Potent, specific MEPicides for treatment of zoonotic staphylococci
Authors:
Rachel L. Edwards aff001; Isabel Heueck aff001; Soon Goo Lee aff002; Ishaan T. Shah aff001; Justin J. Miller aff001; Andrew J. Jezewski aff003; Marwa O. Mikati aff001; Xu Wang aff004; Robert C. Brothers aff004; Kenneth M. Heidel aff004; Damon M. Osbourn aff005; Carey-Ann D. Burnham aff001; Sophie Alvarez aff007; Stephanie A. Fritz aff001; Cynthia S. Dowd aff004; Joseph M. Jez aff008; Audrey R. Odom John aff001
Authors place of work:
Department of Pediatrics, Washington University School of Medicine, St. Louis, Missouri, United States of America
aff001; University of North Carolina-Wilmington, Wilmington, North Carolina, United States of America
aff002; Department of Molecular Microbiology, Washington University School of Medicine, St. Louis, Missouri, United States of America
aff003; Department of Chemistry, George Washington University, Washington, DC, United States of America
aff004; Department of Chemistry, Saint Louis University, St. Louis, Missouri, United States of America
aff005; Department of Pathology and Immunology, Washington University School of Medicine, St. Louis, Missouri, United States of America
aff006; Department of Agronomy and Horticulture, University of Nebraska-Lincoln, Lincoln, Nebraska, United States of America
aff007; Department of Biology, Washington University, St. Louis, Missouri, United States of America
aff008
Published in the journal:
Potent, specific MEPicides for treatment of zoonotic staphylococci. PLoS Pathog 16(6): e32767. doi:10.1371/journal.ppat.1007806
Category:
Research Article
doi:
https://doi.org/10.1371/journal.ppat.1007806
Summary
Coagulase-positive staphylococci, which frequently colonize the mucosal surfaces of animals, also cause a spectrum of opportunistic infections including skin and soft tissue infections, urinary tract infections, pneumonia, and bacteremia. However, recent advances in bacterial identification have revealed that these common veterinary pathogens are in fact zoonoses that cause serious infections in human patients. The global spread of multidrug-resistant zoonotic staphylococci, in particular the emergence of methicillin-resistant organisms, is now a serious threat to both animal and human welfare. Accordingly, new therapeutic targets that can be exploited to combat staphylococcal infections are urgently needed. Enzymes of the methylerythritol phosphate pathway (MEP) of isoprenoid biosynthesis represent potential targets for treating zoonotic staphylococci. Here we demonstrate that fosmidomycin (FSM) inhibits the first step of the isoprenoid biosynthetic pathway catalyzed by deoxyxylulose phosphate reductoisomerase (DXR) in staphylococci. In addition, we have both enzymatically and structurally determined the mechanism by which FSM elicits its effect. Using a forward genetic screen, the glycerol-3-phosphate transporter GlpT that facilitates FSM uptake was identified in two zoonotic staphylococci, Staphylococcus schleiferi and Staphylococcus pseudintermedius. A series of lipophilic ester prodrugs (termed MEPicides) structurally related to FSM were synthesized, and data indicate that the presence of the prodrug moiety not only substantially increased potency of the inhibitors against staphylococci but also bypassed the need for GlpT-mediated cellular transport. Collectively, our data indicate that the prodrug MEPicides selectively and robustly inhibit DXR in zoonotic staphylococci, and further, that DXR represents a promising, druggable target for future development.
Keywords:
Staphylococcus – Zoonoses – Antimicrobial resistance – Staphylococcal infection – Isoprenoids – Esters – Pro-drugs – Phosphonic acids
Introduction
Coagulase-positive staphylococci, such as S. pseudintermedius and S. schleiferi subsp. coagulans, are leading causes of skin, soft tissue, and invasive infections in companion animals such as dogs and cats. In addition, these organisms cause zoonotic infections in humans that are clinically indistinguishable from infections with S. aureus including pneumonia, skin and soft tissue infections, hardware infections, and bacteremia[1–5]. Newer clinical microbiological techniques, such as mass spectrometry, now readily distinguish S. aureus from zoonotic coagulase-positive staphylococci, which were previously often misidentified[3,6,7]. Thus, there is a growing recognition of the importance of zoonotic staphylococci in human disease. Because mecA-mediated methicillin resistance is on the rise in both veterinary and human clinical isolates, new antibacterial strategies to specifically target zoonotic staphylococci are highly desirable[8–10].
