RÉSUMÉ
The p38 mitogen-activated protein kinase (MAPK) is one important member of MAPK family and reported to serve a predominant function in regulating innate immunity after the occurrence of certain infection. In the present study, one novel p38 MAPK gene was acquired from Cyclina sinensis based on the RNA-seq analysis and designated as Csp38 MAPK. This novel gene contained a full length of 1781 bp, 1104 bp of which was deemed as open reading frames and gave rise to a peptide of 367 amino acids with a predicted molecular weight of 42.31 KDa. A conserved serine/threonine protein kinase (S_Tkc) region along with a Thr-Gly-Tyr motif was discovered in the deduced sequence. According to the phylogenetic analysis, there was a close relationship between this kinase and Meretrix petechialis p38 MAPK. As for the expression pattern, this newly-identified Csp38 MAPK was ubiquitously distributed in several tissues throughout the body but with varied abundance. After the challenge of Vibrio anguillarum, both the transcription and phosphorylation level of Csp38 MAPK in hemolymph were coordinately altered with a time-dependent manner. Besides, with the application of double strand RNA homologous to myeloid differentiation factor 88 (MyD88) of C. sinensis, the activation of Csp38 MAPK was found to obviously decrease in hemolymph after the pathogen stimulation. Hence, our experimental data presented evidence for the potential involvement of p38 MAPK in response to bacterial invaders in C. sinensis, possibly facilitating the understanding for pathogen-induced innate immunity in clams.
Sujet(s)
Bivalvia , ADN complémentaire , Vibrio/immunologie , p38 Mitogen-Activated Protein Kinases , Animaux , Bivalvia/génétique , Bivalvia/immunologie , Bivalvia/microbiologie , Clonage moléculaire , ADN complémentaire/génétique , ADN complémentaire/immunologie , p38 Mitogen-Activated Protein Kinases/génétique , p38 Mitogen-Activated Protein Kinases/immunologieRÉSUMÉ
Immuno-PCR (IPCR) is a sensitive antigen detection by means of specific antibody-DNA conjugates. To ensure the successful conjugation of a protein (an antibody) with a reporter DNA, immuno-PCR method based on cDNA display (cD-IPCR) has been introduced. The cDNA display molecule is a 1:1 covalent complex of a polypeptide and its encoding cDNA at the single molecule level, which is directly used for antigen detection and subsequent qPCR. This method can be applied to detect various antigens in biological samples, if sequences of their single-domain antibodies (VHHs) or peptide aptamers are known.
Sujet(s)
Aptamères peptidiques/immunologie , ADN complémentaire/immunologie , Dosage immunologique , Immunoconjugués/immunologie , Réaction de polymérisation en chaîne , Anticorps à domaine unique/immunologie , Protéine A staphylococcique/analyse , Aptamères peptidiques/génétique , ADN complémentaire/génétique , Immunoconjugués/génétique , Anticorps à domaine unique/génétiqueRÉSUMÉ
We have generated polyclonal and monoclonal antibodies by genetic immunization over the last two decades. In this paper, we present our most successful methodology acquired over these years and present the animals in which we obtained the highest rates of success. The technique presented is convenient, easy, affordable, and generates antibodies against mammalian proteins in their native form. This protocol requires neither expensive equipment, such as a gene gun, nor sophisticated techniques such as the conjugation of gold microspheres, electroporation, or surgery to inject in lymph nodes. The protocol presented uses simply the purified plasmid expressing the protein of interest under a strong promoter, which is injected at intramuscular and intradermal sites. This technique was tested in five species. Guinea pigs were the animals of choice for the production of polyclonal antibodies. Monoclonal antibodies could be generated in mice by giving, as a last injection, a suspension of transfected cells. The antibodies detected their antigens in their native forms. They were highly specific with very low non-specific background levels, as assessed by immune-blots, immunocytochemistry, immunohistochemistry and flow cytometry. We present herein a detailed and simple procedure to successfully raise specific antibodies against native proteins.
Sujet(s)
Anticorps monoclonaux/biosynthèse , ADN complémentaire/immunologie , Protéines/immunologie , Animaux , Cellules COS , Chlorocebus aethiops , Cricetinae , Femelle , Cochons d'Inde , Cellules HEK293 , Humains , Immunisation , Souris , Souris de lignée BALB C , Lapins , Rats , Rat Sprague-DawleyRÉSUMÉ
Heterobothrium okamotoi, a monogenean gill parasite, exhibits high host specificity for the tiger puffer, Takifugu rubripes, and it has been experimentally verified that the parasite cannot colonize either closely related species such as the grass puffer Takifugu niphobles or distantly related fish such as the red seabream Pagrus major. Previously, we demonstrated in T. rubripes that immunoglobulin M (IgM) with d-mannose affinity induced deciliation of the oncomiracidia, the first step of parasitism, indicating that the parasite utilizes the molecule as a receptor for infection. In the present study, we purified mannose-specific IgM from 2 nonhost species, T. niphobles and P. major, by affinity and gel-filtration chromatography techniques and compared their deciliation-inducing activity against H. okamotoi oncomiracidia. The IgM of the former showed activity, whereas the latter had no effect, suggesting that in addition to d-mannose-binding ability, the crystallizable fragment domain of IgM, which is not part of the antigen-binding domain, plays an important role in host recognition by the oncomiracidia, such as direct binding to the parasites. It also suggests that the host specificity of H. okamotoi is relatively low upon initial recognition, and the specificity is established by exclusion in nonhosts during a later stage.
