- 1Laboratory of Molecular Vaccinology and Molecular Diagnostics, School of Public Health, Xiamen University, Xiamen, China
- 2School of Basic Medicine, Anhui Medical University, Hefei, China
- 3State Key Laboratory of Pathogen and Biosecurity, Beijing Institute of Microbiology and Epidemiology, Academy of Military Medical Sciences (AMMS), Beijing, China
- 4Qinghai Institute for Endemic Disease Prevention and Control, Xining, China
- 5National Health Commission - Qinghai Co-construction Key Laboratory for Plague Control, Xining, China
- 6Hua Dong Research Institute for Medicine and Biotechniques, Nanjing, China
- 7Department of Laboratory Medicine, First Medical Center of Chinese People’s Liberation Army (PLA) General Hospital, Beijing, China
Plague caused by Yersinia pestis remains a public health threat worldwide. Because multidrug-resistant Y. pestis strains have been found in both humans and animals, phage therapy has attracted increasing attention as an alternative strategy against plague. However, phage resistance is a potential drawback of phage therapies, and the mechanism of phage resistance in Y. pestis is yet to be investigated. In this study, we obtained a bacteriophage-resistant strain of Y. pestis (S56) by continuously challenging Y. pestis 614F with the bacteriophage Yep-phi. Genome analysis identified three mutations in strain S56: waaA* (9-bp in-frame deletion 249GTCATCGTG257), cmk* (10-bp frameshift deletion 15CCGGTGATAA24), and ail* (1-bp frameshift deletion A538). WaaA (3-deoxy-D-manno-octulosonic acid transferase) is a key enzyme in lipopolysaccharide biosynthesis. The waaA* mutation leads to decreased phage adsorption because of the failure to synthesize the lipopolysaccharide core. The mutation in cmk (encoding cytidine monophosphate kinase) increased phage resistance, independent of phage adsorption, and caused in vitro growth defects in Y. pestis. The mutation in ail inhibited phage adsorption while restoring the growth of the waaA null mutant and accelerating the growth of the cmk null mutant. Our results confirmed that mutations in the WaaA–Cmk–Ail cascade in Y. pestis contribute to resistance against bacteriophage. Our findings help in understanding the interactions between Y. pestis and its phages.
Introduction
Phages have long been used in medicine to identify specific bacteria or as alternative treatment for treating bacterial diseases. Because of the global emergence of antibiotic resistance, phage treatment has attracted great attention as an alternative or complement to antibiotic therapy. Y. pestis, the causative agent of plague, is transmitted by fleabite or respiratory droplets (Gage and Kosoy, 2005; Cathelyn et al., 2006). Three plague pandemics have been recorded in history, resulting in approximately 200 million deaths (Sun and Singh, 2019). Although human plague cases have been well controlled in most countries, sporadic cases or outbreaks are occasionally reported in plague foci worldwide. In 2017, a pneumonic plague outbreak in Madagascar caused 209 deaths in 4 months (Tsuzuki et al., 2017). Antibiotics are generally effective in the treatment of plague, but several antibiotic-resistant strains of Y. pestis have been isolated from patients and rodents in recent years (Cabanel et al., 2018; Sebbane and Lemaitre, 2021). In this context, bacteriophage therapy has been suggested as an alternative, the efficacy of which depends on the administration route (e.g., oral, intramuscular, and aerosol spray) or the frequency of phage application (Anisimov and Amoako, 2006; Sebbane and Lemaitre, 2021; Vagima et al., 2022).
The use of phage therapy has many ethical considerations. For instance, discussing the known and unknown risks of phage therapy can be challenging for patients and physicians. Moreover, the development of phage therapy has been hindered by the lack of predefined regulatory pathways for phage production and concerns about intellectual property protection (Kingwell, 2015). However, the main limitation of phage therapy is phage resistance. In natural environments, bacteria are subjected to strong selective pressure by bacteriophages (Vlot et al., 2018). In response, bacteria have developed mechanisms to resist phages, including inhibition of DNA injection, restriction and modification, abortive infection, CRISPR–Cas, and inhibition of adsorption via phase variation of cell surface receptors (Kim et al., 2015; Takeuchi et al., 2016; Reyes-Robles et al., 2018). Although the CRISPR–Cas system has been studied for decades, unknown defense systems in bacteria remain to be discovered (Makarova et al., 2013). For example, Doron et al. have identified several unreported defense systems using microbial pangenome analysis (Doron et al., 2018). Notably, mutations in certain genes may render the host bacterium resistant to phage infection (Laanto et al., 2020).
In this study, we used in vitro culture assays to screen Y. pestis strains with varying degrees of phage resistance and obtained several strains with mild-to-complete resistance to bacteriophages. We examined heritable gene mutations in resistant strains and identified Y. pestis genes involved in resistance to phage lysis, such as waaA, cmk, and ail. waaA encodes 3-deoxy-D-manno-octulosonic acid transferase, which is involved in the synthesis of lipopolysaccharide (LPS) and serves as the phage receptor in Y. pestis (Kiljunen et al., 2011). cmk encodes cytidine monophosphate (CMP) kinase, which catalyzes the transfer of a phosphoryl group from ATP to CMP or dCMP and plays a crucial role in the biosynthesis of nucleoside precursors (Walker et al., 2012). Escherichia coli with the cmk mutation are less susceptible to T7 phage (Qimron et al., 2006). Our previous study indicated that Ail contributes to phage adsorption in Y. pestis by interacting with the phage tail fiber protein (Zhao et al., 2013). By deciphering the evolutionary processes of Y. pestis against phage lysis stress, we have provided insights into the physiological processes involved in receptor recognition, phage DNA replication, and host degradation resistance.
