Abstract
The accurate analytical measurement of binding affinities of polyclonal antibody in sera to heroin, 6-acetylmorphine (6-AM), and morphine has been a challenging task. A simple nonradioactive method that uses deuterium-labeled drug tracers and equilibrium dialysis (ED) combined with ultra performance liquid chromatography/tandem mass spectrometry (UPLC/MS/MS) to measure the apparent dissociation constant (K d) of antibodies to 6-AM and morphine is described. The method can readily detect antibodies with K d in the low nanomolar range. Since heroin is rapidly degraded in sera, esterase inhibitors were included in the assay, greatly reducing heroin hydrolysis. MS/MS detection directly measured the heroin in the assay after overnight ED, thereby allowing the quantitation of % bound heroin in lieu of K d as an alternative measurement to assess heroin binding to polyclonal antibody sera. This is the first report that utilizes a solution-based assay to quantify heroin-antibody binding without being confounded by the presence of 6-AM and morphine and to measure K d of polyclonal antibody to 6-AM. Hapten surrogates 6-AcMorHap, 6-PrOxyHap, MorHap, DiAmHap, and DiPrOxyHap coupled to tetanus toxoid (TT) were used to generate high affinity antibodies to heroin, 6-AM, and morphine. In comparison to competition ED-UPLC/MS/MS which gave K d values in the nanomolar range, the commonly used competition enzyme-linked immunosorbent assay (ELISA) measured the 50 % inhibition concentration (IC50) values in the micromolar range. Despite the differences in K d and IC50 values, similar trends in affinities of hapten antibodies to heroin, 6-AM, and morphine were observed by both methods. Competition ED-UPLC/MS/MS revealed that among the five TT-hapten bioconjugates, TT-6-AcMorHap and TT-6-PrOxyHap induced antibodies that bound heroin, 6-AM, and morphine. In contrast, TT-MorHap induced antibodies that poorly bound heroin, while TT-DiAmHap and TT-DiPrOxyHap induced antibodies either did not bind or poorly bound to heroin, 6-AM, and morphine. This simple and nonradioactive method can be extended to other platforms, such as oxycodone, cocaine, nicotine, and methamphetamine for the selection of the lead hapten design during substance abuse vaccine development.
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Introduction
Therapeutic vaccines to drugs of abuse obstruct the psychoactive effects of the drugs by inducing antibodies that bind and prevent the drugs from traversing the blood-brain barrier [1, 2]. The development of a heroin vaccine presents a particular challenge because heroin rapidly metabolizes in serum to 6-acetylmorphine (6-AM) and morphine [3]. For effective sequestration of the drugs, hapten bioconjugate vaccines must induce both high titer and high affinity antibodies not only to heroin, but also to 6-AM and morphine [4, 5]. Vaccines to drugs of abuse have been increasingly explored as an alternative treatment for drug addiction. Vaccines have been efficacious in blunting the physiological effects of heroin and other abused drugs in animals. Several studies have demonstrated that the affinity and titer of the induced antibodies [1, 2] and hapten density [6, 7] of the hapten-protein conjugates are critical components of vaccine efficacy. There is a general agreement that enzyme-linked immunosorbent assay (ELISA) can readily and reliably quantify antibody titer [8–11]. In contrast, the measurement of hapten antibody affinity to heroin and its metabolites, as well as other substances of abuse, is generally estimated by competition ELISA [12, 13]. Concerns have been raised that competition ELISA does not accurately measure the antibody affinity [7, 14, 15]. Several of these concerns are as follows: (1) In serum, heroin is rapidly deacetylated to 6-AM and morphine by blood esterases (Fig. 1a) [16–20]. The enzymatic degradation of heroin during the assay changes the concentration of the drugs, and therefore, the calculated affinity constant may not be for heroin per se but for mixture of drugs. (2) The accuracy of ELISA is dependent on the hapten density of the coating agents [21]. (3) There is a localized high concentration of the hapten coated on the well, which allows for both arms of the immunoglobulin G (IgG) to bind to the well resulting in the requirement of high concentrations of competitive inhibitor to prevent antibody binding. (4) Similarly, the affinity of the antibody to the immunizing hapten is most likely higher than its affinity to the competitive inhibitor resulting in the further requirement of high concentrations of the competitive inhibitor. Based on these issues, a new methodology for the accurate measurement of the affinity of antibodies to drugs of abuse needs to be developed.
Equilibrium dialysis (ED) is the standard method for measuring the affinity of proteins to small molecules [22]. However, conventional ED between polyclonal sera and drugs cannot be employed to calculate the apparent dissociation constant (K d) because the antibody concentration is unknown. To circumvent this problem, a competition ED utilizing radioactive tracers as competitive inhibitors is often employed (Müller’s method) [23]. For the antibodies induced by heroin vaccines, the use of radioactive tracers to study heroin-antibody binding presents two main challenges. First, radioactive heroin and 6-AM are not commercially available. Second, the short half-life of heroin and its metabolites in sera is not compatible with the long equilibration time required for ED. We posit that (1) by using an alternative probe and detection system and (2) by identifying assay conditions that prevent the degradation of heroin and its metabolites during ED, binding affinities of heroin, 6-AM, and morphine to polyclonal antibody could be assessed.