Sujet(s)
Ectoparasitoses/médecine vétérinaire , Maladies des poissons/parasitologie , Immunoglobuline M/physiologie , Mannose/immunologie , Plathelminthes/immunologie , Takifugu/parasitologie , Séquence d'acides aminés , Animaux , Technique de Western , Cils vibratiles/immunologie , Clonage moléculaire , ADN complémentaire/génétique , ADN complémentaire/immunologie , Ectoparasitoses/immunologie , Ectoparasitoses/parasitologie , Électrophorèse sur gel de polyacrylamide , Maladies des poissons/immunologie , Expression des gènes , Branchies/parasitologie , Spécificité d'hôte , Concentration en ions d'hydrogène , Immunoglobuline M/sang , Immunoglobuline M/génétique , Immunoglobuline M/isolement et purification , Muqueuse/composition chimique , Muqueuse/immunologie , Muqueuse/parasitologie , Plathelminthes/pathogénicité , Spectrométrie de masse MALDI , Takifugu/immunologie , Infections à trématodes/immunologie , Infections à trématodes/parasitologie , Infections à trématodes/médecine vétérinaireRÉSUMÉ
Zika virus (ZIKV) is a mosquito-borne member of the Flaviviridae family that has been known to circulate for decades causing mild febrile illness. The more recent ZIKV outbreaks in the Americas and the Caribbean associated with congenital malformations and Guillain-Barré syndrome in adults have placed public health officials in high alert and highlight the significant impact of ZIKV on human health. New technologies to study the biology of ZIKV and to develop more effective prevention options are highly desired. In this study we demonstrate that direct delivery in mice of an infectious ZIKV cDNA clone allows the rescue of recombinant (r)ZIKV in vivo. A bacterial artificial chromosome containing the sequence of ZIKV strain Paraiba/2015 under the control of the cytomegalovirus promoter was complexed with a commercial transfection reagent and administrated using different routes in type-I interferon receptor deficient A129 mice. Clinical signs and death associated with ZIKV viremia were observed in mice. The rZIKV recovered from these mice remained fully virulent in a second passage in mice. Interestingly, infectious rZIKV was also recovered after intraperitoneal inoculation of the rZIKV cDNA in the absence of transfection reagent. Further expanding these studies, we demonstrate that a single intraperitoneal inoculation of a cDNA clone encoding an attenuated rZIKV was safe, highly immunogenic, and provided full protection against lethal ZIKV challenge. This novel in vivo reverse genetics method is a potentially suitable delivery platform for the study of wild-type and live-attenuated ZIKV devoid of confounding factors typical associated with in vitro systems. Moreover, our results open the possibility of employing similar in vivo reverse genetic approaches for the generation of other viruses and, therefore, change the way we will use reverse genetics in the future.
Sujet(s)
Chromosomes artificiels de bactérie/génétique , ADN complémentaire/génétique , Vecteurs génétiques/administration et posologie , Virémie/prévention et contrôle , Infection par le virus Zika/prévention et contrôle , Virus Zika/génétique , Animaux , Chlorocebus aethiops , ADN complémentaire/immunologie , ADN viral/génétique , ADN viral/immunologie , Modèles animaux de maladie humaine , Femelle , Mâle , Souris , Récepteur à l'interféron alpha-bêta/génétique , Génétique inverse , Vaccins atténués/administration et posologie , Vaccins atténués/immunologie , Cellules Vero , Vaccins antiviraux/administration et posologie , Vaccins antiviraux/immunologie , Virémie/génétique , Virémie/immunologie , Virus Zika/immunologie , Infection par le virus Zika/génétique , Infection par le virus Zika/immunologieRÉSUMÉ
Peptidoglycan recognition proteins (PGRPs) are pattern recognition receptors that can recognize bacterial peptidoglycans and trigger the innate immune response of insects. Here, we identified and characterized a novel short-type Bombyx mori peptidoglycan recognition proteins short-4 (BmPGRP-S4) in a lepidopteran insect, Bombyx mori. BmPGRP-S4 exhibited a cDNA sequence length of 600 bp, encoding 199 aa with a protein molecular weight of 22 kDa. Multiple sequence alignment revealed that BmPGRP-S4 contains a conserved PGRP domain. Quantitative real-time polymerase chain reaction analysis showed that BmPGRP-S4 is highly expressed in the early developmental stages of silkworm larvae and presents tissue-specific expression in hemocytes. Interestingly, BmPGRP-S4 expression is significantly induced by bacterial infection in the midgut, fat body, and hemocytes. Furthermore, a dual luciferase reporter gene assay revealed that BmPGRP-S4 can activate the expression of the antimicrobial peptide genes lebocin, moricin, cecropin D, cecropin B, and attacin. Taken together, these results suggest that BmPGRP-S4 plays an important role in the innate immune response of silkworms.