Materials and methods
Bacterial strains, plasmids, phage, and media
The Y. pestis strains used in this study are described in Table 1. Other bacterial strains and plasmids are described in Supplementary Table S1, and the primers used in the study are described in Supplementary Table S2. The phage Yep-phi used in this study can effectively lyse all tested Chinese isolates of Y. pestis but is unable to lyse other Yersinia species (Zhao et al., 2011). Y. pestis and Yep-phi cultures were incubated at 26°C and E. coli at 37 °C. Luria–Bertani (LB) media were used for bacterial liquid cultures. A soft agar medium was prepared by adding 0.4% (wt/vol) agar to liquid media. Plates were supplemented with ampicillin (Amp, 100 μg/ml), kanamycin (Kan, 100 μg/ml), spectinomycin (Spe, 100 μg/ml), or chloramphenicol (Cm, 34 μg/ml) when required.
Identification of phage-resistant Y. pestis 614F derivates
Different titers (from 1.5 × 108 plaque-forming unit [PFU] to 1.5 × 104 PFU) of 0.5 ml strain 614F (109 CFU/ml) and 5 ml Yep-phi were mixed and incubated at 26°C for 24h. The serial mixtures were separately plated on LB agar and incubated at 26°C for 24h. Colonies on plates were resistant to the corresponding titer of phage and were selected for passages. Bacterial stocks of every passage were stored for future analysis. Coculture passages were performed to obtain a fully resistant Yep-phi derivate of 614F (phage titer 1.5 × 108 PFU). The genomes of resistant and wild-type 614F strains were sequenced and compared. The identified mutations were screened with mismatch–polymerase chain reaction (PCR) in all passage stocks to determine when these mutations occurred during the entire passage process (Supplementary Table S2) (Wangkumhang et al., 2007).
Mutant construction
Scarless genome editing was used to generate gene knockouts and point mutants in Y. pestis (Kim et al., 2014). In brief, selection cassettes containing Spe-resistant genes, flanked by FRT, I-SceI sites, and 120-bp homologous arms, were electroporated into 201/pREDTKI, which encodes meganuclease I-SceI under the control of the an hydrotetracycline-induced tetA promoter and λ-Red recombinase genes under the control of the arabinose-inducible araB promoter as well as a temperature-sensitive replication origin. The knockout strains were confirmed via PCR and sequencing. Using the primers listed in Supplementary Table S2, the PCR fragment containing the SacI/HindIII site of mutant gene S56 was amplified and cloned into the donor plasmid pKSI-1, which with I-SceI recognition sites was digested with SacI and HindIII to produce pKSI-1_waaA*, pKSI-1_cmk*, and pKSI-1_ail*. The donor plasmid was electroporated into knockout strains; transformants were restruck onto LB plates containing Kan, Spe, and Amp and grown overnight at 26°C. Restruck colonies were suspended in LB containing Kan, Spe, and Amp and grown overnight at 26°C. The colonies were repatched twice onto LB supplemented with 10 mmol L-arabinose for inducing lambda red recombinase and 20 mmol IPTG for inducing I-SceI expression to loop out the selection cassette and donor plasmid at 26°C. To verify the loss of the selection cassette, isolates were tested for growth on LB plates with or without Spe and Amp. The sensitive isolates were screened via PCR and sequencing to confirm mutagenesis. Successive passage was performed at 37°C to remove pREDTKI from the strain. The waaA*/cmk*/ail* mutant was constructed via suicide plasmid-mediated genome editing (Philippe et al., 2004). Homologous upstream and downstream fragments flanking the waaA* mutation were amplified from S56 using PCR. The fragments were cloned into the suicide plasmid pDS132, which was digested with SacI and SalI, and replicated in S17-1 λpir. The recombinant plasmids were purified and introduced in cmk*/ail* via conjugation. Plates containing Cm were screened after incubation at 37°C overnight. The clone was selected on a plate containing 7% sucrose following growth at 26°C for 4 days. We selected transformants that grew on plates but not on Cm plates. The strain containing waaA*/cmk*/ail* was detected via PCR and confirmed via sequencing.
Growth curves
The overnight grown strains were cultured to OD620 of approximately 1.0, diluted 1:100 into 20 ml of LB, and cultured at 26°C and 200 rpm. OD620 was determined every 2h using 300 μl of bacterial culture. The OD620 values were used to draw growth curves. Data were obtained in triplicate, and experiments were repeated twice. Area under the curve analysis was used to quantify the differences in growth (Vornhagen et al., 2019).
