Molecular characterization of the PhiKo endolysin from Thermus thermophilus HB27 bacteriophage phiKo and its cryptic lytic peptide RAP-29

Introduction In the era of increasing bacterial resistance to antibiotics, new bactericidal substances are sought, and lysins derived from extremophilic organisms have the undoubted advantage of being stable under harsh environmental conditions. The PhiKo endolysin is derived from the phiKo bacteriophage infecting Gram-negative extremophilic bacterium Thermus thermophilus HB27. This enzyme shows similarity to two previously investigated thermostable type-2 amidases, the Ts2631 and Ph2119 from Thermus scotoductus bacteriophages, that revealed high lytic activity not only against thermophiles but also against Gram-negative mesophilic bacteria. Therefore, antibacterial potential of the PhiKo endolysin was investigated in the study presented here. Methods Enzyme activity was assessed using turbidity reduction assays (TRAs) and antibacterial tests. Differential scanning calorimetry was applied to evaluate protein stability. The Collection of Anti-Microbial Peptides (CAMP) and Antimicrobial Peptide Calculator and Predictor (APD3) were used to predict regions with antimicrobial potential in the PhiKo primary sequence. The minimum inhibitory concentration (MIC) of the RAP-29 synthetic peptide was determined against Gram-positive and Gram-negative selected strains, and mechanism of action was investigated with use of membrane potential sensitive fluorescent dye 3,3′-Dipropylthiacarbocyanine iodide (DiSC3(5)). Results and discussion The PhiKo endolysin is highly thermostable with melting temperature of 91.70°C. However, despite its lytic effect against such extremophiles as: T. thermophilus, Thermus flavus, Thermus parvatiensis, Thermus scotoductus, and Deinococcus radiodurans, PhiKo showed moderate antibacterial activity against mesophiles. Consequently, its protein sequence was searched for regions with potential antibacterial activity. A highly positively charged region was identified and synthetized (PhiKo105-133). The novel RAP-29 peptide lysed mesophilic strains of staphylococci and Gram-negative bacteria, reducing the number of cells by 3.7–7.1 log units and reaching the minimum inhibitory concentration values in the range of 2–31 μM. This peptide is unstructured in an aqueous solution but forms an α-helix in the presence of detergents. Moreover, it binds lipoteichoic acid and lipopolysaccharide, and causes depolarization of bacterial membranes. The RAP-29 peptide is a promising candidate for combating bacterial pathogens. The existence of this cryptic peptide testifies to a much wider panel of antimicrobial peptides than thought previously.


Introduction
An important goal of enzymes' engineering is the enhancement of their thermal stability and activity at elevated temperatures (Huang et al., 2020).Often, the protein's robustness to thermal challenges is a deciding factor for commercialization of a product and thermophiles are sources of many industrially relevant enzymes, such as thermostable α-amylases, lipases, proteases, antimicrobial enzymes and others (Henne et al., 2004).
Bacteriophages (phages for short) are viruses that infect bacteria (Clokie et al., 2011).Thermostable endolysins (enzymes produced by bacteriophages) are attracting increasing attention due to their potent antibacterial activity.Phages produce endolysins at the end of their lytic cycle to cleave specific bonds within peptidoglycan (PG) layer of the bacterial cell wall which together with internal turgor pressure causes the host cell's lysis and release of the progeny virions to the environment (Haddad Kashani et al., 2018).This is called "lysis from within, " but since the first external usage of endolysins to eliminate Streptococcus pyogenes in infected mice (Nelson et al., 2001), endolysins are increasingly being used as potential therapeutic agents.
Endolysins are categorized by their catalytic specificity (Gerstmans et al., 2018).Glucosaminidases, muramidases, and lytic transglycosylases target bonds between N-acetylmuramic acid (NAM) and N-acetylglucosamine (NAG) in the glycan strands of PG.Endopeptidases cleave bonds within the peptide parts, and N-acetylmuramoyl-L-alanine amidases hydrolyze bonds between the lactyl group of NAM and the α-amino group of L-alanine of the stem peptide of PG of most bacterial species (Vollmer et al., 2008;Vermassen et al., 2019).Gram-positive bacteria do not have an outer membrane (OM), therefore endolysins can directly lyse PG from the outside.In Gram-negatives the OM forms a protective barrier that prevents large molecules (>600 Da), such as endolysins, to reach PG (Gutiérrez and Briers, 2020).However, studies concerning enzymes lysing Gramnegative pathogens are on the rise nowadays (Zampara et al., 2020;Islam et al., 2022;Son et al., 2023).Although rare, there are lysins with intrinsic antibacterial activity related to the presence of cryptic antimicrobial peptides (Lai et al., 2011;Lood et al., 2015;Plotka et al., 2019;Raz et al., 2019).For example, mesophilic Acinetobacter baumannii phage endolysin LysAB2 is composed of 185 amino acids (aa) with an N-terminal lysozyme-like domain and a C-terminal positively charged region (Lai et al., 2011).The C-terminal putative amphipathic helix of LysAB2 was proposed to bind the negativelycharged lipopolysaccharide (LPS) of the OM of Gram-negative bacteria, while the N-terminal catalytic domain cleaved specific bonds within PG, leading to bacterial cell lysis.As a proof of concept, a P0 peptide has been synthetized based on the LysAB2 C-terminal sequence (113-145 aa) and the minimum inhibitory concentration (MIC) of P0 against A. baumannii was determined to be 64 μM (Peng et al., 2017).However, the direct interaction of P0 with components of OM was not tested, as well as the activity of P0 against Gram-positive microorganisms was not determined (the parental endolysin LysAB2 has a broad Gram-negative and Gram-positive antibacterial activity).
Another example of a thermostable endolysin is Ts2631 enzyme from Thermus scotoductus bacteriophage vB_Tsc2631, active against A. baumannii and Pseudomonas aeruginosa at 37°C (Plotka et al., 2019).This lysin has intrinsic antibacterial activity based on a protruding N-terminal cationic part, but the exact mechanism of its antibacterial activity is yet to be elucidated (Plotka et al., 2019).The cationic N-terminal region is also characteristic for TSPphg endolysin from Thermus sp.TC4 phage TSP4 (Wang et al., 2020).The 20-residue N-terminal region of TSPphg (MRLPTKTSRFGYVHGQRNHE) containing six positively charged residues (underlined) was proposed to be responsible for exogenous enzyme activity against Gramnegative Salmonella Paratyphi B, Escherichia coli O157 and Klebsiella pneumoniae.Not all endolysins from thermophilic bacteriophages have positively charged regions and not all have a broad antibacterial spectrum (Żebrowska et al., 2022).For example, the TP84_28 endolysin from Geobacillus stearothermophilus phage TP-84 was only moderately active against E. coli DH11S strain (Żebrowska et al., 2022), while a thermophilic lysozyme from Thermus aquaticus phage φIN93 had lysed specifically only the Thermus spp.cells (Matsushita and Yanase, 2008).
Therefore, in this work we characterize an endolysin derived from Thermus thermophilus bacteriophage phiKo with similarity in the primary sequence to two thermostable endolysins previously discovered in our laboratory-Ts2631 and Ph2119 from Thermus scotoductus bacteriophages vB_Tsc2631 and MAT2119, respectively (Plotka et al., 2014(Plotka et al., , 2015)).Molecular analysis of the PhiKo enzyme was performed and its antibacterial property against thermophilic and mesophilic bacteria was tested.Then, based on bioinformatics analysis, a peptide (RAP-29) with a potent antimicrobial function, hidden in the C-terminal region of this protein was found and synthesized ( 105 RAPGWKSLAWLVRELRKHDSGLRLRLVRH 133 ).Here, the bactericidal function and mechanism of action of this peptide were studied in detail.