Liquid chromatography coupled with mass spectrometry is a valid approach for the detection of drug metabolites in biological fluids and could be used to quantify drugs that are bound to the antibody [24]. We rationalized that nonradioactive deuterium-labeled drug tracers (D3-tracers), such as D3-heroin, D3-6-AM, and D3-morphine, instead of radioactive analogs could be used as tracers in ED. In these D3-tracers, the methyl group of nitrogen is replaced by CD3 (see Electronic supplementary material (ESM) Fig. S1). Since the mass difference between the D3-tracer and corresponding unlabeled drug is significant (Δmass = 3.02 amu), mass spectrometry will be able to discriminate these structurally similar molecules. From an analytical standpoint, the obvious advantage of using D3-tracer/liquid chromatography/mass spectrometry as a probe/detection system over radioactive tracer/scintillation counter and unlabeled drug/enzymatic colorimetric method (ELISA) is that the former can evaluate the integrity of the probe during the assay condition and thereby an unambiguous affinity constant can be determined. We herein report a nonradioactive competition ED coupled with ultra performance liquid chromatography tandem mass spectrometry (UPLC/MS/MS) method that we used to assess the accurate binding affinities of heroin hapten antibodies to 6-AM and morphine. Using this method, (1) we demonstrate that different heroin hapten designs can induce antibodies of varying affinities (Fig. 1b), and (2) we substantiate that the concerns raised about competition ELISA are valid and that the simple methodology of competition ED-UPLC/MS/MS should be used to more accurately measure substance abuse vaccine-induced antibody affinity for the abused substance.
Materials and methods
Tritylmercaptopropionic acid (≥98 %) was acquired from Chem-Impex International (Wood Dale, IL, USA). Chemical reagents and solvents were ACS reagent grade, obtained from Sigma-Aldrich Chem. Co., and were used without further purification. N-hydroxysuccinimide (NHS, 98 %), acetic anhydride (Ac2O, ≥99 %), 4-(dimethylamino)pyridine (DMAP, ≥99 %), formic acid for mass spectrometry, tetraisopropyl pyrophosphoramide (iso-OMPA), and bis(4-nitrophenyl) phosphate (BNPP, 99 %) were purchased from Sigma-Aldrich (Saint Louis, MO, USA). Calibrated solutions (1 mg/mL) of heroin.HCl.H2O, D3-heroin.HCl, 6-AM.HCl, D3-6-AM.HCl, morphine.H2O, and D3-morphine that were used for ED were purchased from Lipomed (Cambridge, MA, USA). Calibrated solutions used were Certified Reference Materials. Optima™ LC/MS grade ammonium formate (NH4HCOO), methanol (MeOH), acetonitrile (ACN), and water (H2O) were purchased from Fischer Scientific (Suwanee, GA, USA). Anti-morphine antibody (ab1060) was purchased from Abcam (Cambridge, MA, USA). Single-use equilibrium dialysis plate with 48 inserts was purchased from Thermo Fisher Scientific (Waltham, MA, USA). An insert (dialysis cassette) contains a sample and a buffer chamber separated by a membrane with 12 K molecular weight cutoff. Screw neck total recovery vial with polytetrafluoroethylene/silicone septa was purchased from Waters (Cambridge, MA, USA). Dulbecco’s phosphate buffered saline (DPBS, 10 mM Na2HPO4, 1.8 mM KH2PO4, 2.7 mM KCl, 137 mM NaCl, pH 7.4) that was used for equilibrium dialysis was purchased from Quality Biological Inc. (Gaithersburg, MD, USA).
Synthesis of 6-AcMorHap
6-AcMorHap was synthesized in eight steps (Fig. 2). Triftylated hydromorphone (2), 3-desoxydihydromorphinone (3), 1-chloro-3-desoxydihydromorphinone (4), and 1-chloro-3-nitro-dihydromorphinone (5) were synthesized sequentially from hydromorphone (1) using the procedure described by Li et al. [25]. The detailed synthesis and analytical characterization of 1-chloro-3-nitro-dihydromorphine (6), 3-amino-dihydromorphine (7), 3-tritylthiopropanamide-dihydromorphine (9), and 6-AcMorHap were described in the ESM. The structure of 6-AcMorHap was confirmed by its 1H and 13C nuclear magnetic resonance (NMR) spectra (see ESM Figs. S2 and S3).
Equilibration of D3-morphine and morphine
In a competition ED, the competitive inhibitor is added on one side of the cassette (buffer chamber) and the tracer to the other side (sample chamber). The two chambers are allowed to reach equilibrium prior to measurements. Equilibration time is the incubation period where ∼50 % of competitive inhibitor and tracer are located in both the buffer and sample chambers. Morphine (300 μL, 1333.3 nM in DPBS) and D3-morphine (100 μL, 5 nM in DPBS) were added into the buffer and sample chambers, respectively. Triplicates were allotted for each time interval: 3, 6, 12, and 24 h. The dialysis plate was covered with sealing tape and incubated at 4 °C/300 rpm on a ThermoMixer® C apparatus (Eppendorf AG, Hamburg, Germany). At a given time point, equal volumes (90 μL) were pipetted from both the sample and buffer chambers. The samples were subsequently placed in separate total recovery vials containing 1 μL of 10 % aqueous formic acid for UPLC/MS/MS analysis. The % drug in the sample and buffer chambers was calculated using the formula:
where [drug]sample chamber and [drug]buffer chamber are the concentrations of the drug in the sample and buffer chambers, respectively.
Stability of heroin and its metabolites
For accurate measurement of K d, the drugs must remain stable during the equilibration time. The stability of heroin and its metabolites was assessed at different dilutions of the mouse sera. An aliquot of the drug (5 nM, 400 μL in DPBS) was treated with different dilutions (1:25, 1:50, 1:100, 1:200, and 1:400) of mouse sera. The reaction mixture was incubated at 4 °C and the amount of drug was monitored at a given time interval using UPLC/MS/MS. The % remaining drug was calculated using the formula:
where [drug] t is the concentration of the drug at time t and [drug]initial is the initial concentration of the drug.
