Phage, bacterial strains and media

Phage φ15 and P. putida strains (PpN, PpN3, PpN119, Pput 373, AC522, DSM9278 and PpG1) were isolated as described in Shaburova et al. [25]. PpKT2440 and Pp00S82 were kindly provided by Prof. D. Springael (Division Soil and Water Management, K.U.Leuven, Belgium) and five other P. putida strains (PSE072, PSE072B, PSE106, PSE107 and WGE060) were obtained from Prof. M. Vaneechoutte (Laboratory Bacteriology, Ghent University Hospital, Belgium). Prof. R. De Mot (Centre of Microbial and Plant Genetics, K.U.Leuven, Belgium) provided P. putida strains ATCC23287, GR12-2R3, LMG2257 and a selection of 35 P. putida rice rizosphere strains [27]. P. putida strains were grown in standard LB-medium at 30°C. Expression strain E. coli BL21(DE3) pLysS (Invitrogen Corporation, Carlsbad, CA, USA) was grown at 30°C in 2xTY-medium.

Phage purification

The CsCl ultracentrifugation method was performed as described by Ceyssens et al. [28]. For purification and concentration by Convective Interactive Media (CIM), the diethylamine (DEAE) CIM® disk monolithic column (12 mm×3 mm i.d., bed volume 0.34 ml; BIA Separations, Ljubljana, Slovenia) was used in combination with the Äkta FPLC-system (GE Healthcare, Little Chalfont, UK) and UNICORN™ 5.01 software in a 20 mM Tris buffer system at pH 7.5. The equilibration buffer with 1 M added sodium chloride was used for elution. Shortly, an overnight culture of a susceptible host strain was used to prepare a 2% inoculum, which was incubated with shaking at 30°C. At OD_{600 nm} of 0.45, phage (10⁶ pfu to a 50 ml culture) were added to the culture and incubation continued until lysis was observed. The bacterial lysate was subsequently centrifuged (3,000× g, 30 min, 4°C), passed through a 0.45 µm pore-size membrane filter (Millipore Corporation, Billerica, MA, USA) and adjusted (with HCl or NaOH) to the pH of the buffer system. This cleared, filtered lysate was used as the starting material for phage purification by CIM. In a stepwise gradient profile (20, 30, 100% and 3 ml segment lengths) to the Tris buffer containing 1 M NaCl, the major part of the bound phage were eluted at 30% elution buffer. The DEAE disk, with a capacity of ∼8*10¹⁰ pfu for phage φ15 can purify up to ∼7*10¹⁰ phage particles.

Microbiological characteristics

One-step growth curves of phage φ15 were made for two P. putida strains, PpG1 and RD5PR2 [29]. In short, 5 min after infection of a 1 ml P. putida culture (OD_{600 nm} = 0.45) at a start pfu/CFU ratio of 0.008, the suspension was washed (1 min centrifugation at 16.060× g, followed by resuspension of the pellet in 1 ml LB, prewarmed at 30°C) twice and 10⁻⁴ and 10⁻⁵ dilutions were incubated at 30°C. Samples were taken at regular intervals and titrated immediately using the double agar overlay method. For the adsorption experiments [29], infection parameters of the one-step growth experiments were maintained. At 1 min-time intervals, 100 µl samples were taken from the solution and mixed with 850 µl LB-media and 50 µl CHCl₃. After 10 min of shaking, the supernatant is titrated to determine the number of non-adsorbed or reversibly adsorbed phage.

The pH-stability of the phage was tested by incubating at room temperature 10⁸ pfu in 1 ml of a pH-buffer constituting of 10 mM KH₂PO₄, 10 mM NaCitrate, 10 mM Boric Acid and 150 mM KCl (pH-adjusted with NaOH or HCl to a pH within the pH-range of 1 to 13). Each sample was titrated after a 24 h exposure using the standard double agar overlay method [29], and compared with control samples [10⁸ pfu in a 1 ml standard phage buffer (10 mM MgSO₄, 150 mM NaCl, 10 mM Tris pH 7.5) also incubated at room temperature for 24 h].

