Abstract
The Gram-positive and spore-forming bacterium Brevibacillus laterosporus (Bl) belongs to the Brevibacillus brevis phylogenetic cluster. Isolates of the species have demonstrated pesticidal potency against a wide range of invertebrate pests and plant diseases. Two New Zealand isolates, Bl 1821L and Bl 1951, are under development as biopesticides for control of diamondback moth and other pests. However, due to the often-restricted growth of these endemic isolates, production can be an issue. Based on the previous work, it was hypothesised that the putative phages might be involved. During investigations of the cause of the disrupted growth, electron micrographs of crude lysate of Bl 1821L showed the presence of phages’ tail-like structures. A soft agar overlay method with PEG 8000 precipitation was used to differentiate between the antagonistic activity of the putative phage and phage tail-like structures (bacteriocins). Assay tests authenticated the absence of putative phage activity. Using the same method, broad-spectrum antibacterial activity of Bl 1821L lysate against several Gram-positive bacteria was found. SDS-PAGE of sucrose density gradient purified and 10 kD MWCO concentrated lysate showed a prominent protein band of ~48 kD, and transmission electron microscopy revealed the presence of polysheath-like structures. N-terminal sequencing of the ~48 kD protein mapped to a gene with weak predicted amino acid homology to a Bacillus PBSX phage-like element xkdK, the translated product of which shared >90% amino acid similarity to the phage tail-sheath protein of another Bl published genome, LMG15441. Bioinformatic analysis also identified an xkdK homolog in the Bl 1951 genome. However, genome comparison of the region around the xkdK gene between Bl 1821L and Bl 1951 found differences including two glycine rich protein encoding genes which contain imperfect repeats (1700 bp) in Bl 1951, while a putative phage region resides in the analogous Bl 1821L region. Although comparative analysis of the genomic organisation of Bl 1821L and Bl 1951 PBSX-like region with the defective phages PBSX, PBSZ, and PBP 180 of Bacillus subtilis isolates 168 and W23, and Bacillus phage PBP180 revealed low amino acids similarity, the genes encode similar functional proteins in similar arrangements, including phage tail-sheath (XkdK), tail (XkdO), holin (XhlB), and N-acetylmuramoyl-l-alanine (XlyA). AMPA analysis identified a bactericidal stretch of 13 amino acids in the ~48 kD sequenced protein of Bl 1821L. Antagonistic activity of the purified ~48 kD phage tail-like protein in the assays differed remarkably from the crude lysate by causing a decrease of 34.2% in the number of viable cells of Bl 1951, 18 h after treatment as compared to the control. Overall, the identified inducible phage tail-like particle is likely to have implications for the in vitro growth of the insect pathogenic isolate Bl 1821L.
Keywords: antibacterial protein, contractile phage tail-sheath, defective phage, insect pathogenic bacterium, PBSX
1. Introduction
Brevibacillus laterosporus (Bl) is a Gram-positive and spore-forming bacterium belonging to the Brevibacillus brevis phylogenetic cluster in the family Paenibacillaceae [1]. Globally, various strains of this bacterium have exhibited biocontrol potential against invertebrate pests of different insect orders, including Coleoptera [2,3], Diptera [4,5,6], Lepidoptera [7], and also against nematodes [8] and molluscs [9,10]. The insecticidal action is mostly related to the production of diverse toxins, many of which act post-ingestion in the insect gut [11,12]. Due to the entomocidal action of Bl against diverse insect pests, there has been a surge of interest in using this species in microbial pesticides [13,14,15,16,17]. The New Zealand insect pathogenic isolates Bl 1821L and Bl 1951, originally isolated from brassica seeds, exhibited activity against diamondback moth (Plutella xylostella) and mosquito larvae (Culex pervigilans and Opifex fuscus) [7,11]. These isolates are under development as biopesticides, but often experience stymied growth during culturing, and it was hypothesised that bacteriophage might be involved [18]. Bacteria predominantly harbour prophages in their chromosomes [19], either in true or defective lysogenic forms [20,21]. The common products of defective phage assembly are sheath-like tails with activity against susceptible bacterial species [22,23]. Phage tail-like particles are commonly known as tailocins, defective bacteriophages, or cryptic phages [24,25] due to their potency against sensitive bacteria without injecting DNA [26]. Tailocins or phage tail-like bacteriocins (PTLBs) are bactericidal structures [25] first identified as R-type and F-type pyocins produced by Pseudomonas aeruginosa [27]. They resemble phage tails, with the R-type pyocins corresponding to the contractile tails of myophages such as T4 and the F-type pyocins corresponding to the flexible, non-contractile tails of siphophages such as T1 [27]. The common feature of the two forms is how they perpetuate in nature [28]. The best-studied examples are the colicins produced by Escherichia coli and the R-type pyocins of P. aeruginosa. Colicin gene clusters are encoded on plasmids while pyocins are typically located on chromosomal DNA [26,29]. Tailocins rely on receptor-binding proteins (RBPs) located on tail fibres or spikes for initial and specific interaction with susceptible bacteria [30,31]. Phages kill bacteria through a lytic, replicative cycle, whereas PTLBs kill the target cell through membrane depolarisation in a single hit mechanism [32].
Homologous bactericidal phage-like element PBSX protein defined within the Gram-positive bacteria of the genus Bacillus [33,34] is known to employ a similar killing mechanism to the one perpetrated by the tailocins [28,35]. PBSH, PBSX, PBSV, PBSW, PBSY, PBSZ, and PBP180 are some of the identified defective phages of Bacillus subtilis 168, Bacillus licheniformis, B. subtilis var. vulgatus, B. subtilis S31, B. subtilis W23, and Bacillus pumilus AB94180, respectively [33,36]. Among all of these bactericidal structures, PBSX from B. subtilis 168 has been the most widely studied phage-like element [34]. PBSX prophage is resident in the host chromosome and is inducible upon exposure to various DNA damaging agents such as mitomycin C, ultraviolet light, and hydrogen peroxide [37,38]. Induction releases synthesised structural proteins of phage-like particles ranging in mass from 12 kD to 76 kD [39,40], and is accompanied by the lysis of the cells [36]. Numerous phage tail-like structures with putative antibacterial activities have been identified in the Gram-negative bacteria [26] and in a limited number of Gram-positive bacteria, including Listeria monocytogenes [41], Bacillus pumilus [36], B. subtilis [42], Clostridium difficile [43], and Bacillus aneurinolyticus [44]. However, B. pumilus 15.1, is the only example of an entomopathogenic bacterium from which phage tail-like particle with bacteriocin activity was defined [45].
In this study we isolated, purified, and characterised the putative antibacterial phage tail-like structures of the PBSX-like region from an insect pathogenic isolate Bl 1821L and compared the encoding region to other bacteria, including the closely related strain Bl 1951.