In search of lytic enzymes
The BlastN software was used to identify open reading frames (ORFs) encoding potential lytic proteins, similar to ORFs of two thermostable endolysins Ph2119 and Ts2631 active against Gram-negative bacteria, both derived from T. scotoductus phages, MAT2119 and vB_Tsc2631, respectively.This analysis has revealed in the unpublished genome sequence of T. thermophilus HB27 phage phiKo (accession no MH673671.2),an ORF (coordinates 2,728-3,243 nt) encoding a protein of 171 aa with a putative amidase activity.The calculated molecular mass of the protein is 19.5 kDa and an isoelectric point (pI) is 8.83.The identified enzyme (accession no AYJ74695.1)shows 67.1% primary sequence identity to PG recognition family protein (PGRP) from metagenome of Thermus sp.
Results of Domain Enhanced Lookup Time Accelerated BLAST (DELTA-BLAST) show the PhiKo endolysin similarity to eukaryotic PG recognition proteins (PGRPs), e.g., PGRP SC2-like precursor from Musca domestica (29% primary sequence identity; Figure 1).According to the NCBI BLAST tool, the PhiKo endolysin resembles several uncharacterized N-acetylmuramoyl-L-alanine amidases encoded in the genomes of Terrabacterial group bacterium ANGP1 isolated from soil samples (Diamond et al., 2019), Microgenomates group bacterium Gr01-1014_7 isolated from groundwater well, and thermophilic Anaerolineae bacterium from volcano mud.The primary sequence identity between these proteins was between 31 to 39%, with query coverage of 71%-80%.
The BlastP results show conserved motifs in the primary sequence of PhiKo.Three residues, His27, His133, and Cys141 are predicted to form a Zn 2+ binding site of the PhiKo endolysin that is a hallmark of type 2 N-acetylmuramoyl-L-alanine amidases (Figure 1).The Zn 2+ coordinating residues and two other residues, Tyr55 and Lys140, are proposed to be responsible for the catalytic activity of this protein.A molecular model inferred by ESMFold (Lin et al., 2023) reveals that the overall architecture of the PhiKo endolysin consists of a five-stranded β-sheet that is flanked by six  10.3389/fmicb.2023.1303794Frontiers in Microbiology 04 frontiersin.orghelices (Figure 2).The Zn 2+ ion is placed in a cleft and is anchored to the protein by His27, His133, and Cys141, and through a phosphate group by Tyr55 (Figure 2; bioinformatics supplement available via RePOD; doi: https://doi.org/10.18150/8ZXKT8).However, Lys140, predicted to form the substrate binding site, is not directed toward the other residues in the catalytic center (Supplementary Figure 3A) and is not conserved in the primary sequence of the PhiKo endolysin (Figure 1).Because PhiKo is the most similar to two thermostable endolysins, Ph2119 and Ts2631, active against Gram-negative bacteria, including Pseudomonas aeruginosa and Acinetobacter baumannii, both critical, priority pathogens according to WHO (Tacconelli et al., 2018), our natural choice was to experimentally explore the antibacterial potential of the PhiKo enzyme.

Purification and oligomeric state of the enzyme
The recombinant PhiKo protein was purified by immobilized cobalt affinity chromatography and analyzed via SDS-PAGE electrophoresis.In the polyacrylamide gel, the protein migrated as a single band according to its predicted molecular mass of 21.7 kDa (Figure 3A).Size-exclusion chromatography was performed to analyze the oligomeric state of the PhiKo endolysin.This enzyme migrated as a single peak between carbonic anhydrase (29 kDa) and aprotinin (6.5 kDa), which indicated that this protein is highly pure, not prone to aggregation and migrates in a monomeric form (Figure 3B).
Analytical ultracentrifugation (AUC) was employed to analyze the degree of oligomerization of the PhiKo endolysin and to study the effect of the n-dodecylphosphocholine (DPC) detergent as an analog  of bacterial cells' membranes (Figure 3C).Detergents such as DPC have not previously been used to analyze the oligomerization of endolysins, but they have been successfully applied to induce the oligomerization of antimicrobial peptides interacting with bacterial membranes (Sancho-Vaello et al., 2020;Zeth and Sancho-Vaello, 2021).Therefore, samples of free protein and samples with DPC were centrifuged at 4°C in the course of the same experiment.In an independent, negative control (buffer with DPC, green line on the graph; Figure 3C) one peak was visible around 0.70 S (20,w) which corresponds to sedimentation of DPC micelles.In samples with the PhiKo endolysin (red line) two peaks were present, the first one accounting for 97.7% of the signal and representing a monomer with a globular shape (frictional ratio 1.25).The second one (2.3% of the signal) indicated slight dimerization of the protein.By the nonlinear fittings, the average molecular mass of PhiKo endolysin was determined as 21.5 kDa which corresponds well with the molecular mass of 21.7 kDa calculated based on the recombinant protein sequence.In protein samples with DPC (blue lines), in addition to the peak corresponding to DPC micelles, similarly to the PhiKo endolysin alone, two peaks were present but the second one around 2.91 S (20,w) corresponding to the dimer, was more prominent (15% of the total signal).The increased frictional ratio coefficient of 1.51 most likely explains the slightly slower sedimentation of this population.These results indicate protein tendency to form a dimer upon contact with bacterial cell membranes.