All phage-host combinations were evaluated by spot testing 10⁷ pfu on a air-dried bacterial lawn (200 µl overnight culture plated directly on LB agar plates) in three independent experiments. After overnight incubation at 30°C, plates were checked for the presence of a lysis zone against a negative, uninfected control.

To visualize halo formation, 10 µl of a 10⁸ pfu phage suspension was dropped on a air-dried bacterial lawn (200 µl overnight culture), plated on LB agar. Plates were sealed and incubated at 30°C. For comparison of phage and bacterial count in the three different zones (lysis, halo and bacterial zone), a equally large surface was removed from each zone, suspended in 1 ml LB-medium and vortexed (30 s). Phage counts were determined using the double agar method, while bacterial numbers were counted after plating a dilution series of the supernatant.

Development of phage resistant strains and UV inactivation of phage particles

200 µl of a bacterial overnight culture was plated on a petri dish with solid LB medium. After drying, 10 µl of 10⁸ pfu/ml of a φ15 phage suspension was dropped on this plate, which was sealed after drying and incubated at 30°C until colonies became visible in the lysis zone. Colonies were picked and subjected to single-colony isolation three times. The double agar overlay method was used to verify resistance to phage φ15 of the different selected colonies.

The UV oven (Bio-Link, Vilber Lourmat, France) was equipped with five fluorescent lamps of 8 W each, emitting 180 to 280 nm with a peak at 254 nm. The distance between the lamps and the plates was 14 cm. The UV doses were programmed and controlled by a radiometer which constantly monitors the UV light emission. To inactivate phage particles by UV illumination, 25 µl of phage (10¹¹ pfu/ml) was dropped on an empty petri dish and irradiated in the UV oven (1 kJ/m²).

Capsule staining

Bacterial cells, scraped from a fully grown agar plate, were transferred to a 10 µl drop of 1% aqueous Congo red solution (Sigma-Aldrich, St. Louis, MO, USA). This suspension was spread across a microscopic glass slide to form a thin film, which was air-dried. A 10 µl drop of Maneval's solution [3.33% fenol, 4.44% glacial acetic acid, 2.67% ferric chloride, 0.02% acid fuchsin (Sigma-Aldrich)], distributed across the slide, acidifies the Congo red background into blue [30] and colors cells red. Capsules are not stained and appear white underneath the light-microscope (100×, oil; Leica DM LB microscope; Mc Bain instruments, Simi Valley, CA, USA).

Biofilm assay

The device used for biofilm formation is a platform of 96 polystyrene pegs (Nunc-Immuno TSP, Thermo Fischer Scientific, Tournai, Belgium) that fits as a microtiter plate lid with a peg hanging in each microtiter plate well (Thermo Fischer Scientific) [31]. Overnight cultures were diluted 1/200 in LB-medium in the 96 wells of the microtiter plate. After hanging the pegs in the wells, the microtiter plate was sealed to avoid water loss due to evaporation. Biofilms were allowed to grow for different periods of times at 30°C without shaking. For biofilm growth assays longer than 24 h, media were renewed every 24 h by placing the pegs in a new microtiter plate containing media. For quantitative biofilm analysis, the pegs were washed once in 200 µl LB-medium. The remaining attached bacteria were stained with 200 µl 0.1% (w/v) crystal violet (Merck) in an isopropanol-methanol-PBS solution [1∶1∶18 (v/v)] for 30 min, washed with LB-medium to remove excess stain and air-dried (30 min). Afterwards, the dye bound to the adhered cells was extracted in 200 µl 30% glacial acetic acid. The intensity of the eluted dye in each well was measured at OD_{600 nm} with the Multiskan RC (Thermo Labsystems, Finland). The planktonic survival was determined simultaneously by an optical density measurement (600 nm; Multiskan RC) of 135 µl supernatant removed from the microtiter plate in which the pegs were hanging. Differences in biofilm and planktonic survival compared to the untreated control samples were analyzed using the two-tailed t test, P-values of <0.01 were considered significant.

