Your search keyword '"I Barna-Vetro"' showing total 16 results

1. Simultaneous non-instrumental detection of aflatoxin B1 and ochratoxin A using a clean-up tandem immunoassay column

Author

I Barna-Vetro, Irina Yu. Goryacheva, Marieke Lobeau, Sarah De Saeger, Barbara Delmulle, Sergei A. Eremin, and Carlos Van Peteghem

Subjects

Ochratoxin A, Spectrometry, Mass, Electrospray Ionization, Analyte, Aflatoxin, Aflatoxin B1, Chromatography, medicine.diagnostic_test, Tandem, Chemistry, Enzyme-Linked Immunosorbent Assay, Ochratoxins, Sensitivity and Specificity, Biochemistry, Chromatography, Affinity, Analytical Chemistry, Sepharose, chemistry.chemical_compound, Tandem Mass Spectrometry, Immunoassay, medicine, Environmental Chemistry, Sample preparation, Spices, Ochratoxin, Spectroscopy

Abstract

A set-up and simple method based on the clean-up tandem immunoassay approach was developed for the visual detection of two analytes. The method was based on a 1 mL column with one clean-up layer and two detection immunolayers. As detection immunolayers CNBr-activated Sepharose 4B with coupled secondary rabbit anti-mouse antibodies was used. Different specific antibodies were coupled to each detection immunolayer. The analysis was realised in a competitive ELISA format with visual detection of the developed colour for each detection immunolayer and took 20 min for six sample extracts. The described method was applied to the simultaneous detection of aflatoxin B1 and ochratoxin A in spices with cut-off levels at 5 and 10 μg kg −1 , respectively. Results were confirmed by LC–MS/MS with immunoaffinity column clean-up.

Published

2007

2. Application and validation of a clean-up tandem assay column for screening ochratoxin A in cocoa powder

Author

Liberty Sibanda, Marieke Lobeau, I Barna-Vetro, Carlos Van Peteghem, Sarah De Saeger, Ghent University, Faculty of Pharmaceutical Sciences, Laboratory of Food Analysis, Universiteit Gent = Ghent University [Belgium] (UGENT), TOXI-TEST NV, and Agricultural Biotechnology Center, Diagnostic Laboratory

Subjects

Ochratoxin A, Screening test, Health, Toxicology and Mutagenesis, Food Contamination, Toxicology, 01 natural sciences, Beverages, 03 medical and health sciences, chemistry.chemical_compound, Tandem Mass Spectrometry, medicine, False Positive Reactions, Mycotoxin, False Negative Reactions, Ochratoxin, Chromatography, High Pressure Liquid, Cacao, 0303 health sciences, Chromatography, Tandem, medicine.diagnostic_test, 030306 microbiology, Chemistry, 010401 analytical chemistry, Public Health, Environmental and Occupational Health, Life Sciences, food and beverages, General Chemistry, Mycotoxins, Ochratoxins, 0104 chemical sciences, Clean-up, Visual detection, Chemistry (miscellaneous), Immunoassay, Carcinogens, Food Science

Abstract

A rapid antibody-based assay for the detection of ochratoxin A in cocoa powder is described, involving sequential clean-up and visual detection of the toxin ("clean-up tandem assay column"). The screening test was developed to have a cut-off level of 2 microg kg(-1) and was shown to have false positive and false negative rates of 10 and 2%, respectively. Analysis of six samples can be carried out in the field in approximately 30 min by untrained workers. Using the proposed rapid screening test, 10 retail cocoa powders were found to contain no detectable levels of ochratoxin A (2 microg kg(-1)). These samples were also found to be negative (2 microg kg(-1)) when analysed using an LC-MS/MS method.

