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ORIGINAL RESEARCH

Studies on HBcAg-rBlo t 5-21 Fusion Protein Vaccine That Alleviates Blomia tropicalis Airway Inflammation

Yechun Pei1 School of Life Sciences, Hainan University, Haikou, People’s Republic of China;2 Laboratory of Biopharmaceuticals and Molecular Pharmacology, School of Pharmaceutical Sciences, Hainan University, Haikou, People’s Republic of China;3 One Health Institute, Hainan University, Haikou, People’s Republic of ChinaCorrespondence[email protected]
ORCID Iconhttps://orcid.org/0000-0002-2039-732XView further author information
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Zhengpan Xiao1 School of Life Sciences, Hainan University, Haikou, People’s Republic of China;2 Laboratory of Biopharmaceuticals and Molecular Pharmacology, School of Pharmaceutical Sciences, Hainan University, Haikou, People’s Republic of ChinaView further author information
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Shuangshuang Wei1 School of Life Sciences, Hainan University, Haikou, People’s Republic of China;2 Laboratory of Biopharmaceuticals and Molecular Pharmacology, School of Pharmaceutical Sciences, Hainan University, Haikou, People’s Republic of ChinaView further author information
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Meiqi Peng1 School of Life Sciences, Hainan University, Haikou, People’s Republic of China;2 Laboratory of Biopharmaceuticals and Molecular Pharmacology, School of Pharmaceutical Sciences, Hainan University, Haikou, People’s Republic of ChinaView further author information
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Chenghui Luo1 School of Life Sciences, Hainan University, Haikou, People’s Republic of China;2 Laboratory of Biopharmaceuticals and Molecular Pharmacology, School of Pharmaceutical Sciences, Hainan University, Haikou, People’s Republic of ChinaView further author information
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Dayong Wang2 Laboratory of Biopharmaceuticals and Molecular Pharmacology, School of Pharmaceutical Sciences, Hainan University, Haikou, People’s Republic of China;3 One Health Institute, Hainan University, Haikou, People’s Republic of ChinaCorrespondence[email protected]
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Pages 6343-6355 | Received 16 Jul 2022, Accepted 06 Nov 2022, Published online: 18 Nov 2022

Abstract

Background

In tropical and subtropical areas, allergens from the dust mite species Blomia tropicalis are common causes of allergic rhinitis and asthma. Blomia tropicalis has two main allergens: Blo t 5 and Blo t 21.

Aim

To generate a chimeric virus-like particle containing HBcAg, Blo t 5 and Blo t 21 that can treat allergies caused by Blomia tropicalis.

Methods

To produce allergic asthma in mice, prokaryotic expression and purification of Blomia tropicalis allergens rBlo t 5, rBlo t 21, and recombinant fusion allergen rBlo t 5–21 were utilized in the study. We created a hepatitis B core antigen (HBcAg) and rBlo t 5–21 fusion prokaryotic expression plasmid. HBcAg-rBlo t 5–21 was purified after expression and tested by transmission electron microscopy (TEM). Furthermore, the protein HBcAg-rBlo t 5–21 was employed as a protein vaccination.

Results

In allergy-induced mouse model experiments, the fusion allergen rBlo t 5–21 was more effective than the individual allergens rBlo t 5 and rBlo t 21 at inducing allergy. We found that vaccinating allergic mice with the recombinant fusion protein vaccine HBcAg-rBlo t 5–21 alleviated allergy symptoms elicited by the rBlo t 5–21 allergen. Vaccination with HBcAg-rBlo t 5–21 resulted in a decrease in total serum IgE levels, suppression of anaphylaxis, and reduction of inflammatory cell infiltration into lung tissue as compared to the PBS group.

Conclusion

HBcAg-rBlo t 5–21, a protein vaccine containing both the hepatitis B core antigen and the Blomia tropicalis fusion allergen rBlo t 5–21, could be a suitable vaccination for preventing allergy disorders caused by Blomia tropicalis.

Introduction

The prevalence of allergic diseases and asthma is increasing worldwide, particularly in low- and middle-income countries.Citation1 House dust mite (HDM) is a predominant source of indoor aeroallergen, which induced allergic diseases including allergic rhinoconjunctivitis, allergic asthma, atopic eczema and other allergic skin diseases.Citation2,Citation3 And it is now clear that dust mite allergy is a key contributor to asthma in many parts of the world.Citation4 Blomia tropicalis is a mite that is considered a house dust mite of tropical and sub-tropical areas, sensitization to this mite is very common in South America and Southeast Asia.Citation4 Specific IgE level induced by Blomia tropicalis sensitization was significantly higher in patients with persistent asthma compared to intermittent asthma.Citation5