Competition equilibrium dialysis of monoclonal antibody
Anti-morphine antibody (ab1060) is a mouse monoclonal antibody, supplied as a protein G purified antibody (∼2 mg/mL). The approximate molecular weight of the IgG is 155 kDa. Based on this information, the antibody concentration of the stock solution is ∼12.9 μM. ab1060 has a reported K d value of 2 nM, which was determined by proprietary ultraviolet-visible (UV-VIS) absorption spectroscopy method that correlated absorbance with the concentration of the ligand-antibody complex [26]. Samples for equilibrium dialysis were prepared by diluting the stock solution in DPBS to yield 2.4, 4.8, and 9.6 nM. Inhibition studies were conducted in a single-use equilibrium dialysis plate with inserts following manufacturer’s instruction. A 100-μL aliquot of ab1060 (2.4, 4.8, and 9.6 nM) with a fixed amount of D3-morphine (Table 1) was pipetted into the sample chamber, and a 300-μL aliquot of the morphine solution in dialysis buffer was added to the buffer chamber (1:400, vide infra). Morphine, which is the competitive inhibitor, was prepared at different concentrations. The total volume of the solution in the insert is 400 μL. The dialysis plate was covered with sealing tape and incubated at 4 °C/300 rpm on a ThermoMixer® C apparatus. After 24 h, equal volumes (90 μL) were pipetted from both the sample and buffer chambers and placed in separate total recovery vials containing 1 μL of 10 % aqueous formic acid for UPLC/MS/MS analysis.
Competition equilibrium dialysis of anti-hapten sera
The preparation of anti-hapten sera and the strategy for conventional and competition ED were described in the ESM. Week 0 and week 9 sera were considered as negative and anti-hapten sera, respectively. Anti-hapten sera solutions were prepared by diluting the sera in DPBS (1:400, 1:800, or 1:600). Dialysis buffer was prepared by diluting the corresponding negative sera in DPBS (1:400, 1:800, or 1:600). Competitive inhibitors with different initial concentrations were prepared in the dialysis buffer. For the test samples, anti-hapten sera/D3-tracer was run against the negative sera/inhibitors at the same sera dilution. A 100-μL aliquot of anti-hapten sera containing 5 nM D3-tracer was pipetted into the sample chamber, and a 300-μL aliquot of the competitive inhibitor solution was added to the buffer chamber. For negative controls, negative sera/D3-tracer was run against the negative sera at the same sera dilution. A 100-μL aliquot of negative sera containing 5 nM D3-tracer in dialysis buffer was pipetted into the sample chamber, and a 300-μL aliquot of the dialysis buffer was added to the buffer chamber. Equilibrium dialysis and preparation of samples for UPLC/MS/MS was performed as described above. In the absence of hapten antibodies (i.e., negative sera), there is no selective partitioning of the D3-tracer in the sample chamber as all negative controls have 0 % bound D3-tracer. After equilibrium, the total concentration of the D3-tracer ([T t]) for both test samples and negative controls was ∼1.25 nM.
Determination of b values for 6-AM and morphine
Parameter b is the fraction of bound D3-tracer in the absence of competitive inhibitors. Anti-hapten sera/D3-tracer was run against the negative sera at the same sera dilution. Briefly, a 100-μL aliquot of anti-hapten sera containing 5 nM D3-tracer was pipetted into the sample chamber and dialyzed against 300 μL of the appropriate dialysis buffer (1:25, 1:50, 1:100, 1:200, 1:400, 1:800, 1:1600). Equilibrium dialysis and preparation of samples for UPLC/MS/MS was performed as described above. The calculation of b values is discussed (vide infra) as part of the K d calculation (see ESM Tables S1–S3).
Determination of % bound heroin
Since the hydrolysis of heroin in diluted sera was extensive, the assay was performed in the presence of esterase inhibitors. All sera were diluted in DPBS (1:400) and pretreated with esterase inhibitors (iso-OMPA, 100 μM and BNPP, 100 μM) for 1 h at 4 °C. Briefly, a 100-μL aliquot of pretreated dilute sera with 5 nM heroin was pipetted into the sample chamber and dialyzed against 300 μL of the dialysis buffer (1:400). Equilibrium dialysis and preparation of samples for UPLC/MS/MS was performed as described above. The % bound heroin, which is the % heroin bound to the antibody in the presence of esterase inhibitors, was calculated using the equation:
where [heroin]sample chamber and [heroin]buffer chamber are the concentrations of heroin in the sample and buffer chambers, respectively.
UPLC/MS/MS
The UPLC conditions and mass spectrometry parameters were derived from Gottas et al. with some modifications [27]. The amount of drugs in the sample and buffer chambers was quantified using a Waters Acquity UPLC/TQD system equipped with an Acquity HSS T3 column (2.1 × 100 mm, 1.8 μm particle size) maintained at 65 °C. Samples were injected using full loop injection mode (10 μL) and ran against a 10-mM NH4HCOO pH 3.1/MeOH gradient (flow rate = 0.5 mL/min). The gradient profile is shown in ESM Table S4. The total cycle time was 8 min to ensure column equilibration prior to the next sample. In addition, a weak wash (600 μL, 10 % MeOH in H2O) and a strong wash (200 μL, 90 % ACN in H2O) were performed before each sample to prevent carryover.
Positive ionization was performed in multiple reaction monitoring (MRM) mode. The electrospray and source settings were as follows: 0.7 kV (capillary voltage), 120 °C (source temperature), 500 °C (desolvation temperature), 900 L/h (desolvation gas flow, N2), and 60 L/h (cone gas flow, N2). The collision gas (Ar) flow in the collision cell was maintained at 0.4 mL/min. The unlabeled drug and D3-tracer were differentiated based on their mass spectra (see ESM, Figs. S5–S10). Drugs were identified by comparing the retention times of the respective MRM transitions with the corresponding standards. Data were processed in the QuanLynx™ software and the drug concentrations in the sample and buffer chambers were quantified using peak area.