Two distinct and independent pathways for isoprenoid biosynthesis have evolved, the mevalonate pathway and a mevalonate-independent route that proceeds through methylerythritol phosphate, called the MEP pathway[11]. Unusual among bacteria, the least common ancestor of all Staphylococcus spp. appears to have possessed both pathways. Primate-associated staphylococcal lineages, including S. aureus, possess the mevalonate pathway, and evidence suggests that mevalonate pathway activity is required for peptidoglycan synthesis, growth, and virulence[12–14]. In contrast, nonprimate-associated staphylococcal species, including S. pseudintermedius and S. schleiferi, utilize the MEP pathway for isoprenoid biosynthesis[15]. Importantly, humans and other mammals lack homologs of MEP pathway enzymes, and MEP pathway activity is required for cellular growth in all organisms in which it has been experimentally determined[16–21]. Thus, new chemical inhibitors of MEP pathway enzymes hold promise as effective antimicrobials that may provide a high margin of safety.
The first dedicated enzyme of the MEP pathway, deoxyxylulose phosphate reductoisomerase (DXR; E.C. 1.1.1.267), is rate-limiting for MEP pathway activity. DXR is known to be susceptible to small molecule inhibition. For example, the phosphonic acid antibiotic fosmidomycin (FSM) is a slow, tight-binding, competitive inhibitor of DXR[22]. FSM is safe and well-tolerated in humans and animals[23–25]. Unfortunately, FSM has poor oral bioavailability and a short serum half-life, which has hampered clinical efficacy. Moreover, the charged nature of FSM and its phosphonate analogs has challenged their clinical development as the compounds are excluded from cells unless actively transported. As a result, many microorganisms, such as Mycobacterium tuberculosis and Toxoplasma gondii, are inherently resistant to FSM (due to poor cellular uptake) even though FSM potently inhibits their DXR orthologs in vitro[16,18,26]. In Gram-negative organisms, FSM resistance can be achieved by reduced expression or activity of a glycerol-3-phosphate/Pi antiporter (GlpT) [27,28], presumed to be required for FSM import.
In this work, we use the highly specific inhibitor FSM to chemically validate the MEP pathway enzyme DXR as an essential, druggable antibacterial target for zoonotic staphylococcal infections. Furthermore, we establish the structural and enzymatic mechanism of staphylococcal DXR inhibition by FSM. Using a chemical genomics approach, we define the genetic basis of FSM resistance in zoonotic staphylococci and define the FSM transporter GlpT in these strains. Finally, we reveal that structurally related lipophilic ester prodrugs (called MEPicides) yield substantially increased potency and circumvent the need for GlpT-dependent import. Thus, lipophilic prodrugs provide a promising new approach to combat zoonotic staphylococcal infections.
Results
Anti-staphylococcal activity of canonical MEP pathway inhibitors
Because previous evidence had suggested that zoonotic staphylococci might be sensitive to MEP pathway inhibition, we quantified the dose-dependent antibacterial effects of FSM and FR-900098, a structurally similar DXR inhibitor (Fig 1)[15]. FSM was 5-10-fold more potent against both S. schleiferi (IC50 = 0.78 ± 0.13 μM) and S. pseudintermedius (IC50 = 0.31 ± 0.04 μM), respectively (Table 1), despite modest chemical differences between the two inhibitors. Data indicate that both compounds elicit their effect via a bacteriostatic mechanism-of-action, as neither caused a substantial drop in viable cells (S1 Fig). Because S. aureus does not utilize the MEP pathway for isoprenoid biosynthesis, neither FSM nor FR-900098 inhibit S. aureus growth (Table 1). Together, these data indicate that both S. schleiferi and S. pseudintermedius have a functional MEP pathway that is required for bacterial growth.
Fosmidomycin inhibits isoprenoid metabolism in zoonotic staphylococci
To establish the presence of MEP pathway intermediates and to determine the cellular mechanism-of-action of FSM, we performed targeted metabolic profiling of MEP pathway intermediates in S. schleiferi and S. pseudintermedius, with and without drug treatment. We confirmed that both species contain MEP pathway intermediates, including the DXR substrate, deoxyxylulose 5-phosphate (DOXP) and the downstream metabolites 4-diphosphocytidyl-2-C-methylerythritol (CDP-ME) and methylerythritol cyclodiphosphate (MEcPP) (Fig 2). Upon FSM treatment, intracellular levels of DOXP increase dramatically (23.8-fold; p < 0.05 and 34.8-fold; p < 0.05 for S. schleiferi and S. pseudintermedius, respectively), consistent with DXR inhibition. Similarly, intracellular levels of CDP-ME and MEcPP are substantially reduced following FSM treatment (CDP-ME 5.5-fold; p< 0.05 and 2.6-fold; p < 0.05 and MEcPP 4.5-fold; p < 0.01 and 2.4-fold; p < 0.05 for S. schleiferi and S. pseudintermedius, respectively), consistent with FSM-mediated reduction in MEP pathway metabolism. Together, these data confirm the presence of active MEP pathway metabolism in zoonotic staphylococci and establish that FSM inhibits growth through MEP pathway inhibition.