Characterization of the PhiKo endolysin lytic activity
The lytic activity of the PhiKo endolysin was measured in a turbidity reduction assay against chloroform-treated T. thermophilus HB8 substrate in a universal 20 mM HEPES buffer, pH 7.4.The activity of the enzyme was dose dependent.With the increase of PhiKo concentration (3.125, 6.25, 12.5, 25, 50, and 100 μg/mL), the turbidity of T. thermophilus cells gradually decreased, reaching the lowest level at 100 μg/mL after 10 min of incubation (Figure 4A).The effect of divalent metal ions on the lytic activity of PhiKo endolysin was determined by turbidity reduction assay in the presence or absence of the following ions: Co 2+ , Ni 2+ , Zn 2+ , Fe 2+ , Mn 2+ , Mg 2+ , and Ca 2+ (Figure 4B).No lytic activity of PhiKo was found upon treatment with EDTA, suggesting that this enzyme requires metal ions for efficient functionality.Except for Mg 2+ , all tested ions restored the activity of EDTA-treated PhiKo endolysin.The best effect was obtained after supplementation of the enzyme/bacteria suspension with 0.1 mM Co 2+ and 1 mM Zn 2+ (42.9 and 63.1% of the initial activity was achieved, respectively).
The PhiKo endolysin was most active between pH of 6.0-8.8, when the lysis exceeded 72.5% (Figure 4C).The activity was reduced to 33.6% at pH 5.5 and did not exceed 2.6% at pH 5.0.The PhiKo showed maximum lytic activity in the absence of NaCl but at salt concentrations of 25 to 800 mM this enzyme's effectiveness remained at a similar level and did not drop below 72% (Figure 4D).The temperature optimal for this enzyme's lytic activity was 60°C (Figure 4E).However, the enzyme was also active at 37°C (82.8% lysis) and in a lesser extent at 20°C (61.5% lysis).Moreover, the PhiKo enzyme showed more than 77% of residual activity after 5 h heating at 100°C (Figure 4F).Next, the activity of PhiKo endolysin was measured under optimal conditions, 20 mM Tris-HCl buffer, pH 8.0, without salt addition at 60°C.Again, the activity of the PhiKo endolysin was dose dependent, but already a concentration of 25 μg/mL resulted in a complete lysis of T. thermophilus HB8 substrate within 10 min (Figure 4G).
Transmission electron microscopy of T. thermophilus cells treated with 6.25 μg/mL of PhiKo endolysin for 10 min revealed PG layer degradation and outflow of cytoplasm outside the bacterial cell, contrary to the control where intact cell walls and well-defined PG layer were visible as a dark border (Figure 4H).
To verify experimentally the involvement of the Lys140 residue in the lytic activity of PhiKo endolysin, two variants Y55A and K140A were designed, overproduced, and purified, replacing Tyr55 and Lys140 by alanine.The Tyr55 residue was chosen for mutagenesis because it does not interact directly with the zinc ion in the catalytic center, but through the phosphate group (PO 4 3− ).The activity of the variants compared to the wild-type protein was tested using the turbidity reduction assay.The results showed high activity of the K140A variant, comparable to the wild-type protein, while the Y55A variant was inactive.Therefore, the analyses show the involvement of the Tyr55 residue in the catalytic activity of the enzyme and the lack of such activity regarding Lys140 (Supplementary Figure 3B).

Thermostability of the PhiKo endolysin
Thermal stability of the PhiKo endolysin was assessed by differential scanning calorimetry (DSC; Figure 5).Analysis of the heat-capacity curve of the PhiKo endolysin revealed the heat-capacity peak at Tm = 91.7°C± 0.1°C (Figure 5A).The transition point was estimated by fitting the experimental Cp vs. T curves to a non-two state model using Marquardt non-linear least squares method (Tm denotes the temperature value of the peak, the temperature at which a maximum of the endothermic effect emerges).Subsequent DSC experiments carried out with the addition of EDTA to the PhiKo endolysin showed that the newly formed system is less thermally stable (Tm = 86.0°C± 0.01°C) when compared to the pure PhiKo, where the determined Tm was over five degrees higher (Figure 5B).This shows that the addition of EDTA reduces thermal stability of the PhiKo endolysin.

Regions of PhiKo with antibacterial properties
Recently, in another lytic protein, LysC from Clostridium intestinale URNW, we found a region responsible for interaction with bacterial membranes and having antibacterial properties (Plotka et al., 2020;Szadkowska et al., 2022).Therefore, we employed the prediction tool of the Collection of Anti-Microbial Peptides (CAMP) and Antimicrobial Peptide Calculator and Predictor (APD3) in search of PhiKo protein regions with a potential antibacterial function.The CAMP is based on four different algorithms, three of which report results as numeric values from 0 to 1, and one algorithm designates protein regions as antimicrobial or non-antimicrobial.Few regions with potential activity against bacteria were found in the PhiKo sequence and the region PhiKo 105-133 , with the highest scores according to all algorithms, has been chosen for further analysis (Supplementary Table 2; Figure 7A).The PhiKo endolysin model shows that this region is formed by one α-helix and one β-sheet (Figure 7B).This peptide has been termed RAP-29, based on the first three residues (arginine R, alanine A, and proline P) and the length of 29 aa, has molecular weight of 3,507 Da, hydrophobic ratio of 41% and the net charge +6.5 (Figure 7C).Moreover, as predicted by APD3, RAP-29 may form an α-helix with eight residues on the same hydrophobic surface (underlined in the RAP-29 sequence 105 RAPGWKSLAWLVRELRKHDSGLRLRLVRH 133 ).The most similar peptide in the APD3 database is HD5 (7-32) from Homo sapiens with an identity percentage of 38.24% (accession no AP03065) and activity against Gram-positive and Gram-negative bacteria (Ehmann et al., 2019).

Antibacterial activity of RAP-29 peptide and MIC values
The antibacterial activity of RAP-29 was evaluated using standard antibacterial tests and selected Gram-positive and Gramnegative bacteria (Table 1).The RAP-29 peptide was synthetized based on the protein sequence, and then used to lyse 15 bacterial strains.The bactericidal activity was 3.7-log for Pseudomonas aeruginosa PAO1 and 7.1-log for multidrug-resistant Acinetobacter baumannii KPD 581.This peptide was also active against Grampositive staphylococci exceeding 5.2-log activity against Staphylococcus hominis KPD 910.
Whereas the antibacterial tests were performed in a buffer, which alone may facilitate bacterial lysis due to high internal turgor pressure and low osmolality of the environment, the minimum inhibitory concentrations (MICs) were also determined and conducted in the Mueller Hinton broth.MICs were defined as the peptide concentration at which no bacterial growth was detectable after 24 h.The MICs of RAP-29 ranged from 2.0 to 31 μM, with the lowest MIC against S. hominis KPD 910 and the highest against two strains of Staphylococcus aureus, KPD 470 and KPD 425 (Table 2).The results of antibacterial tests, as well as the MIC values indicate that RAP-29 has antibacterial properties against mesophilic Gram-positive and Gram-negative bacteria.