2. Materials and Methods
2.1. Bacterial Strains and Growth Conditions
The following bacterial strains were used in this study: Bacillus megaterium 3-2, B. megaterium S1, B. subtilis EM-13 (Tp5), Bl 1951, Bl 1821L, Bl Rsp, Bl CCEB 342, Bl NRS 590, Bl NCIMB, Carnobacterium maltaromaticum 3-1, Fictibacillus rigui EM-14 (FJAT 46895), Oceanobacillus sp. EM-12 (R-31213), and Oerskovia enterophila 3-3. All the strains are held at −80 °C in the Bio-Protection Research Centre Culture Collection, Lincoln University, New Zealand except Bl CCEB 342 and Bl NRS 590. The strains Bl CCEB 342 and Bl NRS 590 were kindly provided by Professor Colin Berry, Cardiff University, UK.
Luria-Bertani (LB, Miller) medium broth was routinely used for growing bacteria on an orbital shaker (Conco, TU 4540, Taibei, Taiwan) at 250 rpm and 30 °C overnight for further usage.
2.2. Mitomycin C Induction of Putative Antibacterial Protein
Mitomycin C (Sigma, Sydney, NSW, Australia) was used to induce the putative antibacterial proteins as outlined by [46]. Single colonies of bacteria were used to inoculate 5 mL of LB (Miller, Sigma) broth, which was placed on an orbital shaker (Conco, TU 4540, Taibei, Taiwan) at 250 rpm and 30 °C overnight. Aliquots (500 µL) of the overnight culture were transferred to further inoculate 25 mL of LB broth. The culture was left to grow (~10–12 h) at 250 rpm and 30 °C until it attained turbidity. Two concentrations (1 µg/mL and 3 µg/mL) of mitomycin C (Sigma) were independently added into the flasks, which were then positioned on an orbital platform for incubation with rotation at 40 rpm at ambient temperature (24°C). OD600nm readings were recorded through an Ultrospec-10 spectrophotometer (Amersham Biosciences, Amersham, UK) after 2, 4, 6, and 24 h of mitomycin C (Sigma) addition. The flasks were monitored for signs of cell lysis (clearing of the culture or accumulation of bacterial debris). The flasks without the addition of mitomycin C served as a control. All the treatments in the experiment were technically replicated four times. OD600nm readings at various time intervals were pooled and statistically analysed using the ANOVA (Analysis of Variance) test through the Genstat 20th edition programme.
2.3. Soft-Agar Overlay Method with Polyethylene Glycol (PEG) Precipitation
Antibacterial activity of bacteriophages and phage tail-like structures (bacteriocins) can be differentiated after PEG 8000 precipitation of mitomycin C-induced bacterial cultures and the serial dilution assay testing in the soft-agar overlay [47]. For PEG precipitation, mitomycin C-induced cultures were centrifuged at 16,000× g for 10 min, and the supernatants were passed through a 0.22 µm filter. To the filtered cell free supernatant (CFS), 1M NaCl and 10% PEG 8000 were added and the sample was repeatedly inverted until both the NaCl and PEG 8000 were completely dissolved. The sample was incubated in an ice bath for 60 min and subsequently centrifuged (16,000× g, 30 min, 4 °C). The supernatant was decanted and the pellet was resuspended in 1/10th volume of the original supernatant volume of buffer (10 mM Tris, 10 mM MgSO4, pH 7.0) by repeated pipetting. PEG 8000 residue was removed by two sequential extractions with an equal volume of chloroform, which was combined with the resuspended pellet and vortexed for 10-15 sec. The mixture was centrifuged (16,000× g, 10 min), and the upper aqueous phase was transferred to a fresh 1.5 mL microfuge tube. This extraction process was repeated until no white interface between the aqueous and organic phases was visible. Soft agar (0.5%) was prepared and maintained at 55–60 °C before use. Next, 3 mL of soft agar was transferred into a 15 mL sterile tube and 100 µL of overnight culture was added. The tube was rotated for 10–15 s and then immediately poured over an LB agar plate. LB agar plates were allowed to dry for 20–30 min. Tenfold serial dilutions of PEG 8000 precipitated culture of Bl 1821L were prepared. Once the agar was solidified, 10 µL of PEG 8000 precipitated supernatant of each dilution (undiluted to 10−8) was pipetted at 2 spots on the lawns of host bacterium, and the plates were incubated at 30 °C for 48–72 h. The control comprised spotted sterile LB broth. Three LB agar plates were used for each dilution to find out the antibacterial activity of the PEG 8000 precipitated lysate. Antibacterial activity was evaluated by measuring the diameter of the zone of inhibition (mm) at the spotting point.
2.4. Antimicrobial Spectrum of PEG 8000 Precipitated Culture Filtrates
To assess the antimicrobial spectrum of PEG 8000 precipitated Bl 1821L filtrate after mitomycin C induction against itself and other Gram-positive bacteria (Bl 1951, Bl Rsp, Bl CCEB 342, Bl NRS 590, C. maltaromaticum 3-1, B. megaterium 3-2, B. megaterium S1, O. enterophila 3-3, Paenibacillus sp. 15.12.1, Oceanobacillus sp. R-31213, B. subtilis Tp5, and F. rigui FJAT 46895), the soft agar overlay method was used as outlined above. Ten µL of sterile LB broth pipetted on the plates was used as a negative control. For the antimicrobial spectrum determination assay, three LB agar plates were used. Antimicrobial activity was evaluated by measuring the diameter (mm) of the zone of inhibition at the spotting point.
2.5. Purification of Putative Antibacterial Protein
The crude lysate of Bl 1821L harbouring the putative antibacterial proteins after mitomycin C induction was purified by ultracentrifugation of 7.5 mL of CFS at 35,000 rpm (151,263× g) in a swing bucket rotor (41Ti, Beckman, California, USA) for 70 min. The concentrated pellet was resuspended in 100-150 µL of TBS buffer (40 g NaCl, 1 g KCl, 2.42 g TRIS Base, 16.5 g TRIS-HCl, dH2O 490 mL, pH 7.4 in 500 mL). Sucrose density gradients were formed by applying layers of 1.25 mL of freshly prepared sucrose solution 10%, 20%, 30%, 40%, 50%, and 60% sequentially from the highest to the lowest concentrations. Two hundred μL of the ultracentrifuged preparation was applied on top of the gradients from where the samples were centrifuged at 35,000 rpm (151,263 × g) in a swing bucket rotor (41Ti, Beckman) for 70 min.
After ultracentrifugation, individual gradients were assayed against Bl 1821L and Bl 1951 as the host bacterium using the Kirby–Bauer disc diffusion test [48]. After the disc diffusion assay, each of the gradients was ultracentrifuged to concentrate the pellet. The purified and concentrated solution of 60% sucrose density gradient pellet was then cleaned using an Amicon Ultra-0.5 (10 kD) centrifugal filter (Millipore, Cork, Ireland) for sodium dodecyl sulphate polyacrylamide gel electrophoresis (SDS-PAGE) and transmission electron microscope (TEM) analysis.