Published

2007

3. Approach for ochratoxin A fast screening in spices using clean-up tandem immunoassay columns with confirmation by high performance liquid chromatography–tandem mass spectrometry (HPLC–MS/MS)

Author

I Barna-Vetro, Marieke Lobeau, S. De Saeger, Sergei A. Eremin, I.Yu. Goryacheva, and C. Van Peteghem

Subjects

Ochratoxin A, Chromatography, medicine.diagnostic_test, biology, Chemistry, Extraction (chemistry), food and beverages, Nutmeg, Tandem mass spectrometry, biology.organism_classification, Biochemistry, High-performance liquid chromatography, Analytical Chemistry, chemistry.chemical_compound, Immunoassay, Pepper, medicine, Environmental Chemistry, Sample preparation, Spectroscopy

Abstract

An approach for ochratoxin A (OTA) fast cost-effective screening based on clean-up tandem immunoassay columns was developed and optimized for OTA detection with a cut-off level of 10 microg kg(-1) in spices. Two procedures were tested and applied for OTA detection. Column with bottom detection immunolayer was optimized for OTA determination in Capsicum ssp. spices. A modified clean-up tandem immunoassay procedure with top detection immunolayer was successfully applied for all tested spices. Its main advantages were decreasing of the number of analysis steps and quantity of antibody and also minimizing of matrix effects. The total duration of the extraction and analysis was about 40 min for six samples. Chilli, red pepper, pili-pili, cayenne, paprika, nutmeg, ginger, white pepper and black pepper samples were analyzed for OTA contamination by the proposed clean-up tandem immunoassay procedures. Clean-up tandem immunoassay results were confirmed by HPLC-MS/MS with immunoaffinity column clean-up. Among 17 tested Capsicum ssp. spices, 6 samples (35%) contained OTA in a concentration exceeding the 10 microg kg(-1) limit discussed by the European Commission. All tested nutmeg (n=8), ginger (n=5), white pepper (n=7) and black pepper (n=6) samples did not contain OTA above this action level.

Published

2006

4. Novel developments in rapid mycotoxin detection

Author

Marieke Lobeau, C. Van Peteghem, S. De Saeger, I Barna-Vetro, C. Paepens, Barbara Delmulle, and Liberty Sibanda

Subjects

Screening techniques, chemistry.chemical_compound, Chromatography, Chemistry, technology, industry, and agriculture, food and beverages, Toxicology, Mycotoxin, Microbiology, Biotechnology

Abstract

Rapid antibody-based mycotoxin screening techniques are designed to be used outside a laboratory environment, at the place of sampling. Results are expected immediately, so that commodities can be further processed without delay. Because they are used for mycotoxin analysis, very low levels (ppb and ppt range) should be detected. A further requirement is that the obtained results are accurate with a false negative rate of5% at the level of interest.At first, plastic microtiter plates were used as solid phase materials for immobilizing antibodies (enzyme-linked immunosorbent assays). However, to increase speed and user-friendliness, plastics were replaced by microporous membranes. As an example a flow-through enzyme immunoassay for the detection of fumonisins in cornflakes with a cut-off value of 275 μg/kg is described. No false negative results were observed and the false positive rate was 18%. However, enzyme labels, used to enable visual evaluation of results, did not seem to be completely satisfactory in terms of stability and repeatability of the generated signal. Therefore microparticle labels such as colloidal gold particles are used more and more,e.g. in a lateral flow dipstick immunoassay. When applied to the detection of aflatoxin B1 in pig feed a cut-off value of 5 μg/kg could be reached with no false negative results and a false positive rate of only 10%. Sample pretreatment for screening techniques should be rapid and simple. Preferably a simple solvent extraction is used, followed by a filtration and dilution step. However, for strongly coloured or complex food matrices, this did not seem to work. The combination of clean-up and detection in one single test device is a new approach. When using this clean-up tandem assay column for the detection of ochratoxin A in roasted coffee, a cut-off value of 6 μg/kg was reached. No false positive results were obtained, however, the false negative rate was 8%.

