 dilution) was added and again incubated for 1 h. ABTS substrate solution was added (125 µl per well) and allowed to incubate for 25 min before the absorbance at 405 nm was determined as described.
Acridine orange staining and microscopy
Stainless steel plates, prepared and utilized in bacterial binding studies as described above, were incubated in 1 mM Acridine Orange stain for 1 min, and thoroughly rinsed with distilled water. Coupons were visualized using a Leitz laborlux K microscope equipped with a MSP4 camera, and 40× Neoflour lens with epifluorescent illumination. Micrographs were recorded with Kodak Colormax 35 mm film, processed and digitally scanned immediately after film processing.
This work was supported by an operating grant from the Canadian Institutes for Health Research (MOP-38004) and an RGPIN-Discovery Grant from the Natural Sciences and Engineering Research Council of Canada (to R.T.I) and by Public Health Service Grants grant from the National Institutes of Health (D.J.H., AI-40541, GM-69845, and RSH, AI-48717) and Cystic Fibrosis Foundation (HASSET03P0, D.J.H). The generosity of Jessica Boyd in the provision of some of the strains used in this study is gratefully acknowledged.