2.6. TEM Examination of Crude and Purified Lysates
For TEM analysis of crude lysate of Bl 1821L, 7 mL of CFS of Bl 1821L from mitomycin C-induced culture was ultracentrifuged at 35,000 rpm for 70 min and 4 °C. The concentrated pellet was dissolved in 150 µL of 25 mM TBS. A 5 µL sample was applied to a freshly glow-discharged plastic-coated hydrophilic 200 mesh EM grid (ProSciTech; Thuringowa, Australia) and stained with 3 µL of 0.7% uranyl acetate (UA, pH 5). The Bl 1821L sample was subjected to TEM analysis at 18,000 to 25,000 magnification in Morgagni 268D (FEI, Hillsboro, OR, USA) TEM operated at 80 KeV. The images were photographed using the TENGRA camera.
2.7. SDS-PAGE Analysis
The putative antibacterial proteins of Bl 1821L were subjected to SDS-PAGE analysis using 30% acrylamide [49]. Next, 10 µL of protein ladder (BIO-RAD, Precision Plus ProteinTM Standards) was loaded. Gels were run for 50 min at 200 volts and then washed four times with H2O before staining with RAMA stain (29 mL MQW, 12.5 mL CBB stock (1 gm CBB, 300 MeOH, 200 mL MQW), 3.75 mL ammonium sulphate (200 gm, 500 mL MQW), 5 mL of glacial acetic acid per gel) [50]. Prior to overnight destaining in water, the gel was rinsed in water. However, for silver staining, the protocol of [51] was followed.
2.8. Bactericidal Activity Assay
First, 500 µL crude lysate harbouring the putative antibacterial proteins (ABPs) was pipetted into the overnight culture of the host bacteria. For the control treatment, a similar volume of LB broth was used. All the flasks with/without putative ABPs were maintained at 30 °C on a shaking incubator (Conco, TU 4540, Taibei, Taiwan). Samples were drawn from each treatment after 1, 3, 6, 12, 18, and 24 h of incubation to determine the number of viable cells (CFU/mL) and OD600m. Cell biomass (OD600nm) was measured using the Ultrospec-10 spectrophotometer (Amersham Biosciences). To determine the number of viable cells (CFU/mL), tenfold serial dilutions (10−1 to 10−6) of each time interval were prepared and 100 µL from each dilution was spread in duplicate on two independent LB agar plates. After incubation at 30 °C for 2–3 days, the colonies were counted using a colony counter (Stuart, London, UK) and converted into log10 CFU/mL. To define potential ABPs antagonistic activity, the percentage change in number of viable cells compared to the control treatment (without ABPs) after treatment with the putative ABPs was calculated. Four independent set of experiments with biological replications were performed, and the pooled data were subjected to statistical analysis using the ANOVA (Analysis of Variance) test through the Genstat 20th edition programme. Similar to the above, an experiment with the purified PTLP was performed.
2.9. N-Terminal Sequencing and Bioinformatic Analysis
A prominent band (~48 kD) of the filtered and concentrated supernatant (crude) of Bl 1821L on the SDS-PAGE was subjected to N-terminal sequencing. After the initial assessment, the purified gel bands of the protein of interest from SDS-PAGE were excised for N-terminal sequence analysis. Peptides generated by trypsin (Promega, Madison, WI, USA) cleavage from separated protein bands of interest were analysed using liquid chromatography mass spectrometry (LC-MS) for further identification. The obtained peptides were compared with the predicted proteins from the Bl 1821L genome (NZ_CP033 464.1). Amino acid sequences from the genomes were assessed and characterised using Uniprot database (https://www.uniprot.org; accessed on 25 September 2019), BLASTp (Basic Local Alignment Search Tool) (https://blast.ncbi.nlm.nih.gov; accessed on 23 April 2021), ExPasy (https://www.expasy.org; accessed on 23 April 2021), and the CLUSTALO (https://www.uniprot.org; accessed on 23 April 2021).
The identified ~48 kD putative antibacterial protein of Bl 1821L was analysed using Geneious [52]. Amino acid sequence alignments were performed using CLUSTALO (https://www.uniprot.org; accessed on 23 April 2021). AMPA (Antimicrobial Sequence Scanning System) is a bioinformatic tool that identifies the antimicrobial domains of proteins (http://tcoffee.crg.cat/apps/ampa; accessed on 23 April 2021) [53]. We ran the whole protein sequence in AMPA using a default propensity value of 0.225. Amino acids expressing the propensity value below the threshold level were considered a positive hit for latent bactericidal activity.
3. Results
3.1. Mitomycin C Induction of Putative Antibacterial Proteins
OD600nm reading of the Bl 1821L culture after treatment with the mitomycin C at a concentration of 1 µg/mL or 3 µg/mL significantly declined by 49.7% and 41% after 24 h, respectively. The OD600nm reading of the control treatment (without mitomycin C) revealed a slight increase in cells up to 6 h from where the OD600nm slowly declined from 6–24 h post incubation (hpi) (Figure 1 and Supplementary Table S1).
3.2. Antimicrobial Activity of PEG 8000 Precipitated Culture Filtrates
Assay testing of the PEG 8000 precipitated filtrates in the serial dilutions in our work indicted an increase in turbidity (Figure S1), but this antagonistic activity was lost upon transfer to fresh soft-agar lawn, which is an indication of bacteriocinogenic activity. Bl 1821L PEG 8000 precipitated filtrates showed inhibitory activities against itself at the highest concentration (FS—full strength, undiluted) (Table 1 and Figure S1B) and against Bl 1951 between FS and 10−3 dilution (Table 1 and Figure S1A).
Table 1.
Bl 1821L as the Host Bacterium | Bl 1951 as the Host Bacterium | ||
---|---|---|---|
Dilution Level | Zone of Inhibition Diameter (mm) |
Dilution Level | Zone of Inhibition Diameter (mm) |
FS * | 12.5 | FS | 12.5 |
10−1 | – ** | 10−1 | 10.5 |
10−2 | – | 10−2 | 13.5 |
10−3 | – | 10−3 | 10.5 |
10−4 | – | 10−4 | – |
10−5 | – | 10−5 | – |
10−6 | – | 10−6 | – |
10−7 | – | 10−7 | – |
10−8 | – | 10−8 | – |
Control *** | – | Control | – |
* FS = Full strength. ** = No zone of inhibition. *** = For control LB broth pipetted on the lawn of host bacteria.
Using 1 µg/mL of mitomycin C induced culture of Bl 1821L after PEG 8000 precipitation exhibited high activity against all the tested strains of Bl except against itself and Bl CCEB 342 (Table 2). With the exception of C. maltaromaticum isolate 3-1, which was slightly sensitive to inhibitory action, all other tested Gram-positive bacterial strains were not susceptible to the Bl 1821L PEG 8000 precipitated culture supernatant (Table 2 and Figure S3).
Table 2.