Calculation of apparent dissociation constant (K d)
The K d value can be calculated using Müller’s equation [23, 28]:
[I 50], which is the molar concentration of the competitive inhibitor required for 50 % inhibition, was derived through interpolation on the % inhibition vs [I] curve. [T t] is the total molar concentration of the D3-tracer after equilibrium. The fraction of bound D3-tracer (b) in the absence of competitive inhibitor, I 0, was calculated using the equation:
where \( \left[{\mathrm{D}}_3\hbox{-} \mathrm{tracer}\right]{}_{\mathrm{bound},\ {I}_0} \) is the concentration of the D3-tracer bound to the antibody in the absence of competitive inhibitor, \( \left[{\mathrm{D}}_3\hbox{-} \mathrm{tracer}\right]{}_{\mathrm{total},\kern0.5em {I}_0} \) is the total (bound + free) concentration of the D3-tracer in the absence of competitive inhibitor, [D3-tracer]sample chamber is the concentration of the D3-tracer in the sample chamber, and [D3-tracer]buffer chamber is the concentration of the D3-tracer in the buffer chamber.
For tight-binding antibodies, the b values of the anti-hapten sera were from 0.4 to 0.7 even at high dilutions (1:400, 1:800, and 1:1600). No binding was assigned for anti-hapten sera with b values of ∼0 % at 1:25 dilution. The % inhibition at a given concentration of the competitive inhibitor, [I], was calculated using the equation:
where [D3-tracer]bound, I is the concentration of the D3-tracer bound to the antibody in the presence of competitive inhibitor. The K d was not determined at ≤1:100 dilution due to degradation of heroin, 6-AM, and morphine.
ELISA and competition ELISA
The pooled mice sera were derived from previous animal studies [25, 29, 30]. ELISA was used to measure the serum antibody levels at week 9 against the heroin haptens. Competition ELISA was used to assess the cross-reactivity of the vaccine-induced anti-hapten sera to heroin and its major metabolites: 6-AM and morphine. ELISA and competition ELISA were performed as described previously [7]. The detailed procedures for ELISA and competition ELISA were provided in the ESM.
Data analysis
Statistical analysis was performed using GraphPad Prism Version 6.0c. A t test (paired, two-tailed) was used to compare the concentration of the sample and buffer chambers. A one-way analysis of variance (ANOVA) with Tukey’s correction for multiple comparisons was used to compare the K d values derived from different assay conditions and to compare the % intact heroin after 24 h from different assay conditions. A one-way ANOVA with anti-DiPrOxyHap as the control group and with Dunnett’s correction for multiple comparisons was used to compare the % bound heroin.
Results
Synthesis of heroin hapten 6-AcMorHap
6-AcMorHap was synthesized from hydromorphone 1 using a previously developed procedure for the introduction of the C-3 nitro group (Fig. 2) [25, 31]. Triflation of the C-3 phenol with N-phenyl-trifluoromethansulfonamide followed by palladium-mediated reductive cleavage afforded arene 3 in excellent yield. Direct C-3 nitration was stymied by undesired C-1 regioselectivity of the nitration. Instead, chlorination of the more reactive C-1 position with N-chlorosuccinimide allowed for selective C-3 nitration under mild conditions to give nitro compound 5 in moderate yield [32]. The C-6 ketone was reduced with K-selectride to give alcohol 6. Reduction of the nitro group was affected via palladium-catalyzed hydrogenation under acidic conditions, and it proceeded smoothly with concomitant cleavage of the C-1 chlorine to give amino alcohol 7. The aniline was selectively acylated with 2,5-dioxopyrrolidin-1-yl 3-(tritylthio)propanoate 8 to give amide 9 [33]. Finally, acylation of the hydroxyl moiety (Ac2O, DMAP) afforded heroin hapten 6-AcMorHap in 23 % over eight steps. The syntheses of 6-PrOxyHap, MorHap, DiAmHap, and DiPrOxyHap have been published [25, 30].
Equilibration of D3-morphine and morphine
The dialysis cassette consists of two chambers separated by a semipermeable membrane. The D3-tracer was added to the sample chamber while the competitive inhibitor was added to the buffer chamber. D3-morphine (5 nM, sample chamber) and morphine (1333.3 nM, buffer chamber) were allowed to diffuse in the semipermeable membrane (Fig. 3a, b). At 3 h, 59.68 ± 2.00 and 40.32 ± 2.00 % of D3-morphine partitioned into the sample and buffer chambers, respectively (Fig. 3a), and this difference between the % D3-morphine in the two chambers was significant (**p < 0.01, t test). There was no significant difference in D3-morphine concentrations between the sample and buffer chambers at 6, 12, and 24 h (p = not significant, t test). Also at 3 h, 45.32 ± 0.70 and 54.66 ± 0.70 % of morphine partitioned into the sample and buffer chambers, respectively (Fig. 3b, **p < 0.01, t test). The amount of morphine that partitioned into the sample chamber increased over time thereby decreasing the difference between the two chambers: 46.68 ± 0.17 % (6 h, *p < 0.05), 48.59 ± 0.39 % (12 h, *p < 0.05), and 49.97 ± 2.3 % (24 h, no significant difference compared to the buffer chamber). Based on these data, 24 h was selected as the standard time of incubation.
Stability of the drugs in dilute sera
The degradation of heroin, 6-AM, and morphine was examined at different dilutions of the normal mouse sera for 24 h (Fig. 3c–e). There was an extensive hydrolysis of heroin at all dilutions (Fig. 3c). Thus, the calculation of antibody affinity against heroin was not performed. Hydrolysis of 6-AM was not observed at ≥1:200 dilutions (Fig. 3d). Degradation of morphine was not observed at ≥1:100 dilutions (Fig. 3e). Based on stability data and b values (vide infra), the calculation of antibody affinity against 6-AM and morphine was performed at ≥1:400 dilution.