Cloning, recombinant expression and purification

Purified genomic φ15 DNA served as template for amplification of gene 17 using Pfu DNA polymerase (Fermentas Life Science) and the specific primer pair (5′-ATGGCACGAACTATCGTC-3′ and 5′-CTACCCGACCAGCTCGATCAG-3′; Eurogentec, Seraing, Belgium). The PCR product was cloned in the pEXP5-NT/TOPO® TA expression vector (Invitrogen Corporation) according to the manufacturer's protocol in order to obtain a 6xHis-tag fusion protein for purification. The construct was verified by DNA sequencing using vector-specific primers (5′-TAATACGACTCACTATAGGG-3′ and 5′-TAGTTATTGCTCAGCGGTGG-3′, Eurogentec) and an internal primer (5′-ACGTGGTGTCATCAAC-3′, Eurogentec). Expression occurred at 37°C for 4 h in E. coli BL21(DE3)pLysS (Invitrogen Corporation) after induction with 0.1 mM isopropyl-β-D-thiogalactopyranoside of 0.5 L exponentially growing cells (OD_{600 nm} = 0.6) in 2xTY medium. Protein purification was essentially performed as described previously [32] with a HisTrap™ HP 1 ml column (Amersham Biosciences) in combination with an Äkta FPLC-system (GE Healthcare) and UNICORN™ 5.01 software. Wash and elution buffers were composed of 20 mM NaH₂PO₄ pH 8.5, 0.5 M NaCl and 10% glycerol with 75 mM and 0.5 M imidazole, respectively. Protein purity was at least 95% as estimated by SDS-PAGE. Purified protein was dialyzed overnight against a volume of PBS buffer (137 mM NaCl, 2.7 mM KCl, 10 mM NaHPO₄, 2 mM KH₂PO₄ pH 7.4) that was 1000× the volume of the protein sample using Slide-A-Lyzer® MINI Dialysis units (Pierce Biotechnology, Rockford, IL, USA).

Microbiological characteristics

Bacteriophage φ15 propagates on P. putida strain PpG1 and infects six other strains (PpN, PpN3, RD6PR1, RD5PR2, RD8PR2 and RD8PR3) from a diverse collection of 53 P. putida strains. These seven P. putida strains show very diverse biofilm forming capacities, ranging from a very weak to a moderate biofilm formation (Figure S1). None of the phage-sensitive strains forms thick biofilms.

Transmission electron microscopic imaging revealed φ15 as a typical short tailed member of the Podoviridae family of double-stranded DNA bacteriophages (58.9 nm head; 12×8 nm tails) (Figure S2). Phage φ15 is stable in a relatively narrow pH range (5 to 11) (Figure S3A). The phage exhibits a very efficient infection cycle on its host PpG1: 95.2% of φ15 phage particles are irreversible adsorbed (k = 2.51*10⁻⁸) within the first minute after infection of a bacterial culture (Figure S3B). PpG1 host cells are lysed after 21 min, releasing an average of 95 newly formed phage particles per cell (Figure S3C). However, under the same laboratory conditions, φ15 exhibited a remarkably lower adsorption to strain RD5PR2 (17.38% adsorbed phage particles after 1 min; k = 2.23*10⁻⁹) (Figure S3B). As a consequence, lysis of RD5PR2 cells occurred unsynchronized, which was observed by a gradual release of phage particles starting 90 min post infection (Figure S3D).