Host Bacterium | Host Bacterium Isolate/Strain |
Sensitivity to Induced Bl 1821L CFS |
---|---|---|
Bacillus megaterium | 3-2 | – * |
Bacillus megaterium | S1 | – |
Bacillus subtilis | EM-13 (Tp5) | – |
Brevibacillus laterosporus | 1951 | + ** |
Brevibacillus laterosporus | 1821L | – |
Brevibacillus laterosporus | Rsp | + |
Brevibacillus laterosporus | CCEB 342 | – |
Brevibacillus laterosporus | NRS 590 | + |
Brevibacillus laterosporus | NCIMB | + |
Carnobacterium maltaromaticum | 3-1 | + |
Fictibacillus rigui | EM-14 (FJAT 46895) | – |
Oceanobacillus sp. | EM-12 (R-31213) | – |
Oerskovia enterophila | 3-3 | – |
Paenibacillus sp. | 15.12.1 | – |
* – = No zone of inhibition. ** + = Zone of inhibition.
3.3. TEM and SDS-PAGE Analysis
Electron micrographs of concentrated crude lysate of Bl 1821L showed the presence of incomplete phage structures similar to hollow sheath and contractile tail sheath-like structures as well as the phage capsid-like and cog wheel-like structures (Figure 2B,C). TEM examination of purified and 10 kD MWCO membrane concentrated lysate revealed the presence of polysheath-like structures (Figure 2D,E) which were jointed at some points, with (Figure 2D) or without (Figure 2E) knot-like structures.
A prominent band of ~48 kD was visualised after high-speed centrifugation of the crude lysate on SDS-PAGE (Figure S2) and it was hypothesised to be involved in the putative antibacterial activity. Furthermore, SDS-PAGE of sucrose density gradient (60%) purified and 10 kD MWCO membrane concentrated Bl 1821L lysate authenticated the preliminary findings by showing a prominent band of ~48 kD (Figure 2A).
3.4. Identification of a ~48 kD Putative Antibacterial Protein in Bl 1821L Genome
Alignment of the ~48 kD purified protein N-terminal sequences revealed several hits (covering approximately 34% of the amino acid sequence; Figure S4) to the loci A0A518VEB0 in the Bl 1821L genome (NZ_CP033464.1) encoding a predicted defective phage protein, similar to that encoded by the Bs 168 phage-like element PBSX gene xkdK. Through Uniprot, the predicted ~48 kD XkdK-like protein of Bl 1821L shared high amino acid identity with phage tail, phage tail sheath, and uncharacterised proteins (Table S2). BLASTp analysis of the identified accession (A0A518VEB0) against Uniprot database exhibited 90.3% amino acid similarity to the phage tail-sheath protein of Bl LMG 15441 and a phage tail protein, phage sheath protein, and uncharacterised proteins encoded in various Bl strains (Table 3). Furthermore, these findings validated the preliminary results of the N-terminal sequencing of the prominent band (~48 kD) of the SDS-PAGE (Figure S2).
Table 3.
Accession | Protein | Host Bacterium | Amino Acids (%) Similarity to the Identified Accession A0A518VEB0 |
---|---|---|---|
A0A075R9L5 | Phage tail sheath | Brevibacillus laterosporus LMG 15441 | 90.3 |
M8E4N0 | Uncharacterised | Brevibacillus borstelensis AK1 | 69.9 |
A0A3M8DWU9 | Phage tail | Brevibacillus fluminis | 68.0 |
C0Z5G9 | Uncharacterised | Brevibacillus brevis (strain 47/JCM 6285/NBRC 100599) | 68.1 |
A0A6M1UCS4 | Phage tail | Brevibacillus sp. SYP-B805 | 66.6 |
A0A0X8D434 | Phage tail sheath | Aneurinibacillus sp. XH2 | 49.1 |
A0A2Z2KS77 | Phage tail sheath | Paenibacillus donghaensis | 48.3 |
3.5. Bactericidal Activity of Identified XkdK Protein
The crude lysate containing the identified XkdK protein along with the other putative ABPs after 6 h of incubation at 30 °C caused a non-significant decrease of 30.1% in the number of viable cells of Bl 1821L compared to the control (without ABPs) and preceding time intervals (1 and 3 h) in the liquid assay but showed no effect against Bl 1951 (Table S3 and Figure S7).
AMPA analysis of the Bl 1821L phage-like element PBSX protein XkdK identified a bactericidal stretch (Figure S5) which was found from 360 to 373 amino acids (NKKFAKNIVRVLD) (Figure S6, shown in red) with a propensity value of 0.223 for the sequenced phage tail-like protein of Bl 1821L. In contrast to the activity of crude lysate, the addition of purified ~48 kD phage tail-like protein (PTLP) caused a decline of 22.1% and 34.2% after 12 and 18 h in the number of viable cells of the Bl 1951 compared to the control (without PTLP) (Table S5 and Figure 3). Similar to crude lysate, OD600nm assessments of the treated and untreated cultures revealed no prominent differences across the assessed time points (Tables S4 and S6, Figures S8 and S9).
3.6. Bl 1821L and Bl 1951 Phage-Like Element PBSX Protein XkdK Comparison with the Similar Proteins of Other Gram-Positive Bacteria and Bl Phages
The predicted ~48 kD phage like-element PBSX protein XkdK of Bl 1821L and Bl 1951 was compared with identical XkdK proteins/phage tail-sheath proteins of other Gram-positive bacteria belonging to the genus Aneurinibacillus, Bacillus, Brevibacillus, Clostridioides, and Geomicrobium (Table S7). Amino acid alignment of the Bl 1821L and Bl 1951 XkdK sequence with orthologous proteins provided an insight into their phylogenetic relationships, revealing mainly distant relationships (Table S8 and Figure 4). Despite similar organisation of the operons, the specific Bl 1821L XkdK protein had only 21.2% amino acid similarity with the Bs 168 XkdK protein (Table S10 and Figure 5 and Figure S10). The predicted phage tail-sheath protein XkdK of Bl 1821L and Bl 1951 aligned with the phage tail-sheath proteins of different known Bl phages, including Abouo, Davies, Jimmer2, Powder, and Osiris [54], but only shared 21.9% amino acid similarity (Table S11 and Figure S11). A dendrogram of aligned phage tail sheath proteins of Bl defined phages with the similar protein of Bl 1821L and Bl 1951 also indicated a distant relationship (Table S10 and Figure 6). Furthermore, this analysis was supported through CLUSTALO-based amino acids alignment (Figure S12).
3.7. Bioinformatic Analysis of Regions Adjacent to the Bl 1821L and Bl 1951 Putative Antibacterial Protein Encoding Gene
The identified homolog of the phage-like element PBSX gene xkdK in the Bl 1821L genome (NZ_CP033464.1) is encoded between 5,137,125 bp and 5,138,462 bp. Bioinformatic analysis of genomic regions flanking the xkdK gene (A0A518VEB0) in both Bl 1821L and Bl 1951 revealed some genetic similarities to the PBSX-like region described in Bs 168 (Figures S13 and S14). An ortholog of the Bl 1821L phage tail-sheath encoding gene xkdK was identified in the genome of Bl 1951 (RHPK01000003.1, contig 1; 1,937,150 bp to 1,935,813 bp). In Bl 1951, at the 5′ end of the xkdK gene were two ORFs encoding hypothetical proteins (Figure S14); the one immediately upstream was identical to an uncharacterised protein (A0A502IL32). The adjacent upstream hypothetical protein (A0A502IL09) shared 96% amino acid similarity with the XkdN protein of Bl LMG 15441 (A0A075R977). Furthermore, in the Bl 1951 genome, several other PBSX-like gene orthologues such as xkdT and xkdU, as well as other phage and hypothetical genes are present (Figure S14).