Phage infection assay
The lysis activity of each phage strain was examined using a spot test on Y. pestis (Paul et al., 2011; Zhao et al., 2013). In brief, 100 ml of bacteria cultured to exponential phase (OD620~1.0) were concentrated 10-fold via centrifugation and mixed with 3 ml of liquefied soft agar medium. The mixture was plated on LB plates to create double-layer agar plates. When the medium solidified, 3 μl of serial dilutions of Yep-phi were spotted on the plates. Plates were incubated at room temperature for 10 h and then examined and photographed.
Phage adsorption assay
For phage adsorption, approximately 8 × 105 PFU of Yep-phi in 100 μl was mixed with 500 μl bacteria (OD620~1.0). LB was used as a nonadsorbing control in each assay, and the phage titer in the control supernatant was set to 100%. The mixture was incubated at room temperature for 5 min and centrifuged at 16,000 × g for 3 min. Residual PFU percentage was calculated as described in a previous study (Kiljunen et al., 2011).
Statistical differences were determined using one-way analysis of variance (ANOVA) with three independent data sets. To reveal the temporal phage adsorption kinetics of all strains, residual PFU percentage was tested at different time points (2, 5, 10, and 15 min). Each assay was performed in triplicate and repeated twice. Statistical differences were determined using two-way RM ANOVA with Dunnett’s multiple comparisons to wild-type groups.
Phage efficiency of plating assay
To determine the efficiency of plating (EOP) of Yep-phi on different strains, 300 μl of wild-type and mutant Y. pestis–cultured bacteria (OD620~1.0) were mixed with 100 μl of Yep-phi in 3 ml of 0.4% soft agar and poured onto LB plates. The number of PFUs was counted after 24h–48h. Each strain was verified in triplicate. EOP was calculated as described (Hyman and Abedon, 2010).
Isolation and analysis of LPS
LPS isolation was performed using the phenol–water extraction method (Zhang and Skurnik, 1994). In brief, 9 ml overnight bacterial cultures were collected via centrifugation and resuspended in 1.5 ml distilled water. The bacterial suspensions were incubated at 70°C for 1h and then mixed with water-saturated phenol (pH 4.0) reheated to 70°C for 10 min and then transferred to ice for cooling (< 10°C). Then, the cells were centrifuged at 2,000 × g for 20 min. The uppermost aqueous layer obtained was transferred to a new Eppendorf tube and 2 volumes of acetone were added to precipitate LPS. The LPS pellet was dissolved in 150 μl of water, of which 5 μl of LPS was analyzed via 15% sodium dodecyl sulfate-polyacrylamide gel electrophoresis and silver staining (Zhang and Skurnik, 1994).
Protein expression and purification
The PCR-generated DNA fragment comprising waaA and waaA* was cloned into the BamHI/HindIII site of the pET32a vector. The plasmid was introduced into DH5α cells, and its DNA sequence was confirmed. The plasmid was extracted and introduced into E. coli BL21(DE3) cells. To induce the expression of WaaA and WaaA* in E. coli BL21(DE3) cells, 1 mM IPTG was added when the culture reached the mid-exponential growth phase at an OD600 of approximately 0.8. The bacterial cells were cultured at 37°C for 4h and collected. WaaA and WaaA* were purified via immobilized metal affinity chromatography on a nickel cephalosporin HP column. The proteins were desalted with PBS (pH 7.2) and 20% glycerol and concentrated using a protein concentration column (Mamat et al., 2009). Protein concentrations were determined using a BCA protein assay kit.
Circular dichroism spectroscopy
To compare the circular dichroism (CD) spectra of wild-type WaaA and WaaA*, a Jasco J-815 spectropolarimeter (Greenfield, 1999; Kelly et al., 2005) was used. Protein solutions (0.1–0.35 mg/ml) were quantified at 200–260 nm. Spectra were obtained with a scan speed of 50 nm/min and 0.5-nm data pitch. The percentage of secondary structure was estimated using online software connected to Jasco J-815.
Protein structure analysis
Protein Data Bank (PDB) was used to conduct homology search (Rose et al., 2015). For WaaA, the structure of membrane-embedded monofunctional glycosyltransferase WaaA from Aquifex aeolicus (PDB code: 2XCI.A) was used as the template based on the quality of models produced. Multiple sequence alignment was performed using Clustal Omega from UniProt (Yip et al., 2008). The ESPript server was used to predict the secondary structure of WaaA (Robert and Gouet, 2014). The Alphafold v2.3.1 monomer_casp14 model was used to predict the structures of WaaA and WaaA* (Jumper et al., 2021). The biological and functional insights derived from the predicted models were verified by matching the models with the protein function database.
Results
Continuous phage challenge produced phage-resistant derivates of strain 614F
Yep-phi is routinely used as a diagnostic phage for identifying Y. pestis, and no natural Yep-phi phage-resistant Y. pestis isolate has been reported (Zhao et al., 2011). In this study, we exposed cultures of Y. pestis 614F to serially diluted phage Yep-phi. The surviving clones were selected and amplified continuously. Figure 1A illustrates how resistant mutants were identified by rounds of progressive challenges with different phage titers. Phage spotting assays revealed that after 12 rounds of phage challenge, the derivate of 614F (strain S12) showed decreased phage susceptibility (resistant to phage titer 105 PFU), whereas later derivates (S38 and S56, with 38 and 56 rounds of challenges, respectively) were fully resistant to phage titer 108 PFU (Figure 1B). The EOP assay showed a similar result; the EOP value for S12 was 3.2 × 10−6, whereas the EOP values for S38 and S56 were<1.68 × 10−9 (Figure 1C). Our results confirmed that the 614F strain gradually developed full resistance to phage Yep-phi under continuous stress. Residual PFU percentages were used to evaluate the adsorption capability of 614F and its derivates S12, S38, and S56. All derivate strains lost their ability to adsorb phages (Figure 1D), which was confirmed through the temporal kinetics of adsorption assays (Figure 1E).