The large (5-mm diameter) and clear plaque morphology of φ15 hints a strictly lytic nature. The most distinct plaque feature is the opaque halo zone with an increasing diameter over the course of time, surrounding a plaque with constant diameter (Figure 1). When 10⁸ pfu of phage were dropped on a lawn of host bacteria, the lysis zone caused by infection and subsequent lysis of host cells, kept a constant diameter with prolonged incubation. The halo zone increased up to 3 mm in diameter every 24 h and eventually spread across the whole petri dish. An opaque halo zone surrounding the plaque was observed for each of the seven strains (PpG1, PpN, PpN3, RD6PR1, RD5PR2, RD8PR2, RD8PR3) out of the collection of 53 P. putida strains sensitive for φ15 infection. A halo zone was not observed when phage were dropped on a bacterial lawn resistant to infection, coupling phage sensitivity and halo formation. Phage enumeration of equally large surfaces of the lysis, halo and bacterial zones outside the halo revealed that only a tenfold less phage were found in the halo zone (1.6*10⁶ pfu) compared to the lysis zone (1.9*10⁷ pfu), while phage were completely absent in the outside bacterial zone. A bacterial count of the same samples indicated the absence of viable bacterial cells within the lysis zone, except for the one or two resistant colonies. The halo and the outside bacterial zone harbored an almost equal amount of viable cells (4.56*10⁷ and 4.43*10⁷ CFU, respectively).

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Figure 1. Plaques of P. putida phage φ15 on the host PpG1.

With increasing time of incubation the diameter of the halo zone, surrounding the plaque with constant diameter, increases up to 3 mm every 24 h.

https://doi.org/10.1371/journal.pone.0018597.g001

Phage-mediated biofilm degradation

Phage-mediated biofilm degradation was evaluated for phage φ15 on 24 h and 48 h old single-species biofilms of two P. putida strains PpG1 and RD5PR2, grown under static conditions at 30°C. Infection parameters were varied to determine the most optimal biofilm degradation conditions: time periods for phage infection ranged from 2 to 24 h and the applied phage titers were 10², 10⁴ and 10⁶ pfu/well.

Biofilm degradation of PpG1 biofilms.

A time and dose dependent biofilm degradation is observed for φ15 infection of PpG1 biofilms initially grown for 24 h. A maximal biofilm reduction was reached 8 h after each phage dose was added (e.g. 96% for initially 10⁶ pfu added) (Figure 2A). The planktonic survival decreased in parallel, but more rapidly than the biofilm degradation. Only 2 h after phage exposure, the planktonic survival decreased to 32 and 11% for 10⁴ and 10⁶ pfu of φ15, respectively. The maximum of planktonic decrease was reached already 4 h after addition of the higher phage doses (10⁴ and 10⁶ pfu) and after 8 h for initially 10² phage particles added.

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Figure 2. Phage φ15-mediated biofilm degradation.

24 h (A) and 48 h (B) old biofilm of PpG1. 24 h (C) and 48 h (D) old biofilm of RD5PR2. Biofilms grown on cones for 24 or 48 h, were initially inoculated with 10², 10⁴ and 10⁶ pfu of phage φ15. After 2, 4, 8 and 24 h of phage treatment at 30°C, mean biofilm (BT: biofilm treatment) and planktonic survival (PCT: planktonic culture treatment) for n = 20 cones or corresponding microtiter plate wells, respectively, were scored relative to untreated control samples (100%) and represented on the Y-axes. Five independent experiments were performed, each starting from a different overnight culture and each with four repeats for each parameter combination giving rise to an overall twentyfold repetition. Error bars indicate SEM. Significant values (two-tailed t test; P<0.01) are marked by a asterisk (*).

https://doi.org/10.1371/journal.pone.0018597.g002

Despite this dose and time responsive behavior, phage counts within the planktonic culture rapidly attained the steady state level of about 7.5 log₁₀ for every initial phage titer added (Figure 3A). Even for only a hundred phage particles added, the maximum phage count (±7.5 log₁₀) was already reached after 4 h, at which point also a sharp decrease in planktonic survival (from 128 to 42%) was observed. Surprisingly, biofilm degradation lagged at least 2 h behind, as a sharp increase in biofilm degradation was only observed between 4 and 8 h (11 to 69%) after initial infection. Similar observations were made for higher initial phage titers: the plateau level of phage count was already reached after 2 h at which point the biofilm degradation was still limited to ±11%. A possible explanation is that free living planktonic cells are easier accessible for phage infection than cells associated within and protected by a biofilm environment. Cells within a biofilm environment are also much less metabolic active, hereby slowing down the infection process, and coupled biofilm destruction.

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Figure 3. Phage amplification.

