Antibiotic Capture by Bacterial Lipocalins Uncovers an Extracellular Mechanism of Intrinsic Antibiotic Resistance

Strains and reagents.Table S2 lists the bacteria and plasmids used in this study. Bacteria were grown in LB broth, supplemented with 0.4% rhamnose when required at 37°C. E. coli cultures were supplemented as required with the antibiotics (final concentrations) tetracycline (30 µg/ml), kanamycin (40 µg/ml), and trimethoprim (50 µg/ml). B. cenocepacia cultures were supplemented as required with trimethoprim (100 µg/ml) and tetracycline (100 µg/ml). Antibiotics (Sigma) were diluted in water, except for PmB, which was diluted in 0.2% bovine serum albumin–0.01% glacial acetic acid buffer. Rifampin was dissolved in dimethyl sulfoxide (DMSO).

General molecular techniques.DNA manipulations were performed as previously described (47). T4 DNA ligase (Roche Diagnostics), Antarctic phosphatase (New England Biolabs), and restriction endonucleases were used as recommended by the manufacturers. Transformation of E. coli GT115 and DH5α was performed by the calcium chloride method (48). Mobilization of plasmids into B. cenocepacia was conducted by triparental mating (49) with E. coli DH5α carrying the helper plasmid pRK2013 (50). DNA amplification by PCR was performed with a C1000 thermal cycler (Bio-Rad Laboratories Ltd., Mississauga, Ontario, Canada) using Taq or HotStar HiFidelity DNA polymerase (Qiagen) and optimized for each primer pair. DNA sequencing was carried out at Eurofins, Huntsville, AL. The DNA sequences were analyzed with the BLAST computer program and compared to the sequenced genome of B. cenocepacia strain J2315. The sequence of S. aureus gene SAUSA300_2620 was optimized for B. cenocepacia codon usage and custom synthesized at Eurofins. Cloning, expression, and purification of bacteriocalins were performed as previously described (17). Transcriptional fusions to luxCDABE and the subsequent luminescence expression assays were performed as previously described (37). For site-directed mutagenesis, pOE16 was amplified with Pfu polymerase and the appropriate primer pairs; the PCR products were digested overnight with 1 U of DpnI at 37°C and then introduced into E. coli DH5α competent cells by transformation. Transformants were selected on LB agar plates supplemented with kanamycin; amino acid replacements were confirmed by DNA sequencing.

Protein analysis and Western blotting.Overnight cultures were diluted to an optical density at 600 nm (OD₆₀₀) of 0.03 in 30 ml of fresh LB medium with or without PmB and incubated for 3.5 h at 37°C at 200 rpm. Following incubation, cells equivalent to an OD₆₀₀ of ~0.2 were pelleted, resuspended in 30 µl of SDS-PAGE protein loading dye, and boiled to obtain whole-cell lysates. Secreted proteins were precipitated from the supernatant of the rest of the cultures with 10% trichloroacetic acid as previously described (51). Precipitated proteins were resuspended in Tris buffer at 1 M and pH 7.5. The volume of protein samples loaded onto the 16% SDS-polyacrylamide gel was normalized to the OD₆₀₀ value. After SDS-PAGE, proteins were transferred onto nitrocellulose membranes and the membranes were blocked overnight at 4°C with Western blocking reagent (Roche Diagnostics, Laval, QC, Canada) in TBST (50 mM Tris-HCl [pH 7.5], 150 mM NaCl, 0.1% Tween 20). The primary antibody, anti-FLAG M2 monoclonal antibody (Sigma) or anti-α-subunit RNA polymerase (E. coli) (Neoclone, Madison, WI), was diluted to 1:15,000 in TBST and applied for 1.5 h. The secondary antibody, goat anti-mouse Alexa Fluor 680 IgG antibody (Invitrogen), was diluted to 1:15,000 and applied for 1 h. Western blot assays were developed with the LI-COR Odyssey infrared imaging system (LI-COR Biosciences, Lincoln, NE).

Antibiotic susceptibility testing.The inoculum of B. cenocepacia K56-2, the appropriate mutants, and other bacterial species was prepared by the direct colony suspension method according to CLSI (52). Cultures with an OD₆₀₀ of 0.0008 in fresh cation-adjusted Mueller-Hinton broth (MHB) with or without the antibiotic were incubated at 37°C with medium shaking continuously in a Bioscreen C automated growth curve analyzer (MTX Lab Systems, Vienna, VA). Bacterial growth was assessed turbidimetrically at 600 nm. E-test strips (AB BioMérieux, Solna, Sweden) were applied to agar plates (17 ml of agar in an 85-mm petri dish) inoculated with test bacteria by swabbing overnight cultures diluted to an OD₆₀₀ of 0.04; plates were then incubated at 37°C for 24 h. Alternatively, population profiling analysis was performed turbidimetrically or by CFU counting as previously described (17). For in vitro protection assays, B. cenocepacia bacteriocalins were added to LB broth at a final concentration of 1.5 µM.