Sujet(s)
Bombyx/génétique , Protéines de transport/génétique , Immunité innée/génétique , Séquence d'acides aminés/génétique , Animaux , Peptides antimicrobiens cationiques/génétique , Protéines de transport/composition chimique , Clonage moléculaire , ADN complémentaire/génétique , ADN complémentaire/immunologie , Régulation de l'expression des gènes/génétique , Régulation de l'expression des gènes/immunologie , Protéines d'insecte/génétique , Larve/composition chimique , Larve/génétique , Alignement de séquencesRÉSUMÉ
The diagnostic performance of a cocktail formula consisting of two Babesia (B.) bovis recombinant proteins, including spherical body protein 1 (BbSBP-1) and spherical body protein 4 (BbSBP-4), was evaluated in the present study for the global detection of B. bovis infection in cattle and for the differentiation between B. bovis and B. bigemina infections. The efficacy and the practicality of the rBbSBP-1 and rBbSBP-4 cocktail formula for differentiation between the infection caused by both parasites were assessed using indirect enzyme-linked immunosorbent assay (iELISA) with serum samples collected from cattle experimentally infected by B. bovis (nâ¯=â¯33) or B. bigemina (nâ¯=â¯30). Cocktail antigen exhibited the highest optical density (OD) values with B. bovis-infected sera and the lowest OD values with normal bovine sera or B. bigemina-infected sera in comparison with the single antigen. A total of 581 field serum samples collected from four countries with known B. bovis endemicity: Ghana (nâ¯=â¯154), Egypt (nâ¯=â¯162), Thailand (nâ¯=â¯96), and South Africa (nâ¯=â¯169) were screened also in the current study using iELISA and the results were compared to those of indirect fluorescent antibody test (IFAT) as a reference. A cocktail formula (rBbSBP-1 and rBbSBP-4) exhibited the highest concordance rate (89.90%) and kappa value (0.73). The obtained results revealed the reliability of the rBbSBP-1 and rBbSBP-4 cocktail antigen for the detection of specific antibodies to B. bovis in cattle and demonstrated the usefulness of cocktail antigen for differentiation between B. bovis and B. bigemina infections compared with the single antigen in cattle, which will be useful for epidemiological surveys and control of bovine babesiosis.
Sujet(s)
Antigènes de protozoaire/immunologie , Babesia bovis/immunologie , Babésiose/parasitologie , Maladies des bovins/parasitologie , Protéines recombinantes/immunologie , Animaux , Anticorps antiprotozoaires/sang , Babésiose/diagnostic , Babésiose/immunologie , Technique de Western/médecine vétérinaire , Bovins , Maladies des bovins/diagnostic , Maladies des bovins/immunologie , ADN complémentaire/biosynthèse , ADN complémentaire/immunologie , Égypte , Test ELISA/médecine vétérinaire , Ghana , Protéines recombinantes/génétique , Sensibilité et spécificité , République d'Afrique du Sud , ThaïlandeRÉSUMÉ
This study presents an efficient method to improve TCR affinity, comprising 1) CDR-directed saturation mutation of TCR cDNA, 2) transient TCR display on CD3-expressing HEK293T (CD3-293T) cells by simple plasmid transfection, 3) staining with HLA-tetramers, and 4) multi-round sorting of cells with CD8-independent tetramer binding on a flow cytometer. Using these procedures, we successfully identified mutant TCRs with enhanced binding from an HLA-A*24:02-restricted, human telomerase reverse transcriptase (hTERT)-specific TCR. Two such clones, 2A7A and 2D162, harboring mutations in CDR1 and CDR2 of TCRß, respectively, were isolated with both showing sequential four amino acid substitutions. When expressed on CD3-293T cells along with wild-type TCRα, the TCR molecules of these mutants as well as their combinatory mutation, bound to HLA-A24/hTERT-tetramers more strongly than the wild-type TCRs, without binding to control tetramers. Besides, in order to facilitate a functional study of TCR, we established an artificial T cell line, designated as CD8I-J2, which expresses a human CD8 and IFN-γ producing cassette by modifying Jurkat-derived J.RT3-T3.5 cells. CD8I-J2 cells expressing wild-type or affinity-enhanced hTERT-specific TCRs were analyzed for their recognition of serially diluted cognate peptide on HLA-A*24:02-transduced T2 cells. CD8I-J2 cells expressing each mutant TCR recognized the hTERT peptide at lower concentrations than wild-type TCR. The hierarchy of peptide recognition is concordant with tetramer binding on CD3-293T cells and none of these mutant TCRs were cross-reactive with irrelevant peptides reported to be present on HLA-A*24:02 molecules as far as tested. These methods might thus be useful for obtaining high affinity mutants from other TCRs of interest.