Figure 1 Screening and characterization of phage-resistant mutants of strain 614F. (A) Screening procedures. (B) Ten-fold dilution of lysates of Yep-phi applied to bacterial lawns of 614F wild-type and phage-resistant strains. The maximum titer of bacteriophage is 108 PFU. (C) The efficiency of plating (EOP) of Yep-phi phage on various strains. EOP = (number of PFUs on mutant strain)/(number of PFUs on wild-type strain). The titer of bacteriophage is 1.68 × 109 PFU. (D) Adsorption of Yep-phi on strain 614F and its derivates. The Y-axis represents percentage of residual plaque-forming unit (PFU). Error bars show standard deviations of the mean of three biological replicates. Significance was determined by one-way ANOVA followed by Dunnett’s multiple comparison test. #P< 0.0001. (E) Adsorption kinetics of Yep-phi to strain 614F and its derivates. ***P< 0.001 (two-way RM ANOVA with Dunnett’s multiple comparison test). Error bars indicate standard deviations in triplicate samples.
Genomic analysis revealed mutations in phage-resistant strain S56
To examine the genetic variations responsible for phage resistance, we sequenced the genomes of strain S56 and its ancestor strain 614F. A control strain S88 (56 passages without phage challenges) was sequenced to rule out unrelated mutations. We identified three mutations in S56 (Supplementary Figure S1): a 9-bp in-frame deletion (249GTCATCGTG257) in waaA (gene ID: YPO0055), a 10-bp frame shift deletion (15CCGGTGATAA24) in cmk (gene ID: YPO1391), and a 1-bp frame shift deletion (A538) in ail (gene ID: YPO2905), which are annotated according to Y. pestis CO92. The mutations were named waaA*, cmk*, and ail*, respectively, and mismatch-PCR was used to screen their presence in passage stocks. The findings revealed that waaA* occurred in passage 12 (strain S12), cmk* occurred in passage 38 (strain S38) in addition to waaA*, and ail* occurred in passage 56 (strain S56) in addition to waaA*/cmk*.
waaA*/cmk*/ail* mutations reproduced phage resistance phenotypes in strain 201
To determine whether a similar phage-resistant profile can be reproduced and the roles of mutations in waaA (9-bp deletions), cmk (10-bp deletions), and ail (1-bp deletion), we constructed single, double, or triple mutants derived from strain 201. Strain waaA* was partially resistant to phage Yep-phi (resistant to 3.15 × 103 PFU, Figure 2A), with an EOP value of 5.4 × 10−6 (Figure 2B, phage titer 1.05 × 1010 PFU). Moreover, waaA*/cmk* and waaA*/cmk*/ail* were fully resistant to phages with EOP< 1.05 × 10−10, which is much lower than that for waaA* (Figure 2B). Adsorption assays indicated that all mutants had a significantly lower ability to adsorb phage Yep-phi, and the residual PFU percentages among the three mutants were indistinguishable (Figures 2C, D). These results suggest that the waaA* mutation affects the binding between Y. pestis and its phage.
Figure 2 Reproduction of phage resistance induced by waaA, cmk, and ail mutations in strain 201. (A) Ten-fold dilution of Yep-phi lysates applied to lawns of 201 wild-type and mutant bacterial strains. The maximum titer of bacteriophage is 3.15 × 107 PFU. (B) Efficiency of plating (EOP) for different strains. The titer of bacteriophage is 1.05 × 1010 PFU. (C) Adsorption of 8 × 105 PFU Yep-phi to Y. pestis 201 WT and its single-, double-, or triple-gene mutants shown as residual PFU percentages. Significance was determined by one-way ANOVA. #P< 0.0001. (D) Adsorption kinetics of Yep-phi to wild-type Y. pestis 201 and its mutants (ca. 2 × 106 PFU/108 CFU). **P< 0.01 (Dunnett’s multiple comparison test of two-way RM ANOVA).
The waaA* mutation inhibits phage adsorption by truncating LPS
Phage adsorption defects were found in strain waaA* and strain 614F carrying the waaA* mutation. The waaA* mutant and the waaA null mutant ΔwaaA displayed similarly decreased phage susceptibility (resistant to 4.35 × 103 PFU phage), with decreased EOP (Figure 3A). In the complementation test, the phage susceptibility of waaA* supplemented with plasmid pACYC184_waaA was restored and comparable to that of wild-type strain 201 (Figures 3A, B). In the adsorption kinetics assays, the phage adsorption ability of waaA* was similar to that of ΔwaaA, and waaA* mutant complemented with plasmid pACYC184_waaA showed similar phage adsorption ability to the wild-type strain, confirming the anti-adsorption effect of the waaA* mutation (Figures 3C, D).