Apparent dissociation constant of a monoclonal antibody standard
The K d of ab1060 at different concentrations of the antibody and the D3-morphine was determined (Table 1). Additionally, parameter b, defined as the fraction of the D3-tracer bound to the antibody in the absence of competitive inhibitor, was also considered for the assessment of K d values. The K d (1.96 ± 0.17 nM) derived from the assay condition with b = 0.41 was consistent with the reported K d (2 nM) [34]. Although ED and UPLC/MS/MS have been individually considered as standard methods, this result confirms that the combination of competition ED-UPLC/MS/MS can be accurately used for drug-antibody binding quantification. A dramatic reduction in K d was calculated when b values were outside of this range (Table 1). The results were consistent with the studies of Müller that the performance of competition ED must be done at assay conditions with b values of 0.4–0.7 [23].
Opiate affinities of vaccine-induced antibodies by competition ED
For accurate determination of antibody affinity to 6-AM and morphine, the K d was derived from different dilutions of pooled sera, which were obtained by immunization of the indicated hapten conjugated to TT and mixed with liposomal monophosphoryl lipid A as adjuvant (Table 2 and ESM Fig. S4) [25, 29, 30, 35]. In general, there was no statistical difference in K d values when the assay conditions had a b value between 0.4 and 0.7 (ESM Tables S1 and S2). Antibodies to hapten conjugates 6-AcMorHap, 6-PrOxyHap, and MorHap had high affinities (K d < 5 nM) to 6-AM and morphine (Table 2). Anti-6-AcMorHap had significantly higher affinities for both 6-AM and morphine relative to anti-6-PrOxyHap (p < 0.05, one-way ANOVA). Although anti-6-PrOxyHap and anti-MorHap had similar affinities to morphine, the affinity of anti-6-PrOxyHap to 6-AM was significantly higher than anti-MorHap (p < 0.01, one-way ANOVA). Both anti-DiAmHap and anti-DiPrOxyHap had low affinity for 6-AM and no affinity to morphine. In competition ED, low affinity and no binding were both determined in 1:25 sera dilution also to ensure that the lack of drug-antibody binding was not due to low concentration of the antibody, but due to the affinity of antibody for the drugs. Low affinity is defined as when >5 % of the D3-tracer was bound to the anti-hapten sera at a 1:25 sera dilution but was <5 % at 1:400. No binding is defined as when <5 % of the D3-tracer was bound to the anti-hapten sera at 1:25 sera dilution. Antibodies to DiAmHap and DiPrOxyHap bound 61.5 ± 2.3 and 9.1 ± 1.9 % D3-6-AM, respectively, at 1:25 sera dilution. However, the K d cannot be accurately calculated because 6-AM was relatively unstable at 1:25 sera dilution (Fig. 3d). Both anti-DiAmHap and anti-DiPrOxyHap had 0 % binding to D3-morphine at all dilutions (ESM Tables S2 and S3). At 1:400 sera dilution, preimmune sera (week 0) do not bind D3-6-AM and D3-morphine, confirming that plasma proteins were not binding the opiates used in this study.
Binding of heroin to vaccine-induced antibodies
The K d of polyclonal antibodies to heroin cannot be measured by competition ED-UPLC/MS/MS utilizing D3-heroin because of the extensive degradation of heroin in dilute sera. By extrapolation of the heroin stability data during ED with 1:400 sera dilution (Figs. 3c and 4a), heroin, D3-heroin, 6-AM, and D3-6-AM would be present at equilibrium with 6-AM and D3-6-AM as predominant chemical species. Although K d cannot be accurately calculated, the assessment of heroin binding to polyclonal antibody is feasible if sufficient concentration of heroin is present in the assay. After 24 h, 79.9 ± 2.71 % heroin remained intact in DPBS (Fig. 4a). This observation was consistent with a previous report on the spontaneous hydrolysis of heroin at physiological pH [36]. This indicates that assay conditions must be identified such that the degradation of heroin in given serum dilution is comparable to spontaneous hydrolysis of heroin in buffer. The effect of inhibitors (I) on the stability of heroin was determined by measuring % intact heroin after 24 h in DPBS (− Sera), in dilute sera (+ Sera), and in dilute sera in the presence of OMPA/BNPP (+ Sera/I). The inhibitors did not suppress the spontaneous hydrolysis of heroin in buffer (p = not significant, one-way ANOVA) but did inhibit the extensive degradation of heroin in sera (****p < 0.0001, one-way ANOVA). The binding of heroin to anti-hapten sera was measured in the presence of inhibitors because the inhibitors blocked the serum esterase-mediated heroin degradation allowing for appreciable heroin concentrations that can be measured under these assay conditions. ED performed in the presence of these inhibitors showed that anti-6-AcMorHap, anti-6-PrOxyHap, anti-MorHap, and anti-DiAmHap bound significantly higher amount of heroin with 92.89 ± 0.72 % (****p < 0.0001), 76.66 ± 2.17 % (****p < 0.0001), 13.82 ± 4.66 % (**p < 0.01), and 10.75 ± 5.34 (*p < 0.05, one-way ANOVA), respectively, relative to anti-DiPrOxyHap (1.54 ± 2.66 %) (Fig. 4b, multiple comparisons using one-way ANOVA).