Fosmidomycin is a competitive inhibitor of S. schleiferi DXR
To establish the enzymatic mechanism-of-action of DXR inhibitors against staphylococci, we cloned and purified S. schleiferi DXR (S2 Fig; S1 Table). Enzymatic characterization of DXR confirmed a Michaelis constant (Km) [DOXP] (0.52 ± 0.08 mM), similar to that of other DXR orthologs (Fig 3A)[29,30]. Both FSM and FR-900098 inhibit S. schleiferi DXR in a dose-dependent manner (Table 1). Further, we confirm that DXR inhibition by FSM is competitive with respect to the DOXP substrate, with a Ki [DOXP] of 0.29 ± 0.022 μM (Fig 3B).
Structural basis of fosmidomycin inhibition
To establish the structural basis of FSM action, we solved the three-dimensional structures of S. schleiferi DXR as an apoenzyme and a FSM complex to 2.15 Å and 2.89 Å resolution, respectively (S2 Table; Fig 4). S. schleiferi DXR is a physiologic dimer with each monomer related by crystallographic symmetry (Fig 4A). A DALI search identified multiple DXR from Escherichia coli, Plasmodium falciparum, M. tuberculosis, and other microbes (Z-scores: 49–51; r.m.s.d. ~1.6 Å2 for 370–400 Cα-atoms; 39–40% amino acid sequence identity)[31–36]. The monomer consists of three regions (Fig 4A): an N-terminal α/β-domain with a central 7-stranded β-sheet (β1-β7) and 7 α-helices that serves as the nucleotide binding site; a middle region of the protein that includes a second β-sheet (β8-β11) and 4 α-helices (α8 and α12-α14); and a C-terminal α-helical domain (α9-α11 and α15-α18) that locks FSM into the active site[37].
Clear electron density for FSM was observed in the active site (Fig 4B) and revealed multiple protein-ligand interactions (Fig 4C). Interactions with Ser170, Ser206, Asn211, and Lys212 positions the FSM phosphonate toward the catalytic histidine (His241) and the NADP(H) binding site. The hydroxamic acid of the ligand contacts Asp144, Glu146, and Glu215. Additional van der Waals contacts are provided by Trp196, which resides in the α10-α11 loop. Comparison of the S. schleiferi DXR apoenzyme and FSM complex structures reveals how the C-terminal capping region (α9-α11 and α16–18) shifts position to allow for the α10-α11 loop to position Trp196 adjacent to the inhibitor (Fig 4D). Movement of this flexible loop is a key feature for FSM inhibition of DXR from a variety of microorganisms[38]. The residues that interact with FSM in the S. schleiferi DXR are conserved in the crystal structures of DXR from E. coli, P. falciparum, and M. tuberculosis, with some variation in the sequence of the α10-α11 loop, although the tryptophan that contacts FSM is conserved in all these enzymes [34,36,37].
Resistance selection reveals a candidate FSM transporter, GlpT
To establish the molecular basis of compound uptake, we performed independent, parallel, forward genetic screens for FSM resistance in both S. schleiferi and S. pseudintermedius (Fig 5A). Candidate FSM resistant (FSMR) strains were colony purified and resistance was quantified by MIC determination (Fig 5B and S3 Table). For both S. schleiferi and S. pseudintermedius, FSMR strains possessed FSM MICs >100-fold higher than the wild-type parental lines. We employed whole genome sequencing to characterize the single-nucleotide polymorphisms (SNPs) that were present in the resistant strains (S4 Table). In both species, FSM selective pressure enriched for new nonsynonymous changes in a single homologous locus, RN70_03745 (10/11 S. schleiferi strains) and SPSE_0697 (10/12 S. pseudintermedius strains) (S3A and S3B Fig). These loci are close homologs (>90% sequence identity and 95.4% sequence similarity), which belong to the glycerol-3-phosphate transporter (GlpT) subfamily (Interpro: IPR005267) of the major facilitator superfamily (MFS) family of proteins (Interpro: IPR011701). These data suggest a model in which GlpT mediates FSM import, such that loss of GlpT function confers FSM resistance.
Fosmidomycin-resistance alleles of the candidate transporter, GlpT
We predicted that the FSM-resistance alleles likely reduce GlpT function. In S. schleiferi, nine distinct alleles were found with GlpT changes: two with nonsense mutations and seven others with amino acid variants that are predicted to be highly deleterious (Polyphen-2 score >0.9; S3 Table)[39]. Similarly, in S. pseudintermedius, a total of seven distinct alleles were identified with GlpT sequence changes. Of these, one contained a nonsense mutation and six other GlpT variants contained amino acid substitutions that are strongly predicted to reduce function (Polyphen-2 score >0.9; S3 Table). FSM-resistant variants map along the length of the nearly 50 Kd GlpT transporter, in both S. schleiferi and S. pseudintermedius (S3A and S3B Fig). Altogether, the finding of multiple independent loss-of-function alleles, including nonsense mutations, in two different selections in distinct organisms, strongly suggests that reduced GlpT function is responsible for FSM resistance in these strains.
