Isolation and Characterisation of Bacteriophage Selective for Key Acinetobacter baumannii Capsule Chemotypes

Nineteen bacteriophages against five main capsular types of multidrug-resistant Acinetobacter baumannii were isolated from tertiary care hospital sewage. Eight representative phages from each capsular type were characterized and tested for their biological properties. The biological features revealed that phages T1245, T444, and T515 had a large burst size of more than 420 pfu/mL, together with a short latent period lasting less than 6 min, and were readily adsorbed to a bacterial host within 10 min. Moreover, these phages demonstrated host specificity and stability over a broad range of temperatures (−20 to 60 °C) and pH (5.0–9.0). A whole-genome analysis of six lytic and two temperate phages revealed high genomic similarity with double-stranded DNA between 40 and 50 kb and G + C content of 38–39%. The protein compositions disclosed the absence of toxin-coding genes. The phylogenic results, together with morphological micrographs, confirmed that three selected phages (T1245, T444, and T515) belong to the Podoviridae family within the order Caudovirales. The biological data and bioinformatics analysis indicated that these novel A. baumannii phages possess important enzymes, including depolymerase and endolysin, which could be further developed as promising alternative antibacterial agents to control A. baumannii infections.


Introduction
Acinetobacter baumannii is an emerging opportunistic Gram-negative pathogen that is associated with frequent and severe infections in the immunocompromised and in patients with prolonged hospitalization or long-term exposure to antimicrobials. The high prevalence and incidence of drug-resistant strains of A. baumannii in both developing and developed countries have been increasingly reported [1,2]. The growing resistance of A. baumannii to antimicrobial treatment is a serious challenge, causing adverse clinical effects associated with high economic costs [3]. Some strains of A. baumannii invariably produce capsular polysaccharides, which promote survival and adaptation to various environmental conditions, and may contribute to antimicrobial resistance and the evasion of host immune defenses [4]. K units are assembled on the lipid carrier molecule for growing sugar chains.

Phage Isolation, Purification, and Plaque Characterisation
A total of twenty phage selective for MDR A. baumannii were isolated from sewage water samples derived from major national referral hospitals in Thailand (Supplementary  Table S1). After incubation at 37 • C for 12 h with different primary host strains, lytic phages formed clear plaques with different morphology and zones of lysis between 0.5 and 10.0 mm in diameter (Figure 1). The plaques from some phages, such as P515, were surrounded by translucent halos that increased in diameter over the time of incubation while the plaque size remained constant (Supplementary Figure S1), indicating the production of polysaccharide depolymerases [22]. while the plaque size remained constant (Supplementary Figure S1), indicating the production of polysaccharide depolymerases [22].

Determination of Phage Host Range
In this study, the lytic spectrum was determined by spot tests onto the lawns formed by 49 strains of MDR A. baumannii belonging to the most common capsular types (KL2, KL3, KL6, KL10, KL47, KL49, and KL52) (Supplementary Table S2). Our results further confirmed that most of the A. baumannii phages were host-specific; thus, they could infect or lyse only a single or limited number of different capsular types ( Figure 2). However, plaque formation on the lawn formed by five capsular types (KL3, KL6, KL10, KL47, and KL52) were detected. Some phages demonstrated almost 100% lytic activity, including P1033 and P245 on KL6 strains, P1245, T1245, T55, P521, S419, and P79 on KL10 strains, T17, P92, T92, P515, T515, and P79 on KL47 strains, and T444, P444, P24, and P79 on KL52 strains (Supplementary Table S2). Three phages demonstrated a host range of three different capsule types; P1051 and S419 were active against KL3, KL6, and KL10, while phage P79 was active against KL10, KL47, and KL52 strains. Nine phages that could infect different capsular types of MDR A. baumannii were selected for further study based on the results of the host range determination. baumannii. (a) Big and bright plaque (8-10 mm) on KL10 isolate, (b) medium-size and bright plaque (5-7 mm) on KL10 isolate, (c) small and slightly dim plaque (2-4 mm) on KL6 isolate, and (d) extremely small and slightly dim plaque (0.5-1 mm) on KL52 isolate.

