Serum samples

Serum samples were obtained from 12 subjects (aged 3–17 years) with confirmed clinical history of allergic responses to shrimp and positive skin prick test (Table S1). Specific IgE reactivities to purified recombinant shrimp tropomyosin Pen a 1 and Met e 1 were characterized by ImmunoCAP and ELISA, respectively. None of the recruited subjects have other allergies. Serum samples (n = 8) obtained from healthy, non-atopic volunteers without Met e 1-specific IgE were used as a negative control.

Ethics statement

A written consent was obtained from the parents of the children enrolled in the study (Institutional Review Board of the University of Hong Kong/Hospital Authority Hong Kong West Cluster, Ref. No. UW10-115). The use and storage of human sera were approved by the Joint Chinese University of Hong Kong - New Territories East Cluster Clinical Research Ethics Committee with a written informed consent (CREC Ref. No. CRE-2010-514). All animal protocols were approved by the Animal Experimentation Ethics Committee, The Chinese University of Hong Kong (ref No. 11/006/GRF and 463911), in accordance with the Department of Health (Hong Kong) guidelines in Care and Use of Animals. All experiments were performed under licenses granted from the Government of Hong Kong Special Administrative Region.

Identification of allergenic epitopes

There were three independent methods used to predict the immunodominant allergenic epitopes including 1) computational prediction of IgE binding epitopes, 2) ELISA against overlapping peptides that span the entire Met e 1 sequence, and 3) dot-immunoblotting of overlapping peptides against the entire Met e 1 sequence. 18 overlapping peptides spanning the full-length (274 amino-acids) Met e 1 were commercially synthesized (GenScript). Each peptide had 20 amino acids (except for peptide 18 that contains 19 amino acids) with five amino acids overlapping with the adjacent peptides at the N-terminus. Individual peptides were dissolved in distilled water, aliquoted and stored at −20°C until required.

1. Three computational models from the Immune Epitope Database (IEDB) Analysis Resource were employed to predict the major linear IgE-binding epitopes of Met e 1, including Bepipred Antibody Epitope Prediction, Kolaskar & Tongaonkar Antigenicity model and Emini Surface Accessibility Prediction. Bepipred Antibody Epitope Prediction predicts the location of IgE-binding epitopes based on the hidden Markov model and propensity scale method [33]. The Kolaskar & Tongaonkar Antigenicity model is based on the physiochemical properties of amino acid residues [34]. Emini Surface Accessibility Prediction is based on the calculation of the surface accessibility scale [35].
2. For peptide ELISA, 3 µg of each peptide were coated on 96-well plates (Nunc, maxisorp) in 0.05 M carbonate buffer overnight. After blocking with 1% BSA/PBS for 1.5 h, the plates were incubated with individual serum samples (150 dilution) at room temperature for 2 h. Thereafter, the plates were incubated with biotinylated goat anti-human IgE (Vector) in 11000 dilution for 45 min followed by incubation with Avidin D, Peroxidase labeled antibody (Vector) in 11000 dilution for 30 min. The plates were then developed with TMB substrate reagent set (BD Biosciences) for 15 min and the reaction was terminated by 2 N H₂SO₄. Absorbance was measured at 450 nm using an ELISA plate reader (Bio-Rad). All absorbance values were background-corrected, in which the background absorbance was the OD value of Met e 1-coated wells incubated with secondary and tertiary antibodies only. All the above procedures were performed at room temperature. The plates were washed with PBS/0.5% Tween-20 (PBST) three times and PBS once between each step and all dilutions were made in 1% BSA/PBS.
3. For dot-immunoblotting, 3 µg of each peptide (3 µL) were spotted onto a 0.2 µm nitrocellulose membrane (Bio-Rad). The membrane was allowed to air-dry and thereafter fixed with 2.5% glutaraldehyde/PBS for 10 min [36]. The membrane was incubated with diluted serum (150 dilution) overnight at 4°C after a 2-h blocking in 3% skim milk/TBS. The membrane was incubated with mouse monoclonal anti-human IgE-alkaline phosphatase antibody (Sigma Aldrich) at 12000 dilution for 1 h at room temperature followed by signal development with NBT/BCIP (Roche). All dilutions were made with 3% skim milk/TBS and all washing steps were performed with TBST) once and TBS three times with shaking.