Fosmidomycin-resistant glpT strains fail to import fosmidomycin
To experimentally address whether GlpT mediates FSM import, we developed a novel liquid-chromatography-mass spectrometry (LC-MS/MS) method to quantify intracellular concentrations of FSM in bacteria. Using this method, we evaluated the intracellular concentration of FSM in drug-treated wild-type S. schleiferi compared to FSM-resistant glpT strains. While wild-type S. schleiferi readily accumulates FSM, four independent FSM-resistant S. schleiferi with glpT mutations do not, establishing staphylococcal GlpT as the first experimentally validated phosphonic acid antibiotic transporter (Fig 6). For one of these strains (4494), the nucleotide polymorphism in the GlpT locus is the only genetic change that distinguishes this FSM-resistant strain from its FSM-sensitive parental line (S4 Table).
Lipophilic ester prodrugs with improved anti-staphylococcal potency
Due to their charged nature, phosphonic acid antibiotics have poor cellular penetration and bioavailability, and serum half-lives are relatively brief[23,25,40]. In the ongoing effort to develop new treatments for malaria and tuberculosis by improving upon the drug-like properties of phosphonates, numerous lipophilic ester prodrugs that target DXR have been generated[41–53]. Our phosphonate parent compounds (1 and 3) are similar in anti-staphylococcal potency to FSM and FR-900098 (Fig 1 and Table 1); however, lipophilic modification of either compound dramatically improves potency (in most cases by 100-fold) against both S. schleiferi and S. pseudintermedius (compare compound 1 to its prodrug, compound 2, and compound 3 to its prodrug, compound 4) (Fig 1 and Table 1). As expected, prodrugs 2 and 4 poorly inhibit purified recombinant S. schleiferi DXR in vitro, since cleavage of the prodrug moiety is required for activity (Table 1). Our data suggest that lipophilic ester modifications improves uptake of the DXR inhibitors, and that active phosphonates are released intracellularly for target inhibition.
Lipophilic prodrugs bypass need for GlpT-mediated transport
We anticipated that our lipophilic ester prodrugs do not require active cellular transport. To evaluate whether GlpT is required for prodrug uptake, we characterized the MEPicide sensitivity of four different FSMR glpT mutant S. schleiferi strains. As expected, we find that FSMR glpT strains are cross-resistant to the phosphonate parent drug (compound 3), suggesting a common mechanism of transport (Fig 7). In contrast, FSMR glpT strains remain sensitive to the MEPicide prodrugs compounds 2 and 4, supporting a model in which GlpT mediates phosphonate transport, with the ester modifications substantially improving cellular uptake (Fig 8)[21].
Discussion
S. schleiferi and the Staphylococcus intermedius group (SIG) (including S. pseudintermedius, S. intermedius, and S. delphini) cause pyodermic infections in companion animals, such as dogs and cats[8]. Treatment of these infections is complicated by rising rates of antimicrobial resistance, particularly methicillin-resistance[54]. A growing recognition that SIG species also cause zoonotic human infections, indistinguishable from infections with S. aureus, has led to new urgency in the search for additional therapeutics against these organisms. The non-mevalonate pathway of isoprenoid biosynthesis through MEP has been previously explored for development of targeted therapeutics for malaria and tuberculosis. In this current work, we establish the MEP pathway enzyme DXR as an attractive new therapeutic target for treatment of infections due to zoonotic staphylococci.
The MEP pathway has a number of major advantages as an antimicrobial target for veterinarian applications. Since mammals utilize the mevalonate pathway for isoprenoid biosynthesis, they lack homologs of the MEP pathway enzymes. As a result, MEP pathway inhibition is expected to have a high therapeutic index. Indeed, previous work indicates that the MEPicides are nontoxic to human cell lines and are well-tolerated in animal models (IC50 of compound 2 against HepG2 cells > 100 μM; IC50s of compounds 3 and 4 against HepG2 cells > 50 μM [42, 53]. Moreover, FSM has been well-tolerated in preclinical and Phase I and II human studies[23–25,55,56]. As an additional advantage of these agents, use of antibiotics in animal health and agriculture has been implicated as a major driver of antimicrobial resistance in human pathogens[57–60]. Of particular relevance to treatment of canine and feline infections, the close physical contact between owners and household pets facilitates not only the cross-colonization of organisms but also direct transfer of drug-resistance traits[61–63]. Because human-associated staphylococci, including S. aureus, S. warnerii, and S. epidermidis, use the mevalonate pathway for isoprenoid biosynthesis, they are not susceptible to MEP pathway inhibitors (Table 1). Importantly, while Gram-negative organisms such as E. coli and Klebsiella pneumoniae are modestly susceptible to MEP pathway inhibition, our lipophilic prodrug compound 2 does not inhibit growth of these organisms (S5 Table). Our MEPicide compounds therefore have a highly specific and valuable antimicrobial spectrum, which may help break the cycle of resistance transfer from antibiotic-treated animals to the microbiota of humans.
