RÉSUMÉ
Nanoformulations in vaccinology provide antigen stability and enhanced immunogenicity, in addition to providing targeted delivery and controlled release. In the last years, much research has been focused on vaccine development using virus-like particles, liposomes, emulsions, polymeric, lipid, and inorganic nanoparticles. Importantly, nanoparticle interactions with innate and adaptive immune systems must be clearly understood to guide the rational development of nanovaccines. This review provides a recap and updates on different aspects advocating nanoparticles as promising antigen carriers and immune cell activators for vaccination. Moreover, it offers a discussion of how the physicochemical properties of nanoparticles are modified to target specific cells and improve vaccine efficacy.
Sujet(s)
Antigènes , Vecteurs de médicaments , Nanoparticules , Vaccins , Humains , Vaccins/administration et posologie , Vaccins/immunologie , Animaux , Antigènes/administration et posologie , Antigènes/immunologie , Antigènes/composition chimique , Vecteurs de médicaments/composition chimique , Systèmes de délivrance de médicaments/méthodes , Système d'administration de médicaments à base de nanoparticules/composition chimiqueRÉSUMÉ
In the Americas and specially in Brazil, the Loxosceles intermedia, Loxosceles gaucho and Loxosceles laeta are the three most medically relevant brown spider species, and whose bites can lead to the condition known as loxoscelism. Here, we report the development of a tool capable of identifying a common epitope amongst Loxosceles sp. venom's toxins. A murine monoclonal antibody (LmAb12) and its recombinant fragments (scFv12P and diabody12P) have been produced and characterized. This antibody and its recombinant constructs were able to recognize proteins of Loxosceles spider venoms with specificity. The scFv12P variant was also able to detect low concentrations of Loxosceles venom in a competitive ELISA assay, displaying potential as a venom identification tool. The primary antigenic target of LmAb12 is a knottin, a venom neurotoxin, that has a shared identity of 100 % between the L. intermedia and L. gaucho species and high similarity to L. laeta. Furthermore, we observed LmAb12 was able to partially inhibit in vitro hemolysis, a cellular event typically induced by the Loxosceles sp. venoms. Such behavior might be due to LmAb12 cross-reactivity between the antigenic target of LmAb12 and the venom's dermonecrotic toxins, the PLDs, or even the existence of synergism between these two toxins.
Sujet(s)
Venins d'araignée , Araignées , Animaux , Anticorps monoclonaux/composition chimique , Anticorps monoclonaux/immunologie , Antigènes/composition chimique , Sérums antivenimeux/composition chimique , Réactions croisées , Miniprotéines à noeud de cystine/composition chimique , Phospholipase D/composition chimique , Venins d'araignée/composition chimique , Araignées/composition chimique , Épitopes/composition chimiqueRÉSUMÉ
Fungal infection is an important health problem in Latin America, and in Brazil in particular. Paracoccidioides (mainly P. brasiliensis and P. lutzii) is responsible for paracoccidioidomycosis, a disease that affects mainly the lungs. The glycoprotein gp43 is involved in fungi adhesion to epithelial cells, which makes this protein an interesting target of study. A specific stretch of 15 amino acids that spans the region 181-195 (named P10) of gp43 is an important epitope of gp43 that is being envisioned as a vaccine candidate. Here we show that synthetic P10 forms typical amyloid aggregates in solution in very short times, a property that could hamper vaccine development. Seeds obtained by fragmentation of P10 fibrils were able to induce the aggregation of P4, but not P23, two other peptides derived from gp43. In silico analysis revealed several regions within the P10 sequence that can form amyloid with steric zipper architecture. Besides, in-silico proteolysis studies with gp43 revealed that aggregation-prone, P10-like peptides could be generated by several proteases, which suggests that P10 could be formed under physiological conditions. Considering our data in the context of a potential vaccine development, we redesigned the sequence of P10, maintaining the antigenic region (HTLAIR), but drastically reducing its aggregation propensity.