Design of hypoallergenic shrimp tropomyosins

With the high structural flexibility and spontaneous unfolding property of tropomyosin [37], we believe that the possibility of having only one single amino acid per epitope that is crucial for IgE binding is unlikely. Restricted homologous substitution may not be sufficient to result in tropomyosin variants with greatly reduced IgE reactivity. Therefore, the amino acid sequence of Met e 1 was compared to the non-allergenic fish tropomyosins of four species Salmo salar (Atlantic salmon; GenBank accession number NP_001117128.1), Epinephelus coioides (orange-spotted grouper; ADG29138.1), Siniperca chuatsi (Mandarin fish; AEK21799.1) and Thunnus thynnus (Atlantic bluefin tuna; BAD01050.1) (Fig. S1). All nine identified IgE-binding regions in Met e 1 were converted into the homologous sequence of fish tropomyosins and 49 point mutations in total were introduced to construct the mutation mutant MEM49 (Fig. 1A & B). To construct the deletion mutant, all nine IgE-binding epitopes were deleted (Fig. 1B). This mutant, named MED171, contained only 171 amino acid residues. The amino acid sequences of MEM49 and MED171 were reverse translated using MEGA 5.0 and the encoding sequences of the two mutants were synthesized commercially by GenScript. Synthetic genes of each of the mutants were cloned into pET30(a)+ (Novagen) expression vector via EcoRV and HindIII restriction sites. The sequences and reading frame of MEM49 and MED171 in the plasmid were confirmed by dideoxynucleotide sequencing.

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Figure 1. Design of two hypoallergenic mutants.

MEM49 was constructed by substitution of 49 different amino acid residues within the nine Met e 1 epitopes to the homologous fish tropomyosin sequence. MED171 was constructed by deletion of epitopes E1 to E9 of Met e1. (A) Location of the IgE-binding epitopes in tropomyosin. The IgE epitopes designated as E1–E9 are shown in boxes and the location of the 49 amino acid residues in Met e 1 that are converted in MEM49 are also shown as one letter amino acid code. (B) Schematic representation of Met e 1, MEM49 and MED171. Epitopes E1 to E9 in Met e 1 are represented as black boxes and the number of amino acids in each epitope is indicated. Amino acid residue changes in MEM49 are shown as *. MED171 is a truncated peptide with the epitopes E1–E9 deleted. (C) SDS-PAGE of Met e 1, MEM49 and MED171 after Coomassie Blue staining. Note the 35 kDa molecular weight of Met e 1 and MEM49 and the expected smaller size of MED171 compared to Met e 1.

https://doi.org/10.1371/journal.pone.0111649.g001

Preparation of recombinant wild type and mutant shrimp tropomyosin

cDNA coding for the full length shrimp tropomyosin Met e 1 and the encoding sequences of MEM49 and MED171 were cloned into His-tag expression vector pET30(a)+ (Novagen) and expressed in Escherichia coli BL21 (DE3) (Invitrogen) by culturing in MagicMedia (Invitrogen) at 37°C overnight. His-tagged recombinant Met e 1 (rMet e 1), MEM49 and MED171 were purified using the HisPur Cobalt Spin Column (Thermo Scientific) according to the manufacturer’s instructions. Protein concentration was determined by BCA assay (Sigma Aldrich) while the purity was determined by Sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and Coomassie blue staining.

Mice sensitization and immunization

3–4 weeks old female Balb/c mice were acquired from the Laboratory Animal Services Centre, The Chinese University of Hong Kong. All animals were maintained on a shrimp-free diet and housed in pathogen-free conditions. To induce Met e 1 hypersensitivity in mice, sensitization was performed as described previously by intragastric administration of 0.1 mg of recombinant tropomyosin plus cholera toxin on days 0, 12, 19 and 26 and challenged on day 33 [29]. Mice fed with phosphate-buffered saline plus cholera toxin were included as controls. Blood samples were collected 4 h after the challenge for antibody analysis.