24 h (A) and 48 h (B) old biofilm of PpG1. 24 h (C) and 48 h (D) old biofilm of RD5PR2. Biofilms grown on cones for 24 or 48 h, were initially inoculated with 10², 10⁴ and 10⁶ pfu of phage φ15. After 2, 4, 8 and 24 h of phage treatment with 10², 10⁴ and 10⁶ pfu of phage φ15 at 30°C, mean phage counts recovered from liquid media in n = 4 microtiter plate wells [log₁₀(phage titer)] were scored. Error bars indicate SEM.

https://doi.org/10.1371/journal.pone.0018597.g003

Although also being time and dose dependent, at every time point the measured biofilm degradation and planktonic killing of the 48 h old biofilm were much lower than for the 24 h old biofilm (Figure 2A+B). Like for the 24 h old biofilm, a maximal degradation was reached for the higher phage doses after 8 h, but only 38 and 55% of the biofilm was degraded compared to 87 and 96% for the 24 h old biofilm after initial inoculation with 10⁴ and 10⁶ phage, respectively. When the 48 h grown biofilm was inoculated with only 10² pfu of φ15, no significant biofilm degradation was observed during the 24 h incubation period, in contrast with a maximal biofilm degradation of 69% reached after 8 h for the 24 h old biofilm. In parallel, we noticed higher planktonic survival rates for 48 h old biofilms: as these older biofilms slowly decay, biofilm-freed cells hereby continuously enrich the planktonic culture. Nevertheless, phage amplification occurred as rapidly as observed for the 24 h old biofilm, reaching steady-state values of about 7.5 log₁₀ at the earlier time points for every initial phage titer applied (Figure 3A+B). A gradual biofilm and planktonic regrowth was observed 24 h after phage exposure for the different phage inoculation titers (except for 10⁶ phage added to the 24 h old biofilm) for both the 24 h and 48 h pregrown biofilm implying bacterial resistance development against phage infection.

Identification of the φ15 tail spike protein by genome analysis

Genome sequencing of φ15 revealed a typical T7-like genome, comprising 39,562 bp and bracketed by 264 bp direct terminal repeats. The genome contains 50 predicted ORFs, all orientated in the same direction and leaving only 6.3% of the genome noncoding. It can be functionally divided into three regions involved in (i) host conversion, (ii) nucleotide metabolism and DNA replication, and (iii) morphogenesis and host cell lysis (Figure S4 and Table S1). With a overall G+C average of 58.2%, the highest of all ‘T7-like viruses’, φ15 approaches the high G+C content (61%) of its host. No tRNA genes were predicted, as expected for a member of the ‘T7-like viruses’.

The entire φ15 genome has 55.5% overall DNA similarity to its closest T7-homolog, the P. putida phage gh-1 [33] and shares 34 out of 50 φ15 ORFs with this phage. While 28 ORFs are typical for ‘T7-like viruses’, six ORFs are unique to φ15 and gh-1 and probably result from adaptation to the P. putida host. Five of these genes are encoded in the DNA replication region, while the particle structure genes are highly conserved. Fifteen other ORFs (except φ15/16), unique for φ15 and located in the early and middle region, probably represent a further adaptation to a particular group of P. putida strains. Using ESI-MS/MS analysis on purified and denatured phage particles, fourteen structural phage proteins were identified (Table S2). This analysis delineated the structural region from 6.7 to 17 and identified also two early and two middle gene products as being part of the structural phage particle. A detailed discussion of the φ15 genome is provided in the supplementary data (Text S1, Table S3, Table S4, Figure S5). Based on the genome sequence, a T7-like infection cycle can be predicted for φ15.