Sujet(s)
Récepteurs aux antigènes des cellules T/génétique , ADN complémentaire/génétique , ADN complémentaire/immunologie , Cellules HEK293 , Humains , Mutation , Peptides/génétique , Peptides/immunologie , Récepteurs aux antigènes des cellules T/immunologieRÉSUMÉ
Single-domain antibodies (variable domain of the heavy chain of a heavy chain antibody; VHH) are promising reagents for therapeutics and diagnostics because of their stability, cost-effective production and material workability as a small antibody. Currently, general acquisition of a VHH using immunization of camelids is inconvenient from the standpoint of animal protection, cost and the process is time-consuming. Thus, a straightforward and efficient method for screening VHHs against a target molecule is required. In this study, we examined whether in vitro selection of a VHH against a target protein could be performed by a cDNA display method with an artificial VHH library that had the three complementarity-determining regions (CDRs) randomized by chemical synthesis. The results revealed that a particular VHH against survivin, which is a member of the inhibitor of apoptosis family, was selected with affinity in the range of 10-7 to 10-8â¯M. The in vitro selection of a VHH using cDNA display with an artificial synthesized library without animal immunization was shown to be effective for rapid and inexpensive screening of VHHs against a target protein.
Sujet(s)
ADN complémentaire/génétique , Anticorps à domaine unique/génétique , Séquence d'acides aminés , Animaux , Brevibacillus/génétique , ADN complémentaire/immunologie , Banque de gènes , Liaison aux protéines , Anticorps à domaine unique/immunologie , Résonance plasmonique de surface , Survivine/immunologieRÉSUMÉ
Bovine leukemia virus (BLV) is the causative agent of enzootic bovine leucosis, which results in significant economic losses on many affected farms. BLV infects a wide range of animals as well as cell lines derived from various mammalian species and organs; however, studies show that only some cell lines support sustained production of viral progeny. The differences between cells that produce viral progeny and those that do not are unclear. The aim of this study was to identify the steps of BLV replication that are associated with the capacity of a cell to support a productive infection. Eleven cell lines derived from various species were categorized into two groups, those that produce BLV progeny and those that do not, and the efficiency of viral attachment was compared. In addition, viral entry and reverse transcription were compared for two BLV-producing cell lines and three non-producing cell lines. BLV attached to and entered all of the tested cells. However, synthesis of viral DNA was inhibited in all three non-virus-producing cell lines, suggesting that BLV production was blocked either prior to or at the stage of reverse transcription. These results increase our understanding of the BLV life cycle and should enable better control over the spread of BLV.
Sujet(s)
ADN complémentaire/génétique , Résistance à la maladie/génétique , Cellules épithéliales/virologie , Virus de la leucémie bovine/génétique , ARN viral/génétique , Réplication virale/physiologie , Animaux , Chats , Bovins , Lignée cellulaire , Chiroptera , Chlorocebus aethiops , ADN complémentaire/biosynthèse , ADN complémentaire/immunologie , Chiens , Cellules épithéliales/classification , Cellules épithéliales/immunologie , Humains , Virus de la leucémie bovine/métabolisme , Souris , Spécificité d'organe , ARN viral/métabolisme , Lapins , Rats , Transcription inverse , Spécificité d'espèce , Attachement viral , Pénétration viraleRÉSUMÉ
Background Thrombospondin type 1 domain-containing 7A (THSD7A) has been identified as a pathogenic autoantigen in membranous nephropathy (MN). However, the THSD7A epitopes targeted by patient autoantibodies are unknown.Methods We performed an in silico analysis of the THSD7A multidomain structure, expressed the folded domains in HEK293 cells, and tested for domain reactivity with 31 serum samples from patients with THSD7A-associated MN using Western and native blotting. Immunogenicity of the antigen domains was further investigated by cDNA immunization of rabbits and mice.Results We characterized the extracellular topology of THSD7A as a tandem string of 21 thrombospondin type 1 domains. Overall, 28 serum samples (90%) recognized multiple epitope domains along the molecule. Detailed epitope mapping revealed that the complex consisting of the first and second N-terminal domains (amino acids 48-192) was recognized by 27 of 31 patient serum samples (87%). Serum recognizing one or two epitope domains showed lower anti-THSD7A antibody levels than serum recognizing three or more epitope domains. During follow-up, a loss of epitope recognition was observed in seven of 16 patients, and it was accompanied by decreasing antibody levels and remission of proteinuria. In four of 16 patients, epitope recognition patterns changed during follow-up. Notably, immunization experiments in rabbits and mice revealed that induced antibodies, like patient autoantibodies, preferentially bound to the most N-terminal domains of THSD7A.Conclusions Our data show that the immune response in THSD7A-associated MN is polyreactive and that autoantibodies predominantly target the most N-terminal part of THSD7A.