For immunization experiments, 5–6 weeks old female Balb/c mice were intraperitoneally immunized three times on days 0, 7 and 14 with 0.1 mg purified rMet e 1, MEM49 or MED171 adsorbed to 1 mg Al(OH)₃. Blood was collected 4 h after the last injection for the determination of antibody levels.

Direct ELISA

To examine the IgE reactivity to rMet e 1, MEM49 or MED171, 96-well ELISA plates were coated with 5 µg/mL of either rMet e 1, MEM49 or MED171 in 0.05 M carbonate buffer overnight at 4°C, blocked with 1% BSA/PBS for 2 h and incubated with serum samples from shrimp allergy subjects or Met e 1-sensitized mice (110 dilution) overnight at 4°C. After washing, plates were incubated with biotinylated anti-human (Vector) or anti-mouse IgE antibodies (BD Pharmigen) and Avidin D, Peroxidase labeled antibody (Vector), each at 11000 dilution at room temperature for 1 h and 30 min, respectively. The plates were then developed with TMB substrate reagent set (BD Biosciences) for 15 min and the reaction was terminated by 2 N H₂SO₄.

To determine the reactivity of IgG and IgG_2a antibodies raised in rMet e 1, MEM49 and MED171 immunized mice, sera in serial dilutions (1400 to 125600) were incubated in the rMet e 1, MEM49 or MED171 coated plates (5 µg/mL) for 2 h at room temperature. The plates were then incubated with goat anti-mouse IgG or anti-mouse IgG_2a (Southern Biotech) in 12000 dilution for 45 min followed by incubation with Avidin D, Peroxidase labeled antibody (Vector) in 11000 dilution for 30 min. The plates were then developed with TMB substrate reagent set (BD Biosciences) for 5 min and the reaction was terminated by 2 N H₂SO₄.

Passive cutaneous anaphylaxis

Passive cutaneous anaphylaxis was performed to determine the in vivo allergenicity of MEM49 and MED171. Backs of naïve Balb/c mice were shaved, followed by intradermal injection of Met e 1-specific IgE-containing sera (undiluted sera in a total volume of 100 µL) under isoflurane narcosis. Two hours later, mice were injected intravenously with a mixture of 100 µL of 0.5% Evan’s blue dye (Sigma Aldrich) and 0.1 mg rMet e 1, MEM49 or MED171. Thirty minutes after dye-rMet e 1 administration, mice were sacrificed by cervical dislocation and skins of their backs were immediately inverted for the measurement of blue region diameters.

Competitive inhibition ELISA

Competitive inhibition ELISA was performed to evaluate the blocking capacity of hypoallergen-induced blocking antibodies. Briefly, rMet e 1 was used to coat 96-well plates (5 µg/mL) overnight at 4°C and blocked with 1% BSA/PBS for 2 h. Plates were then washed and blocked with 100 µL of 110 diluted sera from mice immunized MEM49, or MED171 overnight at 4°C. Thereafter, 100 µL of sera from shrimp allergy patients or Met e 1-sensitized mice at a predetermined dilution (110–120 dilution) were added and incubated at room temperature for 2 h. The wells were then washed and followed by the addition of biotinylated anti-human or anti-mouse IgE antibodies, HRP-Avidin D and developed as described above. The blocking ability of the induced IgG antibodies was determined using the equation [(OD_{no inhibitor}–OD_inhibitor)/OD_{no inhibitor}]×100% and expressed as percentage inhibition.

Statistical analysis

Data were presented as mean ± SEM. The statistical comparison was determined by one-way analysis of variance (ANOVA) followed by the Student-Newman-Keuls test using SigmaStat 3.1. The difference was considered statistically significant at p<0.05.

IgE-binding epitopes of Met e 1 and hypoallergen design

By ELISA, sera from patients with shrimp allergy (n = 12) had significantly higher IgE reactivity against five peptides (P3, P5, P10, P13 and P16) when compared with other peptides (p<0.05) (Fig. 2A). None of the sera from control subjects (n = 8) showed IgE-binding activity towards these or other peptides (data not shown).

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Figure 2. Determination of Met e 1 IgE-binding epitopes.