Sujet(s)
Amyloïde/composition chimique , Antigènes néoplasiques/composition chimique , Antigènes/composition chimique , Paracoccidioides/immunologie , Blastomycose sud-américaine/prévention et contrôle , Algorithmes , Animaux , Antigènes fongiques/immunologie , Dichroïsme circulaire , Biologie informatique/méthodes , Simulation numérique , Épitopes , Protéines fongiques/composition chimique , Vaccins antifongiques/immunologie , Glycoprotéines/composition chimique , Humains , Techniques in vitro , Blastomycose sud-américaine/immunologie , Peptides/composition chimique , Conformation des protéines , Pliage des protéines , Logiciel , Solvants/composition chimique , Développement de vaccinRÉSUMÉ
Microbiota acquired during labor and through the first days of life contributes to the newborn's immune maturation and development. Mother provides probiotics and prebiotics factors through colostrum and maternal milk to shape the first neonatal microbiota. Previous works have reported that immunoglobulin A (IgA) secreted in colostrum is coating a fraction of maternal microbiota. Thus, to better characterize this IgA-microbiota association, we used flow cytometry coupled with 16S rRNA gene sequencing (IgA-Seq) in human colostrum and neonatal feces. We identified IgA bound bacteria (IgA+) and characterized their diversity and composition shared in colostrum fractions and neonatal fecal bacteria. We found that IgA2 is mainly associated with Bifidobacterium, Pseudomonas, Lactobacillus, and Paracoccus, among other genera shared in colostrum and neonatal fecal samples. We found that metabolic pathways related to epithelial adhesion and carbohydrate consumption are enriched within the IgA2+ fecal microbiota. The association of IgA2 with specific bacteria could be explained because these antibodies recognize common antigens expressed on the surface of these bacterial genera. Our data suggest a preferential targeting of commensal bacteria by IgA2, revealing a possible function of maternal IgA2 in the shaping of the fecal microbial composition in the neonate during the first days of life.
Sujet(s)
Antigènes/immunologie , Colostrum/composition chimique , Colostrum/immunologie , Microbiome gastro-intestinal/immunologie , Immunoglobuline A/immunologie , Antigènes/composition chimique , Bactéries/immunologie , Fèces/microbiologie , Femelle , Humains , Immunoglobuline A/analyse , Immunoglobuline A/classification , Nouveau-né , Modèles linéaires , Études longitudinales , Grossesse , Études prospectives , ARN ribosomique 16S/génétiqueRÉSUMÉ
Virus-like particles are excellent inducers of the adaptive immune response of humans and are presently being used as scaffolds for the presentation of foreign peptides and antigens derived from infectious microorganisms for subunit vaccine development. The most common approaches for peptide and antigen presentation are translational fusions and chemical coupling, but some alternatives that seek to simplify the coupling process have been reported recently. In this work, an alternative platform for coupling full antigens to virus-like particles is presented. Heterodimerization motifs inserted in both Tobacco etch virus coat protein and green fluorescent protein directed the coupling process by simple mixing, and the obtained complexes were easily taken up by a macrophage cell line.
Sujet(s)
Présentation d'antigène/immunologie , Antigènes , Potyvirus , Vaccins à pseudo-particules virales , Animaux , Antigènes/composition chimique , Antigènes/immunologie , Souris , Potyvirus/composition chimique , Potyvirus/immunologie , Cellules RAW 264.7 , Vaccins à pseudo-particules virales/composition chimique , Vaccins à pseudo-particules virales/immunologieRÉSUMÉ
Abstract The rapid and accurate diagnosis of tuberculosis (TB), especially considering limited resources, is still a challenge. Development of new methodologies and tests are needed to overcome several disadvantages of the available standard tests. We evaluated the diagnostic potential of two antigens specific for Mycobacterium tuberculosis, the CFP10 and ESAT6 recombinant proteins, and developed stable formulations thereof. Sensitivity and specificity of the delayed-type hypersensitivity (DTH) skin testing and the induction of gamma interferon production (IFN-γ) by lymphocytes, as a non-invasive test, were evaluated using the CFP10 and ESAT6 protein formulations. The recombinant proteins produced by our group presented a high DTH response and the ability to differentiate between tuberculosis infection, BCG vaccination, and the contact with non-tuberculous mycobacteria (NTM). The production of IFN-γ by stimulation with individual and combined proteins was detected in a panel of 40 individuals and showed a specificity of 100% and a sensitivity of 90% when the two proteins were used together. Lyophilized formulations were stable under all conditions, while soluble formulations were stable under freezing at -20 ºC and -80 ºC. The proposed formulations containing the ESAT6 and CFP10 recombinant antigens constitute satisfactory tools for TB testing, suitable to be developed and implemented in a large-scale trial.