So far, allergen-specific immunotherapy (AIT) is the only potential disease modification therapy for HDM allergic subjects.Citation5 With the efforts of doctors and researchers in the field of allergy, the efficacy, safety, standardization and strategy of AIT are constantly developing.Citation6–10 At present, the possibility of using recombinant protein as a substitute for crude allergen extract can significantly affect the current AIT regimen.Citation11,Citation12 As a result, various recombinant allergens have been produced for AIT from different allergens (such as pollen, animal dander, mites and various foods).Citation13–17 Blo t 5 and Blo t 21 are known major allergens in Blomia tropicalis, and studies demonstrate that they include key epitopes that can be recognized by IgE antibodies in people allergic to Blomia tropicalis antigens.Citation18 Despite these allergens have very similar three-dimensional (3D) structures, they do not cross-react, although co-sensitization is a common feature.Citation18–21 The major linear IgE epitopes of Der p 5 and Blo t 5 are involved in species-specific recognition.Citation22 Traditionally, OVA, an egg allergen, has been used in animal asthma models (5pc6), but has been almost replaced by respiratory allergens, such as Dermatophagoides pteronyssinusCitation23–25 and Blomia tropicalis.Citation26–28 And a new mouse model of severe asthma caused by Blo t 5 has been developed, which results in extensive lung inflammation, a strong adoptive and host Th2 response, airway remodeling, and the formation of IL4/IL-13-dependent iBALT.Citation29

AIT is only disadvantageous to individuals sensitized by mild allergens because successful treatment is dose-dependent; therefore, successful treatment may be related to allergen concentration.Citation30 Therefore, it is necessary for individuals sensitized by mild allergens to improve the immunogenicity of low-dose allergens. Hepatitis B core antigen (HBcAg) is an efficient, safe and widely used virus-like particles (VLP) vector due to its self-assembly into virus-like particles and strong immunogenicity.Citation31 They cause T-cell-dependent and T-cell-dependent immune responses and can be easily manipulated.Citation21 The fusion of HBcAg immunodominant internal sites reduced the immunogenicity and antigenicity of HBcAg and most significantly enhanced the immunogenicity of inserted foreign epitopes.Citation32 The present study aimed to generate HBcAg-rBlo t 5–21 chimeric virus-like particles, which can potentially treat the allergic reaction caused by Blomia tropicalis.

Materials and Methods

Animals

Adult female BALB/c mice (6–8 weeks old) were purchased from Guangdong Medical Laboratory Animal Center (Guangzhou, China) and housed in a pathogen-free environment with free access to food and water ad lib.

Design of Expression Vectors of Recombinant Allergens of Blomia Tropicalis

The CDS sequences of Blo t 5 and Blo t 21 were obtained from GenBank (GenBank: U59102 and GenBank: DQ788677.1, respectively). After codon optimization, the sequences of rBlo t 5, rBlo t 21, and rBlo t 5–21 were synthesized and inserted into the pQE80L vector between BamHI and SalI restriction sites. A truncated version of HBcAg gene (coding for HBcAg lacking the arginine-rich C-terminal domain, amino acids 1 through 149) was obtained from GenBank (GenBank: GU827636.1). In the truncated HBcAg gene, the corresponding sequences of 79th amino acid residue P and 80th amino acid residue A were replaced by the rBlo t 5–21 gene sequence. Glycine-rich flexible amino acid sequences (G4S)2G4 (Sequence: GGCGGCGGCGGCTCTGGTGGTGGTGGTTCTGGCGGTGGCGGT) are located on either side of rBlo t 5–21. Then, the chimeric HBcAg-rBlo t 5–21 sequence was inserted into the vector pQE80L. The resultant expression vector was named as pQE80L-HBcAg-rBlo t 5–21.

Expression of Recombinant Protein

Expressions of all of the recombinant proteins were induced at 37℃ with 0.1 mM of IPTG. After 4–5 h, cells were harvested, resuspended in native lysis buffer, and disrupted by sonication. The fusion proteins were purified by Ni-NTA agarose (cat. No. 30210; Qiagen, Hilden, Germany). Imidazole was then removed by ultrafiltration. According to the manufacturer’s instruction, bacterial endotoxins were removed using the ToxinEraser™ Endotoxin Removal Kit (Cat. No. L00338, GenScirpt, USA). The endotoxin level was determined using the ToxinSensor™ Chromogenic LAL Endotoxin Assay Kit. Endotoxin-free protein contains less than 0.15 EU/mL of endotoxin. The Endotoxin-free protein was concentrated to 1 mg/mL in PBS.

Transmission Electron Microscopy

The purified rBlo t 5–21 and HBcAg-rBlo t 5–21 protein (2 mg/mL in PBS) were loaded onto a grid and stained with saturated uranyl acetate for 2 min at room temperature. The samples were dried and visualized under a transmission electron microscope (Hitachi, Tokyo, Japan) at a nominal magnification of 100,000–250,000.

Immunization, Sensitization and Vaccination

On Days 0 and 7, native BALB/c mice (6–8 weeks old) were injected intraperitoneally with 200 μg rBlo t 5–21 mixed in 100 μL Alum (50 mg/mL Al(OH)3; Sigma-Aldrich, USA) for rBlo t 5–21 protein vaccination. Intratracheal challenges were then carried out. In brief, mice were anesthetized with isoflurane, and then 100 μg of rBlo t 5–21 was delivered to the back of each animal’s tongue on Days 14–20. Sensitized mice were vaccinated subcutaneously with either PBS or 100 μg of HBcAg-rBlo t 5–21 in 100 μL PBS on day 35 and boosted on day 42.