Determination of Phage Host Range
In this study, the lytic spectrum was determined by spot tests onto the lawns formed by 49 strains of MDR A. baumannii belonging to the most common capsular types (KL2,  KL3, KL6, KL10, KL47, KL49, and KL52) (Supplementary Table S2). Our results further confirmed that most of the A. baumannii phages were host-specific; thus, they could infect or lyse only a single or limited number of different capsular types ( Figure 2). However, plaque formation on the lawn formed by five capsular types (KL3, KL6, KL10, KL47, and KL52) were detected. Some phages demonstrated almost 100% lytic activity, including P1033 and P245 on KL6 strains, P1245, T1245, T55, P521, S419, and P79 on KL10 strains, T17,  P92, T92, P515, T515, and P79 on KL47 strains, and T444, P444, P24, and P79 on KL52 strains  (Supplementary Table S2). Three phages demonstrated a host range of three different capsule types; P1051 and S419 were active against KL3, KL6, and KL10, while phage P79 was active against KL10, KL47, and KL52 strains. Nine phages that could infect different capsular types of MDR A. baumannii were selected for further study based on the results of the host range determination.

Phage Adsorption
The adsorption assay was used to evaluate the ability of phages to bind to primary host bacterial cells ( Figure 3). Within 10 min of the initiation of infection, the adsorption rates for phage T1245, T444, T515, T17, T92, P521, and P1033 ranged from 79 to 99%. Approximately 50% of the phage particles adsorbed to A. baumannii strains were observed for P1051 and P245 at 8 min post-infection.

Life Cycle of Phage
A single growth cycle ( Figure 4) was conducted with the primary host strain to determine the latent period and burst size of individual phages, which are important characteristics of the phage infection process. The analysis showed a latent period of 2, 6, 2, 4, 6, and 4 min for six phages (T1245, T444, T515, T17, T92, and P521, respectively) (Supplementary Figure S2) and 10, 20, and 40 min for three phages (P1051, P1033, and P245, baumannii. Phages P1051, S419, and P79 were able to infect bacteria with three distinct capsular types. Three different color bars indicate phages P1051, S419, and P79 that could infect three capsular types.

Phage Adsorption
The adsorption assay was used to evaluate the ability of phages to bind to primary host bacterial cells (Figure 3). Within 10 min of the initiation of infection, the adsorption rates for phage T1245, T444, T515, T17, T92, P521, and P1033 ranged from 79 to 99%. Approximately 50% of the phage particles adsorbed to A. baumannii strains were observed for P1051 and P245 at 8 min post-infection.

Phage Adsorption
The adsorption assay was used to evaluate the ability of phages to bind to primary host bacterial cells ( Figure 3). Within 10 min of the initiation of infection, the adsorption rates for phage T1245, T444, T515, T17, T92, P521, and P1033 ranged from 79 to 99%. Approximately 50% of the phage particles adsorbed to A. baumannii strains were observed for P1051 and P245 at 8 min post-infection.

Life Cycle of Phage
A single growth cycle ( Figure 4) was conducted with the primary host strain to determine the latent period and burst size of individual phages, which are important characteristics of the phage infection process. The analysis showed a latent period of 2, 6, 2, 4, 6, and 4 min for six phages (T1245, T444, T515, T17, T92, and P521, respectively) (Supplementary Figure S2) and 10, 20, and 40 min for three phages (P1051, P1033, and P245,