Bioinformatic analysis comparing the PBSX-like regions of Bl 1821L and Bl 1951 revealed that Bl 1951 had two glycine rich protein encoding genes with 1700 bp imperfect repeats in one region, while a predicted unnamed phage resides in the analogous region in Bl 1821L genome (Figure 7).
Furthermore, analysis of this genomic region in both the Bl 1821L and Bl 1951 identified genes, the translated products of which are involved in phage lysis activities, including N-acetylmuramoyl-l-alanine amidase and holins. An upstream gene encoding a protein homologous to a putative bacteriocin UviB (BhlA) of Bs 168 along with homologs of other phage-like element PBSX genes xkdT and xkdU also resided in Bl 1821L PBSX-like region (Figure 8 and Figure S13). BLASTp analysis of the holin protein (BhlA) exhibited homology to an uncharacterised protein of Bl LMG 15441, with protein orthologues in several Bl phages (Table S12). A hydrolytic enzyme, N-acetylmuramoyl-l-alanine amidase, a regulating gene, is adjacent to the uviB/holin bhlA (Figure S13). Furthermore, several other phage-like proteins including a tail protein, phage FluMu protein Gp47, and a prophage LambdaBa01 Xpf encoded in the PBSX-like region of Bl 1821L are also annotated. Various genes encoding hypothetical proteins are also localised in the region where xkdK resides in the Bl 1821L genome (Figure 8). Located at the 3′ end of the phage-like element PBSX in Bl 1821L are four (ABC transporter) permease genes yvcR, yvcS, yvcQ, and yvcP (Figure S13). The translated products of these genes have been implicated in the export of lipid II-binding lantibiotics, such as nisin and gallidermin.
3.8. Genomic Comparison of the Bl 1821L and Bl 1951 PBSX-Like Region with the Defective Prophages PBSZ, PBSX, and PBP180
Comparison of the genomic organisation of PBSX-like regions of Bl 1821L and Bl 1951 with the analogous regions of defective prophages PBSZ, PBSX, and PBP180 of B. subtilis W23, B. subtilis 168, and Bacillus phage PBP180 revealed similar architecture (Figure 8). However, despite organisational similarities, significant differences were noted. Located at the 5′ end of Bl 1821L xkdK are two terminase unit (xtmB) and xkdN genes, while at the 3′ end are genes encoding uncharacterised proteins, a prophage LambdaBa01, and positive control factor Xpf reside (Figure 8). Immediately upstream of the Bl 1821L xkdN gene encoding is the tail protein corresponding to xkdO gene of PBSX, PBSZ, and PBP180 genome; but in other Bacillus strains, a gene xkzB encoding an uncharacterised protein is located at the 3′ of the tail protein gene xkdO. The gene encoding XkdP, a murein-binding protein, resides 5′ of the phage tail protein of the Bacillus strains, and several genes encoding the hypothetical proteins (XkdQ, XkdR, XkdS) reside upstream of it (Figure 8).
Similar to Bl 1821L, the encoded PBSX-like region in the Bl 1951 genome was analysed to compare the genomic organisation with that of PBSZ, PBSX, and PBP180 (Figure 8). Located 5′ of xkdK is a gene encoding a hypothetical protein. Within the PBSX-like region of Bl 1821L and Bl 1951, the section which differs (Figure 7) is notable in Bacillus strains due to the presence of genes encoding XkdV (a putative tail fibre protein) and hypothetical proteins (Figure 8). Amino acid alignment of the XkdK protein of Bl 1821L and Bl 1951 sharing 22.9%, 22.9%, and 21.6% amino acid identity exhibited low amino acid identity with the respective protein orthologues PBSZ, PBSX, and PBP180 of strains B. subtilis W23, B. subtilis 168, and Bacillus phage PBP 180 (Table S14 and Figure 9).
The XkdO (A0A518VEA0) tail protein residing in the PBSX-like region of Bl 1821L and Bl 1951 shares 50% amino acid similarity with the corresponding protein of PBSZ prophage but shared no amino acid similarity to the PBSX and PBP180 defective prophage tail proteins. However, the PBSX-like region protein XkdO shared 51.1% and 37% amino acids similarity with the respective PBSZ and PBP180 tail proteins (Table S14).
The holin protein (XhlB) of PBSX shared 89.8% and 61.4% amino acid similarity with the respective PBSZ and PBP180 amino acid sequences. In contrast, the Bl 1821L and Bl 1951 holin protein (BhlA) exhibited a low level of 11.4%, 13.6%, and 13.6% amino acid identity with the PBP180, PBSZ, and PBSX (Table S18 and Figure S19A). Distance matrices generated using Geneious basic (Table S17 and Figure S19B) and amino acid alignment using CLUSTALO (Figure S18) substantiated these findings. N-acetylmuramoyl-l-alanine is an endolysin-related protein (XlyA) localised in the Bl 1821L and Bl 1951 genome, which had a low sequence similarity of 15.4%, 15.4%, and 7.7% to PBSZ, PBSX, and PBP180, respectively. However, these proteins were quite similar to each other; PBSX had amino acids similarity of 95.3% with PBSZ and 53.9% with PBP180 (Table S20 and Figure S21A).
4. Discussion
While deciphering the causes of erratic growth of entomopathogenic strains of Bl, cultures induced with mitomycin C showed a decline in cells biomass that correlated with the presence of bioactive antagonists in Bl 1821L PEG precipitates. Furthermore, serial dilution testing of precipitated filtrates and the electron micrographs of the crude lysates authenticated the absence of phage activity. N-terminal sequencing of a prominent ~48 kD protein in semi-purified bioactivity samples identified a phage-like element PBSX gene xkdK. However, antibacterial activity of the crude lysate harbouring different putative ABPs including the ~48 kD PTLP differed from the purified ones. AMPA analysis predicted the bactericidal potency of the purified protein. TEM analysis of the purified ~48 kD protein showed the presence of polysheath-like structures. In the liquid growth assay, a decrease in the number of viable cells of Bl 1951 was noted after treatment with the purified PTLP, which had genetic similarities to the phage-like element PBSX protein XkdK. In total, our results indicated that a phage tail-like element, encoded by a PBSX-like region of Bl 1821L and Bl 1951 isolates, was antibacterial (bacteriocin) in nature.