In the current study, we establish the cellular, enzymatic, and structural mechanisms-of-action of FSM against zoonotic staphylococci. We confirm that FSM is a competitive inhibitor of staphylococcal DXR, interrupts cellular isoprenoid biosynthesis, and inhibits growth of zoonotic staphylococci. Of note, the staphylococcal DXR enzyme appears somewhat distinct from previously characterized orthologs, particularly in the α10-α11 loop sequence, which could be explored with additional SAR studies (Fig 4). Together, our work provides insights into differences in staphylococcal DXR that may be key to driving future structure-based inhibitor design efforts.
A well-appreciated liability of antibacterial phosphonates, including fosfomycin and FSM, has been the ready acquisition of resistance through loss of transport [27,64–66]. Our work establishes GlpT as the phosphonic acid antibiotic transporter in zoonotic staphylococci (Fig 6). Identification of multiple, independent loss-of-function alleles from independent screens in two separate species is compelling evidence for a role of this locus in FSM-resistance in staphylococci. For several of these strains, GlpT mutations were the only identified genetic changes arising in FSM-resistant staphyloccci. In addition, the homology between staphylococcal GlpT orthologs and Gram-negative phosphonate transporters suggests that the staphylococcal proteins are functionally similar. The finding that lipophilic prodrug MEPicides, which do not require active transport, are still active against the glpT mutant strains indicates that the molecular basis of phosphonate resistance is through loss of GlpT-mediated transport (Fig 7). The prodrug MEPicides circumvent GlpT, a phosphonate transporter that we find to be readily mutated in staphylococci. Future studies to address the potential for resistance to MEPicides will also be important; however, in vitro resistance development alone should not preclude development of this novel class of antibiotics. It has been well documented that S. aureus, when treated with single therapeutic agents, frequently develops in vitro resistance to therapeutics that remain important front-line treatments [67–70]. Instead, great care should be taken when designing treatment regimens for infections by microbes that can rapidly adapt to antimicrobial pressure, such as staphylococci.
It is important to note that while data indicate that the glpT mutants are resistant to phosphonate parent compound 3, the magnitude of resistance is substantially less than that of FSM. These data suggest that compound 3 may preferentially use an alternative transporter, thereby bypassing the dependence on GlpT. Surprisingly, staphylococcal glpT mutants are hypersensitive to MEPicide prodrugs, suggesting that after penetration and cleavage by cellular esterases, the compounds may accumulate intracellularly in the absence of GlpT (Fig 7). Subsequent studies should examine the cellular transport of the MEPicide compounds, and further, explore whether synergy exists between the parent and prodrug varieties of this class of inhibitors. Since serum esterases may act on lipophilic ester prodrugs, understanding the molecular mechanism of prodrug activation in serum and in bacteria will be key to developing prodrugs that remain stable during transport to the site of infection.
The MEPicide prodrugs, including compounds 2 and 4, represent promising leads for ongoing preclinical testing and development of new therapeutics for zoonotic staphylococcal infections. The prodrugs harness the microbial specificity and thus safety of MEP pathway inhibition, while avoiding the dependency on active GlpT-mediated transport. In addition, we find that ester modification has a dramatic effect on anti-staphylococcal potency in vitro, suggesting that phosphonate transport limits the anti-bacterial efficacy of FSM and related compounds. Lipophilic ester modifications have previously been employed to improve pharmacokinetic properties and bioavailability of anti-staphylococcal agents (e.g., cefditoren pivoxil)[71]. Since MEPicide ester modification at the site of infection is necessary to facilitate bacterial cell entry of inhibitors, future studies will aim to understand what chemical features drive intestinal and serum cleavage of the MEPicide prodrugs.
Materials and methods
DXR inhibitors
FSM (Millipore Sigma) and FR-900098 (Millipore Sigma) were resuspended in sterile water. Compounds 1–4 were synthesized and resuspended in DMSO as previously described[41,42,53].
Growth inhibition assays of Staphylococcus species
Overnight cultures were diluted 1:200 in LB media and grown at 37°C until the mid-logarithmic phase (OD600 = 0.5–0.8). Cultures were diluted in a 96-well plate to 1 x 105 in 150 μL LB media and treated with inhibitors at concentrations ranging from 2 nM to 100 μM. Bacteria were grown at 37°C for 20 h with cyclic shaking at 700 rpm in a FLUOstar Omega microplate reader (BMG Labtech). Growth was assessed over 20 h by measuring the OD600 at 20 min increments. The half-maximal inhibitory concentration (IC50) values were determined during logarithmic growth using GraphPad Prism software. All experiments were performed at least in triplicate and data reported represent the mean ± SEM.