Acute Systemic Anaphylaxis

Sensitized mice were challenged intravenously with 50 μg of rBlo t 5–21 per 100 µL PBS to induce anaphylaxis. Body temperatures were taken using a rectal probe digital thermometer shortly after intravenous antigen challenge and monitored for up to 90 minutes. The area above the curve was determined using Prism (GraphPad 6.02 Software, Inc., San Diego, CA, USA).

Ear Prick Tests

Mice were injected intravenously with 200 µL of Evans blue solution (0.5%; Sangon Biotech, Shanghai, China) and anesthetized 30 min later with isoflurane. Afterward, a drop of rBlo t 5–21 solution (10 μg/20 μL PBS) was placed onto the outer ear skin. Pricks were made into the ear skin with 23-gauge needles (SteriLance, Suzhou, China). For intradermal ear prick tests, an rBlo t 5–21 solution (10 μg/10 μL PBS) was injected intradermally into the ears. Extravasations of dye began almost immediately after the antigen challenge. The mice were euthanized an hour later, and their ears were processed for densitometry analysis of dye leakage. For this purpose, the area of dye leakage was defined within the densitometer by gating around the leaked dye. The magnitude of dye leakage per ear was determined by a combination of the size and color intensity of the pricked area, which was reported as net intensity by the densitometer.

Histology and Inflammation Score

Lung samples from mice were collected from each group, fixed in 4% paraformaldehyde and embedded in paraffin blocks. Sections were then cut and fixed. Antigen retrieval was accomplished by boiling the slides in 0.01 M citrate buffer (pH 6.0) followed by hematoxylin and eosin (H&E) staining with for evaluation of cell invasion and analyzed under a light microscope for determining histology changes.

Lung inflammation was blindly scored. A value of 0 to 3 per criterion was adjudged to evaluate the degree of peribronchial inflammation. A value of 0 was for no inflammation, a value of 1 was for occasional cuffing with inflammatory cells, a value of 2 for most bronchi surrounded by thin layer (one to five cells) of inflammatory cells and a value of 3 was for most bronchi surrounded by a thick layer (more than five cells thick) of inflammatory cells. Each group used 5 mice for H&E staining and scoring analysis.

Determination of Antigen-Specific IgG, IgG1, IgG2a, and IgE

For determination of rBlo t 5–21-specific IgG/IgG1/IgG2a, 96-well ELISA plates (Sangon Biotech, Shanghai, China) were coated with 10 µg of rBlo t 5–21 in carbonate buffer at 4℃ overnight. The plates were rinsed five times with PBS containing 0.05% Tween (PBST), then blocked with 2% nonfat milk solution for 2 hours before being washed five times more with PBST. Serial dilutions of sera were added to the plates and incubated for 2 h at 37℃. The plates were then washed five more times with PBST. Thereafter, HRP-conjugated rabbit anti-mouse IgG (Sangon Biotech, Shanghai, China), HRP-conjugated goat anti-mouse IgG1 (cat. No. PA1-74421, Thermo Fisher Scientific, Waltham, MA, USA), and HRP-conjugated goat anti-mouse IgG2a (cat. No. A10685, Thermo Fisher Scientific, Waltham, MA, USA) antibodies were incubated at 37℃ for 2 h. Plates were washed five times with PBST, followed by the addition of the substrate 3,3’,5,5’-tetramethylbenzidine (Cat. No. C520026, Sangon Biotech, Shanghai, China) and incubated in the dark for 30 min. Then, the stop solution is added to the 96-well plates (Buffer D of EL-TMB Chromogenic Reagent kit, Cat. No. C520026, Sangon Biotech, Shanghai, China). Optical densities were measured at 450 nm.

For the determination of rBlo t 5–21-specific IgE, 96-well plates were coated with 10 µg of rBlo t 5–21 in carbonate buffer at 4℃ overnight. After washing with PBST and blocking with 2% nonfat milk solution for 2 h at 37℃, the sera of individual mice were diluted 1:5 and incubated for 2 h at 37℃. Goat anti-mouse IgE (cat. No. ab19967; Abcam, Cambridge, UK) antibody was added and incubated at 37℃ for 2 h. After washing five times with PBST, plates were incubated with an HRP-conjugated rabbit anti-goat IgG (Sangon Biotech, Shanghai, China) antibodies for 2 h at 37℃. Thereafter, plates were washed five times with PBST, followed by the addition of the substrate 3.3’,5,5’-tetramethylbenzidine (Cat. No. C520026, Sangon Biotech, Shanghai, China) and incubated in the dark for 30 min. Then, added stop solution to stop raction (Buffer D of EL-TMB Chromogenic Reagent kit, Cat. No. C520026, Sangon Biotech, Shanghai, China). Optical densities were measured at 450 nm.

Statistical Analysis

All statistical analysis comparing two different groups were performed with two tailed Student’s t-tests. The resulting p values are either indicated in figure legends or with asterisks in figures (*p < 0.05; **p < 0.01).