Occasionally, the incomplete phage particles may not fit well with the description of R-type or F-type bacteriocins but could correspond to phage killer particles [21]. Interestingly, these elements behave like bacteriocins but are very diverse genetically, displaying features ranging from streamlined PTLBs to nearly complete phages [26]. Therefore, for the defective prophages the term “phage killer particles or protophages” was coined to include PBSX and other non-infectious defective phage particles acting as de facto bacteriocins [33,55]. Numerous defective phage-like elements including PBSX are inducible via the SOS response [36,38], and the induction is suicidal for the bacterial cells, as it results in lysis [56,57]. Turbidimetry is one of the established methods used to monitor bacterial growth since optical density (OD600nm) measurements make it possible to follow bacterial population growth in real time. Some authors have attempted to derive growth parameters from optical density measurements [58,59]. In our study, using mitomycin C at 1 µg/mL significantly decreased the cell biomass (OD600nm) of Bl 1821L by 49.7% after 24 h compared to the control. Following the induction, the lysate was examined under TEM and structures resembling to incomplete phage particles were observed. The findings were in agreement with the work of [45] on an insect pathogenic strain B. pumilus 15.1. Through this study, we have defined the concentration of mitomycin C for the induction of phage tail-like structures of Bl 1821L. Phage-induced bacterial lysis relies on the concerted action of two proteins (lytic enzymes), holin and endolysin [60,61]. Bioinformatic analysis identified a holin protein (BhlA) similar to that found in Bs prophage SPβ than the PBSX holin XhlA, a sign of genomic plasticity that phages and phage-related particles have [45]. The timing of lysis, which is critical for viral reproduction, is somehow “programmed” into the structure of the holin [62]. Localisation in the region of lysis genes holin (bhlA) and endolysin enzyme N-acetylmuramoyl-l-alanine amidase (xlyA) suggests that the predicted lysis genes of the Bl 1821L PBSX-like region may follow a pathway similar to the phages in host cell lysis. Hypothetical proteins resided at 3′ of the holin (BhlA) protein of Bl 1821 and Bl 1951 PBSX-like region. While analysing the genome of different B. pumilus strains [45], speculated that these hypothetical proteins might be the part of the lysis module, based on the location of the similar proteins near holins and endolysins. Typically, fully functional prophages tend to undergo a round of lytic growth, resulting in plaque formation, while a substantial number of phage-like entities present in bacterial genomes only produce phage tail-like structures [63]. Phage tail-like particles are devoid of the phage genome and cannot multiply and form plaques [47]. Therefore, in the present study, the soft-agar overlay method with PEG 8000 precipitation was used to differentiate between the activities of bacteriophages and bacteriocins [47]. Assay test findings were in accordance with previous work, which demonstrated that performing a serial dilution on a supernatant containing bacteriophages will result in individual plaques becoming less in number with greater dilution, whereas in the former it will result in a clearing zone that becomes uniformly more turbid with greater dilution [47,64]. Furthermore, a bacteriophage will produce a clearing zone when spotted onto a fresh soft-agar overlay seeded with the same strain, whereas a bacteriocin will not produce a clearing zone when transferred to a fresh soft agar lawn, owing to the dilution of the bacteriocin [47]. Using the same method, bacteriocin-like activity of the phage tail-like particles from different Gram-positive bacteria were defined [43,45].
Bacterial genomes often harbour genes encoding a toxin–antitoxin (TA) system [65]. Within this system, the toxin may inhibit the producing cell’s own cell growth by halting essential cellular processes [66], but its cognate antitoxins can block this activity [67]. In our study, the crude lysate harbouring the different putative ABPs including the ~48 kD PTLP, statistically caused a non-significant decrease of 30.1% in the number of viable cells of Bl 1821L and no effect against the Bl 1951. However, the addition of purified ~48 kD PTLP into the culture of Bl 1951 decreased the number of viable cells by 34.2%, 18 h after treatment, compared to the control (without PTLP). Variation in the bactericidal activity of crude lysate and the purified PTLP suggests that a TA system might be operational in a crude form that neutralises the lethal effect of one protein against the other. The killing mechanism of phage tail-sheath proteins (bacteriocins) is related to the mechanism in which Myoviridae phages translocate DNA into the cell after binding, but instead of DNA entering the cell, a pore is created [26,30]. These findings are in agreement with previous work, which showed that defective phages such as phage-like element PBSX containing the protein XkdK [45] and R-type tailocins [35] act as specialised weapons against kin bacteria.
N-terminal sequence of ~48 kD purified protein band identified a gene with low homology (34%) to the phage-like element PBSX gene xkdK similar to that encoded in the Bs 168. PBSX of Bs 168, is one of the most widely studied defective phages [36]. The region flanking xkdK encoded a phage-like element and resembled a PBSX-like encoding region. The PBSX phage particle is composed of at least 26 polypeptides. XkdG is the main capsid protein; XkdK and XkdM are the tail sheath and core proteins, respectively. XkdV is the fibre subunit that is involved in the killing of susceptible strains [39,68]. In phages, long tails may be contractile (Myoviridae) or non-contractile (Siphoviridae), and the morphogenesis of the tail is largely dependent on the production of the tail assembly chaperon protein, which is XkdN in PBSX [69]. XtmB proteins (phage terminase large subunit) in other PBSX-like structures reside in the capsid region and often accompany the small terminase subunit protein XtmA. However, in the Bl 1821L putative PBSX-like region, their location in the upstream region suggests a possible role in the adhesion of tail protein with the putative phage tail-sheath protein. Temperate phages integrating into the genome of the susceptible host attach themselves with an enzyme known as integrase [70]. An integrase-encoding gene was found in the Bl 1821L region and is presumed to be a site of attachment of xkdK gene in the Bl 1821L genome.
Another New Zealand isolate, Bl 1951, which has been shown to harbour the specific phage-like element PBSX gene xkdK, exhibited a similar genomic organisation around the gene. However, PBSX-like regions in both the isolates differed with the insertion of 4458 bp at the 3′ end of xkdT gene in Bl 1821L compared to Bl 1951. In Bl 1951, in the upstream region of xkdT and xkdU, are genes encoding imperfect repeats within glycine rich proteins. The tips of phage tail fibres are reported to be rich in glycine [71,72]. Glycine-rich proteins are considered vital in sustaining the unusual conformations found in the tail fibre structures [73]. Based on this information, it is likely that the glycine-rich proteins of Bl 1951 might be involved in conformations of tail fibres for adhesion to its host and have a role in defining the antimicrobial spectrum. Phage tails are the molecular machines that play a decisive role in determining the host specificity and infection process of respective phages [73,74]. Tail fibres, tail spikes, and tail tips located at the distal end of tailed phages act as receptor binding proteins (RBPs) to interact with the bacterial cell surface receptors [75]. This initial recognition subsequently leads to infection of the bacterium by phages or the depolarisation of its membrane by PTLBs [30,76]. Typically, phages and PTLBs exhibit a narrow host range [77] and employ the same primary determinant of specificity, i.e., one or more RBPs used to bind to the cell surface of the sensitive host bacterium [74]. For instance, PBSX-like particles isolated from an entomopathogenic bacterium B. pumilus 15.1 in the spot assay test displayed putative antibacterial activity against the closely related strains (narrow spectrum) [45]. In this study, PEG 8000 precipitated lysate harbouring the putative phage tail-sheath protein exhibited broad-spectrum antagonistic activity that included the kin strains Bl 1951, Bl Rsp, Bl NRS 590, Bl NCIMB, and an unrelated species, C. maltaromaticum. The sensitivity of Brevibacillus strains and the other Gram-positive bacteria implied that these might share similar RBPs. These findings align with the previous studies where the putative antibacterial activity of R-type pyocins against other bacteria like Campylobacter sp. [78]; Haemophilus influenzae [79]; Haemophilus ducreyi [80]; Neisseria gonorrhoeae [81]; and Neisseria meningitidis [82] was attributed to the common receptor sites on P. aeruginosa [83]. There are several examples in the past where the host range of bacteriophages and PTLBs has been expanded due to modifications in the tail fibre proteins [32,84].