Minimum bactericidal (MBC) assay
Overnight cultures were diluted 1:200 in LB media and grown at 37°C until reaching mid-logarithmic phase of growth. Compounds were added to cultures at their respective IC50 and at 10 x IC50, and the bacteria were incubated at 37°C for 24 h while shaking. Cultures were serially diluted in 1 X Dulbecco’s Phosphate Buffered Saline (PBS; Gibco) and plated on LB agar. Colonies were enumerated after overnight growth at 37°C. Values reflect the mean and standard deviations of at least three independent experiments.
Sample preparation for mass spectrometry analysis
Overnight cultures of Staphylococcus spp. were diluted 1:200 in LB media and grown at 37°C until reaching mid-logarithmic phase. Cultures were then treated for 2 h with FSM at 10x their IC50 while shaking at 37°C. For normalization, the OD600 was determined after 2 h of treatment with the DXR inhibitors. Cells were pelleted by centrifugation for 5 min at 3000 x g at 4°C. The supernatants were removed and cells were washed twice with 1 x PBS (Gibco). The supernatants were removed and the pellets stored at -80°C until analysis. MEP intermediates were extracted from the samples using glass beads (212–300 u) and 600 μL chilled H2O: chloroform: methanol (3:5:12 v/v) spiked with PIPES (piperazine-N,N′-bis(2-ethanesulfonic acid) as internal standard. The cells were disrupted with the TissueLyser II instrument (Qiagen) using a microcentrifuge tube adaptor set pre-chilled for 2 min at 20 Hz. The samples were then centrifuged at 16,000 x g at 4°C for 10 min, the supernatants collected, and pellet extraction repeated once more. The supernatants were pooled and 300 μL chloroform and 450 μL of chilled water were added to the supernatants. The tubes were vortexed and centrifuged. The upper layer was transferred to a 2 mL tube PVDF filter (ThermoFisher, F2520-5) and centrifuged for 5 min at 4,000 x g at 4°C. The samples were transferred to new tubes and dried using a speed-vac. The pellets were re-dissolved in 100 μL of 50% acetonitrile.
LC-MS/MS analysis
For LC separation, Luna-NH2 column (3 μm, 150 x 2 mm, Phenomenex) was used flowing at 0.4 mL/min. The gradient of the mobile phases A (20 mM ammonium acetate, pH 9.8, 5% acetonitrile) and B (100% acetonitrile) was as follows: 60% B for 1 min, to 6% B in 3 min, hold at 6% B for 5 min, then back to 60% B for 0.5 min. The LC system was interfaced with a Sciex QTRAP 6500+ mass spectrometer equipped with a TurboIonSpray (TIS) electrospray ion source. Analyst software (version 1.6.3) was used to control sample acquisition and data analysis. The QTRAP 6500+ mass spectrometer was tuned and calibrated according to the manufacturer’s recommendations. The metabolites were detected using MRM transitions that were previously optimized using standards. The instrument was set-up to acquire in negative mode. For quantification, an external standard curve was prepared using a series of standard samples containing different concentrations of metabolites and a fixed concentration of the internal standard. The limit of detection for 1-deoxy-D-xylulose 5-phosphate (DOXP), 4-diphosphocytidyl-2-C-methylerythritol (CDP-ME), and 2-C-methyl-D-erythritol 2,4-cyclopyrophosphate (MEcPP) was 0.0064 μM for a 10 μL injection volume. Data reflect the mean and SD of at least three independent experiments. Student’s t-tests were used to test for significance between untreated (UNT) and drug-treated bacteria (Prism).
Recombinant expression and purification of DXR
Wild-type dxr from S. schleiferi was amplified from genomic DNA using the forward primer 5’-CTCACCACCACCACCACCAT ATGAAAAATATAGCAATTTTAGGCGC-3’ and the reverse primer 3’-ATCCTATCTTACT CACCTACACCTCATATGATTTTGTTTTATAAT-5’ The PCR product was cloned into vector BG1861 by ligation-independent cloning to introduce a N-terminal 6xHis tag, and transformed into Stellar chemically competent cells (Clontech Laboratories)[72]. The sequence was confirmed by Sanger sequencing and the plasmid was transformed into E. coli BL21(DE3) pLysS (Life Technologies). Gene expression was induced for 2 h with 1 mM isopropyl-β-D-thiogalactoside (IPTG) and cells were harvested by centrifugation at 4274 x g for 10 min at 4°C. The cell pellet was lysed by sonication in lysis buffer containing 25 mM Tris HCl (pH 7.5), 100 mM NaCl, 20 mM imidazole, 10% glycerol, 1 mM MgCl2, 1 mM dithiothreitol (DTT), 1 mg/mL lysozyme, 75 U benzonase and 1 Complete Mini EDTA-free protease inhibitor tablet (Roche Applied Science). The hexahistidine-tagged DXR protein was affinity purified from soluble lysate via nickel agarose beads (Gold Biotechnology). Bound protein was eluted in 300 mM imidazole, 25 mM Tris HCl (pH 7.5), 1 mM MgCl2 and 100 mM NaCl. Purified protein was dialyzed in buffer containing 10% glycerol without imidazole prior to analysis. The enzyme was frozen in liquid nitrogen and stored permanently at -80°C.