Sujet(s)
Antigènes de surface/immunologie , Autoanticorps/sang , Épitopes/immunologie , Glomérulonéphrite extra-membraneuse/immunologie , Protéines membranaires/immunologie , Domaines protéiques/immunologie , Thrombospondines/immunologie , Sujet âgé , Animaux , Antigènes de surface/génétique , Simulation numérique , ADN complémentaire/immunologie , Femelle , Glomérulonéphrite extra-membraneuse/complications , Cellules HEK293 , Humains , Mâle , Protéines membranaires/génétique , Souris , Adulte d'âge moyen , Protéinurie/étiologie , Lapins , Thrombospondines/métabolismeRÉSUMÉ
High-throughput immune repertoire sequencing is promising to lead to new statistical diagnostic tools for medicine and biology. Successful implementations of these methods require a correct characterization, analysis, and interpretation of these data sets. We present IGoR (Inference and Generation Of Repertoires)-a comprehensive tool that takes B or T cell receptor sequence reads and quantitatively characterizes the statistics of receptor generation from both cDNA and gDNA. It probabilistically annotates sequences and its modular structure can be used to investigate models of increasing biological complexity for different organisms. For B cells, IGoR returns the hypermutation statistics, which we use to reveal co-localization of hypermutations along the sequence. We demonstrate that IGoR outperforms existing tools in accuracy and estimate the sample sizes needed for reliable repertoire characterization.
Sujet(s)
Lymphocytes B/immunologie , Récepteurs pour l'antigène des lymphocytes B/génétique , Récepteurs aux antigènes des cellules T/génétique , Logiciel , Lymphocytes T/immunologie , Recombinaison V(D)J , Lymphocytes B/cytologie , Séquence nucléotidique , Référenciation , ADN complémentaire/génétique , ADN complémentaire/immunologie , Expression des gènes , Séquençage nucléotidique à haut débit , Humains , Immunité innée , Annotation de séquence moléculaire , Récepteurs pour l'antigène des lymphocytes B/immunologie , Récepteurs aux antigènes des cellules T/immunologie , Lymphocytes T/cytologieRÉSUMÉ
We describe novel plasmid DNA that encodes the full-length Japanese encephalitis virus (JEV) genomic cDNA and launches live-attenuated JEV vaccine in vitro and in vivo. The synthetic cDNA based on the sequence of JEV SA14-14-2 live-attenuated virus was placed under transcriptional control of the cytomegalovirus major immediate-early promoter. The stability and yields of the plasmid in E. coli were optimized by inserting three synthetic introns that disrupted JEV cDNA in the structural and nonstructural genes. Transfection of Vero cells with the resulting plasmid resulted in the replication of JEV vaccine virus with intron sequences removed from viral RNA. Furthermore, a single-dose vaccination of BALB/c mice with 0.5 - 5µg of plasmid resulted in successful seroconversion and elicitation of JEV virus-neutralizing serum antibodies. The results demonstrate the possibility of using DNA vaccination to launch live-attenuated JEV vaccine and support further development of DNA-launched live-attenuated vaccine for prevention of JEV infections.
Sujet(s)
Anticorps neutralisants/immunologie , Anticorps antiviraux/immunologie , ADN complémentaire/immunologie , Virus de l'encéphalite japonaise (espèce)/génétique , Plasmides/génétique , Animaux , ADN complémentaire/génétique , Encéphalite japonaise/prévention et contrôle , Souris , Souris de lignée BALB C , Vaccins à ADN/immunologie , Vaccins antiviraux/immunologie , Réplication viraleRÉSUMÉ
CD28 is the major costimulatory receptor on T cells regulating proliferation, survival and effector function. Acquired mutations in the extracellular domain of CD28 have been identified in patients with cutaneous T cell lymphoma, angioimmunoblastic T cell lymphoma and other T cell neoplasms, suggesting it may contribute to disease pathogenesis. We used a heterologous system in which mutant human CD28 was expressed on primary murine T cells deficient in CD28 to ascertain how specific mutations identified in a genetic screen of patients with cutaneous T cell lymphoma affected normal T cell function. All three mutant CD28 proteins examined enhanced CD28-dependent T cell proliferation and effector function. These data suggest that the mutant CD28 isoforms could accelerate tumor cell growth and increase tumor burden in affected patients. Interruption of CD28:ligand interactions may be an effective, targeted therapy for a subset of patients whose tumors bear the mutant CD28 receptor.