Comparative analysis of the genomic architecture of the Bl 1821L PBSX-like region with the defective prophages PBSZ, PBSX, and PBP180 demonstrated some shared features, while showing low homology for individual genes. Despite sharing low protein similarity with the different Bacillus defective prophages, the regions perform a similar function (bactericidal). These findings are in agreement with the work of [36], who deliberated that in spite of similar genomic organisation, XkdV, a putative tail fibre protein of the PBSX region, differed from the defective prophage PBP180 corresponding operons ORF30, ORF33, and ORF35. Based on the similarities in operon architecture and differences of Bl 1821L with the identical regions, it is likely that these regions were acquired from a common distant ancestor.
Bacteria seldom exist in isolation, and generally reside within diverse microbial communities [85]. A fundamental requirement for survival in these complex environments is to gain access to scarce resources, i.e., nutrients and space, by competing with the other inhabitants. The bacteria are not only in competition with distantly related microorganisms, but also with phylogenetically related kin bacteria, which are likely the contenders for the same ecological niche [85,86]. Therefore, competition with the kin bacteria requires highly specific mechanisms to outcompete—but not to kill—individuals from the same clonal population (strains which have identical genomes). Hence, the arsenal employed against kin needs to be highly specialised, with a narrow spectrum of activity [87,88]. The findings of the antibacterial spectrum of putative phage-tail like structures (bacteriocins) of Bl 1821L against itself and the kin strains (Bl 1951, Bl Rsp, Bl CCEB 342, Bl NRS 590, Bl NCIMB) were significant in the context of interbacterial competition. Importantly, the expression of broad-spectrum activity of the Bl 1821L putative ABPs may provide an insight into complex relationships within bacterial communities.
5. Conclusions
Initially, it was hypothesised that the Tectivirus-like structures might be involved in the loss of virulence of entomopathogenic strain Bl 1821L [18]. However, no plausible evidence was found in this work. Overall, this research was the first to identify, purify, and characterise an inducible and bactericidal phage-like element PBSX gene xkdK encoded in an entomopathogenic bacterium Bl 1821L genome and compare the encoding region to other bacteria, including the closely related strain Bl 1951. Despite the broad spectrum of activity of the PEG 8000 precipitated lysate of Bl 1821L, the absence of bioactivity against a kin strain Bl CCEB 342 can provide an insight into the interbacterial competition at the community level. Furthermore, the decrease in the number of viable cells of the Bl 1951 due to the antibacterial activity of identified phage tail-like particles is likely to have implications with regard to harnessing the insecticidal potential of these strains in future.
Acknowledgments
We thank Colin Berry, Cardiff University (UK) for provision of the strains Bl CCEB 342 and Bl NRS 590, Evelyne Maes of Proteomics Platform AgResearch, Lincoln, New Zealand for LC-MS analyses, and. Marina Richena for her expertise in TEM analysis. We are also thankful to the laboratory manager, Karl Gately, RFH building, Lincoln University, New Zealand for providing ultracentrifugation facility for the uninterrupted scientific work.
Supplementary Materials
The following supporting information can be downloaded at: https://www.mdpi.com/article/10.3390/biom12081154/s1, Figure S1: Antibacterial activity of Bl 1821L cell free supernatant after PEG 8000 precipitation in the serial dilutions assay test against Bl 1951 as the host bacterium (A) and Bl 1821L as the host bacterium (B). Arrows (red colour) denote the zones of inhibition due to the activity of PEG 8000 precipitated putative antibacterial proteins. LB broth was used as a negative control against both the strains (Bl 1951 and Bl 1821L) (C). Figure S2: SDS-PAGE of mitomycin C induced culture of Bl 1821L showing a prominent band of ~48 kD (shown with dark arrow). Figure S3: Antibacterial activity of Bl 1821L-induced culture cell free supernatant after PEG 8000 precipitation against various Gram-positive bacteria. Arrows (red colour) denote the zone of inhibition due to the activity of PEG 8000 precipitated putative antibacterial proteins. Figure S4: N-terminal sequenced short amino acid match hits to the putative phage tail protein (~48 kD) encoded in Bl 1821L genome. Figure S5: AMPA analysis of identified phage tail-sheath protein of Bl 1821L. Identified bactericidal motif is indicated is pointed with red arrow. Figure S6: AMPA analysis of identified phage-like element PBSX protein XkdK of Bl 1821L. Amino acids (360–373) corresponding to the bactericidal stretch are highlighted in red colour. Figure S7: Number of viable cells (log10 CFU/mL) of Bl 1821L and Bl 1951 with/without treatment of crude Bl 1821L putative antibacterial proteins (ABPs) after incubation at 30 °C over 24 h. Figure S8: Effect of crude Bl 1821 putative antibacterial proteins (ABPs) on the OD600nm reading of Bl 1821L and Bl 1951 after incubation at 30 °C for various time intervals. Figure S9: Effect of purified Bl 1821 putative phage tail-like protein (~48 kD) on the OD600nm reading of Bl 1821L and Bl 1951 after incubation at 30 °C for various time intervals. Figure S10: Amino acids alignment of identified Bl 1821L and Bl 1951 phage like-element PBSX protein XkdK (A0A518VEB0) with the similar proteins of other Gram-positive bacteria (See SM Table S7) using the programme CLUSTALO. Figure S11: Amino acids alignment and percentage identity of identified putative phage tail-sheath protein (A0A518VEB0, shown with red arrow) of Bl 1821L and Bl 1951 with similar proteins of different Bl phages including Abouo (S5MUG6), Jimmer1 (S5MNC1), Davies (S5MCF5), Jimmer2, (S5MBG7), Powder (A0A0K2FLW7), and Osiris (A0A0K2CNL4) using Geneious basic. Figure S12: Amino acids alignment of identified Bl 1821L and Bl 1951 putative phage tail-sheath protein (A0A518VEB0) with the phage tail-sheath protein of different Bl phages using the programme CLUSTALO. Figure S13: Schematic of the genomic architecture of Bl 1821L PBSX-like region encoding the identified gene xkdK. The red shaded box denotes Bl 1951 region absent in Bl 1821L. Figure S14: Genomic architecture of Bl 1951 PBSX-like region encoding the identified gene xkdK. The filled red wedge points to the integration of the red shaded region of Bl 1821L (Figure S13) in the Bl 1951 genome. Figure S15: Amino acids alignment of identified Bl 