Mechanistic insight into the function of RAP-29
To assess the possibility of the RAP-29 interaction with bacterial membrane components, isothermal titration calorimetry (ITC) measurements were performed with the use of lipoteichoic acid (LTA) isolated from Gram-positive S. aureus.The thermodynamic parameters of the RAP-29-LTA interaction, namely logK ITC = 6.77 ± 0.16 and ΔH ITC = −10.86± 0.26 kcal mol −1 , were obtained directly from the measurements by fitting isotherms (using nonlinear least-squares procedures) to a model that assumes one set of binding sites (Figure 8A).Then, the standard thermodynamic relationships: ΔG ITC = −RTlnK ITC = ΔH ITC − TΔS ITC were used to calculate the free energy of binding (ΔG ITC = −9.24± 0.21 kcal mol −1 ), and the entropy change (TΔS ITC = −1.62 ± 0.33 kcal mol −1 ).
Many antimicrobial peptides have a random coil structure in solution while in the presence of bacterial membranes they adopt an α-helical conformation (Sarkar et al., 2021).To verify this hypothesis, circular dichroism was performed for RAP-29 without or in the presence of micelles of Lauryl-β-D-maltoside (DDM), Dodecylphosphocholine (DPC), Lauryldimethylamine N-oxide (LDAO) and Sodium dodecyl sulfate (SDS).The RAP-29 peptide forms an α-helical structure in the presence of all tested microbial membrane mimics (Figure 8C) which suggests that this peptide acquires its secondary structure in the presence of a bacterial cell membrane.Next, the membrane potential was investigated upon addition of RAP-29 (Figure 8D).LL-37, the human cathelicidin peptide that dissipate the membrane potential, served as a positive control in these tests.The fluorescent carbocyanine dye DISC 3 (5) has been used to monitor bacterial membrane depolarization.This dye loses fluorescence intensity in polarized membranes and becomes highly fluorescent once polarization is lost.RAP-29 was able to rapidly depolarize the cytoplasmic membrane in a concentration-dependent manner.At the highest concentration of RAP-29 tested (10 μM), the level of depolarization appeared to reach a maximum at 5 min after peptide addition (Figure 8D).In summary, the RAP-29 peptide binds to the bacterial cell wall components, shows an α-helical structure in the presence of detergents DDM, DPC, LDAO, and SDS, and causes collapsing of the membrane potential which altogether leads to dysfunction of the bacterial cell.