Stability Tests
The desirable characteristics of candidate phages for therapeutic applications should include stability under different conditions of temperature and pH as well as the ability to maintain infectivity after long-term storage. The phage stability was investigated at different temperatures and pH conditions. As shown in Figure 5, most phages were stable at temperatures ranging from −20 to 60 °C when exposed for 2 h. At 60 °C, a significant decrease of more than >50% in the survival rate was observed for phage P1033 when compared with the control at 37 °C. However, no phage showed lytic activity after incubation at 70 °C. Most phages showed greater than 80% viability over a broad pH range (5.0 to 9.0) after incubation for 2 h. However, 47.6% survival was observed for phage P1033 at pH 9 ( Figure 6). The results suggested that the infectivity of the phage remained intact when exposed to broad temperature and pH conditions. Stock titers were stable for at least two years in SM buffer at 4 °C. However, a slight decrease was observed in titers for some phages (Table S1).

Stability Tests
The desirable characteristics of candidate phages for therapeutic applications should include stability under different conditions of temperature and pH as well as the ability to maintain infectivity after long-term storage. The phage stability was investigated at different temperatures and pH conditions. As shown in Figure 5, most phages were stable at temperatures ranging from −20 to 60 • C when exposed for 2 h. At 60 • C, a significant decrease of more than >50% in the survival rate was observed for phage P1033 when compared with the control at 37 • C. However, no phage showed lytic activity after incubation at 70 • C. Most phages showed greater than 80% viability over a broad pH range (5.0 to 9.0) after incubation for 2 h. However, 47.6% survival was observed for phage P1033 at pH 9 ( Figure 6). The results suggested that the infectivity of the phage remained intact when exposed to broad temperature and pH conditions. Stock titers were stable for at least two years in SM buffer at 4 • C. However, a slight decrease was observed in titers for some phages (Table S1).

Genome Annotation and Analysis
The complete genome sequences were determined by high-throughput sequencing. The phylogenetic tree figure represents the DNA relatedness among nineteen phages based on whole-genome sequences ( Figure 7) and the distance matrix between two DNA sequences (Supplementary Table S3). The dendrogram for nineteen phages was drawn based on sequence comparison with 138 Acinetobacter Caudvirales phages in GenBank assemblies to examine the distribution of A. baumannii phages ( Figure 8) and a tab-delimited matrix of the MASH distances between each pair of isolates was presented as supplementary data (Supplementary Table S4). The results from taxonomy-based phylogeny, together with TEM images (Supplementary Figure S3), confirmed that eight phages (P444, P24, P105, P1033, P245, P1257, P373, and P79) and eleven phages (P1245, T1245, T444, P515, T515, T55, T17, P92, T92, P521, and P45) were designated to the Myoviridae and Podoviridae (Autographivirinae subfamily) family, respectively, as members of order Caudovirales, following the current guidelines of the ICTV (International Committee on

Genome Annotation and Analysis
The complete genome sequences were determined by high-throughput sequencing. The phylogenetic tree figure represents the DNA relatedness among nineteen phages based on whole-genome sequences ( Figure 7) and the distance matrix between two DNA sequences (Supplementary Table S3). The dendrogram for nineteen phages was drawn based on sequence comparison with 138 Acinetobacter Caudvirales phages in GenBank assemblies to examine the distribution of A. baumannii phages ( Figure 8) and a tab-delimited matrix of the MASH distances between each pair of isolates was presented as supplementary data (Supplementary Table S4). The results from taxonomy-based phylogeny, together with TEM images (Supplementary Figure S3), confirmed that eight phages (P444, P24, P105, P1033, P245, P1257, P373, and P79) and eleven phages (P1245, T1245, T444, P515, T515, T55, T17, P92, T92, P521, and P45) were designated to the Myoviridae and Podoviridae (Autographivirinae subfamily) family, respectively, as members of order Caudovirales, following the current guidelines of the ICTV (International Committee on