Sujet(s)
Antigène CD28/génétique , Antigène CTLA-4/génétique , Lymphome T cutané/génétique , Mutation , Lymphocytes T/immunologie , Séquence d'acides aminés , Animaux , Antigène CD28/immunologie , Antigène CTLA-4/immunologie , Prolifération cellulaire , Survie cellulaire , ADN complémentaire/génétique , ADN complémentaire/immunologie , Expression des gènes , Humains , Activation des lymphocytes , Lymphome T cutané/immunologie , Lymphome T cutané/anatomopathologie , Souris , Souris de lignée BALB C , Souris knockout , Protéines chimériques mutantes/génétique , Protéines chimériques mutantes/immunologie , Culture de cellules primaires , Lymphocytes T/anatomopathologie , Transfection , TransgènesRÉSUMÉ
To develop safe vaccines for inducing mucosal immunity to major pulmonary bacterial infections, appropriate vaccine antigens (Ags), delivery systems and nontoxic molecular adjuvants must be considered. Such vaccine constructs can induce Ag-specific immune responses that protect against mucosal infections. In particular, it has been shown that simply mixing the adjuvant with the bacterial Ag is a relatively easy means of constructing adjuvant-based mucosal vaccine preparations; the resulting vaccines can elicit protective immunity. DNA-based nasal adjuvants targeting mucosal DCs have been studied in order to induce Ag-specific mucosal and systemic immune responses that provide essential protection against microbial pathogens that invade mucosal surfaces. In this review, initially a plasmid encoding the cDNA of Flt3 ligand (pFL), a molecule that is a growth factor for DCs, as an effective adjuvant for mucosal immunity to pneumococcal infections, is introduced. Next, the potential of adding unmethylated CpG oligodeoxynucleotide and pFL together with a pneumococcal Ag to induce protection from pneumococcal infections is discussed. Pneumococcal surface protein A has been used as vaccine for restoring mucosal immunity in older persons. Further, our nasal pFL adjuvant system with phosphorylcholine-keyhole limpet hemocyanin (PC-KLH) has also been used in pneumococcal vaccine development to induce complete protection from nasal carriage by Streptococcus pneumoniae. Finally, the possibility that anti-PC antibodies induced by nasal delivery of pFL plus PC-KLH may play a protective role in prevention of atherogenesis and thus block subsequent development of cardiovascular disease is discussed.
Sujet(s)
Adjuvants immunologiques/administration et posologie , Cellules dendritiques/immunologie , Immunité muqueuse/immunologie , Infections à pneumocoques/prévention et contrôle , Vaccins antipneumococciques/immunologie , Streptococcus pneumoniae/génétique , Streptococcus pneumoniae/immunologie , Vaccins à ADN/immunologie , Administration par voie nasale , Animaux , Anticorps antibactériens/immunologie , Antigènes bactériens/administration et posologie , Antigènes bactériens/génétique , Antigènes bactériens/immunologie , Protéines bactériennes/administration et posologie , Protéines bactériennes/immunologie , ADN complémentaire/immunologie , Hémocyanine/administration et posologie , Hémocyanine/immunologie , Humains , Protéines membranaires/génétique , Protéines membranaires/immunologie , Oligodésoxyribonucléotides/administration et posologie , Oligodésoxyribonucléotides/immunologie , Phosphoryl-choline/administration et posologie , Phosphoryl-choline/immunologie , Vaccins antipneumococciques/administration et posologie , Vaccins à ADN/administration et posologieRÉSUMÉ
BACKGROUND: CD20-based targeting of B-cells in hematologic malignancies and autoimmune disorders is associated with outstanding clinical outcomes. Isolation and characterization of VH and VL cDNAs encoding the variable regions of the heavy and light chains of monoclonal antibodies (MAb) is necessary to produce next generation MAbs and their derivatives such as bispecific antibodies (bsAb) and single-chain variable fragments (scFv). OBJECTIVE: This study was aimed at cloning and characterization of the VH and VL cDNAs from a hybridoma cell line producing an anti-CD20 MAb. METHODS: VH and VL fragments were amplified, cloned and characterized. Furthermore, amino acid sequences of VH, VL and corresponding complementarity-determining regions (CDR) were determined and compared with those of four approved MAbs including Rituximab (RTX), Ibritumomab tiuxetan, Ofatumumab and GA101. RESULTS: The cloned VH and VL cDNAs were found to be functional and follow a consensus pattern. Amino acid sequences corresponding to the VH and VL fragments also indicated noticeable homologies to those of RTX and Ibritumomab. Furthermore, amino acid sequences of the relating CDRs had remarkable similarities to their counterparts in RTX and Ibritumomab. CONCLUSIONS: Successful recovery of VH and VL fragments encourages the development of novel CD20 targeting bsAbs, scFvs, antibody conjugates and T-cells armed with chimeric antigen receptors.
