Systematic epitope analysis of the p26 EIAV core protein

The major core protein of equine infectious anemia virus (EIAV), p26, is one of the primary immunogenic structural proteins during a persistent infection of horses and is highly conserved among antigenically variants of viral isolates. In order to investigate its immune profile in more detail for a...

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Veröffentlicht in:Journal of molecular recognition 2007-07, Vol.20 (4), p.227-237
Hauptverfasser: Soutullo, Adriana, Santi, María N., Perin, Juan C., Beltramini, Leila M., Borel, Ileana Malan, Frank, Ronald, Tonarelli, Georgina G.
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container_end_page 237
container_issue 4
container_start_page 227
container_title Journal of molecular recognition
container_volume 20
creator Soutullo, Adriana
Santi, María N.
Perin, Juan C.
Beltramini, Leila M.
Borel, Ileana Malan
Frank, Ronald
Tonarelli, Georgina G.
description The major core protein of equine infectious anemia virus (EIAV), p26, is one of the primary immunogenic structural proteins during a persistent infection of horses and is highly conserved among antigenically variants of viral isolates. In order to investigate its immune profile in more detail for a better diagnostic, an epitope mapping was carried out by means of two libraries of overlapping peptide fragments prepared by simultaneous and parallel SPPS on derivatized cellulose membranes (SPOT synthesis). Polyclonal equine sera from infected horses were used for the biological assay. Particularly two promising continuous epitopes (NAMRHL and MYACRD) were localized on the C‐terminal extreme of p26, region 194–222. A cyclic synthetic fragment of 29 amino acid residues containing the identified epitopes was designed and studied. A significant conformational change towards a helical structure was observed when the peptide was cyclized by a bridge between Cys198 and Cys218. This observation correlated with an improvement of its ability to be recognized by specific antibodies in an EIA (Enzyme‐linked Immunosorbent assay). These results suggest that the conformationally restricted synthetic antigen adequately mimics the native structure of this region of p26 core protein. Copyright © 2007 John Wiley & Sons, Ltd.
doi_str_mv 10.1002/jmr.825
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In order to investigate its immune profile in more detail for a better diagnostic, an epitope mapping was carried out by means of two libraries of overlapping peptide fragments prepared by simultaneous and parallel SPPS on derivatized cellulose membranes (SPOT synthesis). Polyclonal equine sera from infected horses were used for the biological assay. Particularly two promising continuous epitopes (NAMRHL and MYACRD) were localized on the C‐terminal extreme of p26, region 194–222. A cyclic synthetic fragment of 29 amino acid residues containing the identified epitopes was designed and studied. A significant conformational change towards a helical structure was observed when the peptide was cyclized by a bridge between Cys198 and Cys218. This observation correlated with an improvement of its ability to be recognized by specific antibodies in an EIA (Enzyme‐linked Immunosorbent assay). These results suggest that the conformationally restricted synthetic antigen adequately mimics the native structure of this region of p26 core protein. 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Mol. Recognit</addtitle><description>The major core protein of equine infectious anemia virus (EIAV), p26, is one of the primary immunogenic structural proteins during a persistent infection of horses and is highly conserved among antigenically variants of viral isolates. In order to investigate its immune profile in more detail for a better diagnostic, an epitope mapping was carried out by means of two libraries of overlapping peptide fragments prepared by simultaneous and parallel SPPS on derivatized cellulose membranes (SPOT synthesis). Polyclonal equine sera from infected horses were used for the biological assay. Particularly two promising continuous epitopes (NAMRHL and MYACRD) were localized on the C‐terminal extreme of p26, region 194–222. A cyclic synthetic fragment of 29 amino acid residues containing the identified epitopes was designed and studied. A significant conformational change towards a helical structure was observed when the peptide was cyclized by a bridge between Cys198 and Cys218. This observation correlated with an improvement of its ability to be recognized by specific antibodies in an EIA (Enzyme‐linked Immunosorbent assay). These results suggest that the conformationally restricted synthetic antigen adequately mimics the native structure of this region of p26 core protein. 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subjects Amino Acid Sequence
circular dichroism
conformation
ELISA
epitope analysis
Epitope Mapping - methods
equine anemia virus
Models, Molecular
molecular recognition
Molecular Sequence Data
p26 core protein
Peptide Fragments - analysis
Protein Array Analysis
Protein Structure, Secondary
Protein Structure, Tertiary
spot synthesis
Viral Core Proteins - analysis
Viral Core Proteins - chemistry
Viral Core Proteins - immunology
Viral Core Proteins - metabolism
title Systematic epitope analysis of the p26 EIAV core protein
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