Epitopes were determined by ELISA, dot-immunoblotting and three prediction models Emini Surface Accessibility Prediction Kolaskar & Tongaonkar Antigenicity model and Bepipred Antibody Epitope Prediction. (A) Histogram of the IgE binding reactivity against the Met e 1 peptides as determined by ELISA. (B) Histogram of IgE binding reactivity against the Met e1 peptides as determined by dot-immunoblotting. (C) Alignment of Met e 1 IgE-binding epitope sequences as determined by ELISA, dot-immunoblotting and each of the three prediction models.

https://doi.org/10.1371/journal.pone.0111649.g002

Allergenic regions on Met e 1 were also defined based on the intensity of peptide spots and the frequency of recognition in dot-immunoblotting (Fig. 2B). A peptide with >50% recognition (6 out of 12 patients) or an epitope score (calculated by the summation of the IgE reactivity score (strong reactivity: 3; median: 2; low: 1)) higher than the mean intensity score (8.83, calculated by adding all epitope scores and dividing by 18 peptides) was defined as a major IgE-binding epitope. Based on these criteria, eight peptides (P1, P3, P10, P11, P15, P16, P17 and P18) were identified as the major Met e 1-specific IgE-binding sequences. The discrepancy in epitopes determined by ELISA and dot-immunoblotting (Fig. 2C) was apparently due to assay sensitivity and peptide presentation on different materials in the two assays.

Three online immunoinformatics models were applied to define the IgE epitopes. (Fig. 2C & Fig. S2). Seven epitopes, with six to 16 amino acid residues in length, were identified using Emini Surface Accessibility Prediction based on the surface probability score (Fig. S2A). Ten allergenic regions, between six to 19 amino acid residues in length, were defined under the Kolaskar & Tongaonkar Antigenicity model based on the antigenic propensity score (Fig. S2B). Using Bepipred Antibody Epitope Prediction, 15 regions from one to 28 amino acid residues in length were recognized as IgE-binding epitopes (Fig. S2C). In comparing the predictions by these three models, Emini Surface Accessibility Prediction and Bepipred Antibody Epitope Prediction yielded very similar epitope results (>85% similarity, calculated as the degree of overlapping amino acid residues), while the prediction by Kolaskar & Tongaonkar Antigenicity deviated from those of the other two models. Only six regions resulted in consensus between Emini Surface Accessibility Prediction and Kolaskar & Tongaonkar Antigenicity, but with a low degree of overlap ranging between 14% and 37%.

Data obtained by ELISA and dot-immunoblotting, as well as from the three predictions models, were combined and equally weighted for defining the major IgE-binding epitopes (Fig. 2C). Logically, sequences that are determined as IgE reactive both experimentally and by modeling studies are more likely to represent IgE-binding epitopes in the native protein. Therefore, only regions that were suggested as IgE reactive by at least one of the experimental assays, and at least two other of the above assays or models, were considered as major epitopes [38]. Altogether, nine major IgE-binding epitopes of Met e 1 ranging from five to twenty-one amino acid residues in length were identified, namely E1–E9, with positions at Met e 1^25–30, Met e 1^43–60, Met e 1^87–103, Met e 1^146–154 Met e 1^161–165, Met e 1^191–211, Met e 1^236–241, Met e 1^247–255 and Met e 1^269–281, respectively (Fig. 1A). Based on these epitopes, we constructed two tropomyosin mutants, by site-directed mutagenesis (MEM49) and epitope deletion (MED171). The locations of the IgE epitopes and their corresponding amino acid changes in mutants MEM49 and MED171 are shown in Fig. 1A and B. Approximately 4 mg of purified soluble recombinant proteins of MEM49 and MED171 could be obtained from 1 liter of E.coli culture. SDS-PAGE analysis of purified recombinant proteins of the mutation mutant MEM49 and the deletion mutant MED171 showed a 35-kDa MEM49 band and a 27-kDa MED171 band, compared to a 35 kDa rMet e 1 band (Fig. 1C).