Sujet(s)
Clonage moléculaire/méthodes , Régions déterminant la complémentarité/génétique , ADN complémentaire/immunologie , Chaines lourdes des immunoglobulines/génétique , Chaines légères des immunoglobulines/génétique , Séquence d'acides aminés , Animaux , Anticorps monoclonaux/composition chimique , Anticorps monoclonaux/génétique , Anticorps monoclonaux/métabolisme , Anticorps monoclonaux humanisés/composition chimique , Anticorps monoclonaux humanisés/génétique , Anticorps monoclonaux humanisés/métabolisme , Antigènes CD20/génétique , Antigènes CD20/immunologie , Lymphocytes B/cytologie , Lymphocytes B/immunologie , Séquence nucléotidique , Lignée cellulaire , Régions déterminant la complémentarité/composition chimique , Régions déterminant la complémentarité/métabolisme , ADN complémentaire/composition chimique , ADN complémentaire/génétique , Escherichia coli/génétique , Escherichia coli/métabolisme , Expression des gènes , Vecteurs génétiques/composition chimique , Vecteurs génétiques/métabolisme , Humains , Hybridomes/cytologie , Hybridomes/immunologie , Chaines lourdes des immunoglobulines/métabolisme , Chaines légères des immunoglobulines/métabolisme , Souris , Protéines recombinantes/composition chimique , Protéines recombinantes/génétique , Protéines recombinantes/métabolisme , Rituximab/composition chimique , Rituximab/génétique , Rituximab/métabolisme , Alignement de séquences , Similitude de séquences d'acides aminésRÉSUMÉ
BACKGROUND: The assignment of human leukocyte antigen (HLA) null alleles is clinically relevant in the setting of stem cell transplantation. Cell surface expression profiling and mRNA processing analysis of the HLA-B allele previously designated as B*07:44, have been performed. MATERIALS AND METHODS: Cell surface expression of HLA-B*07:44 was determined using flow cytometry. Genomic full-length and HLA-B*07-specific cDNA sequencing were carried out by Sanger procedure. RESULTS: Flow cytometric analysis confirmed previous serologic results and demonstrated a lack of cell membrane expression of the HLA-B protein. The mRNA processing, studied using direct HLA-B*07-specific cDNA sequencing, revealed the presence of a unique, aberrantly spliced mRNA, with a deletion of the last 43 bp on the 5'-end of exon 4. The substitution from T to G at genomic position 1799 compared to B*07:02:01 introduced a new and stronger splice donor site at exon 4. This alternative splicing produced an mRNA containing a premature stop codon at position 280, explaining the absence of mature HLA-B7 protein on the cell surface. CONCLUSION: These findings led us to consider this HLA-B variant as a HLA null allele. The World Health Organization (WHO) Nomenclature Committee has since renamed this variant B*07:44N .
Sujet(s)
Épissage alternatif , Séquence nucléotidique , Antigène HLA-B7/génétique , ARN messager/génétique , Délétion de séquence , Allèles , Transplantation de moelle osseuse , Clonage moléculaire , Codon stop , ADN complémentaire/génétique , ADN complémentaire/immunologie , Exons , Cytométrie en flux , Antigène HLA-B7/immunologie , Humains , ARN messager/immunologie , Alignement de séquences , Analyse de séquence d'ADN , Terminologie comme sujet , Donneurs de tissusRÉSUMÉ
The Toll pathway is one of the most important signaling pathways regulating insect innate immunity. Spatzle is a key protein that functions as a Toll receptor ligand to trigger Toll-dependent expression of immunity-related genes. In this study, a novel spatzle gene (ApSPZ) from the Chinese oak silkworm Antheraea pernyi was identified. The ApSPZ cDNA is 1065 nucleotides with an open reading frame (ORF) of 777 bp encoding a protein of 258 amino acids. The protein has an estimated molecular weight of 29.71 kDa and an isoelectric point (PI) of 8.53. ApSPZ is a nuclear and secretory protein with no conserved domains or membrane helices and shares 40% amino acid identity with SPZ from Manduca sexta. Phylogenetic analysis indicated that ApSPZ might be a new member of the Spatzle type 1 family, which belongs to the Spatzle superfamily. The expression patterns of several genes involved in the Toll pathway were examined at different developmental stages and various tissues in 5th instar larvae. The examined targets included A. pernyi spatzle, GNBP, MyD88, Tolloid, cactus and dorsalA. The RT-PCR results showed that these genes were predominantly expressed in immune-responsive fat body tissue, indicating that the genes play a crucial role in A. pernyi innate immunity. Moreover, A. pernyi infection with the fungus Nosema pernyi and the gram-positive bacterium Enterococcus pernyi, but not the gram-negative bacterium Escherichia coli, activated the Toll signaling pathway. These results represent the first study of the Toll pathway in A. pernyi, which provides insight into the A. pernyi innate immune system.