Opiate affinities of vaccine-induced antibodies by competition ELISA
The most commonly used method for measuring the affinity of anti-hapten sera to small molecules has been competition ELISA because of its facile nature. In competitive ELISA, binding affinity is reported in terms of 50 % inhibition concentration (IC50). Analysis of the anti-hapten sera by competition ELISA indicated that anti-6-AcMorHap and anti-6-PrOxyHap had the highest relative affinities (IC50 < 10 μM) to heroin, 6-AM, and morphine (Table 3 and ESM Fig. S11). Anti-MorHap showed more modest affinity (IC50 ∼ 21 μM) to 6-AM, higher affinity for morphine (9.2 μM), and no affinity (IC50 > 103 μM) to heroin. Anti-DiAmHap had no affinity for heroin and its metabolites. Anti-DiPrOxyHap displayed modest affinity to heroin, lower affinity to 6-AM (IC50 ∼ 145 μM), and no affinity to morphine. Comparison of these affinities with those obtained by competition ED-UPLC/MS/MS indicated that the affinity (IC50) derived from competition ELISA underestimated the actual K d value by a factor of 103–104. Competition ELISA did not determine if the antibodies bind the drug of interest or if the degradation product was responsible for the binding (i.e., heroin degrading to 6-AM).
Discussion
Drugs of abuse are too small to elicit antibody production and, therefore, require conjugation of structural analogs (haptens) to immunogenic proteins [37, 38]. Hapten bioconjugate vaccines are frequently used to generate functional antibodies against small molecules. The chemical structure of the hapten generally dictates the cross-reactivity of the anti-hapten sera, and thus, the hapten surrogate must be rationally designed [30, 39, 40]. To be efficacious, the hapten antibodies must cross-react with high affinity to the target drug(s).
For heroin vaccines, the hapten design must mimic the key epitopes of heroin and its metabolites [4]. Currently, there has been no established rule that predicts whether a given hapten design would induce anti-hapten sera that target multiple chemical structures. To better understand the relationship between structure and cross-reactivity, the binding affinity of the antibodies induced by immunization with heroin haptens 6-AcMorHap, 6-PrOxyHap, MorHap, DiAmHap, and DiPrOxyHap conjugated to TT (Fig. 2) was assessed using competition ED-UPLC/MS/MS and competition ELISA (Fig. 5). We hypothesized that these hapten designs will induce antibodies with different cross-reactivities that will guide the future optimization of hapten structure. In terms of linker point attachment, the hapten design can be assigned into three groups: C3-linked haptens (6-AcMorHap and 6-PrOxyHap), C6-linked hapten (MorHap), and N-linked haptens (DiAmHap and DiPrOxyHap). The importance of linker point attachment was previously discussed by Matyas’ concept on facial recognition [30]. The conjugation of the haptenic surrogates to TT confines their freedom of motion, and thus, the hapten’s molecular structure bisects into two immunologically defined “faces.” The “front face” is defined as the key epitopes exposed to the immune system, while the “back face” is the sterically blocked moieties that cannot induce antibodies. Using the concept of facial recognition, 6-AcMorHap is particularly interesting because it preserves the C6-ester group that is the common moiety for both heroin and 6-AM [30]. Animals immunized with C3-linked hapten conjugates induced antibodies that bind morphine [41, 42]. In contrast to 6-AcMorHap, the haptens that were used by Spector and Koida contain a C6-alcohol group. We hypothesized that 6-AcMorHap has a “front face” that mimics heroin, 6-AM, and morphine, and thus, TT-6-AcMorHap bioconjugates will induce antibodies that cross-react with these three drugs (Fig. 1a, b) [30]. We also hypothesized that modification of an acetyl group to a propan-2-one group at the C6 position (i.e., 6-PrOxyHap) will reduce the binding affinity, but will not change the pattern of cross-reactivity because haptens 6-AcMorHap and 6-PrOxyHap have similar overall molecular shapes. Previously, we were not able to accurately measure the affinity of the anti-hapten sera due to the inherent limitations of competition ELISA [30]. Now that we can more accurately measure the affinity, we are able to demonstrate that our hypothesis of facial recognition has greater relevance [30].
In this study, competition ED utilizing D3-tracers has been developed to address the inherent constraints of competition ELISA. The main challenge in ED is to maintain the stability of the heroin and its metabolites during the assay. To address this problem, the equilibration time and the degradation of the drugs in dilute sera were investigated. Equilibration between the competitive inhibitor and the D3-tracer were attained at 24 h (Fig. 3a, b). However, this long equilibration time is not compatible with the short half-life of heroin and its metabolites in “neat” sera. We believed that by diluting the mouse sera, the concentration of the enzymes involved in heroin metabolism would be reduced. Consequently, the degradation of heroin and its metabolites would be suppressed. The degradation of the drugs in different dilutions of the sera was monitored for 24 h (Fig. 3c–e). At all dilutions, extensive degradation of heroin was observed. This suggests that the activity of the esterases, which are responsible for C3-ester group cleavage, cannot be suppressed by simple dilution. After 24 h, degradation of 6-AM and morphine was observed at lower dilutions but not at higher dilutions of sera. This indicates that the activity of the enzymes responsible for C6-ester group hydrolysis is concentration dependent. In general, morphine metabolism occurs in the liver. However, extrahepatic metabolism of morphine has been also reported [43]. The degradation profiles of the drugs seem to reach a plateau after 12 h, which might be due to loss of enzymatic activity. Collectively, ≥1:400 sera dilutions can be used to measure antibody affinities to 6-AM and morphine but not to heroin.