Immunoreactivity of tropomyosin mutants

Sera from 8/8 shrimp allergy patients and Met e 1-sensitized mice showed a marked decrease in IgE reactivity to MEM49 and MED171 (Fig. 3). Reactivity of MEM49 and MED171 towards patient IgE decreased by an average of 71.4% and 77.4% relative to Met e 1, respectively (Fig. 3A & B), while that to mouse IgE decreased by an average of 90.5% and 97.6%, respectively (Fig. 3C & D). Notably, the IgE-binding reactivity of MED171 was significantly lower than that of MEM49 (p<0.05) when tested with mouse sera. In addition to in vitro reduction in IgE reactivity, both MEM49 and MED171 did not trigger mast cell degranulation in passive cutaneous anaphylaxis assays. In contrast to a >2.5 cm blue region induced by intradermal injection of Met e 1-specific IgE and intravenous injection of Met e 1 with Evan’s blue dye, no Evan’s blue dye extravasation could be induced by intravenous injection of either hypoallergens (Fig. 3E). More importantly, none of the MEM49- or MED171-immunized mice produced Met e 1-recognizing IgE antibodies (OD 0.071±0.001 and 0.092±0.003, respectively) and hypoallergen-specific IgE antibodies, comparing to an IgE level of OD 0.405±0.056 upon Met e 1 immunization (Table 1). These clearly demonstrated that both MEM49 and MED171 had marked reduction in their in vivo allergenicity.

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Figure 3. In vitro and in vivo IgE reactivity and allergenicity of the hypoallergens.

Reactivity of (A) MEM49 and (B) MED171 to IgE from shrimp allergy patients (n = 8) and reactivity of (C) MEM49 and (D) MED171 to IgE of Met e 1-sensitized mice (n = 8) in ELISA. (E) In vivo IgE reactivity and allergenicity of Met e 1, MEM49 and MED171 as determined by PCA assay. Note that the in vitro and in vivo IgE reactivity and allergenicity of MEM49 and MED171 are significantly lower than those of Met e 1, as shown by the significantly lower absorbance value at 450 nm and absence of Evan’s blue dye extravasation.

https://doi.org/10.1371/journal.pone.0111649.g003

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Table 1. Immunoreactivity of mutants as hypoallergen vaccines in mouse.

https://doi.org/10.1371/journal.pone.0111649.t001

Hypoallergen-immunized mice produced Met e 1-specific IgG antibodies and inhibited IgE binding to Met e 1

Mice immunized with either rMet e 1, MEM49 or MED171 produced robust IgG antibodies that recognized rMet e 1 with OD 1.778±0.037, 0.571±0.082 and 1.089±0.085, respectively (Table 1). Moreover, IgG antibodies induced by MED171 exhibited better rMet e 1 recognition when compared to those induced by MEM49 at all tested dilutions (Fig. 4A). It is noteworthy that only the hypoallergens MEM49 and MED171, but not Met e 1, could induce the production of Met e 1-specific IgG_2a antibodies (Fig. 4B). We further examined if the sera IgG antibodies from hypoallergen-immunized mice were able to block Met e 1-specific IgE from binding to rMet e 1 by competitive inhibition ELISA. Serological IgG from MEM49 and MED171 were able to inhibit 46.2±3.41% and 45.9±3.54% of IgE from shrimp allergy patients from binding to Met e 1, respectively (Fig. 4C). MEM49- and MED171-IgG could better inhibit mouse IgE binding to Met e 1 with average of 82.5±3.24% and 87.6±2.84%, respectively (Fig. 4D).

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Figure 4. Immuno-reactivity of hypoallergens and inhibitory potential of the induced IgG antibodies.

Reactivity of the rMet e 1-, MEM49- and MED171-induced (A) IgG and (B) IgG_2a antibodies towards the wild type allergen rMet e 1. Note that specific IgG_2a could only be induced by the hypoallergens. Inhibitory potential of the induced IgG towards Met e 1-specific IgE from (C) shrimp allergy subjects (n = 8) and (D) Met e 1-sensitized mice (n = 8) determined by competitive inhibition ELISA. Percentage inhibition was calculated by [(OD_{no inhibitor}–OD_inhibitor)/OD_{no inhibitor}]×100%. Note that the MEM49- and MED171-induced IgG antibodies could significantly inhibit IgE of shrimp allergy patients and Met e 1-sensitized mice from binding to Met e 1.

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