Results

Expression and Validation of Recombinant Fusion Proteins

The recombinant plasmids PQE80L-rBlo t 5, PQE80L-rBlo t 21, and PQE80L-rBlo t 5–21 were constructed as shown in . The recombinant plasmid was digested by BamHI and SalI and detected by gel electrophoresis (). All positive bands were detected in the corresponding location (rBlo t 5, Lane 1; rBlo t 21, Lane 2; and rBlo t 5–21, Lane 3). Blomia tropicalis recombinant allergens were expressed and purified as full-length fusion proteins containing N-terminal His-tags (6×His). Once the fusion proteins were purified, their tags were not removed. Each His-tagged protein (rBlo t 5, rBlo t 21, and rBlo t 5–21) produced an expected band in sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) (). Validation of recombinant fusion proteins (rBlo t 5 and rBlo t 5–21) was detected by Western blotting using biotin4D9 anti-Blo t 5 ().

Figure 1 Expression, purification, and Western blotting identification of recombinant tropical mite allergens. (A) Construction diagram of recombinant protein. (B) Double enzyme digestion of recombinant plasmid: M, DNA marker (DL5000, Takara, Japan); 1, PQE80L-rBlo t 5 digested with BamHI and SalI; 2, PQE80L-rBlo t 21 digested with BamHI and SalI; 3, PQE80L-rBlo t 5–21 digested with BamHI and SalI. (CE) Prokaryotic expression and purification of recombinant proteins rBlo t 5, rBlo t 21, and rBlo t 5–21: M, prestained protein marker (26612, ThermoFisher, USA); IPTG (−), bacterial lysate with no IPTG induction; IPTG (+) 1, bacterial lysate with IPTG induction; IPTG (+) 2, supernatant of bacterial lysate with IPTG introduction; E1–E3, protein purified for different times by nickel column. (F) Western blotting analysis of protein: M, prestained protein marker (26616, ThermoFisher, USA); 1, rBlo t 5–21 protein purified by nickel column; 2, rBlo t 5 protein purified by nickel column.

Figure 1 Expression, purification, and Western blotting identification of recombinant tropical mite allergens. (A) Construction diagram of recombinant protein. (B) Double enzyme digestion of recombinant plasmid: M, DNA marker (DL5000, Takara, Japan); 1, PQE80L-rBlo t 5 digested with BamHI and SalI; 2, PQE80L-rBlo t 21 digested with BamHI and SalI; 3, PQE80L-rBlo t 5–21 digested with BamHI and SalI. (C–E) Prokaryotic expression and purification of recombinant proteins rBlo t 5, rBlo t 21, and rBlo t 5–21: M, prestained protein marker (26612, ThermoFisher, USA); IPTG (−), bacterial lysate with no IPTG induction; IPTG (+) 1, bacterial lysate with IPTG induction; IPTG (+) 2, supernatant of bacterial lysate with IPTG introduction; E1–E3, protein purified for different times by nickel column. (F) Western blotting analysis of protein: M, prestained protein marker (26616, ThermoFisher, USA); 1, rBlo t 5–21 protein purified by nickel column; 2, rBlo t 5 protein purified by nickel column.

Establishment of the Allergic Mouse Model

To investigate the efficacy of the virus-like particle vaccine constructed in our study, we established an allergic mouse model. BALB/c mice were sensitized and intratracheal challenged with rBlo t 5, rBlo t 21 and rBlo t 5–21 (). Since the significant increase in IgE level is a typical feature of type I hypersensitivity, we measured the total IgE level in the serum of sensitized mice (). Compared with the groups induced by PBS, rBlo t 5, and rBlo t 21, the total IgE level of the sensitized mice induced by rBlo t 5–21 was significantly increased.

Figure 2 Allergic model mice induced by allergen rBlo t 5–21. (A). Flowchart of induced allergic mice model. After induction of mice allergic model, blood was collected on day 21 to prepare serum for IgE detection (red text). (B). The IgE levels of total serum in mice (n = 5). (C). The temperature change curve (n = 3). (D). Temperature variation curve area statistic chart (n = 3). (E). Mouse lung sections stained with hematoxylin and eosin staining. (F). Statistical chart of lung cell infiltration score in mice (n = 5). *, p < 0.05; **, p < 0.01.

Abbreviation: ns, no significant difference.
Figure 2 Allergic model mice induced by allergen rBlo t 5–21. (A). Flowchart of induced allergic mice model. After induction of mice allergic model, blood was collected on day 21 to prepare serum for IgE detection (red text). (B). The IgE levels of total serum in mice (n = 5). (C). The temperature change curve (n = 3). (D). Temperature variation curve area statistic chart (n = 3). (E). Mouse lung sections stained with hematoxylin and eosin staining. (F). Statistical chart of lung cell infiltration score in mice (n = 5). *, p < 0.05; **, p < 0.01.