Another challenge that must be addressed in ED is the potential impact of plasma protein binding of the drugs. Recently, Zhang et al. reported the plasma protein binding of 222 drugs, of which 50 % showed 90–100 % binding [44]. In “neat” plasma/sera, heroin and morphine have ∼35 % plasma binding [45]. Presumably, 6-AM will also have ∼35 % plasma binding due to structural similarity to both drugs. If the binding of the D3-tracers to plasma protein is significant, the distinction of bonafide antibody-drug interactions from nonspecific protein binding becomes challenging. However, we believed that the effect of plasma binding could be reduced by sera dilution. At ≥1:400 dilution of the week 0 sera (i.e., preimmunized sera), D3-6-AM and D3-morphine showed ∼0 % binding to the plasma proteins. The binding of heroin to plasma proteins cannot be accurately assessed due to esterase-mediated degradation of heroin in dilute sera. However, extrapolation of the % bound heroin for anti-DiPrOxyHap sera conveys that the binding of heroin to plasma proteins is negligible in 1:400 sera dilution (Fig. 4b). Collectively, these data suggest that competition ED-UPLC/MS/MS can be used to measure antibody affinities to 6-AM and morphine in the dilute sera. For other drugs, where plasma protein binding is still significant even in dilute sera, the K d values would difficult to calculate.
We tested the applicability of the competition ED-UPLC/MS/MS method for evaluating small drug-antibody interactions by measuring the dissociation constant of commercially available morphine monoclonal antibody ab1060. According to Müller, competition equilibrium dialysis should be carried out under the following conditions: (1) the b value of the antibody/tracer system should be ∼0.4–0.7, and (2) the specific radioactivity of the tracer should be optimal to prevent large deviations in the antibody affinity [23]. The effects of b values and D3-morphine concentrations on K d were investigated using different assay conditions. Our results were consistent with the findings of Müller. A K d of 1.96 nM, which is in agreement with the reported value of 2 nM [34], is obtained for ab1060 when b is 0.41 (Table 1 and ESM Fig. S4). At 2.4 nM ab1060/2.5 nM D3-morphine, a large deviation in K d was observed. This most likely was because b was >0.7 and 2.5 nM D3-morphine was not an optimal tracer concentration. Considering the accuracy of affinity is dependent on both b values and specific concentration of the tracer, we utilized the b limit range of 0.4–0.7 and 5 nM D3-tracer for determining the K d values of the anti-hapten sera.
Since antibody concentration is not required for the calculation of affinity, the competition ED-UPLC MS/MS could be extended to polyclonal sera [23]. As the polyclonal sera have high antibody titer (Table 3), we hypothesized that the concentration of hapten antibodies in dilute sera is still amenable for binding studies. The b values of anti-hapten sera were determined at both low and high sera dilutions (ESM Tables S1–S3). Anti-6-AcMorHap, anti-6-PrOxyHap, and anti-MorHap had b values of 0.4–0.7 at the range of 1:400–1:1600 dilutions. This suggests that K d for 6-AM and morphine can be only calculated within a specific dilution range. At low sera dilution (≤1:100), 6-AM and morphine were prone to degradation, while at high sera dilution (≥1:1600, b < 0.4), the concentration of antibody was insufficient for reliable quantification. Anti-6-AcMorHap, anti-6-PrOxyHap, and anti-MorHap bound 6-AM and morphine with K d values of <5 nM (Table 2 and ESM Fig. S4). Both anti-DiAmHap and anti-DiPrOxyHap have low affinity for 6-AM and no affinity for morphine. In contrast to the affinity values derived from ab1060, the K d values of anti-hapten sera were not prone to large deviations when b ≥ 0.7. Based on the results, “pure” monoclonal antibody was more sensitive to variation in K d, when the b values were outside of the limit range. As the study of Müller was performed using anti-hapten polyclonal sera, the b limits of 0.4–0.7 might have limitations when applied to monoclonal antibodies. It is also possible that the optimal range of b values and D3-tracer concentrations vary from a given specific monoclonal antibody/drug system to another, and therefore, these values have to be determined empirically. In the case of the polyclonal anti-hapten sera that were used in this study, the b limit range of 0.4–0.7 was congruent with the findings of Müller, and the 5-nM D3-tracer concentration was optimal enough to prevent large deviation in K d values.
To suppress the hydrolysis of heroin at 1:400 sera dilution, the specific esterase inhibitors iso-OMPA and BNPP were added to the reaction mixture [46–48]. The addition of iso-OMPA and BNPP increased the amount of intact heroin to ≥80 %, which was comparable to hydrolysis of heroin in DPBS in the absence of sera (Fig. 4a). This suggests that although K d could not be calculated, the amount of % bound heroin to the antibody in lieu of K d could be used to assess binding. Anti-6-AcMorHap and anti-6-PrOxyHap had 92.89 ± 0.72 and 76.66 ± 2.17 % of the heroin bound, respectively (Fig. 4b), suggesting that hapten designs 6-AcMorHap and 6-PrOxyHap can mimic crucial epitopes of heroin.
While competition ED is a solution-based assay, competition ELISA depends on interactions at the solid-liquid interface (Fig. 5). In contrast to the competition ED-UPLC/MS/MS method, the IC50 values calculated from competition ELISA were in the micromolar range, which suggest low affinity antibodies (Table 3 and ESM Fig. S11). Collectively, the IC50 values derived from competition ELISA were 103–104 higher than the K d from competition ED-UPLC/MS/MS. However, we believe that these IC50 values are not true reflections of drug-antibody interactions. In competition ELISA, hapten-antibody interactions occur at the solid-liquid interface and, thus, are prone to avidity effects. It could be envisioned that the two arms of the IgG antibodies were tightly engaged to the haptens of the coating antigen; thus, higher concentrations of the competing drugs are needed to disrupt the hapten-antibody interactions. Besides underestimation of antibody affinity (i.e., high IC50), another limitation associated with competition ELISA is ambiguity in the interpretation of results. In the case of anti-DiAmHap, there are at least two interpretations for IC50 >103 μM. As we originally proposed for anti-DiAmHap and anti-DiPrOxyHap, either the hapten antibodies simply do not cross-react with the competing drugs, or the affinity of the hapten antibodies to the original hapten design is extremely high [25, 30]. The latter interpretation is consistent with our previous findings [30] and the findings of Pravetoni et al., which demonstrated the higher affinity of hapten antibodies to haptenic surrogate than the target drugs [15]. In addition, the avidity effects associated with competition ELISA further increase the interactions between the haptenic surrogate and the hapten antibodies. This ambiguity can be resolved by considering the b values derived from competition ED-UPLC/MS/MS (ESM Tables S1–S3). Extending those findings, the IC50 values of anti-DiAmHap and anti-DiPrOxyHap to 6-AM and morphine are simply due to weak drug-antibody interactions.