Sujet(s)
Tuberculose/diagnostic , Interféron gamma , Mycobacterium tuberculosis/isolement et purification , Antigènes/composition chimiqueRÉSUMÉ
BACKGROUND: Several studies have evaluated the effect of infectious diseases and vaccine protocols during pregnancy on maternal milk immunoglobulin (Ig) levels, to understand the protection conferred by lactation on newborns. Colostrum is the primary source of maternal IgA for the newborn. IgA participates in protection mechanisms in the neonate's mucosa. In humans, IgA has two subclasses with differential anatomical distribution among mucosal compartments. Total IgA levels in maternal milk vary after antigen stimulation and have differential affinities in function of the chemical composition of the antigens. We studied the effect of antigenic stimulation during pregnancy on the concentrations of specific IgA1 and IgA2 subclasses in human colostrum. METHODS: We analyzed data from 113 women in Mexico City and compared the amount of IgA subclasses in colostrum against three antigens: two from vaccine protocols (tetanus toxoid and pneumococcal polysaccharides) and lipopolysaccharide, a ubiquitous antigen in the gastrointestinal tract. RESULTS: In agreement with the previous reports, we showed that IgA1 from colostrum mainly recognized protein antigens; in sharp contrast, IgA2 was mostly directed against polysaccharide antigens. These levels increased in women who had previous contacts through vaccination or infections during pregnancy. CONCLUSIONS: Antigen interaction during pregnancy increased the amount of specific IgA subclasses, depending on the chemical composition of the antigen.
Sujet(s)
Antigènes/composition chimique , Antigènes/immunologie , Colostrum/immunologie , Immunoglobuline A/classification , Immunoglobuline A/immunologie , Adulte , Réaction antigène-anticorps , Colostrum/composition chimique , Femelle , Humains , Immunoglobuline A/analyse , GrossesseRÉSUMÉ
ABSTRACT Background: Several studies have evaluated the effect of infectious diseases and vaccine protocols during pregnancy on maternal milk immunoglobulin (Ig) levels, to understand the protection conferred by lactation on newborns. Colostrum is the primary source of maternal IgA for the newborn. IgA participates in protection mechanisms in the neonate's mucosa. In humans, IgA has two subclasses with differential anatomical distribution among mucosal compartments. Total IgA levels in maternal milk vary after antigen stimulation and have differential affinities in function of the chemical composition of the antigens. We studied the effect of antigenic stimulation during pregnancy on the concentrations of specific IgA1 and IgA2 subclasses in human colostrum. Methods: We analyzed data from 113 women in Mexico City and compared the amount of IgA subclasses in colostrum against three antigens: two from vaccine protocols (tetanus toxoid and pneumococcal polysaccharides) and lipopolysaccharide, a ubiquitous antigen in the gastrointestinal tract. Results: In agreement with the previous reports, we showed that IgA1 from colostrum mainly recognized protein antigens; in sharp contrast, IgA2 was mostly directed against polysaccharide antigens. These levels increased in women who had previous contacts through vaccination or infections during pregnancy. Conclusions: Antigen interaction during pregnancy increased the amount of specific IgA subclasses, depending on the chemical composition of the antigen.