To assess acute systemic anaphylactic reactions, sensitized mice were challenged intravenously with corresponding allergens to induce anaphylactic syndromes as documented by a rapid drop in temperature (eg rBlo t 5-induced allergic mouse model group, mice were injected with rBlo t 5 through tail vein). However, mice in the PBS group were injected with rBlo 5–21 recombinant allergen. As shown in and , rBlo t 5–21-induced allergic mouse model group experienced anaphylaxis with severe drops in body temperature.

Airway inflammation was evaluated with hematoxylin and eosin staining. The mice were sacrificed, and their lung tissue was removed and fixed by 4% paraformaldehyde. The tissues were then stained with hematoxylin and eosin after paraffin sectioning. According to , the infiltration of inflammatory cells in rBlo t 5–21-, rBlo t 21-, and rBlo t 5-induced mice were significantly higher than that in the PBS group. The Invading cells in the rBlo t 5–21 induce group was significantly higher than those in the rBlo t 5-induced or rBlo t 21-induced group (). The results showed that the best induction effect in mouse allergic model was rBlo t 5–21, followed by rBlo t 5 and rBlo t 21.

Expression and Validation of Recombinant Fusion Protein HBcAg-rBlo t 5-21

We displayed the major Blomia tropicalis recombinant fusion protein rBlo t 5–21 in a highly ordered fashion on HBcAg particle. The details of the constructs are schematically shown in and . The HBcAg-rBlo t 5–21 protein was purified (lane 3, ) and characterized by were detected by Western blotting using biotin4D9 anti-Blo t 5 (Cat. No, MA-4D9, Indoor Biotechnologies, USA) (). To confirm that fusion protein HBcAg-rBlo t 5–21 can form virus-like particles (VLP) structures, the purified HBcAg-rBlo t 5–21 protein was analyzed by transmission electron microscopy (TEM). TEM micrographs confirmed the presence of spherical, capsid-like particles (, middle and right, black arrow), whereas no such structures were observed in the preparation of rBlo t 5–21 protein (, left).

Figure 3 Establishment of recombinant virus-like particles. (A). Structural features of the constituent components of HBcAg. The bar represents the primary sequence of the full-length core protein c1–183 and the sequence of amino acids DPASRE indicates the c/e1 epitope. Additionally, the C-terminal basic domain (clusters of Arg residues) is symbolized by + signs. (B). Chimeric HBcAg-rBlo t 5–21 protein. Amino acids 1 to 149 of HBcAg are retained, then amino acids Pro-79 and Ala-80 of the central c/e1 epitope were replaced by the fusion protein rBlo t 5–21, flanked on both sides by Gly-rich linkers (G4S)2G4 and a 6×His tag was added to the N terminus. (C). prokaryotic expression and purification of recombinant protein HBcAg-rBlo t 5–21: M, Non-prestained protein marker (26610, ThermoFisher, USA); 1, bacterial lysate with no IPTG induction control; 2, bacterial lysate with IPTG induction; 3, chimeric HBcAg-rBlo t 5–21 protein purified by nickel column. (D). Western blotting analysis. M, prestained protein marker (26612, ThermoFisher, USA); 1, HBcAg-rBlo t 5–21 protein; 2, rBlo t 5–21 protein; 3, rBlo t 5 protein. (E). Protein detection by transmission electron microscopy. rBlo t 5–21 protein (left), HBcAg-rBlo t 5–21 protein (middle and right. Right: enlarge the black box.). The black arrows indicate virus-like particles formed by the HBcAg-rBlo t 5–21 protein. (F). The IgG levels of total serum in mice (serum diluted by 1:105, n = 6). Normal mice were randomly divided into two groups. The mice were immunized with different recombinant protein on day 0 and day 7, respectively, and sera were collected on day 21. (G). Curve of temperature change in mice. Asthmatic mice were induced by rBlo t 5–21 and randomly divided into two groups. The allergic mice were subcutaneously immunized with rBlo t 5–21 and HBcAg-rBlo t 5–21 twice with an interval of one week. A week after the treatment ended, allergic mice were challenged intravenously with 50 μg of rBlo t 5–21 per 100 µL PBS to induce anaphylaxis. Body temperatures were measured at regular intervals. (n = 3) (H). Temperature variation curve area statistic chart (n = 3). *, p < 0.05; **, p < 0.01.