Figure 3 The waaA mutation inhibits phage adsorption by disrupting LPS. (A) Ten-fold dilution of Yep-phi lysates applied to bacterial lawns of wild-type and mutant Y. pestis strains. The maximum titer of bacteriophage is 4.35 × 107 PFU. (B) Efficiency of plating (EOP) of 2 × 102 PFU phage for different strains. (C) Adsorption of Yep-phi to Y. pestis 201 and waaA mutant strains, expressed as a percentage of residual PFU. Significance was determined by one-way ANOVA; **P< 0.01. ns, non-significant. (D) Adsorption kinetics of Yep-phi to Y. pestis and waaA mutant strains expressed as percentages of residual PFU. Two-way RM ANOVA was used to determine significance between the mutant and wild-type groups; ** P< 0.01. (E) Analysis of isolated LPS fractions from Y. pestis 201 and waaA mutants using SDS/PAGE. The gel was silver stained for visualization. (F) CD spectra of WaaA and WaaA*. (G) The build-in software of the spectropolarimeter predicted the conformations ratio between WaaA and WaaA* of Y. pestis 201.
Because the waaA gene, encoding 3-deoxy-D-mannooctulosonic acid (KDO) transferase, is involved in LPS synthesis (Chung and Raetz, 2010), we hypothesize that the mutation in waaA* affects the adsorption of Yep-phi phage because of failure to synthesize LPS, which is the phage adsorption receptor. At 26°C, Y. pestis expresses rough LPS, which does not contain the O-polysaccharide that is considered the phage receptor (Kiljunen et al., 2011). Rough LPS was expressed in 201 WT but was not stained on the gel by silver (a characteristic of a core-lacking LPS) in either ΔwaaA or waaA* (Figure 3E), which confirmed the failure of complete LPS core synthesis in the two mutants (Meredith et al., 2006; Dentovskaya et al., 2011). CD spectra assays demonstrated that wild-type WaaA has two negative absorption bands at 209 and 222 nm, which are characteristic of α-helical proteins, and the CD spectrum of WaaA* protein is slightly different from that of wild-type strain (Figure 3F). Meanwhile, the build-in software of the spectropolarimeter predicted decreased α-helix and increased β-sheet in WaaA* protein comparing with the wild-type WaaA (Figure 3G).
The 9-bp (249GTCATCGTG257) in-frame deletion in waaA resulted in the 84TMT86 deletion in WaaA. To further determine the consequence of the 84TMT86 deletion in WaaA, we compared the predicted structures of wild-type WaaA and mutated WaaA*. Sequence alignment of WaaA and WaaA* showed the presence of charged residue matching the monofunctional glycosyltransferase WaaA of A. aeolicus (PDB code: 2XCI.A) (Schmidt et al., 2012; Rose et al., 2015). In A. aeolicus, residues S54 and R56 of WaaA had been proven vital for its KDO transferase activity, and these two residues together with S28 and E31 provide necessary hydrogen bonds to bind tetraacyl-4'-phosphate lipid A during KOD transferring process as part of the receptor-substance binding site of WaaA (Schmidt et al., 2012). Secondary structure predictions of WaaA and WaaA* indicated that the 84TMT86 deletion occurred in the junction of β-sheet 2 (β2) and α-helix3 (α3), right next to residues S54 and R56 of A. aeolicus WaaA (Supplementary Figure S2). Sequence alignment of multiple bacterial WaaA showed that the 84TMT86 region is conserved among multiple bacterial species (Supplementary Figure S3). Additionally, Alphafold analysis of WaaA and WaaA* proteins demonstrated that their predicted structures are slightly different from each other (Supplementary Figures S4A–C). The 84TMT86 is located at an α helix-loop-β turn connection in WaaA protein, and the deletion of 84TMT86 of resulted in a shorter length of the α helix, followed by a shift of approximately 2.7 Å in the loop and a 6.8° deflection of the in the β turn (Supplementary Figure S4D).
Our results suggest that the 84TMT86 deletion in WaaA hinders its binding to the precursor of lipid A, and causes the loss of its glycosyltransferase function. The three amino acids in-frame deletion in waaA* resulted in a core-lacking LPS of Y. pestis, leading to phage resistance similar to ΔwaaA.
cmk*-related phage resistance is independent of adsorption
cmk encodes a cytidylate kinase that catalyzes phosphoryl transfer from ATP to (d)CMP (Tsao et al., 2015). Mutant waaA*/cmk* was more resistant to phage lysis than waaA*. However, the role of the cmk mutation against phage lysis remains unknown. To address this, we constructed cmk*, which contains a frameshift mutation (15CCGGTGATAA24 deletion). We performed infection assays using cmk*, C_cmk* (a complementary strain), and Δcmk (cmk null mutant) simultaneously and found that cmk* and Δcmk were resistant to a high phage titer (3.15 × 107 PFU) (Figure 4A), with EOP values of 5.8 × 10−5 and 4.5 × 10−5, respectively (Figure 4B). C_cmk* restored susceptibility, comparable with wild-type 201. Notably, cmk* and Δcmk have similar adsorption capacity compared with WT 201 (Figures 4C, D), suggesting that cmk*-mediated phage resistance is irrelevant for the adsorption of Y. pestis and phage particles. The 10-bp (15CCGGTGATAA24) deletion of cmk led to premature termination of Cmk translation. The mechanism of Cmk-related phage resistance needs further investigation.