Sujet(s)
Humains , Femelle , Grossesse , Adulte , Colostrum/immunologie , Antigènes/immunologie , Antigènes/composition chimique , Colostrum/composition chimique , Réaction antigène-anticorpsRÉSUMÉ
BACKGROUND: The use of biomaterials has been expanded to improve the characteristics of vaccines. Recently we have identified that the peptide PH(1-110) from polyhedrin self-aggregates and incorporates foreign proteins to form particles. We have proposed that this peptide can be used as an antigen carrying system for vaccines. However, the immune response generated by the antigen fused to the peptide has not been fully characterized. In addition, the adjuvant effect and thermostability of the particles has not been evaluated. RESULTS: In the present study we demonstrate the use of a system developed to generate nano and microparticles carrying as a fusion protein peptides or proteins of interest to be used as vaccines. These particles are purified easily by centrifugation. Immunization of animals with the particles in the absence of adjuvant result in a robust and long-lasting immune response. Proteins contained inside the particles are maintained for over 1 year at ambient temperature, preserving their immunological properties. CONCLUSION: The rapid and efficient production of the particles in addition to the robust immune response they generate position this system as an excellent method for the rapid response against emerging diseases. The thermostability conferred by the particle system facilitates the distribution of the vaccines in developing countries or areas with no electricity.
Sujet(s)
Antigènes/immunologie , Immunoglobulines/métabolisme , Protéines de la matrice du corps d'occlusion/composition chimique , Peptides/composition chimique , Vaccins/immunologie , Animaux , Antigènes/composition chimique , Stabilité de médicament , Femelle , Protéines à fluorescence verte/composition chimique , Protéines à fluorescence verte/immunologie , Immunisation , Souris , Nanoparticules , Taille de particule , Agrégats de protéines , Protéines de fusion recombinantes/immunologie , Thermodynamique , Vaccins/composition chimiqueRÉSUMÉ
Biosensors presenting high sensitivity for the detection of biomolecules are very promising for diseases diagnosis. Nowadays, there is a need for the development of biosensors with fast, trustworthy diagnosis and mostly with low cost, mainly for applications in developing countries. Label-free plasmonic biosensors are good candidates to reach out all these characteristics due to the possibility of spectral tunability, fast sensor response, real-time detection, strong enhancement of the local electric field and excellent adaptability to assemble different nanobiotechnology architectures. In this paper, two different configurations for LSPR based biosensor were developed by using solution-phase gold nanorods (S-P-AuNRs) and AuNRs-chip. The LSPR sensitivities were evaluated by monitoring shifts in the longitudinal plasmon band with changes in the refractive index of the medium surrounding the nanoparticles. AuNRs-chip presented higher sensitivity of 297â¯nm RIU-1 (refractive index unit) against 196â¯nm RIU-1 for S-P-AuNRs. Figure of merit (FOM) for AuNRs-chip and S-P-AuNRs were 3.0 and 2.2 RIU-1, respectively. This result was assigned to the coupling of the lower energy longitudinal LSPR mode of propagation for AuNRs-chip among nearby nanoparticles in the film. In addition, an improvement of at least 18% in sensitivity was obtained comparing to others AuNRs based assay with similar aspect ratio. FOM is more appropriate to compare different approaches, in this case, the proposed biosensor reached improvements of at least 114%, presenting higher values even when compared to AuNRs of higher aspect ratio. As a proof of concept, AuNRs surface was chemically modified using mercaptoundecanoic acid followed activation with ethylcarbodiimide and N-hidroxysuccinimide to allow the interaction between Bovine Serum Albumin (BSA) antibody and correspondent antigen. Both configurations studied resulted in efficient plasmonic biosensors, presenting high sensitivity for changes in the refractive index and for surface binding with anti-BSA.
Sujet(s)
Anticorps/composition chimique , Antigènes/composition chimique , Techniques de biocapteur , Or/composition chimique , Nanotechnologie , Nanotubes/composition chimique , Animaux , Bovins , Sérumalbumine bovine/composition chimique , Propriétés de surfaceRÉSUMÉ
Transdermal immunization is highly attractive because of the skin's accessibility and unique immunological characteristics. However, it remains a relatively unexplored route of administration because of the great difficulty of transporting antigens past the outermost layer of skin, the stratum corneum. In this article, the abilities of three poly( N-vinylcaprolactam) (PVCL)-based thermoresponsive assemblies-PVCL hydrogels and nanogels plus novel film forming PVCL/acrylic nanogels-to act as protein delivery systems were investigated. Similar thermal responses were observed in all systems, with transition temperatures close to 32 °C, close to that of the skin surface. The investigated dermal delivery systems showed no evidence of cytotoxicity in human fibroblasts and were able to load and release ovalbumin (OVA), a well-studied antigen, in a temperature-dependent manner in vitro. The penetration of OVA into ex vivo human skin following topical application was evaluated, where enhanced skin delivery was seen for the OVA-loaded PVCL systems relative to administration of the protein alone. The distinct protein release and skin penetration profiles observed for the different PVCL assemblies were here discussed on the basis of their structural differences.