Genome Annotation and Analysis
The complete genome sequences were determined by high-throughput sequencing. The phylogenetic tree figure represents the DNA relatedness among nineteen phages based on whole-genome sequences (Figure 7) and the distance matrix between two DNA sequences (Supplementary Table S3). The dendrogram for nineteen phages was drawn based on sequence comparison with 138 Acinetobacter Caudvirales phages in GenBank assemblies to examine the distribution of A. baumannii phages ( Figure 8) and a tab-delimited matrix of the MASH distances between each pair of isolates was presented as supplementary data (Supplementary Table S4). The results from taxonomy-based phylogeny, together with TEM images (Supplementary Figure S3), confirmed that eight phages (P444, P24, P105, P1033, P245, P1257, P373, and P79) and eleven phages (P1245, T1245, T444, P515, T515,  T55, T17, P92, T92 Eight phages (T1245, T444, T515,  T17, T92, P521, P1033, and P245) were selected for further study as the results of the host range determination (phages against different KL strains) and genomes have been fully sequenced. Based on life cycle, phages were grouped as virulent or temperate. Six of the phages were classified as lytic or virulent, including T1245, T444, T515, T17, T92, and P521. According to the turbid plaques and the presence of integrase genes in their genomes, P1033 and P245 were considered as temperate phages. The analysis of the whole-genome sequence revealed that seven of the eight phages (T1245, T444, T515, T17, T92, P521, and P245) had a genome length between 40 and 50 kb, while P1033 had a genome of 136 kb. The genome of phages had an average G + C content of 38-39% and showed a similar pattern of 39% of the host's average genome. The correlation between the host and phage genomic G + C content is involved in phage and host evolution, indicating that they occurred during the same period. It is now accepted that horizontal gene transfer regularly occurs between bacteriophages and their hosts. This study is similar to the 39.15% G + C content reported for the genome of Abp1 (GenBank Acc. No. NC_021316), a lytic phage against A. baumannii. Phages T1245, T444, T515, T717, T92, and P521 displayed more than 90% homology to four phages belonging to the Autographiviridae subfamily, including Acinetobacter IME200 (GenBank Acc. No. NC_028987), Acinetobacter phiAB1 (GenBank Acc. No. NC_028675), Acinetobacter vB_AbaP_AS12 (GenBank Acc. No. NC_041914), and Acinetobacter phage Fri1 (GenBank Acc. No. NC_028848.1). A high percentage of the genomes of the sequenced phages, 80-90%, are represented by coding sequences (CDSs). According to the identification of coding sequences, the six lytic phages consisted of 47-54 CDSs, and 49-63% of genes were predicted as putative functional proteins. The genomes of phage P245 and P1033 were found to contain 59 and 180 CDSs, respectively, of which 28% and 24% of genes were predicted to encode proteins of known function, respectively (Supplementary Table S5). The known functions of CDSs encoding proteins were divided into several groups, including structure and morphogenesis, tRNA nucleotidyltransferase, DNA synthesis, regulation and replication, lysis, and homing endonuclease (Supplementary Table S6). Among these phages, no gene associated with antibiotic resistance or toxin production was found. The commonly presented genes in more than 50% of phages in this study are presented in Table 1. The results of the conserved sequence segments by a progressive Mauve alignment indicated that most of the protein functions were similar within six phages (T1245, T515, T17, T92, P521, and T444) and two phages (P1033 and P245), but the CDSs organization and direction were different (Supplementary Figure S4).      Whole-genome neighbor-joining phylogeny inferred from MASH distances of assemblies in the GenBank data set. The isolated phages used in this study are in red color, the family/genus of each phage is represented as a colored background, and a tab-delimited matrix of the MASH distances between each pair of isolates is presented as supplementary data.