In vitro binding assays.In vitro binding assays were performed as previously described (23), with a few modifications. Purified BCNs were prepared in phosphate-buffered saline (PBS, pH 7.4). Phospholipids and Nile red were prepared in DMSO. The binding of each fluorescent probe to BCNs was measured by titrating 100 µl of BCNs (1.5 µM) in a flat-bottom 96-well microtiter plate (LUMITRAC 200 White; Greiner Bio-One, Monroe, NC) with aliquots of increasing concentrations of probe until the fluorescence intensity reached a plateau, indicating that all of the binding sites were occupied. All spectra were corrected for background fluorescence determined from probe-into-buffer titrations. Fluorescence was measured with a Cary Eclipse fluorescence spectrophotometer (Varian) set at an excitation wavelength (λ_ex) specific for each probe, as follows: Nile red, 550 nm; BODIPY phospholipids, 500 nm for fatty acyl BODIPY-labeled phosphocholine and 505 nm for head group BODIPY-labeled phosphoethanolamine. The emission spectrum for each probe was collected across the following wavelengths (λ_em): Nile red, 590 to 750 nm; BODIPY phospholipids, 510 to 665 nm. The background-corrected binding fluorescence with each probe was fitted to a one-site binding model as previously described for human AGP (23). The equilibrium binding affinity constant for the probe-BCN complex (K_d), the probe concentration needed to achieve half-maximum binding at equilibrium, was determined by nonlinear least-squares regression analysis of the binding isotherms with GraphPad Prism v 5.0 software (GraphPad Software, Inc.).

For probe displacement experiments, antibiotic solutions and fat-soluble vitamins (prepared in DMSO) diluted in PBS, pH 7.4, were titrated against a BCN-probe complex at a saturating concentration necessary to obtain the maximum fluorescence when bound. Probe displacement was measured as the corresponding decrease in fluorescence upon the progressive increase in the antibiotic concentration. The binding inhibition constants (K_is) of the test compounds were determined by nonlinear regression analysis with competition-binding equations for one-site binding calculated by GraphPad Prism v 5.0 software. The lower the K_i values, the higher the affinity of the molecule for BcnA. All fluorometric assays were conducted in duplicate three independent times.

G. mellonella larva in vivo infection.Larval infection assays were performed as previously described (53), with modifications. Overnight cultures were diluted in PBS, pH 7.4, with or without B. cenocepacia BCNs at a 1.5 µM final concentration to the following OD₆₀₀s: B. cenocepacia and P. aeruginosa PAO1, 0.00004; K. pneumoniae Kpn18, 0.04; A. baumannii AB1, 0.4; S. aureus USA300, 0.004. The larvae were injected with 10 µl of the bacterial suspensions or sterile PBS (10 larvae/group in each experiment) with 10-µl MICROLITER syringes (Hamilton). The larvae were incubated at 30°C, and their viability was checked at regular time intervals. In similar assays, five larvae/group were sacrificed at 200 min postinfection and the hemolymph was extracted as previously described (53). The hemolymph was immediately serially diluted in PBS and plated on LB agar supplemented with 0.3% cetrimide or 200 µg/ml ampicillin–25 µg/ml PmB to quantify the CFU of P. aeruginosa PAO1 or B. cenocepacia, respectively, recovered from the infected larvae.