Sujet(s)
Antigènes/composition chimique , Vecteurs de médicaments , Hydrogels/composition chimique , Nanoparticules/composition chimique , Administration par voie cutanée , Antigènes/administration et posologie , Azépan-2-one/composition chimique , Derme/effets des médicaments et des substances chimiques , Derme/anatomopathologie , Épiderme/effets des médicaments et des substances chimiques , Épiderme/anatomopathologie , Humains , Hydrogels/administration et posologie , Nanoparticules/administration et posologie , Ovalbumine/administration et posologie , Ovalbumine/composition chimique , Polyéthylène glycols/synthèse chimique , Polyéthylèneimine/composition chimique , Polymères/administration et posologie , Polymères/composition chimique , Peau/métabolisme , Absorption cutanée/effets des médicaments et des substances chimiques , Température , VaccinationRÉSUMÉ
There is a need for new vaccine adjuvant strategies that offer both vigorous antibody and T-cell mediated protection to combat difficult intracellular pathogens and cancer. To this aim, we formulated class-B synthetic oligodeoxynucleotide containing unmethylated cytosine-guanine motifs (CpG-ODN) with a nanostructure (Coa-ASC16 or coagel) formed by self-assembly of 6-0-ascorbyl palmitate ester. Our previous results demonstrated that mice immunized with ovalbumin (OVA) and CpG-ODN formulated with Coa-ASC16 (OVA/CpG-ODN/Coa-ASC16) elicited strong antibodies (IgG1 and IgG2a) and Th1/Th17 cellular responses without toxic systemic effects. These responses were superior to those induced by a solution of OVA with CpG-ODN or OVA/CpG-ODN formulated with aluminum salts. In this study, we investigated the capacity of this adjuvant strategy (CpG-ODN/Coa-ASC16) to elicit CD8+ T-cell response and some of the underlying cellular and molecular mechanisms involved in adaptive response. We also analyzed whether this adjuvant strategy allows a switch from an immunization scheme of three-doses to one of single-dose. Our results demonstrated that vaccination with OVA/CpG-ODN/Coa-ASC16 elicited an antigen-specific long-lasting humoral response and importantly-high quality CD8+ T-cell immunity with a single-dose immunization. Moreover, Coa-ASC16 promoted co-uptake of OVA and CpG-ODN by dendritic cells. The CD8+ T-cell response induced by OVA/CpG-ODN/Coa-ASC16 was dependent of type I interferons and independent of CD4+ T-cells, and showed polyfunctionality and efficiency against an intracellular pathogen. Furthermore, the cellular and humoral responses elicited by the nanostructured formulation were IL-6-independent. This system provides a simple and inexpensive adjuvant strategy with great potential for future rationally designed vaccines.
Sujet(s)
Antigènes/immunologie , Lymphocytes T CD4+/immunologie , Lymphocytes T CD4+/métabolisme , Lymphocytes T CD8+/immunologie , Lymphocytes T CD8+/métabolisme , Interféron de type I/métabolisme , Oligodésoxyribonucléotides/immunologie , Adjuvants immunologiques , Animaux , Antigènes/composition chimique , Cytokines/métabolisme , Humains , Immunité humorale , Souris , Souris knockout , Nanostructures , Oligodésoxyribonucléotides/composition chimique , Ovalbumine/immunologie , Transduction du signal , Sous-populations de lymphocytes T/immunologie , Sous-populations de lymphocytes T/métabolismeRÉSUMÉ
Diagnosis of Taenia solium cysticercosis in endemic rural communities depends on serological tests, as typically there is no access to imaging facilities. The HP10 antigen ELISA (HP10 Ag ELISA), which detects a high molecular weight secreted protein of viable metacestodes, has been employed for the diagnosis of both human and porcine cysticercosis in such communities. In this communication, we formally demonstrate that the HP10 Ag ELISA, already known to function for the detection of T. saginata and T. solium cysticercosis, also detects a similar high molecular weight antigen of T. hydatigena. Thus, the HP10 Ag assay, while specific for human cysticercosis, may not be recommended for the diagnosis of porcine cysticercosis where there is co-infection of pigs with T. solium and T. hydatigena.