Sujet(s)
Protéines d'insecte/génétique , Larve/génétique , Papillons de nuit/génétique , Protéines nucléaires/génétique , Cadres ouverts de lecture/immunologie , Transduction du signal/immunologie , Séquence d'acides aminés , Animaux , Séquence nucléotidique , Protéines de transport/génétique , Protéines de transport/immunologie , Clonage moléculaire , ADN complémentaire/génétique , ADN complémentaire/immunologie , Enterococcus/pathogénicité , Enterococcus/physiologie , Corps gras/immunologie , Corps gras/microbiologie , Régulation de l'expression des gènes au cours du développement , Immunité innée , Protéines d'insecte/immunologie , Point isoélectrique , Larve/immunologie , Larve/microbiologie , Manduca/génétique , Manduca/immunologie , Manduca/microbiologie , Masse moléculaire , Papillons de nuit/immunologie , Papillons de nuit/microbiologie , Facteur de différenciation myéloïde-88/génétique , Facteur de différenciation myéloïde-88/immunologie , Nosema/pathogénicité , Nosema/physiologie , Protéines nucléaires/immunologie , Phosphoprotéines/génétique , Phosphoprotéines/immunologie , Alignement de séquences , Transduction du signal/génétique , Récepteurs de type Toll/génétique , Récepteurs de type Toll/immunologie , Tolloid-Like Metalloproteinases/génétique , Tolloid-Like Metalloproteinases/immunologie , Facteurs de transcription/génétique , Facteurs de transcription/immunologieRÉSUMÉ
Myeloid differentiation protein 2 (MD2) regulates bacterial lipopolysaccharide (LPS) triggered anti-bacterial immune response as a broker between LPS and Toll-like receptor 4 (TLR4). In this study, we identified a novel naturally occurring spliceosome of human MD2, termed as MD2-T3. This transcript lacked two exons of MD2 gene. By protein structure analysis and literature review, we predicted that MD2-T3 isoform might execute regulatory biological effects such as limiting LPS-triggered TLR4 signaling.
Sujet(s)
Épissage alternatif , Antigène lymphocytaire-96/génétique , Monocytes/immunologie , ARN messager/génétique , Transcription génétique , Séquence d'acides aminés , Séquence nucléotidique , Lignée cellulaire , Clonage moléculaire , ADN complémentaire/génétique , ADN complémentaire/immunologie , Escherichia coli/génétique , Escherichia coli/métabolisme , Cellules HeLa , Humains , Lipopolysaccharides/pharmacologie , Antigène lymphocytaire-96/immunologie , Monocytes/cytologie , Monocytes/effets des médicaments et des substances chimiques , Cadres ouverts de lecture , Isoformes de protéines/génétique , Isoformes de protéines/immunologie , Structure secondaire des protéines , ARN messager/immunologie , Protéines recombinantes/génétique , Protéines recombinantes/immunologie , Transduction du signal , Splicéosomes/génétique , Splicéosomes/immunologie , Récepteur de type Toll-4/génétique , Récepteur de type Toll-4/immunologieRÉSUMÉ
A full-length infectious cDNA clone of the genome of a foot-and-mouth disease virus isolated from the 2010 epidemic in Japan was constructed and designated pSVL-f02. Transfection of Cos-7 or IBRS-2 cells with this clone allowed the recovery of infectious virus. The recovered virus had the same in vitro characterization as the parental virus with regard to antigenicity in neutralization and indirect immunofluorescence tests, plaque size and one-step growth. Pigs were experimentally infected with the parental virus or the recombinant virus recovered from pSVL-f02 transfected cells. There were no significant differences in clinical signs or antibody responses between the two groups, and virus isolation and viral RNA detection from clinical samples were similar. Virus recovered from transfected cells therefore retained the in vitro characteristics and the in vivo pathogenicity of their parental strain. This cDNA clone should be a valuable tool to analyze determinants of pathogenicity and mechanisms of virus replication, and to develop genetically engineered vaccines against foot-and-mouth disease virus.