Published

2006

5. Development of a new clean-up tandem assay column for the detection of ochratoxin A in roasted coffee

Author

Marieke Lobeau, Liberty Sibanda, I Barna-Vetro, C. Van Peteghem, and S. De Saeger

Subjects

Ochratoxin A, Analyte, Chromatography, medicine.diagnostic_test, Color reaction, food and beverages, Contamination, Biochemistry, Analytical Chemistry, Clean-up, chemistry.chemical_compound, chemistry, Immunoassay, medicine, Environmental Chemistry, Mycotoxin, Ochratoxin, Spectroscopy

Abstract

As the mycotoxin ochratoxin A (OTA) can occur in roasted coffee, regulations and maximum limits are necessary. The need for simple, rapid and inexpensive detection methods which require a minimum of equipment led to the development of a clean-up tandem assay column for the detection of OTA in roasted coffee. In this study the column comprised two superposed layers: a layer capable of adsorbing at least part of the interfering fraction of the sample and a detection layer containing antibodies that were able to capture the analyte. No expensive instruments were needed as results were visually evaluated. The cut-off level, i.e. the smallest mycotoxin concentration resulting in no colour development, was 6 μg kg−1. Assay validation was performed using samples fortified with OTA. The method gave a low percentage of false negative results and no false positive results. Assay performance was evaluated by screening naturally contaminated samples using the clean-up tandem assay column. The described method offers a rapid, simple and cost-effective screening tool, contributing to more effective quality control procedures.

Published

2005

6. Development of an Immunoassay-Based Lateral Flow Dipstick for the Rapid Detection of Aflatoxin B1 in Pig Feed

Author

Carlos Van Peteghem, Liberty Sibanda, Barbara Delmulle, I Barna-Vetro, and Sarah De Saeger

Subjects

Immunoassay, Aflatoxin, Analyte, Aflatoxin B1, Chromatography, medicine.diagnostic_test, Swine, Chemistry, Reproducibility of Results, General Chemistry, Dipstick, Animal Feed, Matrix (chemical analysis), Colloidal gold, Reagent, Solvents, medicine, Animals, General Agricultural and Biological Sciences, Reagent Strips, Conjugate

Abstract

The aim of this work was to develop an immunoassay-based lateral flow dipstick for the rapid detection of aflatoxin B(1) in pig feed. The test consisted of three main components: conjugate pad, membrane, and absorbent pad. The membrane was coated with two capture reagents, that is, aflatoxin B(1)-bovine serum albumin conjugate and rabbit anti-mouse antibodies. The detector reagent consisted of colloidal gold particles coated with affinity-purified monoclonal anti-aflatoxin B(1) antibodies, which saturated the conjugate pad. A comparison of several extraction methods for the pig feed matrix is presented. A mixture of methanol/water (80:20, v/v) gave the best recoveries. After sample extraction and dilution, the dipstick was put in the sample solution at the conjugate pad side and developed for 10 min. Analyte present in the sample competed with the aflatoxin B(1) immobilized on the membrane for binding to the limited amount of antibodies in the detector reagent. Thus, the line color intensity of an aflatoxin B(1)-positive dipstick is visually distinguishable from that of an aflatoxin B(1)-negative sample. The visual detection limit for aflatoxin B(1) is 5 microg/kg. The major advantages of this one-step striptest are that results can be obtained within 10 min and that all reagents are immobilized on the lateral flow dipstick.

Published

2005

7. A flow-through enzyme immunoassay for the screening of fumonisins in maize

Author

S. De Saeger, Liberty Sibanda, C. Van Peteghem, I. Léglise, F. Van Hove, I Barna-Vetro, and C. Paepens

Subjects

Detection limit, Chromatography, medicine.diagnostic_test, Chemistry, Coefficient of variation, Color reaction, Contamination, Biochemistry, High-performance liquid chromatography, Analytical Chemistry, chemistry.chemical_compound, Immunoassay, Fumonisin, medicine, Environmental Chemistry, Mycotoxin, Spectroscopy

Abstract

The format of an existing flow-through enzyme immunoassay has been optimised for the detection of fumonisin B-1 (FB1) and B-2 (FB2) in maize. The visual detection limit i.e. the smallest mycotoxin concentration resulting in no colour development, is 1000 mug/kg. Assay validation was performed using samples spiked with respectively only FBI and a FB1 + FB2 mixture (ratio 1:1). Results showed that within-day and between-day coefficients of variation ranged from respectively 0.4-10.2% and 1.1-9.0%. Naturally contaminated samples were screened with the developed flow-through method and results were compared with fumonisin contamination values obtained by a validated HPLC method. The assay was demonstrated to be accurate and reliable giving no false compliant and only a low percentage of false non-compliant results. The described method offers a simple, rapid and cost-effective screening tool, thus contributing to a better consumers' health protection. (C) 2004 Elsevier B.V. All rights reserved.