Intraperitoneal infection of mice.A clinical isolate of P. aeruginosa (strain Q502) was grown overnight in nutrient broth at 37°C with constant agitation. The bacteria were centrifuged at 2,000 × g and washed three times in sterile, endotoxin-free PBS. The bacteria were resuspended in sterile, injection-grade saline, and the inoculum was adjusted to an OD of 0.5 (A₅₅₀). Female adult (8- to 12-week-old) C57BL6 mice were infected i.p. with 100 μl of the bacterial suspension. Subsequent growth of the inoculum on nutrient agar demonstrated that each animal received 10⁶ CFU. Six mice per treatment were used. This was determined by GraphPad StatMate 2.0 to ensure 80% power to detect statistically significant effects between antibiotic-treated and untreated animals at a significance level (alpha) of 0.05, two tailed. The actual power was >99%. Mice were selected at random from open stock cages (10 per cage), earmarked to allow individual identification, and then sequentially placed into treatment groups. During the course of the experiment, mice were housed in individually ventilated cages. This method of assigning animals to groups ensures an approximately equal distribution of mice from different stock cages in each group to minimize the influence of cage-to-cage variability. At the time of inoculation, the mice were treated with the standard pediatric PmB dose of 20,000 U/kg (n = 6), PmB and 100 µl of 25 µM BCN (n = 6), BCN only (n = 6), or a saline control (n = 6) by i.p. injection. The individual components injected into mice were added to the same syringe immediately before i.p. injection. Animals were culled by cervical dislocation 4 h postinoculation. That time point was selected because by that time point and under the infection conditions used, the untreated mice reach the humane endpoint and need to be culled, as defined within the UK Home Office license under which the experiments were carried out (PLL 2700). Because of the virulence of the clinical isolate and the dose of the bacterial inoculum and because the bacteria are delivered i.p., the mice rapidly succumb to the infection. In contrast, those given effective antibiotic treatment rapidly clear the infection and remain perfectly healthy. The vast divergence between the responses seen in this model provides us with the statistical power to robustly assess the microbial response to antibiotic therapies without requiring the use of a very large number of mice per group. We are therefore adhering to the reduction principle of the three R’s. The peritoneal cavity was lavaged with 3.5 ml of ice-cold, sterile, endotoxin-free PBS, and the volume recovered was recorded. Serial dilutions of the lavage fluid were plated onto cetrimide agar; and bacterial colonies were counted after 24 h of growth at 37°C. Harvesting of the samples and quantification of the bacterial burdens in the mice were done while blinded to the treatment groups. Data were not normally distributed, and there was no equal variance between groups; therefore, a nonparametric Kruskal-Wallis test was used. The mouse infection experiments carried out were assessed by the Queen’s University Belfast animal welfare and ethical review body (AWERB) committee and conducted under a license issued by the UK Home Office under the Animals (Scientific Procedures) Act 1986, amended in 2012.

Antibiotic bioassay.Antibiotic test solutions with or without 1.5 µM BcnA were incubated for 30 min at 37°C with rotation. The solutions were filtered through filter units with a 10-kDa cutoff by centrifugation at 7,500 × g, at 4°C for 10 min. The antibiotic concentrations in the filtrates were determined by spotting 5 µl onto sterile filter discs placed on agar plates swabbed with the test bacteria. Petri dishes (15-cm diameter) containing 40 ml of LB agar were swabbed with bacterial suspensions with an OD₆₀₀ of 0.04. The plates were incubated at 37°C for 24 h. Each plate included four discs containing standard concentrations of the antibiotic alongside the discs impregnated with test and control antibiotic solutions. E. coli DH5α was used for bioassays of PmB, norfloxacin, ceftazidime, and gentamicin, and S. aureus USA300 was used for bioassays of rifampin. The theoretical disc contents of the test antibiotic solutions were 10, 5, 2, 30, and 10 µg for PmB, rifampin, norfloxacin, ceftazidime, and gentamicin, respectively. Standard antibiotic discs contained a 2-fold higher concentration than, the same concentration as, or a 2- or 4-fold lower concentration than the test antibiotic discs. After incubation, the clear zones of inhibition were measured and the antibiotic concentrations were determined from standard curves constructed from the standard antibiotic discs.

Structure determination.BcnA and BcnB were purified by fast protein liquid chromatography and concentrated to ~20 mg/ml in a mixture of 20 mM Tris (pH 7.5) and 100 mM NaCl (1% DMSO for BcnB) with >95% purity. Protein solutions were mixed 1:1 with mother liquor, and crystals were grown at room temperature. BcnA crystals grew with 0.1 M Tris (pH 8.5) and 2.4 M ammonium sulfate (final pH of 8.0) as the mother liquor. BcnB crystals grew with 0.1 M HEPES (pH 6.5)–26% polyethylene glycol 6000 as the mother liquor. Data sets were collected on beamline 08ID-1 at Canadian Light Sources (54), integrated with iMOSFLM (55), and scaled with AIMLESS (56) from CCP4. Phases for BcnA and BcnB were obtained with Phaser.MRage (57) from PHENIX with PDB accession no. 2FGS and 1WUB, respectively, as the search models. Both structures were initially built with AutoBuild (58) from PHENIX and then manually built with Coot (59). The BcnA and BcnB structures were refined with phenix.Refine (60) from PHENIX and REFMAC5 (61) from CCP4, respectively, with translation-libration-screw motion refinement for both. Figures were generated with Pymol, version 1.8 (https://www.pymol.org/). Data collection and refinement statistics are provided in Table S1 in the supplemental material. SEC-MALS experiments were conducted to assess the oligomeric solution state of BcnA and BcnB as previously described (62) with proteins diluted to 1 mg/ml in 20 mM Tris (pH 7.5)–100 mM NaCl.