Figure 3 Establishment of recombinant virus-like particles. (A). Structural features of the constituent components of HBcAg. The bar represents the primary sequence of the full-length core protein c1–183 and the sequence of amino acids DPASRE indicates the c/e1 epitope. Additionally, the C-terminal basic domain (clusters of Arg residues) is symbolized by + signs. (B). Chimeric HBcAg-rBlo t 5–21 protein. Amino acids 1 to 149 of HBcAg are retained, then amino acids Pro-79 and Ala-80 of the central c/e1 epitope were replaced by the fusion protein rBlo t 5–21, flanked on both sides by Gly-rich linkers (G4S)2G4 and a 6×His tag was added to the N terminus. (C). prokaryotic expression and purification of recombinant protein HBcAg-rBlo t 5–21: M, Non-prestained protein marker (26610, ThermoFisher, USA); 1, bacterial lysate with no IPTG induction control; 2, bacterial lysate with IPTG induction; 3, chimeric HBcAg-rBlo t 5–21 protein purified by nickel column. (D). Western blotting analysis. M, prestained protein marker (26612, ThermoFisher, USA); 1, HBcAg-rBlo t 5–21 protein; 2, rBlo t 5–21 protein; 3, rBlo t 5 protein. (E). Protein detection by transmission electron microscopy. rBlo t 5–21 protein (left), HBcAg-rBlo t 5–21 protein (middle and right. Right: enlarge the black box.). The black arrows indicate virus-like particles formed by the HBcAg-rBlo t 5–21 protein. (F). The IgG levels of total serum in mice (serum diluted by 1:105, n = 6). Normal mice were randomly divided into two groups. The mice were immunized with different recombinant protein on day 0 and day 7, respectively, and sera were collected on day 21. (G). Curve of temperature change in mice. Asthmatic mice were induced by rBlo t 5–21 and randomly divided into two groups. The allergic mice were subcutaneously immunized with rBlo t 5–21 and HBcAg-rBlo t 5–21 twice with an interval of one week. A week after the treatment ended, allergic mice were challenged intravenously with 50 μg of rBlo t 5–21 per 100 µL PBS to induce anaphylaxis. Body temperatures were measured at regular intervals. (n = 3) (H). Temperature variation curve area statistic chart (n = 3). *, p < 0.05; **, p < 0.01.

In order to evaluate whether HBcAg-rBlo t 5–21 has strong immunogenicity, normal mice were randomly divided into two groups. Mice were subcutaneously immunized with rBlo t 5–21 and HBcAg-rBlo t 5–21 on day 0 and day 14, respectively, and serum samples were collected on day 21 to detect IgG levels. As shown in , the HBcAg-rBlo t 5–21 immunized group was able to induce higher levels of IgG than the rBlo t 5–21 immunized group. Furthermore, the rBlo t 5–21-induced allergic mice were randomly divided into two groups, which were immunized with rBlo t 5–21 and HBcAg-rBlo t 5–21, respectively. We found that HBcAg-rBlo t 5–21 could alleviate the decrease of body temperature caused by acute systemic anaphylaxis. However, the body temperature of mice immunized with rBlo t 5–21 protein decreased significantly ( and ). These results indicated that HBcAg-rBlo t 5–21 has good immunogenicity and may be used to inhibit anaphylaxis induced by Blomia tropicalis.

Vaccination with HBcAg-rBlo t 5-21 Can Alleviate rBlo t 5-21-Induced Allergic Symptoms

To investigate whether the HBcAg-rBlo t 5–21 vaccine could treat the established allergic inflammation, BALB/c mice were sensitized and intratracheal challenged with rBlo t 5–21 allergen, then randomly divided into two groups and immunized with PBS or HBcAg-rBlo t 5–21. Naïve mice were negative control (). Mice in naive group have very low IgE levels and sensitive mice have very high IgE levels on day 34 (). The allergic mice vaccinated with HBcAg-rBlo t 5–21 led to a significant decrease in IgE titers at Days 41 and 48 (). However, the titers of IgE were still at a high level. To assess whether vaccinated mice were protected from allergic reactions, all groups were challenged intravenously with rBlo t 5–21, and body temperature was monitored for a maximum of 90 min after challenge. A severe drop in body temperature was observed in mice that had been treated with PBS ( and ). In contrast, HBcAg-rBlo t 5–21-treated allergic mice were completely protected from anaphylactic reactions.

Figure 4 Treatment of allergic mice with HBcAg–rBlo t 5–21. (A). Flowchart of vaccination in allergic model mice. The red font indicates the time point at which the sera were collected. (B). The IgE levels of total serum in mice (Naive group, n = 3; Asthma-PBS group, n = 6; Asthma-HBcAg-rBlo t 5–21 group, n = 6). (C). Curve of temperature change in mice. (Naive group and Asthma-PBS group, n = 6; Asthma-HBcAg-rBlo t 5–21 group, n = 8) (D). Statistical map of body temperature change in mice. (Naive group and Asthma-PBS group, n = 6; Asthma-HBcAg-rBlo t 5–21 group, n = 8) (E). The IgG levels of total serum in mice (serum diluted by 1:105; Naive group, n = 3; Asthma-PBS group, n = 9; Asthma-HBcAg-rBlo t 5–21 group, n = 12). (F). The IgG1 levels of total serum in mice (serum diluted by 1:106; Naive group, n = 3; Asthma-PBS group, n = 9; Asthma-HBcAg-rBlo t 5–21 group, n = 12). (G). The IgG2a levels of total serum in mice (serum diluted by 1:104; Naive group, n = 3; Asthma-PBS group, n = 9; Asthma-HBcAg-rBlo t 5–21 group, n = 12). (H). Changes in IgG1/IgG2a (serum diluted by 1:105; Naive group, n = 3; Asthma-PBS group, n = 9; Asthma-HBcAg-rBlo t 5–21 group, n = 9). (I). Ears prick test. (J). Statistical map of auricle prick test in mice (n = 3). *, p < 0.05; **, p < 0.01.