1821L and Bl 1951 phage-like element PBSX protein XkdK (A0A518VEB0) with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180 using programme CLUSTALO. Figure S16: Dendrogram showing alignment of the identified phage-like element PBSX protein XkdK (A0A518VEB0) of Bl 1821L and Bl 1951 with similar proteins of defective prophages of Bs W23 (E0U1S9), Bs 168 (P54331), and Bacillus phage PBP180 (R4JQA6). Key is 0.2 nt substitutions per site. Figure S17: Amino acids alignment of tail protein (A0A518VEA0) encoded in PBSX-like region of Bl 1821L and Bl 1951 with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180 using programme CLUSTALO. Figure S18: Amino acids alignment of holin protein (A0A075R9K7) encoded in PBSX-like region of Bl 1821L and Bl 1951 with the similar protein of the defective prophages PBSZ, PBSX, and PBP180 using programme CLUSTALO. Figure S19: Schematic presentation of amino acids alignment of holin protein (A0A075R9K7) encoded in PBSX-like region of Bl 1821L and Bl 1951 with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180 using programme Geneious basic (A) and CLUSTALO (B). Figure S20: Amino acids alignment of N-acetylmuramoyl-l-alanine amidase protein (A0A518VEA4) encoded in PBSX-like region of Bl 1821L and Bl 1951 genome with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180 using the programme CLUSTALO. Figure S21: Schematic presentation of amino acids alignment of N-acetylmuramoyl-l-alanine amidase protein (A0A518VEA4) encoded in PBSX-like region of Bl 1821L and Bl 1951 with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180 using programme Geneious basic (A) and CLUSTALO (B). Table S1: Spectrophotometer reading (OD600nm) of Bl 1821L culture after treatment with the mitomycin C at various concentrations. Table S2: Similar proteins to the ~48 kD identified putative phage tail protein of Bl 1821L in the Uniprot database. Table S3: Effect of crude Bl 1821L putative antibacterial proteins (ABPs) on the number of viable cells of Bl 1821L and Bl 1951 after incubation at 30 °C for various time intervals. Data present the mean values of four experiments. Values of % decrease/increase in the number of viable cells are calculated from CFUs values of corresponding time intervals. Table S4: Effect of crude Bl 1821 putative antibacterial proteins (ABPs) on the OD600nm reading of Bl 1821L and Bl 1951 after incubation at 30 °C for various time intervals. Data present the mean values of four experiments. Table S5: Effect of purified Bl 1821L putative ~48 kD phage tail-like protein (PTLP) on the number of viable cells of Bl 1821L and Bl 1951 after incubation at 30 °C for various time intervals. Data present the mean values of one experiment. Values of % decrease/increase in the number of viable cells are calculated from CFUs values of corresponding time intervals. Table S6: Effect of purified Bl 1821L ~48 kD putative phage tail-like protein (PTLP) on the OD600nm reading of Bl 1821L and Bl 1951 after incubation at 30 °C for various time intervals. Data present the mean values of one experiment. Table S7: Phage-like element PBSX protein XkdK and phage tail-sheath proteins from different Gram-positive bacteria. Table S8: Distance matrices of identified Bl 1821L and Bl 1951 phage-like element PBSX protein XkdK (A0A518VEB0) with the similar proteins of other Gram-positive bacteria. Table S9: Amino acids alignment % of identified Bl 1821L and Bl 1951 phage-like element PBSX protein XkdK (A0A518VEB0) with the similar proteins of other Gram-positive bacteria. Table S10: Distance matrices of identified Bl 1821L and Bl 1951 putative phage tail-sheath protein (A0A518VEB0) with the phage tail-sheath proteins of different Bl phages. Table S11: Amino acids alignment (%) of identified Bl 1821L and Bl 1951 putative phage tail-sheath protein (A0A518VEB0) with the phage tail-sheath proteins of different Bl phages. Table S12: Protein orthologues of Bl 1821L UviB (BAGEL)/Holin BhlA protein in Uniprot. Table S13: Distance matrices of identified Bl 1821L and Bl 1951 phage-like element PBSX protein XkdK (A0A518VEB0) with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180. Table S14: Amino acids alignment (%) of identified Bl 1821L and Bl 1951 phage-like element PBSX protein XkdK (A0A518VEB0) with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180. Table S15: Distance matrices of tail protein (A0A518VEA0) encoded in PBSX-like region of Bl 1821L and Bl 1951 with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180. Table S16: Amino acids alignment (%) of tail protein (A0A518VEA0) encoded in PBSX-like region of Bl 1821L and Bl 1951 with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180. Table S17: Distance matrices of holin protein (A0A075R9K7) encoded in PBSX-like region of Bl 1821L and Bl 1951 with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180. Table S18: Amino acids alignment (%) of holin protein (A0A075R9K7) encoded in PBSX-like region of Bl 1821L and Bl 1951 with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180. Table S19: Distance matrices of N-acetylmuramoyl-l-alanine amidase protein (A0A518VEA4) encoded in PBSX-like region of Bl 1821L and Bl 1951 with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180. Table S20: Alignment (%) of N-acetylmuramoyl-l-alanine amidase protein (A0A518VEA4) encoded in PBSX-like region of Bl 1821L and Bl 1951 with the similar proteins of the defective prophages PBSZ, PBSX, and PBP180.
Author Contributions
Conceptualization, T.K.B. and T.R.G.; Data curation, T.K.B.; Investigation, T.K.B.; Methodology, T.K.B., T.R.G., M.R.H.H. and J.O.N.; Software, T.K.B. and T.R.G.; Supervision, T.R.G., J.G.H., M.R.H.H. and J.O.N.; Validation, T.K.B., T.R.G., J.G.H., M.R.H.H. and J.O.N.; Visualization, T.K.B. and T.R.G.; Writing—original draft, T.K.B.; Writing—review and editing, T.R.G., J.G.H., M.R.H.H. and J.O.N. All authors have read and agreed to the published version of the manuscript.
Institutional Review Board Statement
Not applicable.
Informed Consent Statement
Not applicable.
Data Availability Statement
All data generated or analysed during this study are included in this published manuscript and its supplementary materials.
Conflicts of Interest
The authors declare no conflict of interest.
Funding Statement
The corresponding author pursued PhD under the “Faculty Development Programme of Bahauddin Zakariya University, Multan, Punjab, Pakistan” at the Bioprotection Research Centre, Lincoln University, Christchurch, New Zealand.
Footnotes
Publisher’s Note: MDPI stays neutral with regard to jurisdictional claims in published maps and institutional affiliations.
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