Figure 4 cmk* resists phage lysis without impacting phage adsorption. (A) Ten-fold dilution of Yep-phi lysates applied to bacterial lawns of wild-type and cmk mutant Y. pestis strains. The maximum titer of bacteriophage is 4.35 × 107 PFU. (B) Efficiency of plating (EOP) for different strains. (C) Adsorption of Yep-phi to Y. pestis 201 and its cmk mutant strains expressed as a percentage of residual PFU. ns, non-significant (one-way ANOVA). (D) Adsorption kinetics of Yep-phi to Y. pestis and cmk mutant strains, expressed as percentages of residual PFU. ns, non-significant (Dunnett’s multiple comparison test of two-way RM ANOVA).
The ail* mutation affects the phage adsorption ability of Y. pestis
In Y. pestis, Ail is an outer membrane protein that contains 182 amino acids. Our previous study revealed that Ail interacts with the phage tail fiber protein and contributes to phage adsorption in Y. pestis (Zhao et al., 2013). In this study, we identified the A538 deletion in ail in strain S56 (ail*, Table 1), which is at the very end of the ail coding region. ail* or Δail was as susceptible to phages as wild-type 201, with comparable EOP values (Figures 5A, B). Moreover, the ail* mutant showed similar phage adsorption defects as the null mutant Δail (Figures 5C, D). The addition of waaA* or cmk* to ail* did not make a difference in phage adsorption (Figures 5C, D); however, it significantly increased resistance to phage compared with the ail* null strain (Figures 4B, 5B). Our results indicate that ail* (1-bp deletion at A538) exhibited phage adsorption resistance, consistent with the effects of disrupting phage adsorption in Δail.
Figure 5 The ail mutation confers resistance to phages in Y. pestis. (A) Ten-fold dilution of Yep-phi lysates applied to bacterial lawns of wild-type and mutant strains. The maximum titer of bacteriophage is 4.35 × 107 PFU. (B) Efficiency of plating (EOP) for different strains. (C, D) Yep-phi adsorption and adsorption kinetics to Y. pestis 201 and its mutant strains. #P< 0.0001. ns, non-significant.
Interplays of waaA*/cmk*/ail* mutations restore the growth of the mutants
The waaA*/cmk* mutant is resistant to high-titer phage attacks (Figures 2A, B), and the ail* mutant is somewhat sensitive to phages even though it adsorbs phages less effectively. We wondered whether the evolution of phage resistance due to the waaA*/cmk* mutations was a liability that was compensated by the ail mutation or why the weakly lysis-resistant ail* mutation occurred in Y. pestis when the waaA*/cmk* mutation already renders the strain completely phage resistance. The 614F derivate S12 grows slower in LB than 614F. The growth of S38 is even slower than that of S12, which suggests the great fitness costs accompanying the phage resistance phenotype of these two derivates. Interestingly, S56 grew much better than S38, and its growth recovered to the level of 614F (Figure 6A and Supplementary Figure S5A). Because waaA*/cmk*/ail* mutations occurred sequentially in S12, S38, and S56, we assumed that waaA* and cmk* mutations influence the growth of the mutants in addition to conferring phage resistance onto them. Growth curves showed a deceleration of bacterial growth for cmk*, especially for waaA*, while the subsequent ail* mutation restored the mutant growth, as measured by calculating area under the curve (Figures 6B, C; Supplementary Figures S5B, C). Our results indicate that the growth deficiency in waaA*/cmk* mutants can be compensated by the A538 deletion of ail.
Figure 6 Growth attenuation caused by waaA* and/or cmk* mutations can be restored by ail* in Y. pestis. (A) Growth curve of Y. pestis 614F and its derivates. (B) ail* restored growth of waaA*. (C) ail* restored growth of cmk*. Data represent the average of three biological replicates; error bars indicate SEM.
Discussion
In this study, we obtained phage-resistant Y. pestis mutants by continuously challenging strain 614F with the Yep-phi phage. Characterization of these mutants identified successive mutations in waaA, cmk, and ail.
The waaA null mutant not only demonstrated resistance to eight types of phages but was also greatly attenuated in mice (Filippov et al., 2011). Our previous study revealed that the waaA null mutant lost most of its phage-binding activity in an adsorption assay while remaining sensitive to high titers of Yep-phi (Zhao et al., 2013). Crystal structure analysis of WaaA from A. aeolicus suggested that the N-terminal domain functions as the acceptor–substrate binding site for the lipid A precursor (Schmidt et al., 2012). In contrast, the waaA* mutant harbors a 9-bp in-frame deletion (249GTCATCGTG257, resulting in the 84TMT86 deletion in WaaA) that is located at the junction of the N-terminal β2 sheet and α2 helix (Supplementary Figure S2). Basic amino acids on the N-terminal α2 helix have been shown to be crucial for facilitating the entry of the lipid A precursor into the acceptor–substrate binding site of WaaA (Schmidt et al., 2012). Here, we found that the phage-induced 9-bp in-frame deletion in waaA had similar effects to the waaA null mutation in Y. pestis regarding truncated LPS and phage resistance.