Discussion
The versatile use of bacteriophages or their components, such as endolysins, e.g., in combating antibiotic-resistant bacteria or protecting food against bacterial contamination, most often refers to operating in a temperature range of 4°C-40°C (Liu et al., 2023).Advances in research on thermophilic bacteriophages and their proteins have opened new research avenues for their applications at elevated temperatures, e.g., in food processing conditions, including pasteurization.A limited number of thermostable endolysins has been described in the literature, but their number grows constantly and this work fits well into this trend (Matsushita and Yanase, 2008;Ye and Zhang, 2008;Plotka et al., 2014Plotka et al., , 2015;;Wang et al., 2020;Choi and Kong, 2023;Jasilionis et al., 2023).Here, we characterize the PhiKo endolysin derived from extremophilic T. thermophilus HB27 bacteriophage phiKo.According to the NCBI BLAST, this protein possesses an amidase catalytic site with Zn 2+ binding motif and cuts the amide bond between the glycan moiety (NAM) and the peptide moiety (L-alanine) of bacterial PG.
The group of thermostable endolysins includes, among others, LysGR1 endolysin from Geobacillus stearothermophilus phage GR1.This enzyme retains more than 60% of lytic activity after 15 min incubation at 70°C and several foodborne pathogens, such as Clostridium perfringens, Listeria monocytogenes, and Escherichia coli O157:H7 (Choi and Kong, 2023).Another extremophilic enzyme, the Ts2631 endolysin of Thermus scotoductus phage vB_Tsc2631, caused 1.07-3.71log 10 reduction of A. baumannii and P. aeruginosa multidrug-resistant strains in antibacterial assays (Plotka et al., 2019).Subsequently, the MMPphg endolysin derived from thermophilic phage MMP17 was efficacious against Gram-positive and Gramnegative bacteria including nine antibiotic-resistant strains of Klebsiella pneumoniae (Wang et al., 2020).However, not all thermostable endolysins exhibit a broad spectrum of antimicrobial activity.The PhiKo endolysin, described herein, has a narrow spectrum.Similarly, the thermophilic lysozyme from bacteriophage φIN93 lyses specifically only the Thermus sp. cells (Matsushita and Yanase, 2008).The mechanism of such specificity is unknown and requires further studies.However, the T. thermophilus peptidoglycan represents a rare A3β chemotype with L-ornithine at position 3 of the stem peptide subunit (Schleifer and Kandler, 1972;Quintela et al., 1995), which may determine the high specificity of PhiKo endolysin of the Thermus bacteriophage.Gram-positive bacteria have mostly lysine (Lys) at position 3 of the stem peptide and Gram-negative bacteria mostly diaminopimelic acid (DAP; Schleifer and Kandler, 1972).The PhiKo endolysin is thermally stable and its melting temperature is 91.70°C (Figure 5A).The Ts2631 endolysin that shows 49.0% primary sequence identity to PhiKo endolysin has T m = 99.82°C(Plotka et al., 2015), and the Ph2119 endolysin (52.4% primary sequence identity with PhiKo) has T m = 103.56°C(unpublished results).The melting temperature of another thermostable endolysin AmiP of Thermus parvatiensis prophage is 102.6°C(Jasilionis et al., 2023).As can be observed, the melting temperature of all mentioned endolysins differs only by a few degrees and is in a range of 91.70°C-103.56°C.For comparison, the newly discovered AbLys2 endolysin from metavirome of marine biofilm sample that shows lytic activity against mesophilic bacteria A. baumannii has a T m of 47.1°C (Premetis et al., 2023).The addition of EDTA to PhiKo endolysin decreases the T m to 86.0°C (Figure 5B).Since EDTA is a known metal ions chelator, and Zn 2+ ion is present in the catalytic center of the PhiKo enzyme (Figure 2), its removal may result in destabilization of the enzyme structure or/and its inactivation.
The PhiKo endolysin displays its optimum lytic activity at pH 8.0 at 60°C without addition of NaCl.However, it retains more than 72% of initial activity in the presence of NaCl up to 800 mM.For example, Pseudomonas aeruginosa endolysins KZ144 from the giant phage φKZ tolerated high concentrations of NaCl and at a concentration of 500 mM the lytic activity of the enzyme was above 100% (Briers et al., 2007).On the other hand, increasing concentrations of NaCl inhibited the activity of LysB4 endolysin from Bacillus cereus phage B4 resulting in ~60% decrease in activity at 200 mM (Son et al., 2012).These results suggest that the effect of salt concentration on the enzyme activity is a unique property of a particular protein, and not a general trend related to endolysins.Under optimal conditions, PhiKo causes complete lysis of chloroform-treated T. thermophilus substrate within 10 min at a concentration of 25 μg/mL.Nevertheless, the narrow substrate specificity of the PhiKo endolysin precludes its usage as a potential antibacterial agent.
Recent research conducted in our laboratory on the thermostable Ts2631 endolysin revealed an N-terminal highly positively charged region in its amino acid sequence, most probably responsible for permeabilization of the outer membrane of Gram-negative bacteria (Plotka et al., 2019).A similar region with antibacterial properties was found in another lytic protein LysC derived from Gram-positive mesophilic bacterium Clostridium intestinale (Plotka et al., 2020;Szadkowska et al., 2022).Therefore, we decided to screen the amino acid sequence of PhiKo in search for similar regions.With use of the CAMP algorithm, several PhiKo regions with potential antibacterial activities were identified (Supplementary Table 2), and the region with the highest probability of antibacterial properties was selected for synthesis and further analysis.
The synthesized peptide, named RAP-29, is the first AMP derived from a thermophilic protein.In contrast to its parental enzyme PhiKo, RAP-29 showed strong antibacterial properties and lysed all Grampositive and Gram-negative strains used in antibacterial assays with 3.7-7.1 log 10 reduction of bacterial counts.Also, the MIC values ranged from 2 μM for S. hominis KPD 910 and 31 μM for S. aureus KPD 470 and S. aureus KPD 425.The obtained MICs for the RAP-29 peptide were significantly lower when compared to the MICs of another peptide derived from the lytic protein sequence, Intestinalin (P30) where the MIC values were often ≥124 μM (Szadkowska et al., 2022).Moreover, MICs values for peptide HD5 (7-32), which shares 38.24% primary sequence identity with RAP-29 were in a range of 25 μM (for Acinetobacter baumannii 4-MRGN and Enterococcus faecium 475747), and 50 μM for Pseudomonas aeruginosa ATCC 27853 (Ehmann et al., 2019).
The antimicrobial peptides are widespread in nature (Huan et al., 2020), and the cryptic peptides are AMPs that are embedded in larger proteins.An example of such a peptide is human lactoferricin which is released from the iron-binding glycoprotein lactoferrin through proteolysis by pepsin present in the gut.Lactoferricin consists of the N-terminal 49 residues of lactoferrin and similarly to RAP-29, possesses stronger antimicrobial activity than the parental enzyme (Gifford et al., 2005;Hunter et al., 2005).Human lactoferricin has the ability to bind LPS from the outer membrane of Gram-negative bacteria, and bovine lactoferricin (residues 17-41 of bovine lactoferrin) can bind teichoic acid originating from Gram-positive bacteria (Vorland et al., 1999).By the ITC analysis, similar properties of RAP-29 were revealed, as this peptide is able to bind both, the lipopolysaccharide and the lipoteichoic acid.Based on ITC data, it has been proven that LPS, in contrast to LTA, possesses two different sites capable of binding RAP-29.Moreover, the RAP-29 peptide causes bacterial membrane depolarization, as shown by fluorometric measurement with the use of membrane potential-sensitive dye DiSC 3 (5).Loss of membrane potential was also observed for lactoferricin and other antimicrobial peptides, such as gramicidin D (Boix-Lemonche et al., 2020;Gruden and Poklar, 2021).
Recently, cryptic peptides are gaining more attention.By using different algorithms, Nandi et al. (2022) predicted antimicrobial peptides from the protein sequences of A. baumannii specific phages.Anti-biofilm, anti-fungal, and cell-penetrating capacity of these peptides was predicted in silico and three peptides were selected as promising for experimental analysis (Nandi et al., 2022).In 2023, the American company ContraFect Corporation patented lysin polypeptides active against Gram-negative bacteria, such as Pseudomonas aeruginosa, Klebsiella spp., Enterobacter spp., Escherichia coli, Citrobacter freundii, Salmonella typhimurium, Yersinia pestis, and Franciscella tulerensis (Schuch et al., 2023).The peptide sequences were derived from five potential lysins GN2, GN4, GN14, and GN43 produced by phages.Studies have shown that in the presence of polymyxin B, the total pool of peptides named: PGN4, FGN4-1, FGN4-2, FGN4-3, and FGN4-4 (each at a concentration of 25 μg/mL) reduced the number of P. aeruginosa PAO1 cells in human serum by at least 2 log CFU/mL greater than the antibiotic alone.
To the best of our knowledge, our study is the first report on the presence of a peptide, hidden in the sequence of a larger thermophilic protein, with lytic properties against mesophilic Gram-positive and Gram-negative bacteria.These findings are especially important in the era of urgent search for new, effective antibacterial tools.As our results show, the cryptic antimicrobial peptide may have a broader antibacterial spectrum than the parental protein.That sheds new light on antibacterial peptides, indicating that the panel of effective antibacterial peptides may be broader than commonly thought.Therefore, studies of antibacterial peptides as an alternative strategy for antibiotics are still an inexhaustible and interesting direction of research in the light of growing drug resistance among pathogenic bacteria.

Bacterial strains and culture conditions
Staphylococcal strains were cultured at 37°C in tryptic soy broth (TSB; Graso Biotech, Starogard Gdanski, Poland) or solid TSB medium containing 1.5% agar.All other mesophilic bacterial strains were grown at the same temperature in Luria-Bertani (LB) broth or LB agar.Thermophilic bacteria were grown in Thermus 162 medium [see the 878 position on the List of recommended media for microorganisms of the German Collection of Microorganisms and Cell Cultures GmbH (DSMZ)] at 60°C.All bacterial strains were received either from the American Type Culture Collection (ATCC), Collection of Plasmids and Microorganisms, University of Gdansk, Gdansk, Poland (KPD), DSMZ, or MATIS collection of microorganisms, Reykjavík, Iceland (MAT).Pattern of antibiotic resistance for each clinical strain is provided in Supplementary Table 3.