Sujet(s)
Anticorps monoclonaux/composition chimique , Cysticercose/épidémiologie , Maladies des porcs/épidémiologie , Taenia solium/composition chimique , Animaux , Antigènes/composition chimique , Cysticercose/diagnostic , Test ELISA , Tests sérologiques , Suidae , Maladies des porcs/diagnosticRÉSUMÉ
BACKGROUND: The development of safe and reliable protocols for the transplantation of the face and hands may be accomplished with animal modeling of transplantation of vascularized composite allografts (VCA). Previously, we demonstrated that tolerance to a VCA could be achieved after canine recipients were simultaneously given marrow from a dog leukocyte antigen-identical donor. In the present study, we extend those findings across a dog leukocyte antigen mismatched barrier. METHODS: Eight recipient dogs received total body irradiation (4.5 cGy), hematopoietic cell transplantation (HCT), either marrow (n = 4) or granulocyte-colony stimulating factor mobilized peripheral blood stem cells (n = 4), and a VCA transplant from the HCT donor. Post grafting immunosuppression consisted of mycophenolate mofetil (28 days) and cyclosporine (35 days). RESULTS: In 4 dogs receiving bone marrow, 1 accepted both its marrow transplant and demonstrated long-term tolerance to the donor VCA (>52 weeks). Three dogs rejected both their marrow transplants and VCA at 5 to 7 weeks posttransplant. Dogs receiving mobilized stem cells all accepted their stem cell transplant and became tolerant to the VCA. However, 3 dogs developed graft-versus-host disease, whereas 1 dog rejected its stem cell graft by week 15 but exhibited long-term tolerance toward its VCA (>90 weeks). CONCLUSIONS: The data suggest that simultaneous transplantation of mobilized stem cells and a VCA is feasible and leads to tolerance toward the VCA in a haploidentical setting. However, there is a higher rate of donor stem cell engraftment compared with marrow HCT and an increase in the incidence of graft-versus-host disease.
Sujet(s)
Cellules de la moelle osseuse/métabolisme , Allogreffes de tissus composites/immunologie , Survie du greffon , Mobilisation de cellules souches hématopoïétiques/méthodes , Transplantation de cellules souches hématopoïétiques , Animaux , Antigènes/composition chimique , Ciclosporine/pharmacologie , Chiens , Rejet du greffon/immunologie , Maladie du greffon contre l'hôte , Facteur de stimulation des colonies de granulocytes/pharmacologie , Immunosuppression thérapeutique , Leucocytes/immunologie , Acide mycophénolique/pharmacologie , Reproductibilité des résultats , Transplantation de peau , Conditionnement pour greffe , Tolérance à la transplantation , Transplantation homologueRÉSUMÉ
Computational methods have traditionally struggled to predict the effect of mutations in antibody-antigen complexes on binding affinity. This has limited their usefulness during antibody engineering and development, and their ability to predict biologically relevant escape mutations. Here we present mCSM-AB, a user-friendly web server for accurately predicting antibody-antigen affinity changes upon mutation which relies on graph-based signatures. We show that mCSM-AB performs better than comparable methods that have been previously used for antibody engineering. mCSM-AB web server is available at http://structure.bioc.cam.ac.uk/mcsm_ab.