DXR enzyme activity and inhibitory constant determination
Oxidation of NADPH to NADP+ as a result of substrate turnover was monitored at 340 nm in a POLARstar Omega microplate reader (BMG Labtech)[73]. The standard reaction had a final concentration of 62.5 nM purified DXR protein, 0.5 mM NADPH, 100 mM NaCl, 25 mM Tris pH 7.5, 10% glycerol, 1 mM MgCl2 and 0.09 mg/mL BSA in 50 μL volume per assay. Reactions were initiated by the addition of DOXP after 15 min incubation of the reaction mixture without DOXP at 37°C. Absorption at 340 nm was measured continuously for up to 45 min. For Km [DOXP] determination, DOXP concentrations between 0 and 2 mM were tested at 0.5 mM NADPH. The linear range of enzyme activity was determined by varying the DXR concentration at 1 mM DOXP and 1 mM NADPH. IC50 assays were performed using the standard reaction conditions with the respective amount of DXR inhibitor added to obtain the given final concentrations. Data points from at least three independent replicates were analyzed by nonlinear regression using GraphPad Prism software. Slopes of changing absorbance values were converted to (μM DOXP)(mg enzyme)-1 s -1 using a NADPH standard curve (data not shown). For the determination of the inhibitory constant Ki [FSM] of DXR, enzyme activity over a range of DOXP substrate concentrations between 0 and 2 mM was measured for FSM between 0 mM to 4 mM. Data points from at least three independent replicates were analyzed as described above.
Protein crystallography
Crystals of S. schleiferi DXR were grown at 4°C using the vapor diffusion method in hanging drops of a 1:1 mixture of protein (10 mg mL-1) and crystallization buffer (2 M ammonium sulfate, 100 mM sodium citrate/citric acid, pH 5.5). Crystals of the S. schleiferi DXR•FSM complex were obtained in 100 mM HEPES/MOPS (pH 7.5), 20 mM D-glucose, 20 mM D-mannose, 20 mM D-galactose, 20 mM L-fucose, 20 mM D-xylose, 20 mM N-acetyl-D-glucosamine, 20% glycerol, 10% PEG 4000, and 2 mM FSM. Prior to data collection, crystals were stabilized in cryoprotectant (mother liquor supplemented with 30% glycerol) before flash freezing in liquid nitrogen for data collection at 100 K. All diffraction images were collected at beamline 19-ID of the Argonne National Laboratory Advanced Photon Source at Argonne National Laboratory. HKL3000 was used to index, integrate, and scale the data sets[74]. For phasing of the apoenzyme structure, molecular replacement was performed in PHASER using the x-ray crystal structure of E. coli DXR (PDB: 1T1S) as a search model[31,75]. Two monomers were found in the asymmetric unit, with each forming a physiological dimer by crystallographic symmetry. For iterative rounds of model building and refinement, COOT and PHENIX were used, respectively[76,77]. The resulting model was used to solve the structure of the FSM complex by molecular replacement with PHASER. Two molecules were found in the asymmetric unit with crystallographic symmetry completing each dimer. Data collection and refinement statistics are summarized in S2 Table. Atomic coordinates and structure factors of S. schleiferi DXR (PDB:6MH4) and the S. schleiferi DXR•FSM complex (PDB:6MH5) were deposited in the RCSB Protein Data Bank.
Generation of FSM-resistant mutants in S. schleiferi and S. pseudintermedius
Clinical isolates of S. schleiferi (S53022327s) and S. pseudintermedius (H20421242p) were cloned and adapted to laboratory media via four rounds of sequential colony isolation and growth on LB agar plates. The isolated FSM-sensitive parental clones were incubated overnight on LB agar containing FSM (32 μM). Surviving single colonies were re-struck onto LB agar for clonal isolation. FSM resistance of isolated clones was confirmed by overnight growth on LB agar containing FSM (32 μM). The FSM-sensitive parental clones were used as a control to confirm growth and antibiotic-resistance.
Quantification of MEPicide potency
Minimum Inhibitory Concentration (MIC) assays were conducted by microtiter broth dilution in clear 96-well plates[78]. MEPicides were serially diluted in duplicate at concentrations ranging from 1.5 mM– 19.5 nM in 75 μL of LB broth. Bacteria cultured without drug were used as a positive control for growth. The plates were inoculated with 75 μL bacteria diluted to 1 x 105 CFU/mL in LB. Plates were incubated for 18–20 h while shaking at 200 RPM at 37°C. The plates were then visually inspected, and the MIC value was defined as the lowest concentration of MEPicide that prevented visual growth.