Bioinformatics analysis
A sequence-similarity search was performed using the Basic Local Alignment Search Tool (BLASTN for nucleotide and BLASTP for protein sequence) available at the National Center for Biotechnology Information web page. 1 Protein sequences were aligned with CLUSTAL Omega software (Sievers et al., 2011).The isoelectric point (pI) and molecular weight of the PhiKo endolysin were determined using the IPC 2.0 tool (Kozlowski, 2021).The antibacterial properties of the C-terminal region of PhiKo endolysin and physicochemical properties of the RAP-29 peptide were predicted with the use of Antimicrobial Peptide Calculator and Predictor APD3 (Wang et al., 2016).The antimicrobial activity of the RAP-29 peptide was predicted by the use of Collection of Anti-Microbial Peptides CAMP which is 1 https://blast.ncbi.nlm.nih.gov/blast.cgibased on four different algorithms: Support Vector Machine (SVM), Random Forest (RF), Artificial Neural Network (ANN), and Discriminant Analysis (DA; Thomas et al., 2010).The protein models were predicted by multiple methods, such as ESMFold (Lin et al., 2023), AlphaFold2 (Mirdita et al., 2022), OmegaFold (Sievers et al., 2011), RGN2 (Chowdhury et al., 2022), and RoseTTAFold (Baek et al., 2021) showing only minor differences (the critical residues were modeled consistently regardless of the method used).Furthermore, the models were processed, analyzed and visualized using USCF Chimera viewer (Pettersen et al., 2004).
Bacteria carrying the overexpression plasmid were cultivated at 37°C in 1 L of LB medium supplemented with 100 μg/mL ampicillin to an optical density at 600 nm (OD 600 ) of 0.5.At that point, overproduction of the PhiKo endolysin or its substitution variants was induced by adding isopropyl-β-Dthiogalactopyranoside (IPTG) to a final concentration of 1 mM.Induction proceeded for 4 h at 37°C.Cells were harvested by centrifugation (10,000 × g for 20 min, 4°C) and resuspended in 20 mL of the NPi buffer (50 mM NaH 2 PO 4 , pH 8.0, 300 mM NaCl, 0.1% Triton X-100, 10% glycerol and 1 mM phenylmethylsulfonyl fluoride; PMSF) with 10 mM imidazole.The resuspended cells were sonicated (30 bursts of 10 s at an amplitude of 12 μm), followed by centrifugation and supernatant was loaded onto 1 mL HiTrap TALON crude column coupled to an HPLC chromatography system ÄKTA™ pure 25 (Cytiva).The protein was eluted with 150 mM imidazole in NPi buffer and dialyzed overnight against the HEPES buffer (20 mM HEPES, pH 7.4, 50% glycerol).The purity of the protein was assessed with the use of 12% sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and the concentration was determined by Bradford assay (Bradford, 1976).The protein was stored at −80°C until further analysis.The RAP-29 peptide synthesis was carried out exactly as previously described (Plotka et al., 2020).Size exclusion chromatography (SEC) analysis was performed using a Superdex 75 10/300 GL column on ÄKTA™ pure 25 chromatography system equilibrated with 25 mM

Turbidity reduction assays
The peptidoglycan degrading activity of PhiKo enzyme was evaluated against outer membrane-permeabilized Gram-negative bacterial cells by measuring reductions in optical density at 600 nm (OD 600 ).Substrates of Thermus strains were prepared using chloroform-Tris-HCl technique.Briefly, cells were grown at 60°C to an OD 600 between 0.6-1.0,pelleted, and resuspended in 50 mM Tris-HCl, pH 7.7 saturated with chloroform.Samples were incubated for 45 min at room temperature with gentle shaking, washed with 50 mM Tris-HCl, pH 7.7, and lyophilized.Substrates were kept at −80°C, and before use were suspended in 20 mM HEPES, pH 7.4 (or indicated buffer) to an OD 600 of 1.0.PhiKo endolysin (10 μL) was combined with chloroform-treated cells (190 μL) to achieve protein final concentration range of 1.56 to 100 μg/mL, and the change in OD 600 was measured over time using EnSpire multimode plate reader (PerkinElmer).The lytic activity of PhiKo endolysin was calculated at specific condition as follows: (ΔOD 600 control − ΔOD 600 sample with endolysin)/initial OD 600 , as previously described (Plotka et al., 2015).
To evaluate the effect of divalent metal ions on PhiKo endolysin function, Thermus thermophilus substrate was prepared as described above and suspended in 20 mM HEPES, pH 7.4 buffer with or without 0.1 mM and 1.0 mM ions (CoCl 2 , NiCl 2 , ZnCl 2 , FeCl 2 , Mn(CH 3 COO) 2 , MgCl 2 , and CaCl 2 ).To chelate metal ions attached to the PhiKo endolysin, 5.0 mM EDTA was added to 5 μg of the enzyme and incubated for 30 min at 60°C.Subsequently, the endolysin was dialyzed overnight against 20 mM HEPES, pH 7.4.The lytic activity of EDTAtreated enzyme was compared to the one without EDTA treatment and without cation substitution.In all negative controls, 20 mM HEPES, pH 7.4 buffer instead of the PhiKo endolysin was added to the cell suspension.All experiments were performed in triplicate.

Antibacterial tests
The antibacterial activity of PhiKo endolysin was assayed against mesophilic bacteria listed in Supplementary Table 1.Briefly, bacterial cells were grown in TSB (staphylococci) or LB broth (other mesophilic bacteria) at 37°C to OD 600 of 0.5.Bacterial cultures were harvested (4,000 × g for 15 min, 4°C), washed with 20 mM HEPES, pH 7.4 and diluted 100-fold in the same buffer to a final density of ~10 6 cells/ mL.Fifty μL of PhiKo endolysin or RAP-29 peptide were added to 400 μL of cells to achieve the final concentrations of 500 μg/mL and 20 μg/mL of the protein and peptide, respectively.After 90 min of incubation at 37°C, the mixtures were serially diluted and spread onto TSB or LB plates to determine the colony forming units (CFUs).The antibacterial activity was presented as the relative inactivation in logarithmic units (=log10 (N 0 /N i ), where N 0 = the number of residual cells (in the negative control) and N i = the number of viable cells counted after incubation).For the negative control, the same volume of buffer was added instead of PhiKo endolysin or RAP-29 peptide.All experiments were performed in triplicate.

Minimum inhibitory concentrations
The MIC of the RAP-29 peptide was determined by the microdilution method in Difco™ Mueller-Hinton broth (MHB; ThermoFisher Scientific), as indicated by the Clinical and Laboratory Standards Institute (CLSI).Briefly, bacteria were grown overnight at 37°C and next day the number of mid-logarithmic bacterial cells was adjusted to 0.5 McFarland standard, diluted 100× to a density of 10 6 CFU/mL and transferred into a 96-well round-bottom microtiter plate (90 μL/well).Two-fold serial dilutions of PhiKo peptide were prepared in MHB and placed in triplicate in a plate (10 μL/well) to achieve the final concentrations of the peptide ranging from 124 to 1.95 μM.The assays were incubated at 37°C for 24 h.MIC was determined as the lowest concentration of PhiKo peptide which completely prevented visible growth of the tested bacterial strain.