Tail spike protein

For most ‘T7-like viruses’ (T3, T7, φA1122, φYeO3-12 and gh-1), the viral tail spike (Gp17) recognizes and adsorbs to specific sugars of the host lipopolysaccharide (LPS) [34], [35]. For example, φYeO3-12 is specific for the O3 antigen of Yersinia enterocolitica, T3 binds to glucose residues in the outer core of rough E. coli strains, while T7 binds to more inner moieties. In contrast, E. coli K1 phage K1F encodes a tail-associated endosialidase which recognizes and depolymerizes the K1 polysialic acid capsule instead of LPS structures [36]. Within the classified ‘T7-like viruses’, a conserved N-terminal head-binding domain is present, which is reasonably similar in length (±149 AA) and necessary for association with the tail structure (Figure 4) [37]. Gp17 of φ15 (728 AA) shares a 49.7% amino-acid identity in this N-terminal region with gh-1, while the C-terminal two-third of the tail spike is only 18.3% homologous. Also for other members of the ‘T7-like viruses’, these C-termini differ markedly in amino-acid sequence and length. They form the distal part of the tail spike protein and are involved in recognition of and binding to the host cell receptor.

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Figure 4. ClustalW alignment of the conserved N-terminal domain of the tail spike proteins (Gp17) of all classified ‘T7-like viruses’.

Identical residues are marked in black and similar residues are shaded in two different gray scales, the darker gray marking the higher chemical and physical similarity. Numbering starts at the N-terminal methionine. Gaps, indicated by horizontal lines, were introduced into the sequences to maximize the alignment.

https://doi.org/10.1371/journal.pone.0018597.g004

It was expected that the φ15 tail spike (Gp17) serves EPS degrading activity. However, homology on the level of the primary amino-acid sequence (BlastP) is limited to the conserved N-terminal domain of the ‘T7-like viruses’. Further analysis of Gp17 of φ15 using Phyre [38] indicated that there is a significant chance (75%) that Gp17 of φ15 has right-handed β-helical folds, similar to pectin lyases (E-value 0.77). These right-handed β-helical structural elements were so far only identified in carbohydrate binding (and depolymerizing) enzymes of microbial or viral origin and in an autotransporter family of secreted bacterial proteins [39]. Large-scale recombinant expression of the 80 kDa φ15 tail spike protein allowed purification of low yet pure amounts of this protein. Dropping 10 µl of this solution in parallel with a 10⁸ pfu phage suspension on a bacterial PpG1 lawn confirmed the presence of the EPS degrading activity within the tail spike protein of φ15, as the recombinantly purified tail spikes formed identical looking opaque halo zones as those found around the lytic zone caused by phage infection. Further microscopical analysis of these halo zones and the outside bacterial zone clearly shows that the EPS material keeps bacteria closely associated within small cell clusters. In contrast, virtually all bacteria within the halo zone are separated from each other, their EPS material is reduced and sometimes completely removed (Figure 5).

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Figure 5. Capsule staining of bacteria in the outside bacterial (A) and in the halo (B) zone.

Within the outside bacterial zone bacteria are all encircled by white capsule and packed closely together, while in the halo zone bacteria are lying separately and have sometimes lost their white capsule.

https://doi.org/10.1371/journal.pone.0018597.g005

Role of the viral tail spike in biofilm degradation

To differentiate between the individual contributions of φ15 in bacterial cell lysis and EPS depolymerization to biofilm degradation, we attempted to isolate PpG1 strains which are resistant to phage infection, but susceptible for halo formation. However, all of twelve infection resistant strains were also resistant for halo formation. This observation indicates that, although resistance development can occur through various mechanisms (deletion or mutation of receptor sites, host DNases, …), modification or loss of the EPS receptor must be the most straightforward. This again suggest that the EPS receptor is probably a primary and essential receptor for φ15 infection, as supported by the specific host range of the phage.

In a last step, phage φ15 particles were inactivated by UV radiation mutagenesis, which rendered the particle non-infective but left the enzymatic activity of viral tail spike proteins unharmed. When these particles were dropped onto a bacterial lawn, an opaque halo zone appeared after overnight incubation at 30°C. Further capsule staining of bacteria isolated from these halo zones confirmed the individual arrangement of cells within these zones. Finally, addition of UV inactivated particles (10², 10⁴ and 10⁶ pfu) to 24 h old PpG1 and RD5PR2 biofilms did not influence the pregrown biofilm at the different time points measured after inoculation (2, 4, 8 and 24 h; data not shown).