Published

2004

8. Glycoprotein B of Aujeszky's disease virus: topographical epitope mapping and epitope-specific antibody response

Author

Istvan Fodor, A Gyöngyösi-Horvath, B Siklodi, O S Morenkov, I Barna-Vetro, and M M Zaripov

Subjects

Swine, medicine.drug_class, Blotting, Western, Immunology, Pseudorabies, Enzyme-Linked Immunosorbent Assay, Antibodies, Viral, Monoclonal antibody, Epitope, Immunoenzyme Techniques, Mice, Viral Envelope Proteins, Antigen, Antibody Specificity, Neutralization Tests, Glycoprotein complex, Virology, medicine, Animals, Antigens, Viral, Swine Diseases, biology, Immunodominant Epitopes, Immunogenicity, Antibodies, Monoclonal, biology.organism_classification, Herpesvirus 1, Suid, Precipitin Tests, Molecular biology, Epitope mapping, biology.protein, Antibody, Epitope Mapping

Abstract

A panel of 26 monoclonal antibodies (mAbs) against glycoprotein B (gB) of Aujeszky's disease (pseudorabies) virus (ADV), a glycoprotein complex consisting of three glycoproteins, gBa, gBb, and gBc, was produced by two research groups and was used for the topographical epitope mapping of gB. An epitope map was constructed in which the identified epitopes of gB were situated in 14 topologically distinct antigenic domains; ten antigenic domains represented by 22 mAbs were localized on gBc, while four antigenic domains represented by four mAbs resided on gBb of the gB complex. All the epitopes located on gBc appeared to be conformation-dependent, whereas all the epitopes on gBb were conformation-independent. The identified epitopes of gB were conserved among laboratory, vaccine and field ADV strains. Conformation-dependent epitopes were shown to contribute largely to the overall antibody response to gB in naturally infected swine and immunized mice. Moreover, it was found that most of the infected animals responded relatively weakly to the identified conformation-independent epitopes of gB, while a group of immunodominant epitopes that induced a strong antibody response was represented exclusively by conformation-dependent epitopes from different antigenic domains. The results clearly demonstrated that conformation-dependent epitopes of gBc play a crucial role in inducing the humoral immune response to gB of ADV during the natural infection of swine and immunization of mice. The application of mAbs of our panel as research and diagnostic tools is discussed.

Published

1998

9. Evaluation of fumonisin contamination in cornflakes on the Belgian market by 'flow-through' assay screening and LC-MS/MS analyses

Author

Yvan Larondelle, Carlos Van Peteghem, M Anselme, Liberty Sibanda, I Barna-Vetro, C. Paepens, and Sarah De Saeger

Subjects

Screening test, Food Handling, Enzyme immunoassay method, Analytical chemistry, Organic production, Agriculture, Food Contamination, General Chemistry, Contamination, Fumonisins, Zea mays, Mass Spectrometry, Immunoenzyme Techniques, chemistry.chemical_compound, Animal science, chemistry, Belgium, Fumonisin, Lc ms ms, Food, Organic, General Agricultural and Biological Sciences, Analysis method, Chromatography, Liquid