Transmission electron microscopy
Overnight culture of T. thermophilus HB8 cells was used to inoculate 20 mL of the 162 medium at 60°C and grown until exponential growth was reached.The cells were centrifuged, washed and resuspended in 20 mM Tris-HCl, pH 8.0 to a final concentration of ~10 7 cells in a volume of 500 μL.The bacteria were incubated at 60°C for 10 min with PhiKo endolysin (6.25 μg/mL).As a control, buffer without protein was used.After incubation, bacteria were centrifuged and the pellet was fixed with 2.5% glutaraldehyde and post-fixed with 1% osmium tetroxide (Polysciences Inc.).Samples were dehydrated with ethanol and embedded in Epon 812 resin (Sigma-Aldrich).Ultrathin sections (60 nm) were obtained with ultramicrotome (Leica UC7), and stained with lead citrate and uranyl acetate (Sigma-Aldrich).TEM analyses were performed at the Laboratory of Electron Microscopy (Faculty of Biology, University of Gdansk, Poland).Bacteria were visualized using Tecnai Spirit BioTwin electron microscope (FEI Company).

Sedimentation velocity analytical ultracentrifugation
The SV-AUC experiments were performed using a ProteomeLab XL-I analytical ultracentrifuge (Beckman-Coulter, Inc.), equipped with An-50, 8-hole analytical rotor and double-sector charcoal-Epon cells (12 mm path length).The experiments were carried out at 50,000 rpm, in 20 mM MES, 150 mM NaCl, pH 6.0 in the presence or absence of 10.3389/fmicb.2023.1303794Frontiers in Microbiology 14 frontiersin.org20 mM DPC (dodecylphosphocholine) detergent at 4°C, using continuous scan mode and radial spacing 0.003 cm. 100 scans were collected with 8 min intervals between scans, both in the absorbance (280 nm) and interference mode.Cells were loaded with 400 μL of PhiKo endolysin (1.2 mg/mL) and 410 μL of buffer.Solvent densities (1.00851 g/cm 3 without DPC and 1.00871 g/cm 3 with DPC) and viscosities (1.581 without and 1.611 mPa s with DPC) were measured at 4°C using Anton Paar (Graz, Austria) DMA 5000 densitometer and Lovis 2000 M rolling-ball viscometer, respectively.Partial specific volume and extinction coefficients for proteins were calculated using the SEDNTERP software (Philo, 2011).Data were analyzed using the "Continuous c(s) distribution" model of the SEDFIT program (Schuck, 2000), with confidence level (F-ratio) specified to 0.68.The result were plotted using GUSSI graphical program (Brautigam, 2015).

Differential scanning calorimetry
For calorimetric experiments, the untreated or 5 mM EDTAtreated PhiKo endolysin was dialyzed against 20 mM MES, pH 6.0.The measurements were conducted on a VP-DSC microcalorimeter (MicroCal Inc.) with a scan rate of 90°C/h, a filtering period of 20 s, and with a prescan thermostat time of 15 min.To perform a DSC measurement of the protein unfolding process, the reference cell was filled with buffer, and the sample cell was filled with the PhiKo endolysin at a concentration of 1 mg/mL in 0.5 mL volume (before the mentioned step, the reproducibility of the baseline scan was done).PhiKo samples and buffers were degassed (5 min vacuum treatment) before loading into the calorimeter.All of the scans were run at a temperature range of 5°C to 110°C.The reversibility of the transition was checked by cooling and reheating the same sample and the measurements were recorded three times.The Origin 7.0 software for measuring instruments from MicroCal, was used for data analysis.The quantity measured by DSC is the difference between the heat capacity of MES buffer-protein solution and that of pure MES buffer.During DSC measurements, heat absorption causes a temperature difference (ΔT) between the cells when a protein unfolds.

Isothermal titration calorimetry
The ITC experiments were performed using the AutoITC isothermal titration calorimeter (MicroCal Inc.) at 25°C.The procedure was performed according to Panuszko et al. (2009).Briefly, lipoteichoic acid (LTA) from S. aureus or lipopolysaccharide (LPS) from P. aeruginosa 10 (both from SIGMA-Aldrich) and RAP-29 peptide were dissolved in 20 mM potassium phosphate buffer, pH 8.0, 10% glycerol.The RAP-29 peptide at concentration of 0.5 mM was gradually injected (29 injections for at 4-min intervals, 2 μL for the first injection only) into the reaction cell containing 0.05 mM solution of LTA or LPS.A background titration, consisting of the identical titrant solution but only the buffer solution in the sample cell, was subtracted from each experimental titration to account for heat of dilution.Mixing was carried out at constant 300 rpm.The standard procedure (CaCl 2 − EDTA titration) was performed to validate the apparatus and the stoichiometry, K, ΔH results were compared with those obtained for the test kit from Malvern Instruments Ltd. (Malvern, United Kingdom).

Circular dichroism spectroscopy
To study the secondary structure of RAP-29 peptide, circular dichroism (CD) spectroscopy was performed with the use of Spectropolarimeter J-815 (Jasco) equipped with a 1-mm path length quartz cell.The spectra of RAP-29 (43 μM) were recorded at 25°C from 185 to 260 nm at 0.1-nm intervals.The peptide was dissolved in water or 20 mM micelles of Lauryl-β-D-maltoside (DDM), Dodecylphosphocholine (DPC), Lauryldimethylamine N-oxide (LDAO) and Sodium dodecyl sulfate (SDS).Each spectrum corresponded to the mean of six scans.The CD results were expressed as mean residue ellipticity (θ) in degree × cm 2 × dmol -1 .

Determination of membrane potential
Cells of mid-log phase S. aureus ATCC 25923, suspended at 1 × 10 6 CFU/mL in 20 mM HEPES, pH 7.4, were incubated with 1 μM 3,3-Dipropylthiadicarbocyanine iodide dye DiSC 3 (5) in the presence of 1% DMSO.Cell suspension in a volume of 200 μL was added in triplicate to the wells of a black 96-well polystyrene microtiter plate (OptiPlate, PerkinElmer), and the plate was preincubated at 37°C for 25 min in the dark.Subsequently, fluorescence was monitored (excitation 652 nm, emission 672 nm) at 1 min intervals using EnSpire multimode plate reader (PerkinElmer).When the readings were stabilized, the plate was ejected, and RAP-29 peptide was added in triplicate to a final concentration between 0.5 μM to 10 μM.The fluorescence was measured again for 15 min at 1 min intervals.10 μM LL-37 peptide (Sigma-Aldrich) served as a positive control.

Protein sequence accession numbers
The GenBank accession number for the protein sequence of the PhiKo endolysin is AYJ74695.