Discussion
The global prevalence of drug resistance in clinical isolates of A. baumannii is a public health concern. Therefore, alternative strategies to treat infections caused by MDR A.
baumannii are urgently needed. Phage therapy, the use of bacteriophage viruses to treat bacterial infections, is widely being reconsidered as an alternative to antibiotics. The host range of a bacteriophage is an important feature to be considered in the selection of phages for potential therapeutic applications. The range of bacterial hosts that can be infected by an individual phage may vary considerably and some phages, such as those active against Klebsiella spp, may infect bacteria of different genera [23,24]. In contrast, phages against A. baumannii have been reported to infect only Acinetobacter spp. [25]. A limited host range is beneficial in restricting the killing of other bacterial species and preventing the disruption of the microbiota. The narrow host specificity of phage could mitigate the development of resistance, which is an advantage over antibiotics [26]. Previous studies revealed that two A. baumannii lytic phages belonging to Myovirus and Podovirus were able to propagate on approximately 53% (15 of 28) of tested strains [27]. In this study, phages were isolated against five common capsular types of A. baumannii. Lytic phages including T1245, T444, and T515 could infect all strains of their host KL type. None of the isolated phages in this study were active against A. baumannii KL2 and KL49 capsule types, indicating the absence of phage-specific receptors on host cell surfaces, which predominantly influences the host range of phages. Within 10 min of the initiation of infection, the adsorption rate for phages T1245, T444, and T515 ranged from 80 to 99%. These phages had larger burst sizes with shorter latent periods, compared with previously isolated Acinetobacter phages of the order Caudovirales [27]. Furthermore, the selected phages are relatively stable over a wide range of pH and temperatures, which are important in both storage conditions and transportation for use in a clinical scenario. The genome sequences of three lytic phages (T1245, T444, and T515) showed more than 90% homology to other genomes annotated as Acinetobacter phages, including IME200, phiAB1, vB_AbaP_AS12, and Fri1. Phages T1245, T444, and T515 have evolved various virion-associated proteins with depolymerase activity and endolysin. Bacteriophages have specific recognition for receptors located on the bacterial cell surface, such as capsular polysaccharides and extracellular polysaccharides. The presence of depolymerases is described and characterized in the phage virion within the tail fibers or tailspikes. The genes encoding tail fiber proteins were presented in all the selected A. baumannii phages. Phage-encoded capsule depolymerases from a tail fiber protein of IME200 was previously reported [28]. Certain studies have represented the relationship of these genes with the capsular polysaccharides function as primary receptors on the bacterial surface [29][30][31]. Moreover, in this study, the genome sequences of three lytic phages disclosed no protein toxin-coding genes.
As natural killers of bacteria, phages are recognized as promising alternatives to antibiotics in treating pulmonary bacterial infections. Phage therapy has been applied in personalized therapy in the treatment of CRAB in a patient with chronic obstructive pulmonary disease [32]. The development of phage-based therapy combined with antibiotics has been demonstrated to enhance the antibacterial effects in Gallerai mellonella models [33,34]. Recently, the use of phage cocktails with antibiotics resulted in the reduction in A. baumannii biofilm in human urine models [35]. Due to the ability of phage-derived systems to integrate plasmid DNA into the host's chromosomes, phages containing the integrase gene can be used as a viral vector-mediated gene therapy [36]; therefore, the temperate phages in this study (P1033 and P245) could be candidates. Moreover, phage therapy could be used in secondary A. baumannii infections in critical coronavirus disease (COVID-19) patients with antibiotic treatment failure [37]. However, further evaluation in well-designed clinical trials is required to confirm the potential of phage in future studies.

Isolation of Bacteriophages
The protocol described by Clokie and Kropinski (2009) was used for phage isolation, with minor modifications [38]. Briefly, sewage water samples were collected from hospitals in Thailand. Ten milliters of sewage water sample was mixed with 0.3 g of TSB powder and then inoculated with 100 µL of overnight bacterial culture. After overnight incubation at 37 • C with continuous shaking, the mixture was centrifuged at 5000× g for 20 min. The supernatant was filtered through a 0.45 µm membrane filter (Millipore) and kept at 4 • C until use. An agar overlay method was used for the examination of bacteriophage activity; an overnight bacterial culture was mixed with molten soft nutrient agar (0.75% agar) and immediately poured onto a 1.5% agar plate. Ten milliters of supernatant was dropped onto the plate, and the plate was incubated overnight at 37 • C.