Previous research has revealed that Yersinia pseudotuberculosis with the cmk null mutation has a growth defect and is highly attenuated in mice (Walker et al., 2012). Our data indicate that the phage-induced cmk* mutation (with a 15CCGGTGATAA24 frameshift deletion leading to the failure of Cmk translation) displays a similar phage-resistant phenotype as Δcmk. However, how defects in cmk confer phage resistance to Y. pestis is unclear. Because T7-like phages depend on the nucleoside monophosphate kinase of the host (Qimron et al., 2006), we propose that the loss of Cmk impacts nucleoside synthesis pathways and hinders the replication of phages in the host. In this study, other genes encoding nucleoside monophosphate kinases, such as adk, tmk, gmk, and pyrH (Qimron et al., 2006), were found to be unaffected in the phage-resistant S56 strain, likely due to the high fitness costs associated with mutations in these essential genes. Notably, cmk* showed growth deficiency in addition to phage resistance, similar to waaA*. This finding suggests that bacterial resistance to lytic phages comes at a cost to growth fitness.
Previous research has demonstrated that laboratory passages of Y. pestis may result in the disruption or premature truncation of Ail expression (Leiser et al., 2015). Ail is a critical virulence factor of Y. pestis, playing a central role in promoting immune resistance to human host defense (Zhang et al., 2020; Kent et al., 2021). We have reported that ail* with a frameshift mutation in ail (A538 deletion) and Δail have similar phenotypes, indicating that the A538 deletion affects the functional integrity of Ail. Both waaA* and ail* attenuated phage adsorption, and the phage resistance of waaA*/ail* was additive compared with that of ail* or waaA* alone. Thus, we speculate that the phage primarily relies on LPS as an adsorption receptor, whereas ail is a secondary receptor, thereby affecting the reduction in viral progeny through different loadings onto host bacteria (Zhao et al., 2013).
The ail* mutation, which was observed only in S56 (the final passage), plays a minor role in phage resistance. However, the mutation in ail restores the growth of Y. pestis that was disrupted by a single mutation in waaA or cmk. In the phospholipid biosynthesis pathway, CTP and dCTP are downstream products of Cmk and may affect outer membrane lipids (Langley and Kennedy, 1978). In addition, the mutation in waaA can result in the accumulation of tetraacylated precursor lipid IV A (Tzeng et al., 2002). In contrast, the deletion of ail has been reported to cause an abnormal flow of phospholipids into the outer leaflet of the outer membrane (Kolodziejek et al., 2021), which might counterbalance the detrimental effects of accumulating mutations in waaA and cmk. One plausible explanation is that the ail mutation rebalances the changes in lipid content of the outer membrane caused by waaA and cmk mutations, thereby modifying cell shape and accelerating growth. Our data suggest that mutations in waaA* and cmk* may be advantageous to Y. pestis in the presence of phages but come at the cost of growth defects when phages are absent. Notably, waaA* and cmk* could recover their fitness through the ail mutation.
In this study, we identified successive mutations in waaA, cmk, and ail of Y. pestis that were induced by continuous phage challenges. Although these genes have individually been shown to be related to phage resistance in Y. pestis and other bacteria, they have not been observed simultaneously in one strain. Based on our findings, we propose a scenario in which Y. pestis developed a phage-resistant phenotype through mutations in waaA, cmk, and ail under continuous phage pressure. Initially, when phage stress was imposed on Y. pestis, the cells prevented phage adsorption through the waaA mutation, which truncates LPS. As phage pressure persisted, waaA*/cmk* mediated stronger phage resistance reinforced by the cmk mutation, which enhances resistance to phage lysis but leads to growth defects. Finally, the growth of waaA*/cmk* was restored by the ail mutation, and waaA*/cmk*/ail* prevented phage attachment because the Ail receptor was damaged. The interplay between mutations in the WaaA–Cmk–Ail cascade illustrates a tradeoff strategy during the development of phage-resistant phenotypes in Y. pestis (Figure 7).
Figure 7 Proposed scenario of interplay between mutations in Y. pestis leading to resistance to Yep-phi phage infection. (A) Inhibition of phage adsorption to the surface of bacterial cells due to alterations in the surface receptor LPS by waaA* and ail*. (B) Inhibition of phage replication through secondary bacterial metabolites by cmk*. (C) Restoration of growth by ail*.
All three genes responsible for phage resistance in Y. pestis discussed in this study are known to be virulence-related factors for pathogenic Yersinia. In the case of CO92, the waaA null mutant exhibited an LD50 nearly 4 million times lower than that of its wild-type counterpart (Filippov et al., 2011). In mice, the KIM5 ail null mutant showed > 3,000-fold increase in LD50 (Felek et al., 2010). The cmk null mutant in Y. pseudotuberculosis was > 400 times attenuated in the mice model (Walker et al., 2012). These findings suggest that phage pressure may have an impact on virulence and fitness in other niches of Y. pestis, which could partially explain the scarcity of natural phage-resistant isolates of Y. pestis.