FIGURE 1
FIGURE 1Multiple sequence alignment of PhiKo endolysin with similar proteins from the NCBI GeneBank database.Sequences of PhiKo endolysin (accession no AYJ74695.1),two thermostable endolysins Ph2119 and Ts2631 (accession no AHF20915.1 and AIM47292.1,respectively), PGRP from metagenome of Thermus sp.(accession no MDM7323587.1),PGRP SC2-like protein from Musca domestica (accession no NP_001295936.1),and T7 lysozyme (accession no AAB32819.1)were aligned with use of CLUSTAL Omega program.Black background represents 100% amino acid sequence identity, while gray shading reflects the amino acid conservation at 70% consensus.Red triangles indicate residues involved in Zn 2+ binding: His27, His133 and Cys141.Yellow triangles highlight two additional residues, Tyr55 and Lys140 potentially responsible for PhiKo enzyme catalytic function.The sequence of RAP-29 peptide investigated within this work is marked with a red box.

FIGURE 3
FIGURE 3 Purification and oligomeric state of the enzyme.(A) 12.5% SDS-PAGE gel of the purified PhiKo endolysin after dialysis into storage buffer (20 mM HEPES, pH 7.4, 50% glycerol).Predicted molecular mass of the recombinant enzyme with N-terminal His-tag is 21.7 kDa.M-marker proteins (PageRuler Prestained Protein Ladder, Thermo Scientific).The molecular masses of reference proteins (in kilodaltons) are indicated on the left.(B) Elution profile of PhiKo endolysin on Superdex 75 10/300 GL column.The position of molecular mass standards are shown as arrows, conalbumin 75 kDa, carbonic anhydrase 29 kDa, and aprotinin 6.5 kDa.mAU-milli-Absorbance Units (C) Degree of oligomerization of the PhiKo endolysin in the absence (red line) or presence (blue line) of n-dodecylphosphocholine (DPC) detergent.Green line corresponds to the control-buffer with DPC.

FIGURE 4
FIGURE 4 Lytic activity of PhiKo endolysin.(A) Dose dependent reduction in turbidity of chloroform-treated Thermus thermophilus HB8 cells suspended in 20 mM HEPES, pH 7.4.Increase in the enzyme activity was proportional to the enzyme concentration until saturation was achieved (100 μg/mL of endolysin within 10 min of assay).Error bars represent means ± standard deviations.Each experiment was repeated in triplicate.(B) Effect of divalent metal ions on PhiKo endolysin activity.The addition of 1 mM ZnCl 2 restored the activity of the EDTA-treated enzyme to 63.1% compared to the control (C) Influence of pH on the PhiKo endolysin specific activity.Endolysin showed optimum activity at pH 8.0.(D) Effect of NaCl concentrations was assessed and maximum activity was achieved without salt addition and activity was above 70% at 25-800 mM of NaCl.(E) PhiKo endolysin withstands temperatures up to 100°C with above 80% activity at temp.Between 37°C and 100°C.(F) Activity of the PhiKo endolysin after heating at 100°C for 1 to 5 h in comparison to the untreated control.PhiKo residual activity was at the level of 77.3% ± 1.5% after 5 h heat-treatment.(G) Dose dependent reduction in Thermus thermophilus HB8 cell suspension turbidity under optimal conditions of 20 mM Tris-HCl, pH 8.0 at 60°C without salt addition.(H) Transmission electron microscope (TEM) observation of cell morphology of PhiKo-treated T. thermophilus HB8 cells.The scale bar represents 1 μm.

FIGURE 5
FIGURE 5Heat-capacity curves of the PhiKo endolysin determined by DSC (black line) and the fit to the non-two state model (red solid line) in the absence (A) or presence (B) of 0.5 mM EDTA recorded in 20 mM MES, pH 6.0.Tm-melting temperature, the temperature at which 50% of the protein is unfolded.

FIGURE 6
FIGURE 6 Substrate specificity of the PhiKo endolysin.Chloroform permeabilized Gram-negative bacteria Thermus thermophilus HB8, T. thermophilus HB27, Thermus flavus ATCC 1087, Thermus parvatiensis DSM 21745, T. scotoductus MAT2631, and Gram-positive Deinococcus radiodurans ATCC 13939 were prepared and used as a substrate in turbidity reduction assay.The 100% activity corresponds to the highest decrease obtained among the dataset.Experiments were performed in triplicate; error bars indicate standard deviations.

FIGURE 7 C
FIGURE 7 C-terminal region of the PhiKo endolysin with potential antibacterial properties (A) Antimicrobial peptide prediction of the C-terminal region of PhiKo endolysin with the use of Collection of Anti-Microbial Peptides (CAMP R3 ).A peptide is predicted to be antimicrobial if the probability is ≥0.5 (B) Structural model of PhiKo endolysin with the position of the peptide sequence highlighted in black (C) Physicochemical properties of the RAP-29 peptide analyzed by the Antimicrobial Peptide Calculator and Predictor (APD3).

FIGURE 8
FIGURE 8 Mechanistic insights into the activity of RAP-29.Calorimetric titration isotherms of the binding interactions between RAP-29 and (A) lipoteichoic acid (LTA) of Staphylococcus aureus and (B) lipopolysaccharide (LPS) of Pseudomonas aeruginosa in 20 mM potassium phosphate buffer, pH 8.0 at 25°C.(C) Circular dichroism spectra of RAP-29 peptide show α-helical conformation of the peptide in the presence of 20 mM detergents DDM, LDAO, SDS, and DPC.Without addition of detergents RAP-29 is in a randomly coiled state; DDM-Lauryl-β-D-maltoside; LDAO-Lauryldimethylamine N-oxide; SDS-Sodium dodecyl sulfate; DPC-n-dodecylphosphocholine.(D) Bacterial membrane potential monitored with DiSC 3 (5) in the absence (control) or in the presence of 10 μM LL-37 (positive control) and increasing concentrations of RAP-29 (0.5 to 10 μM).The membrane potential sensitive dye DiSC 3 (5) was incubated with bacteria until a stable baseline was formed.The time point of RAP-29 and LL-37 addition is highlighted with an arrow.Fluorescence increase upon addition of peptides was measured at excitation wavelength of 652 nm and an emission wavelength of 672 nm as a function of time.Experiments were performed in triplicate; error bars indicate standard deviations.

TABLE 1
Bactericidal activity of the RAP-29 peptide against Grampositive staphylococci and Gram-negative bacteria.
NaH 2 PO 4 , pH 8.0, 150 mM NaCl.The column was with 300 μL of PhiKo endolysin at a concentration of 1 mg/mL and the flow rate was set to 0.8 mL/min.The absorbance was measured at 280 nm (mAU, milli-absorbance units).Gel Filtration Calibration Kit Low Molecular Weight (Cytiva) was used to calibrate the column prior experiment.