Abstract

A total of 205 cornflake samples collected in Belgian retail stores during 2003-2004 were surveyed for the natural occurrence of fumonisin B1 (FB1), B2 (FB2), and B3 (FB3). These cornflake samples, originating from conventional as well as from organic production, were analyzed using an intralaboratory-validated LC-MS/MS method. Additionally, 90 cornflake samples were subjected to rapid screening using a flow-through enzyme immunoassay method to demonstrate the practicability of a screening test coupled to a validated confirmatory LC-MS/MS method for the management of food safety risks. FB(1) concentrations ranged from not detected (nd) [LOD (FB1) = 20 microg/kg] to 464 microg/kg with mean and median concentrations of respectively 104 +/- 113 and 54 microg/kg. For FB2 and FB3, the concentration ranges varied respectively from nd [LOD (FB2) = 7.5 microg/kg] to 43 microg/kg and from nd [LOD (FB3) = 12.5 microg/kg] to 90 microg/kg. Mean concentrations for FB2 and FB3 were respectively 12 +/- 8 and 21 +/- 15 microg/kg, while the median concentration was 11 microg/kg for FB2 and 19 microg/kg for FB3. From the statistical tests (chi2 and ANOVA model III), it could be concluded that the agricultural practice did not have any significant effect on the fumonisin concentrations but that the variation between different batches was significant (p0.0001).

Published

2005

10. Clinical and pathological effects of the dermonecrotic toxin of Bordetella bronchiseptica and Pasteurella multocida in specific-pathogen-free piglets

Author

L Papp, P. Gergely, B. Éliás, P. Rafai, I. Barna Vetro, G Boros, E Molnar, M. Albert, and s. Tuboly

Subjects

medicine.medical_specialty, Pathology, Bordetella, Swine, animal diseases, Bacterial Toxins, Biology, Turbinates, Weight Gain, Microbiology, Pathogenesis, Necrosis, otorhinolaryngologic diseases, medicine, Animals, Pasteurella multocida, Specific-pathogen-free, Swine Diseases, Bordetella bronchiseptica, Osteoid, Stomach, Muscles, Rhinitis, Atrophic, General Medicine, respiratory system, biology.organism_classification, Specific Pathogen-Free Organisms, Microscopy, Electron, Nasal Mucosa, Lymphatic system, medicine.anatomical_structure, Animals, Newborn, Thigh, Microscopy, Electron, Scanning, Histopathology, Pasteurella

Abstract

The role of dermonecrotic toxin (DNT) of Bordetella bronchiseptica and Pasteurella multocida, purified by repeated chromatography in Sephacryl S-200 gel, in the pathogenesis of atrophic rhinitis (AR) of swine was studied bacteriologically, clinically and pathologically. Two-week-old specific pathogen-free (SPF) piglets were parenterally treated with 30 micrograms of DNT 3 times at 2-day interval and 7-week-old piglets were treated with 15 micrograms of DNT twice a week for 5 weeks. In 2- to 3-week-old piglets, both B. bronchiseptica DNT and P. multocida DNT produced nasal turbinate lesions with similar severity, characterized by damage of the cilia, epithelial metaplasia, intensive proliferation of osteoblasts, regressive changes, and diffuse osteocytic osteolysis. In 7- to 12-week-old piglets, treatment with B. bronchiseptica DNT failed to produce progressive changes in the nasal turbinates. Histopathological examination revealed osteogenic processes and osteoid synthesis besides the proliferation of osteoblasts and mild osteocytic osteolysis. Moreover, severe gross pathological lesions developed in the stomach, liver, kidneys, and lymphoid organs. The piglets' appetite and body weight gain gradually decreased during the DNT treatment and in the last week when the toxic signs appeared. Treatment of 7- to 12-week-old piglets with P. multocida DNT resulted in progressive AR. Histopathologically, diffuse osteocytic osteolysis was observed in the nasal turbinates. Neither clinical signs nor pathological lesions of the visceral organs developed in these piglets. The authors emphasize that the DNT of B. bronchiseptica basically differs from that of P. multocida in biological properties, though there are certain similarities between the DNTs.

Published

1990

11. USE OF PEROXIDASE LABELLED ANTIBODIES FOR DETECTION OF PLUM POX VIRUS

Author

R. Varro, I. Barna-Vetro, V. Schuster, and B. Gyorgy

Subjects

biology, biology.protein, Pox virus, Horticulture, Antibody, Virology, Peroxidase

Published

1981

12. Novel developments in rapid mycotoxin detection.

Author

De Saeger S, Sibanda L, Paepens C, Lobeau M, Delmulle B, Barna-Vetro I, and Van Peteghem C