A caveat to consider is whether these mutations are involved in antibiotic resistance in Y. pestis. Studies have suggested that LPS regulated by WaaA plays a role in polymyxin resistance, and an Ail-like protein imparts ceftriaxone resistance to Salmonella enterica (Hu et al., 2005; Moffatt et al., 2019). In Y. pestis, the minimal inhibitory concentration of polymyxin B for the waaA null mutant is 250 times lower than that of its wild-type counterpart, possibly due to the less efficient incorporation of 4-amino-4-deoxyarabinose into lipid A (Dentovskaya et al., 2011). Furthermore, reduced Cmk activity may increase the tolerance of Staphylococcus aureus to vancomycin through effects on cell wall biosynthesis (Matsuo et al., 2013). Notably, all these antibiotics target the bacterial membrane, which suggests that phage resistance likely relies on changes in membrane characteristics. Fortunately, there is no evidence linking the WaaA–Cmk–Ail cascade to resistance against first-line antibiotics used to treat plague (Barbieri et al., 2020). Studies using animal models and clinical studies have identified tradeoffs between resistance and virulence. These findings bode well for improving treatment effectiveness despite the development of phage resistance (Oechslin, 2018; Mangalea and Duerkop, 2020).
In this study, we examined the microevolutionary processes of Y. pestis under phage stress and found that phage exposure resulted in complex changes in Y. pestis, particularly perturbations of the cell membrane. The findings of the present study provide valuable insights into the molecular mechanisms underlying Y. pestis resistance to bacteriophage and may aid ongoing investigations into phage therapies for plague. Notably, as a facultative intracellular pathogen with a complex life cycle, Y. pestis is likely to develop phage resistance through different pathways under different conditions, such as in natural environments, fleas, and hosts if exposed to phage pressure. We acknowledge that these three genes (waaA, cmk, and ail) were identified through continuous in vitro selection with phage pressure and caution against using our data to predict or interpret what may happen in human or rodent hosts. Investigating the relationship between phage resistance and virulence characteristics of Y. pestis during long-term phage therapies will be valuable, although ethical and technical obstacles need to be addressed. Additional genetic factors related to phage resistance in Y. pestis should be discovered through parallel passages under phage pressure. Moreover, conditions more closely resembling the host environment may help identify pathways of phage resistance in Y. pestis.
Data availability statement
The datasets presented in this study can be found in online repositories. The names of the repository/repositories and accession number(s) can be found in the article/Supplementary Material.
Author contributions
LX, ZQ, and KS conducted the experiments, analyzed the data, and authored the paper. The phage adsorption experiments were carried out by KS and RL. HZ, HW, CL, and YX took part in the screening of phage-resistant strains. YJ, XL, XX, and XuZ contributed to the development curve of the 614F strain. RC, YT, ZD, and YC contributed to the interpretation of the data. RY, XiZ, and YS designed the experiments and contributed to the production and revision of the text. All authors contributed to the article and approved the submitted version.
Funding
This research was supported by the National Natural Science Foundation of China (81660349, U22A20526), and the National Health Commission (2019PT310004). The funders had no role in study design, data collection, and interpretation, or the decision to submit the work for publication.
Acknowledgments
The authors are grateful to Dr. Guoqiang Li for AlphaFold analysis of WaaA and WaaA* proteins. We are also grateful to Medelite Corp. for language polishing.
Conflict of interest
The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.
Publisher’s note
All claims expressed in this article are solely those of the authors and do not necessarily represent those of their affiliated organizations, or those of the publisher, the editors and the reviewers. Any product that may be evaluated in this article, or claim that may be made by its manufacturer, is not guaranteed or endorsed by the publisher.
Supplementary material
The Supplementary Material for this article can be found online at: https://www.frontiersin.org/articles/10.3389/fcimb.2023.1174510/full#supplementary-material
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Keywords: Yersinia pestis, phage, phage resistance, fitness cost, waaA, cmk, ail
Citation: Xiao L, Qi Z, Song K, Lv R, Chen R, Zhao H, Wu H, Li C, Xin Y, Jin Y, Li X, Xu X, Tan Y, Du Z, Cui Y, Zhang X, Yang R, Zhao X and Song Y (2023) Interplays of mutations in waaA, cmk, and ail contribute to phage resistance in Yersinia pestis. Front. Cell. Infect. Microbiol. 13:1174510. doi: 10.3389/fcimb.2023.1174510
Received: 26 February 2023; Accepted: 04 May 2023;
Published: 26 May 2023.
Edited by:
Xihui Shen, Northwest A&F University, ChinaReviewed by:
Lotta Johanna Happonen, Lund University, SwedenChao Pan, Beijing Institute of Biotechnology, China
Bo Pang, National Institute for Communicable Disease Control and Prevention (China CDC), China
Copyright © 2023 Xiao, Qi, Song, Lv, Chen, Zhao, Wu, Li, Xin, Jin, Li, Xu, Tan, Du, Cui, Zhang, Yang, Zhao and Song. This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) and the copyright owner(s) are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
*Correspondence: Yajun Song, c29uZ3lqQGJtaS5hYy5jbg==; Xilin Zhao, emhhb3g1QG5qbXMucnV0Z2Vycy5lZHU=
†These authors have contributed equally to this work and share first authorship