Purification of Bacteriophages
Single plaques were picked from the plate with a sterile pipette tip, transferred to sterile SM buffer (100 mM NaCl, 8 mM MgSO 4 • 7H 2 O, 50 mM Tris-Cl; pH 7.5), and stored at 4 • C. The solution was diluted tenfold in SM buffer and mixed with TSB containing 200 µL of log-phase bacterial culture at an optical density (OD) 600 of 0.8-0.9. An agar overlay method was used for the purification and determination of the phage titer [39]. The single plaque isolation procedure was repeated three times to obtain purified bacteriophage.

Phage Lysate Preparation
The plate containing purified phage with a high phage titer was mixed with 5 mL of SM buffer and incubated overnight at 4 • C. The supernatant was collected and centrifuged at 5000× g for 30 min at 4 • C. The pellet was discarded and the phage lysate was filtered through a sterile 0.45 µm filter. Subsequently, 1 µL/mL of chloroform was added and the bacteriophage stock was kept at 4 • C until used.

Determination of Phage Host Range
The host range of each phage was determined by spotting onto each of the 49 A. baumannii as described previously [40]. In brief, a TSA plate was overlaid with molten soft nutrient agar (0.8% agar) containing 200 µL of each log-phase A. baumannii isolate and spotted with 10 µL of phage lysate. Plates were dried and incubated at 37 • C to assess the lytic activity.

Phage Adsorption
The adsorption of phages to the bacterial host was examined as described by Hua et al. (2018) [41], with minor modifications. Exponentially grown A. baumannii was adjusted to 10 8 cfu/mL and mixed with phage lysate at an MOI of 0.01. After incubation at 37 • C for 10 min, 100 µL of sample was added into 900 µL of cold TSB, centrifuged at 13,000× g for 5 min to eliminate debris, and the supernatant was filtered through a sterile 0.45 µm membrane filter. The supernatants were used for plaque assays to determine the titers of the non-adsorbed phages. Adsorption curves were constructed based on the percentage of non-adsorbed phages at different time intervals. Each experiment was performed in triplicate.

One-Step Growth Parameters
The phage growth characteristics (latent period and burst size) were determined as described by Drulis-Kawa et al. (2011) [42], with some modifications. Briefly, the exponential phase A. baumannii cultures were adjusted to 10 8 cfu/mL and incubated with phage lysate at a multiplicity of infection (MOI) of 0.001. A bacteriophage was allowed to adsorb to the bacterial surface at 37 • C for 10 min prior to determine the latency period. The mixture was centrifuged and the pellet was washed twice in 10 mL of LB broth. The samples were collected and the soft agar overlay method was used to determine the phage titer. The time interval between initiation of phage infection and release of progeny was defined as the latent period. The ratio of phage titer to the number of infected bacterial cells for one cycle was calculated as the burst size. Each experiment was performed in triplicate.

Sensitivity of Phage Particles to Temperature and pH
The thermal and pH stabilities of phages were examined according to the method of Yang et al. (2019) [43]. Briefly, 10 5 pfu/mL of phages were incubated at different temperatures (−20, 4, 25, 37, 40, 50, 60, and 70 • C), and at various pH values (3, 5, 7, 9, and 11). For both experiments, samples were taken at 2 h and the surviving phage were quantified by titration. Phage incubated at 37 • C and pH 7 were used as the control for the temperature and pH variation experiments, respectively. Each experiment was performed in triplicate. Statistical analysis between the test and control sets were performed by an unpaired t-test using GraphPad Prism v8, p < 0.05 for significance.

Phage Stock Stability
The titer of each phage stock was prepared from a 10-fold dilution in SM buffer and determined by the double agar overlay method after preparation of the stock. Stock titers were also determined after two years storage at 4 • C.

