Chimeric swine vesicular disease viruses produced by fusion PCR: a new method for epitope mapping

Chimeric swine vesicular disease viruses produced by fusion PCR: a new method for epitope mapping

A new method of epitope mapping based on chimeric swine vesicular disease (SVD) viruses produced by fusion PCR (polymerase chain reaction). Seven out of 16 neutralising and non-neutralising newly produced monoclonal antibodies (MAbs) discriminated between SVD isolate ITL/1/66 and NET/1/92. Using fus...

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Veröffentlicht in:Journal of virological methods 2000-05, Vol.86 (2), p.131-141
Hauptverfasser: Dekker, A, Leendertse, C.H, van Poelwijk, F, Rebel, J.M.J, Moormann, R.J.M
Format: Artikel
Sprache:eng
Schlagworte:
Animals
Antibodies, Monoclonal
Antibodies, Viral
Antibody Specificity
ANTICORPS MONOCLONAL
ANTICUERPOS MONOCLONALES
Antigens, Viral - immunology
Base Sequence
Biological and medical sciences
CHIMAERAS
CHIMERE
Chimeric virus
Enterovirus - classification
Enterovirus - genetics
Enterovirus - immunology
Enterovirus - isolation & purification
Epitope mapping
Epitope Mapping - methods
EPITOPES
Fundamental and applied biological sciences. Psychology
fusion PCR
ID Lelystad, Institute for Animal Science and Health
ID-Lelystad, Instituut voor Dierhouderij en Diergezondheid
Microbiology
Molecular Sequence Data
MONOCLONAL ANTIBODIES
Mutation
Neutralization Tests
PCR
Picornavirus
Polymerase Chain Reaction - methods
QUIMERA
Sequence Analysis, DNA
Swine
Swine vesicular disease
Swine Vesicular Disease - virology
SWINE VESICULAR DISEASE VIRUS
Techniques used in virology
Virology
VIRUS DEL MAL VESICULAR PORCINO
VIRUS MALADIE VESICULEUSE DU PORC
WIAS
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Beschreibung
Zusammenfassung:A new method of epitope mapping based on chimeric swine vesicular disease (SVD) viruses produced by fusion PCR (polymerase chain reaction). Seven out of 16 neutralising and non-neutralising newly produced monoclonal antibodies (MAbs) discriminated between SVD isolate ITL/1/66 and NET/1/92. Using fusion PCR eight chimeric viruses were produced containing different supplementary pieces of the P1 region of both parent strains. Using these chimeric viruses we were able to map the epitope regions recognised by these seven neutralising and non-neutralising Mabs. This new method, using chimeric viruses produced by fusion PCR, is particularly valuable for the epitope mapping of non-neutralising MAbs.
ISSN:0166-0934
1879-0984
DOI:10.1016/S0166-0934(00)00142-7