Computational methods.All of the following codes can be obtained under license agreement: AMBER 12 and AmberTools (http://www.ambermd.org), Maestro Suite (Schrödinger, Cambridge, MA), AutoDock 4.2.2, and AutoDockTools (http://autodock.scripps.edu; free software). Amber and Maestro have Academic fees. We studied the stability of the two X-ray structures of BcnA and BcnB, as well as the D82A-D93A mutant, by MD simulations as implemented in AMBER 12. The initial model of D82A-D93A was built with AmberTools. Missing hydrogen atoms were added, and the protonation state of ionizable groups was computed by using Maestro Protein Preparation Wizard, version 9.3 (Schrödinger, Cambridge, MA). Atom types and charges were assigned according to AMBER ff10 force field (63). The three molecular systems were hydrated by using cubic boxes containing explicit TIP3P water molecules extending 10 Å away from any protein atom for simulating the aqueous environment with the help of AmberTools with added counterions to neutralize the system. Before the MD simulations, the two systems were equilibrated under the following protocol: an initial 8,000 steps of steepest-descent minimization, followed by heating of the system with position restraint (force constant of 20 kcal mol⁻¹ Å⁻²) for all protein atoms during 10 ps of MD simulation increasing the temperature from 100 K to 300 K plus an additional 15 ps at a constant temperature of 300 K. Position restraint was gradually decreased for 100 ps at a constant 300 K, until the full system was under no restraint with constant temperature (300 K) and pressure (1 atm). After equilibration, 20 ns of MD simulation was run at a constant temperature (300 K) and pressure (1 atm). Short- and long-range forces were calculated every one and two time steps, respectively (each time step was 2.0 fs), constraining the covalent bonds involving hydrogen atoms to their equilibrium values. Long-range electrostatic interactions were accounted for by means of the particle mesh Ewald approach applying periodic boundary conditions. The RMSD as a function of time with respect to the starting structure of the α-C atoms was computed with CPPTRAJ (64). The three-dimensional (3D) coordinates of the structures of BcnA and BcnB subjected to the equilibration protocol described above were used for docking purposes. The two models were prepared for docking calculations by adding Kollman charges (65) with the help of AutoDockTools.

3D coordinates of norfloxacin, PmB, ceftazidime, gentamicin, Nile red, and α-tocopherol were built in Corina (66) from the SMILES code. The 3D structure of rifampin was extracted from the crystallographic structure PDB accession no. 1LSV. The structures of the seven ligands were protonated at pH 7.0 with Epik (67) and then optimized with MMFFs force field by with MacroModel version 9.9 (Schrödinger, Cambridge, MA). Additionally, the structure of PmB was subjected to 100 ps of MD simulation at 300 K. Ligands were prepared for docking calculations with AutoDockTools by adding Gasteiger charges (68) and setting all rotatable bonds free to move during the docking calculation.

Docking calculations of all compounds were performed by means of AutoDock 4.2.2 (69). Analysis was performed with the help of AutoDockTools. The grid point spacing was set at 0.375 angstroms, and a hexahedral box was built with x, y, and z dimensions of 21.00, 26.25, and 27.75 angstroms centered in the binding site of the protein. Two hundred runs with the Lamarckian genetic algorithm were performed with a population size of 100 and 250,000 energy evaluations. Side chains of residues Y85, W94, and Q41 were considered flexible during the docking protocol.

BCN consensus motif determination.A subset of 187 curated BcnA homologues from different bacterial species and families were used to obtain a consensus motif generated by the Gapped Local Alignment Motifs GLAM2 tool (70). This motif was verified by analyzing an alignment of 1,995 BCN homologues with CLUSTAL-omega and visualized with JalView. In addition, upon submitting the predicted motif to the GLAM2Scan database (70) against B. cenocepacia, P. aeruginosa PAO1, M. tuberculosis H37Rv, and S. aureus USA300, the correct homologues only were detected as BCNs for each of the organisms.

Statistical analyses.Statistical analyses were conducted with GraphPad Prism 5.0. All of the results shown are the mean ± the standard error of the mean (SEM) unless otherwise stated. Unless otherwise stated, data were assumed to follow a Gaussian distribution as determined by the D’Agostino-Pearson omnibus K2 normality test whenever possible, and hence, t tests and analysis of variance (ANOVA) were used. An unpaired t test was used to compare the means of two unmatched groups. A paired t test was used to compare the means of two matched groups, assuming that the before-and-after differences follow a Gaussian distribution. The sample size was chosen with GraphPad StatMate 2.0 to ensure a minimum of 80% power to detect statistically significant effects at a significance level (alpha) of 0.05, two tailed. However, the actual power of most of the assays was ≥90% and in many cases exceeded 99%. In the case of MIC assays, the experiments were repeated three independent times and the experiment showing the lowest fold change (if applicable) was reported.