Transmission Electron Microscopy (TEM)
The phage morphology was determined by TEM. Purified phage particles (10 7−10 pfu/mL) were allowed to adsorb to formvar-coated 200-mesh copper grids for 10 min and washed twice for 1 min in double-distilled water (ddH 2 O). The particles were negatively stained with 2% (wt/vol) uranyl acetate for 5 min and allowed to air dry. The samples were observed under TEM (JEOL, JEM-2010).

Extraction of Genomic DNA
The phage lysate was precipitated using 8% (wt/vol) polyethylene glycol 8000 (PEG 8000) and 1 M NaCl precipitation according to Sambrook and Russell (2001) [44]. The phage lysate was added with 0.9 mL of PEG/NaCl, and incubated overnight at 4 • C. The culture was centrifuged at 17,000× g for 20 min and the pellet was suspended in 0.5 mL of PBS (phosphate buffered saline; pH 7.4). The phage DNA was prepared by the Phase Lock Gel System (phenol-chloroform method) of Pickard (2009) [45]. Briefly, contaminants were removed by incubation with 1 mg/mL of DNase I and 12.5 mg/mL of RNase A for 30 min at 37 • C. The mixture was added to 20% SDS and 10 mg/mL of proteinase K and incubated for a further 30 min at 37 • C. The mixture was aliquoted into 500 µL volumes in 1.5 mL Phase Lock gel Eppendorf tubes and extracted with 0.5 mL of phenol:chloroform:isoamyl alcohol (IAA) (25:24:1), followed by centrifugation at 5000× g for 5 min in order to separate the phases. The top aqueous phase was transferred into a fresh Phase-lock gel tube and the above step was repeated, chloroform:isoamyl alcohol (24:1) was added, and the mixture was centrifuged at 5000× g for 5 min. To precipitate phage DNA, the aqueous phase was transferred into a 1.5 mL Eppendorf tube, and then 45 µL of 3 M sodium acetate (pH 5.2) and two volumes of absolute ethanol were added to the mixture and incubated at room temperature for 20 min. The precipitated DNA was collected by centrifugation at 17,000× g for 20 min, washed twice with 70% ethanol, and air dried. The DNA pellet was suspended to a final volume of 30 µL with TE buffer (10 mM Tris HCl, 1.0 mM EDTA).

Accession Number
The whole-genome sequencing data generated in this study have been deposited into the European Nucleotide Archive (ENA; https://www.ebi.ac.uk/ena (accessed on 21 January 2022)) under study accession number PRJEB33567. Sample accession numbers for each sequenced bacteriophage are listed in Supplementary Table S7.

Conclusions
The gene-encoded depolymerase and endolysin identified in the newly isolated lytic A. baumannii phages, together with the absence of virulence-associated genes, render further studies for potential applications. Moreover, these lytic phages demonstrated a short generation and adsorption time, high degree of host specificity, ability to produce high numbers of virions, and physical stability over a wide range of temperature, pH, and storage conditions. Supplementary Materials: The following supporting information can be downloaded at: https: //www.mdpi.com/article/10.3390/ph15040443/s1, Table S1: Isolated phage. A total of 20 phages against multidrug-resistant isolates of Acinetobacter baumannii; Table S2A: Cross-infectivity of the isolated bacteriophages; Table S2B: Summary table of phage infectivity on different KL Types; Table S3: Corresponding matrix of the DNA distances; Table S4: A tab-delimited matrix of MASH distances between each pair of isolates; Table S5: The list of CDSs/gene in the genome of phages and their putative functions; Table S6: The common presence of genes in study; Table S7: Sample accession numbers of sequenced bacteriophages; Figure S1: The presence of phage-encoded polysaccharide depolymerases; Figure S2: A single growth cycle of six phages showed a short latent period (2-6 min); Figure S3: Morphology of T444 (a) and P1033 (b) by transmission electron microscopy; Figure S4: The genome organization of eight phage and reference Acinetobacter phage IME200 were compared using a progressive Mauve progressive alignment.