Sujet(s)
Anticorps/génétique , Anticorps/immunologie , Affinité des anticorps/génétique , Antigènes/immunologie , Internet , Mutation , Logiciel , Anticorps/composition chimique , Affinité des anticorps/immunologie , Complexe antigène-anticorps/composition chimique , Complexe antigène-anticorps/génétique , Complexe antigène-anticorps/immunologie , Antigènes/composition chimique , Antigènes/génétique , Référenciation , Jeux de données comme sujet , Anticorps anti-VIH/composition chimique , Anticorps anti-VIH/génétique , Anticorps anti-VIH/immunologie , Ingénierie des protéines , Vaccins/composition chimique , Vaccins/génétique , Vaccins/immunologieRÉSUMÉ
Single domain heavychain binders (nanobodies) obtained from camelid antibody libraries hold a great promise for immunoassay development. However, there is no simple method to select the most valuable nanobodies from the crowd of positive clones obtained after the initial screening. In this paper, we describe a novel nanobody-based platform that allows comparison of the reactivity of hundreds of clones with the labeled antigen, and identifies the best nanobody pairs for two-site immunoassay development. The output clones are biotinylated in vivo in 96-well culture blocks and then used to saturate the biotin binding capacity of avidin coated wells. This standardizes the amount of captured antibody allowing their sorting by ranking their reactivity with the labeled antigen. Using human soluble epoxide hydrolase (sEH) as a model antigen, we were able to classify 96 clones in four families and confirm this classification by sequencing. This provided a criterion to select a restricted panel of five capturing antibodies and to test each of them against the rest of the 96 clones. The method constitutes a powerful tool for epitope binning, and in our case allowed development of a sandwich ELISA for sEH with a detection limit of 63 pg/mL and four log dynamic range, which performed with excellent recovery in different tissue extracts. This strategy provides a systematic way to test nanobody pairwise combinations and would have a broad utility for the development of highly sensitive sandwich immunoassays.
Sujet(s)
Test ELISA , Anticorps à domaine unique/immunologie , Anticorps à domaine unique/isolement et purification , Réaction antigène-anticorps , Antigènes/composition chimique , Antigènes/métabolisme , Epoxide hydrolase/composition chimique , Epoxide hydrolase/métabolisme , Humains , Protéines recombinantes/composition chimique , Protéines recombinantes/métabolisme , SolubilitéRÉSUMÉ
Antibody engineering must be accompanied by mapping strategies focused on identifying the epitope recognized by each antibody to define its unique functional identity. High throughput fine specificity determination remains technically challenging. We review recent experiences aimed at revisiting the oldest and most extended display technology to develop a robust epitope mapping platform, based on the ability to manipulate target-derived molecules (ranging from the whole native antigen to antigen domains and smaller fragments) on filamentous phages. Single, multiple and combinatorial mutagenesis allowed comprehensive scanning of phage-displayed antigen surface that resulted in the identification of clusters of residues contributing to epitope formation. Functional pictures of the epitope(s) were thus delineated in the natural context. Successful mapping of antibodies against interleukin-2, epidermal growth factor and its receptor, and vascular endothelial growth factor showed the versatility of these procedures, which combine the accuracy of site-directed mutagenesis with the high throughput potential of phage display.
Sujet(s)
Antigènes/immunologie , Techniques d'exposition à la surface cellulaire/méthodes , Cartographie épitopique/méthodes , Banque de peptides , Antigènes/composition chimique , Antigènes/génétique , Épitopes/composition chimique , Épitopes/génétique , Épitopes/immunologie , Humains , Modèles moléculaires , Mutagenèse dirigée/méthodes , Structure tertiaire des protéinesRÉSUMÉ
Although multiple different procedures to characterize the epitopes recognized by antibodies have been developed, site-directed mutagenesis remains the method of choice to define the energetic contribution of antigen residues to binding. These studies are useful to identify critical residues and to delineate functional maps of the epitopes. However, they tend to underestimate the roles of residues that are not critical for binding on their own, but contribute to the formation of the target epitope in an additive, or even cooperative, way. Mapping antigenic determinants with a diffuse energetic landscape, which establish multiple individually weak interactions with the antibody paratope, resulting in high affinity and specificity recognition of the epitope as a whole, is thus technically challenging. The current work was aimed at developing a combinatorial strategy to overcome the limitations of site-directed mutagenesis, relying on comprehensive randomization of discrete antigenic regions within phage-displayed antigen libraries. Two model antibodies recognizing epidermal growth factor were used to validate the mapping platform. Abrogation of antibody recognition due to the introduction of simultaneous replacements was able to show the involvement of particular amino acid clusters in epitope formation. The abundance of some of the original residues (or functionally equivalent amino acids sharing their physicochemical properties) among the set of mutated antigen variants selected on a given antibody highlighted their contributions and allowed delineation of a detailed functional map of the corresponding epitope. The use of the combinatorial approach could be expanded to map the interactions between other antigens/antibodies.