Abstract

Rapid antibody-based mycotoxin screening techniques are designed to be used outside a laboratory environment, at the place of sampling. Results are expected immediately, so that commodities can be further processed without delay. Because they are used for mycotoxin analysis, very low levels (ppb and ppt range) should be detected. A further requirement is that the obtained results are accurate with a false negative rate of <5% at the level of interest.At first, plastic microtiter plates were used as solid phase materials for immobilizing antibodies (enzyme-linked immunosorbent assays). However, to increase speed and user-friendliness, plastics were replaced by microporous membranes. As an example a flow-through enzyme immunoassay for the detection of fumonisins in cornflakes with a cut-off value of 275 μg/kg is described. No false negative results were observed and the false positive rate was 18%. However, enzyme labels, used to enable visual evaluation of results, did not seem to be completely satisfactory in terms of stability and repeatability of the generated signal. Therefore microparticle labels such as colloidal gold particles are used more and more,e.g. in a lateral flow dipstick immunoassay. When applied to the detection of aflatoxin B1 in pig feed a cut-off value of 5 μg/kg could be reached with no false negative results and a false positive rate of only 10%. Sample pretreatment for screening techniques should be rapid and simple. Preferably a simple solvent extraction is used, followed by a filtration and dilution step. However, for strongly coloured or complex food matrices, this did not seem to work. The combination of clean-up and detection in one single test device is a new approach. When using this clean-up tandem assay column for the detection of ochratoxin A in roasted coffee, a cut-off value of 6 μg/kg was reached. No false positive results were obtained, however, the false negative rate was 8%.

Published

2006

13. Development of an immunoassay-based lateral flow dipstick for the rapid detection of aflatoxin B1 in pig feed.

Author

Delmulle BS, De Saeger SM, Sibanda L, Barna-Vetro I, and Van Peteghem CH

Subjects

Animals, Reproducibility of Results, Solvents, Aflatoxin B1 analysis, Animal Feed analysis, Immunoassay methods, Reagent Strips, Swine

Abstract

The aim of this work was to develop an immunoassay-based lateral flow dipstick for the rapid detection of aflatoxin B(1) in pig feed. The test consisted of three main components: conjugate pad, membrane, and absorbent pad. The membrane was coated with two capture reagents, that is, aflatoxin B(1)-bovine serum albumin conjugate and rabbit anti-mouse antibodies. The detector reagent consisted of colloidal gold particles coated with affinity-purified monoclonal anti-aflatoxin B(1) antibodies, which saturated the conjugate pad. A comparison of several extraction methods for the pig feed matrix is presented. A mixture of methanol/water (80:20, v/v) gave the best recoveries. After sample extraction and dilution, the dipstick was put in the sample solution at the conjugate pad side and developed for 10 min. Analyte present in the sample competed with the aflatoxin B(1) immobilized on the membrane for binding to the limited amount of antibodies in the detector reagent. Thus, the line color intensity of an aflatoxin B(1)-positive dipstick is visually distinguishable from that of an aflatoxin B(1)-negative sample. The visual detection limit for aflatoxin B(1) is 5 microg/kg. The major advantages of this one-step striptest are that results can be obtained within 10 min and that all reagents are immobilized on the lateral flow dipstick.

Published

2005

14. Development of a solid-phase cleanup and portable rapid flow-through enzyme immunoassay for the detection of ochratoxin a in roasted coffee.

Author

Sibanda L, De Saeger S, Barna-Vetro I, and Van Peteghem C

Subjects

Chromatography, High Pressure Liquid, False Positive Reactions, Sodium Bicarbonate, Solvents, Coffea chemistry, Hot Temperature, Immunoenzyme Techniques methods, Ochratoxins analysis, Seeds chemistry

Abstract

A membrane-based flow-through enzyme immunoassay (patent application pending) for the detection of ochratoxin A (OA) in roasted coffee was developed. First, an extraction and solid-phase cleanup method was developed. A high partition coefficient for OA in the mobile phase was achieved by using methanol/5% aqueous NaHCO(3) as the sample extraction and cleanup solvent. The solid-phase (aminopropyl) cleanup was developed to chromatographically elute OA but retain cross-reacting compounds. Without using aminopropyl cleanup, cross-reacting compounds resulted in 100% false positives for both flow-through enzyme immunoassay and HPLC methods. However, after cleanup with aminopropyl, no false positives were observed. The flow-through results were visually evaluated. The sensitivity achieved for the flow-through was 4 microg kg(-1) in spiked roasted coffee. The assay was used to screen roasted coffee samples. Results were confirmed with HPLC with a detection limit of 1 microg kg(-1).