Figure 4 Treatment of allergic mice with HBcAg–rBlo t 5–21. (A). Flowchart of vaccination in allergic model mice. The red font indicates the time point at which the sera were collected. (B). The IgE levels of total serum in mice (Naive group, n = 3; Asthma-PBS group, n = 6; Asthma-HBcAg-rBlo t 5–21 group, n = 6). (C). Curve of temperature change in mice. (Naive group and Asthma-PBS group, n = 6; Asthma-HBcAg-rBlo t 5–21 group, n = 8) (D). Statistical map of body temperature change in mice. (Naive group and Asthma-PBS group, n = 6; Asthma-HBcAg-rBlo t 5–21 group, n = 8) (E). The IgG levels of total serum in mice (serum diluted by 1:105; Naive group, n = 3; Asthma-PBS group, n = 9; Asthma-HBcAg-rBlo t 5–21 group, n = 12). (F). The IgG1 levels of total serum in mice (serum diluted by 1:106; Naive group, n = 3; Asthma-PBS group, n = 9; Asthma-HBcAg-rBlo t 5–21 group, n = 12). (G). The IgG2a levels of total serum in mice (serum diluted by 1:104; Naive group, n = 3; Asthma-PBS group, n = 9; Asthma-HBcAg-rBlo t 5–21 group, n = 12). (H). Changes in IgG1/IgG2a (serum diluted by 1:105; Naive group, n = 3; Asthma-PBS group, n = 9; Asthma-HBcAg-rBlo t 5–21 group, n = 9). (I). Ears prick test. (J). Statistical map of auricle prick test in mice (n = 3). *, p < 0.05; **, p < 0.01.

Vaccination with HBcAg-rBlo t 5–21 led to a significant increase in rBlo t 5–21-specific IgG, IgG1, and IgG2a titers at Days 41 and 48 (). In addition, the ratio of IgG1 to IgG2a in HBcAg–rBlo t 5–21 immunized group gradually decreased significantly, but there was no significant difference in PBS immunized group on days 34, 41 and 48 ().

To inquire into the effects of vaccination on local allergic reactions, ear skin prick tests with rBlo t 5–21 were performed in a different set of mice. Extravasations of Evans blue began almost immediately after the allergen challenge. We can observe that the dye leakage was very obvious in the asthma model group and the asthma-PBS group, while the dye leakage circle was significantly reduced in the asthma-HBcAg-rBlo t 5–21 group (). Statistical analysis of Evans blue leakage circle also showed that asthma-HBcAg-rBlo t 5–21 group was significantly smaller than the other two groups ().

We next sought to assess whether vaccinated animals have improved pulmonary inflammation. As shown in , as compared with the asthma model group () and asthma-PBS group (), the infiltration of cells in lung tissue of the HBcAg-rBlo t 5–21-treated group () was significantly lower. The cell infiltration of lung tissue in the PBS-treated group was similar to that in the untreated asthma model mice ().

Figure 5 Mouse lung sections stained with hematoxylin and eosin. (A). Untreated model mice (asthma model). (B). PBS-treated model mice (asthma-PBS). (C). Model mice treated with HBcAg–rBlo t 5–21 (asthma–HBcAg-rBlo t 5–21). (D). Lung inflammation was defined as the peribronchial inflammation score (n = 5). Values are expressed as mean ± SEM, ** p < 0.01.

Figure 5 Mouse lung sections stained with hematoxylin and eosin. (A). Untreated model mice (asthma model). (B). PBS-treated model mice (asthma-PBS). (C). Model mice treated with HBcAg–rBlo t 5–21 (asthma–HBcAg-rBlo t 5–21). (D). Lung inflammation was defined as the peribronchial inflammation score (n = 5). Values are expressed as mean ± SEM, ** p < 0.01.

Discussion

In the present study, an allergic mice model was successfully induced using the recombinant allergen rBlo t 5–21 of Blomia tropicalis (), which provides a mouse model for further studies on vaccines and drugs against anaphylaxis induced by Blomia tropicalis. We also describe a therapy for a Blomia tropicalis allergy based on immunization with the recombinant Blomia tropicalis allergen rBlo t 5–21 displayed on VLPs derived from the hepatitis B virus (HBcAg-rBlo t 5–21). One advantage of the HBcAg-VLP is that it can be successfully expressed in multiple prokaryotic and eukaryotic expression systems. For example, expressed in an Escherichia coli expression system,Citation33 in a yeast expression system,Citation34 in an adenoviral vector expression system,Citation35 in human HeLa cells,Citation36 and expressed in plants,Citation37 and the like. Furthermore, foreign antigens fused into the most exposed region on the capsid surface,Citation38 encompassing the immunodominant c/e1 B cell epitope of HBcAg,Citation39 are particularly immunogenic for B cells. In this study, we generated fusions of the HBcAg protein with rBlo t 5–21 protein flanked by flexible linkers in the c/e1 epitope (). The chimeric protein, termed HBcAg-rBlo t 5–21, was observed to form VPLs by transmission electron microscopy (). Foreign antigens, fused into the c/e1 epitope of HBcAg, can be displayed outside the core particles and did not prohibit the formation of VLPs, such as the green fluorescent protein (GFP),Citation40 and the outer surface protein C (OspC) of B. Burgdorferi.Citation41