Sujet(s)
Facteur de croissance épidermique/génétique , Facteur de croissance épidermique/immunologie , Cartographie épitopique/méthodes , Mutagenèse , Séquence d'acides aminés , Animaux , Anticorps monoclonaux/immunologie , Réaction antigène-anticorps , Antigènes/composition chimique , Antigènes/génétique , Antigènes/immunologie , Lignée cellulaire tumorale , Facteur de croissance épidermique/composition chimique , Épitopes/composition chimique , Épitopes/génétique , Épitopes/immunologie , Humains , Souris , Modèles moléculaires , Données de séquences moléculaires , Mutagenèse dirigée , Banque de peptides , Conformation des protéinesRÉSUMÉ
B-1 lymphocytes comprise a unique subset of B cells that differ phenotypically, ontogenetically and functionally from conventional B-2 cells. A frequent specificity of the antibody repertoire of peritoneal B-1 cells is phosphatidylcholine. Liposomes containing phosphatidylcholine have been studied as adjuvants and their interaction with dendritic cells and macrophages has been demonstrated. However, the role of B-1 cells in the adjuvanticity of liposomes composed of phosphatidylcholine has not been explored. In the present work, we studied the contribution of B-1 cells to the humoral response against ovalbumin (OVA) encapsulated into dipalmitoylphosphatidylcholine (DPPC) and cholesterol-containing liposomes. BALB/X-linked immunodeficient (xid) mice, which are deficient in B-1 cells, showed quantitative and qualitative differences in the anti-OVA antibody response compared with wild-type animals after immunization with these liposomes. The OVA-specific immune response was significantly increased in the BALB/xid mice when reconstituted with B-1 cells from naive BALB/c mice. Our results indicate the internalization of DPPC-containing liposomes by these cells and their migration from the peritoneal cavity to the spleen. Phosphatidylcholine significantly contributed to the immunogenicity of liposomes, as DPPC-containing liposomes more effectively stimulated the anti-OVA response compared with vesicles composed of dipalmitoylphosphatidylglycerol. In conclusion, we present evidence for a cognate interaction between B-1 cells and phosphatidylcholine liposomes, modulating the immune response to encapsulated antigens. This provides a novel targeting approach to assess the role of B-1 cells in humoral immunity.
Sujet(s)
Antigènes/immunologie , Sous-populations de lymphocytes B/immunologie , Adjuvants immunologiques , Animaux , Anticorps/immunologie , Production d'anticorps/immunologie , Spécificité des anticorps , Antigènes/composition chimique , Sous-populations de lymphocytes B/métabolisme , Mouvement cellulaire , Femelle , Immunisation , Liposomes , Souris , Ovalbumine/immunologie , Phosphatidylcholines/composition chimique , Phosphatidylcholines/immunologie , Rate/immunologieRÉSUMÉ
Sea lice (Copepoda, Caligidae) are the most widely distributed marine pathogens in the salmon industry. Vaccination could be an environmentally friendly alternative for sea lice control; however, research on the development of such vaccines is still at an early stage of development. Recent results have suggested that subolesin/akirin/my32 are good candidate antigens for the control of arthropod infestations, including sea lice, but background knowledge about these genes in crustaceans is limited. Herein, we characterize the my32 gene/protein from two important sea lice species, Caligus rogercresseyi and Lepeophtheirus salmonis, based on cDNA sequence isolation, phylogenetic relationships, three dimensional structure prediction and expression analysis. The results show that these genes/proteins have the main characteristics of akirins from invertebrates. In addition, immunization with purified recombinant my32 from L. salmonis elicited a specific antibody response in mice and fish. These results provide an improvement to our current knowledge about my32 proteins and their potential use as vaccine candidates against sea lice in fish.