Published

2002

15. Glycoprotein B of Aujeszky's disease virus: topographical epitope mapping and epitope-specific antibody response.

Author

Zaripov MM, Morenkov OS, Siklodi B, Barna-Vetro I, Gyöngyösi-Horvath A, and Fodor I

Subjects

Animals, Antibodies, Monoclonal biosynthesis, Antibodies, Monoclonal immunology, Antibody Specificity, Blotting, Western, Enzyme-Linked Immunosorbent Assay, Immunodominant Epitopes immunology, Immunoenzyme Techniques, Mice, Neutralization Tests, Precipitin Tests, Swine, Antibodies, Viral biosynthesis, Antigens, Viral immunology, Epitope Mapping, Herpesvirus 1, Suid immunology, Pseudorabies immunology, Swine Diseases immunology, Viral Envelope Proteins immunology

Abstract

A panel of 26 monoclonal antibodies (mAbs) against glycoprotein B (gB) of Aujeszky's disease (pseudorabies) virus (ADV), a glycoprotein complex consisting of three glycoproteins, gBa, gBb, and gBc, was produced by two research groups and was used for the topographical epitope mapping of gB. An epitope map was constructed in which the identified epitopes of gB were situated in 14 topologically distinct antigenic domains; ten antigenic domains represented by 22 mAbs were localized on gBc, while four antigenic domains represented by four mAbs resided on gBb of the gB complex. All the epitopes located on gBc appeared to be conformation-dependent, whereas all the epitopes on gBb were conformation-independent. The identified epitopes of gB were conserved among laboratory, vaccine and field ADV strains. Conformation-dependent epitopes were shown to contribute largely to the overall antibody response to gB in naturally infected swine and immunized mice. Moreover, it was found that most of the infected animals responded relatively weakly to the identified conformation-independent epitopes of gB, while a group of immunodominant epitopes that induced a strong antibody response was represented exclusively by conformation-dependent epitopes from different antigenic domains. The results clearly demonstrated that conformation-dependent epitopes of gBc play a crucial role in inducing the humoral immune response to gB of ADV during the natural infection of swine and immunization of mice. The application of mAbs of our panel as research and diagnostic tools is discussed.

Published

1998

16. In vitro neutralization of T-2 toxin toxicity by a monoclonal antibody.

Author

Minervini F, Gyongyosi-Horvath A, Lucivero G, Visconti A, Barna-Vetro I, and Solti L

Subjects

Animals, Antibody Specificity, Cells, Cultured, Enzyme-Linked Immunosorbent Assay, Female, Humans, Immunoglobulin G, Lymphocytes drug effects, Mice, Neutralization Tests, T-2 Toxin immunology, T-2 Toxin toxicity, Trichothecenes pharmacology, Antibodies, Monoclonal pharmacology, T-2 Toxin antagonists & inhibitors

Abstract

A T-2 toxin specific monoclonal antibody, IgG1 K, with a low level of ELISA cross-reactivity to Acetyl T-2, HT-2, and iso T-2 toxins has been produced. The ability of this monoclonal antibody to neutralize the cytotoxicity of T-2 toxin in PHA stimulated cultures of human lymphocytes was determined by the MTT method. The complete neutralization of the toxic effect of 0.02 microM T-2 toxin was obtained with 0.03 microM of MoAb, whereas the 50% neutralizing dose (ND50) was observed at 0.009 microM of MoAb. Partial neutralization was observed with Acetyl T-2 toxin (ND50 = 0.038 microM) and HT-2 (ND50 = 0.94 microM). These results could represent a rational for clinical use of T-2 toxin specific monoclonal antibody in prophylaxis and therapy of T-2 toxemia.

Published

1994