Allergic diseases mainly depend upon the response of Th2 cells, which leads to the production of IL-4 and IgE.Citation42 The imbalance of Th1/Th2 is the main immunological mechanism of allergic diseases. To change the balance of Thl/Th2 by enhancing Th1 or canceling Th2 reaction has always been the main direction of the immune pathway for the prevention and treatment of allergies and asthma. The most direct pathways include injecting cytokines to induce the activation of the Th1 pathway [eg, interferon (IFN) γ, IL-12, and IL-18] or blocking antibodies that inhibit the action of Th-2-related cytokines (eg, anti-IL-4, anti-IL-5, anti-IL-9, and anti-IL-13).Citation43 IFN-γ and IL-2 in the local environment are the key factors to guide the differentiation of Th0 into Th1 cells. Th1 cells can secrete IFN-γ, IL-2, and tumor necrosis factor and mainly promote cellular immune responses.

IFN-γ can promote the transformation of antibodies synthesized by B-cells into IgG2a and IgG3, while IFN-γ can inhibit the production of IgG1 and IgE. Additionally, Th2 can induce B-cells to produce IgG1, and IL-4 can inhibit the production of IgG2a.Citation44 In this study, after the allergic model mice were treated with HBcAg–rBlo t 5–21 protein, it was found that the levels of IgG1 and IgG2a in the model mice were significantly increased ( and ), indicating that the Th1 and Th2 reactions in the model mice were enhanced, while the ratio of IgG1/IgG2a was decreased significantly (), indicating that the Th1 type reaction in mice was stronger than that of the Th2 type. Acute systemic stress anaphylaxis and ear prick tests showed that HBcAg-rBlo t 5–21 immunization relieved the symptoms of allergic reaction in mice when reexposed to the same allergen ( and ). At the same time, it was found that the invasion of inflammatory cells in the HBcAg–rBlo t 5–21-treated group was significantly lower than that in the untreated group and PBS-treated model mice (). These results suggest that the recombinant virus-like granule protein HBcAg–rBlo t 5–21 has a certain effect on allergic symptoms in mice. It also provides an idea for the prevention and treatment of inhaled and ingested allergens.

However, HBcAg-rBlo t 5–21 can alleviate the allergic symptoms induced by rBlo t 5–21. Whether HBcAg-rBlo t 5–21 can inhibit the allergic reactions induced by Blomia tropicalis remains to be further verified. This is one limitation in this paper. The main reason is that it is difficult to raise Blomia tropicalis in Hainan. Another reason is that the whole extract of Blomia tropicalis commercially available is not very effective. We may solve this problem by means of in-house cultivation in our next article. It was also observed that HBcAg-rBlo t 5–21 could alleviate allergic symptoms induced by rBlo t 5–21, including inhibition of body temperature drop (), reduction of lung cell invasion, etc. However, IgE remained at a high level (). This is mainly because IgE takes longer time to fall. This is the defect of protein desensitization by multiple small injections,Citation45–47 not the deficiency of this article itself. This article is intended as a basic exploration to build a more complex tolerant vaccine, and our subsequent work will focus on vaccine research and development around more rapid IgE decline.

Conclusions

In summary, HBcAg-rBlo t 5–21, a protein vaccine containing both the hepatitis B core antigen and the Blomia tropicalis fusion allergen rBlo t 5–21, can alleviate the allergic symptoms induced by rBlo t 5–21. It could be a novel AIT vaccine candidate for preventing allergy disorders caused by Blomia tropicalis.

Data Sharing Statement

All data generated or analysed during this study are included in this article. Further enquiries can be directed to the corresponding author Yechun Pei.

Statement of Ethics

This study protocol was reviewed and approved by the Animal Ethics Committee of Hainan University, approval number [HNUAUCC-2022-000113], guided by the national law of Regulations for the Administration of Affairs Concerning Experimental Animals (Revision 2017).

Author Contributions

All authors made a significant contribution to the work reported, whether that is in the conception, study design, execution, acquisition of data, analysis and interpretation, or in all these areas; took part in drafting, revising or critically reviewing the article; gave final approval of the version to be published; have agreed on the journal to which the article has been submitted; and agree to be accountable for all aspects of the work.

Disclosure

The authors have no conflicts of interest to declare in this work.

Acknowledgment

We sincerely thank Shuang Geng (Tsinghua University) and Qingyun Li (Washington University, St. Louis) for their valuable suggestions on this article.

Additional information

Funding

The study was financially supported by the grants from Science and Technology Project of Hainan Province (ZDYF2022SHFZ059) and National Natural Science Foundation of China (31860726; 32160837) to Yechun Pei, and the grants from Natural Science Foundation of Hainan Province (821RC1053) and National Natural Science Foundation of China (32160214) to Dayong Wang.

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