Whole genome sequencing and variant discovery
Genomic DNA was isolated from overnight cultures of S. pseudintermedius and S. schleiferi using a standard phenol-chloroform extraction and ethanol precipitation protocol. Sequencing libraries were prepared and sequenced by the Washington University Genome Technology Access Center (GTAC). 1 μg of DNA was sonicated to an average size of 175 bp. Fragments were blunt ended and had an A base added to the 3´ end. Sequence adapters were ligated to the ends and the sequence tags were added via amplification. Resulting libraries were sequenced on an Illumina HiSeq 2500 to generate 101 bp paired end reads. DNA quantity and quality were assessed by GTAC using Agilent Tapestation.
For WGS, sequences from GenBank were retrieved from the following organisms: S. pseudintermedius ED99 (accession number CP002478) and S. schleiferi 1360–13 (CP009740) assemblies were downloaded from NCBI (ftp://ftp.ncbi.nlm.nih.gov). Paired-end reads were aligned to each of the available genomes using Novoalign v3.03. (Novocraft Technologies). Duplicates were removed and variants were called using SAMtools[79]. SNPs were filtered against parent variants and by mean depth value and quality score (minDP = 5, minQ = 37)[80]. Genetic variants were annotated using SnpEff v4.3 (S4 Table)[81]. For all samples, at least 90% of the genome was sequenced at 20x coverage. All whole genome sequencing data is available in the NCBI BioProject database and Sequence Read Archive. Point mutations found in the GlpT domain were mapped onto the predicted transmembrane topology of GlpT using Protter[82].
Sanger Sequencing of S. schleiferi and S. pseudintermedius glpT
Reference sequences for glpT in S. schleiferi (WP_016426432.1) and S. pseudintermedius (WP_014613322.1) were found with the Basic Local Alignment Search Tool (BLAST, v. 2/2/22). The regions of interest were amplified from S. pseudintermedius and S. schleiferi using gene-specific primers (S1 Table). Amplicons were sequenced by the Washington University Protein and Nucleic Acid Laboratory using BigDye Terminator v3.1 Cycle Sequencing reagents (Life Technologies). Representative traces for all strains are available through the NCBI Trace Archive.
Quantification of Intracellular FSM
Overnight cultures of Staphylococcus spp. were diluted in LB media and grown at 37°C until reaching mid-logarithmic phase. Cultures were then treated with FSM at 10x the WT IC50 (7.8 μM) while shaking at 37°C. At the time points indicated, 15 mL of each culture was transferred to fresh tube and the cells were pelleted by centrifugation for 10 min at 3000 x g at 4°C. The supernatants were removed and the pellets resuspended by vortexing in 200 μL acetonitrile with 100 ng/mL enalapril. Samples were stored at -80°C until LC-MS analysis.
The intracellular concentration of FSM was determined by LC-MS (AB Sciex API4000, Foster City, CA) operated in MRM mode with negative electrospray ionization. The monitored mass transitions for FSM and enalapril were m/z: 181.909>135.700 and 375.090>114.100, respectively. Samples were injected onto an Armor C18 column (3 cm x 2.1 mm x 5 um, Analytical Sales and Services, Flanders, NJ), and eluted with a gradient. Mobile phase A was 0.1% formic acid in water and mobile phase B was 0.1% formic acid in acetonitrile. Samples of cells were thoroughly mixed in acetonitrile containing enalapril as an internal standard to precipitate proteins and then centrifuged at 3200 rpm for 5 min. The acetonitrile was transferred to a 96-well plate and allowed to evaporate to dryness under nitrogen. The samples were reconstituted in 150 μL of mobile phase A before analysis. The gradient program for the LC held mobile phase B at 2% for 0.1 min before ramping to 100% mobile phase B in 1 min at a flow rate of 0.4 mL/min. Data analysis was performed using Analyst software (AB Sciex, Foster City, CA). Standards were prepared by addition of FSM to blank cellular preparations over a concentration range of 1 ng/mL to 500 ng/mL.
Supporting information
S1 Fig [eps]
DXR inhibitors are bacteriostatic.
S2 Fig [m]
SDS-PAGE of purified . DXR.
S3 Fig [a]
Membrane topology of GlpT.
S1 Table [xlsx]
Primers.
S2 Table [xlsx]
Summary of crystallographic data collection and refinement statistics.
S3 Table [docx]
FSM MICs, alleles, GlpT protein changes, and Polyphen-2 scores for FSM strains.
S4 Table [xls]
SNP calls from FSM . and . strains.
S5 Table [xlsx]
Inhibitory effect of MEPicides against a panel of Gram-negative bacteria.
S1 File [docx]
Supplemental methods.
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