Although there was an underestimation of binding affinities (i.e., high IC50) with competition ELISA [14], it is noteworthy to mention that both methods gave similar trends, i.e., polyclonal antibody with high binding affinities for heroin, 6-AM, and morphine was consistently predicted by both methods. In light of the results, we have observed recurring themes that could serve as guiding principles in the design of a heroin vaccine (Fig. 1b). First, when linker is at the C3 position, the induced antibodies (anti-6-AcMorHap and anti-6-PrOxyHap) cross-reacted with heroin, 6-AM, and morphine. Second, when linker is at the C6 position, the induced antibodies (anti-MorHap) cross-reacted with both 6-AM and morphine, but poorly with heroin. Third, when the linker is at the bridge nitrogen, the induced antibodies (anti-DiAmHap and anti-DiPrOxyHap) had low cross-reactivity to both 6-AM and morphine. Heroin contains two acetyl groups at the C3 and C6 position, while DiAmHap and DiPrOxyHap have acetamide and propan-2-one groups, respectively. The binding affinity data suggest that modifications at this position dramatically affect the cross-reactivity of the induced antibodies to heroin. These results are in agreement with previous reports that hydrolytically stable N-linked haptens tended to generate antibodies that were highly specific to the parent hapten and had no cross-reactivity to other drugs [49–52]. It has been postulated that antibody titer and antibody affinity are crucial for the efficacy of drug of abuse vaccines [1, 2]. Previously, we demonstrated that mice immunized with TT-DiAmHap and TT-DiPrOxyHap showed partial protection and no protection against heroin challenge, respectively [25, 30]. In terms of binding affinity, anti-DiAmHap is superior to anti-DiPrOxyHap (Fig. 4b and ESM Table S3). The protection against heroin challenge could be attributed to the presence of high titer, but low affinity antibodies to heroin and 6-AM. Based on IC50 and antibody titer from ELISA and K d and % heroin bound from competition ED-UPLC/MS/MS, it is clear that 6-AcMorHap and 6-PrOxyHap are the lead hapten designs.
Despite the ability of competition ED-UPLC/MS/MS to measure K d, the assay system does have some limitations. Due to the use of dilute sera, the method cannot measure the affinity of polyclonal antibodies that poorly bind 6-AM and morphine. Within the context of a heroin vaccine, it can be argued that the determination of antibodies with high K d values (>1 μM, low affinity antibodies) is unimportant, since these antibodies are expected to bind low amounts of heroin and its metabolites and, consequently, have little role in efficacy. The competition ED-UPLC/MS/MS also cannot be used for drugs that have a significant binding to plasma proteins even at high sera dilutions. Overall, competition ED-UPLC/MS/MS is a simple method for determining the binding affinities of antibodies. It is a convenient method because it does not involve the use of radioactive tracers, and all the reagents for the assay are commercially available. This nonradioactive method only requires 5–10 μL of anti-hapten sera to generate a binding curve and has the potential applications for studying the binding affinities of antibodies induced by small molecule hapten-based immunogens. In addition, competition ED-UPLC/MS/MS resolved the ambiguity of the IC50 values derived from competition ELISA.
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Acknowledgments
The work of JFGA, FL, AEJ, and KCR was supported by the NIH Intramural Research Programs of the National Institute on Drug Abuse and the National Institute of Alcohol Abuse and Alcoholism. The work of OBT, RJ, CRA, and GRM was supported through a Cooperative Agreement Award (no. W81XWH-07-2-067) between the Henry M. Jackson Foundation for the Advancement of Military Medicine and the U.S. Army Medical Research and Materiel Command (MRMC). The work was partially supported by an Avant Garde award to GRM from the National Institute on Drug Abuse (NIH grant no. 1DP1DA034787-01). We thank Noel Whittaker and Dr. John Lloyd (Mass Spectrometry Facility, NIDDK) for the mass spectral data and Drs. Klaus Gawrisch and Walter Teague (Laboratory of Membrane Biochemistry and Biophysics, NIAAA) for NMR spectroscopic data. We also thank Dr. Kejun Cheng (FDA) for providing some of the initial compounds and Mr. Marcus Gallon, Ms. Caroline Kittinger, Ms. Courtney Tucker, and Mr. Alexander Duval for providing outstanding technical assistance. Research was conducted in compliance with the Animal Welfare Act and other federal statutes and regulations relating to animals and experiments involving animals and adhered to the principles stated in the Guide for the Care and Use of Laboratory Animals, NRC Publication, 1996 edition.
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The authors declare that they have no competing interests. However, Gary R. Matyas, Kenner C. Rice, Arthur E. Jacobson, and Carl R. Alving are coinventors in a related patent application that is owned by Walter Reed Army Institute of Research, National Institute on Drug Abuse, and Henry M. Jackson Foundation.
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Torres, O.B., Antoline, J.F.G., Li, F. et al. A simple nonradioactive method for the determination of the binding affinities of antibodies induced by hapten bioconjugates for drugs of abuse. Anal Bioanal Chem 408, 1191–1204 (2016). https://doi.org/10.1007/s00216-015-9223-z
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DOI: https://doi.org/10.1007/s00216-015-9223-z