Mapping of two immunodominant antigenic epitopes conserved among the major inner capsid protein, VP7 of five bluetongue viruses

Joseph Kali; Yi Yuan Yang

doi:10.1016/0042-6822(90)90353-S

Mapping of two immunodominant antigenic epitopes conserved among the major inner capsid protein, VP7 of five bluetongue viruses

Joseph Kali, Yi Yuan Yang

Research output: Contribution to journal › Article › peer-review

23 Citations (Scopus)

Abstract

A combination of polyclonal, monoclonal, and oligoclonal antibodies was used in Western blot to analyze intact VP7 proteins and their proteolytic peptide fragments of five bluetongue viruses found in the United States. Two linear immunodominant antigenic determinants were located and identified on this major inner capsid protein. One of the antigenic epitopes, which consisted of 11 residues (LTRAIARAAYV), was mapped by polyclonal antibody to the carboxyl terminus of the viral protein (residues 339 through 349). The second epitope (ARQPYGFFLETEEVYQPG) was located by both monoclonal and oligoclonal antibodies and mapped between residues 122 through 139. The exact locations of these two linear and continuous epitopes were also confirmed by competition with sequence-specific synthetic peptides. These epitopes were highly conserved among the VP7 proteins of all five U.S. bluetongue viruses.

Original language	English
Pages (from-to)	552-559
Number of pages	8
Journal	Virology
Volume	178
Issue number	2
DOIs	https://doi.org/10.1016/0042-6822(90)90353-S
Publication status	Published - Oct 1990
Externally published	Yes

ASJC Scopus subject areas

Virology

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10.1016/0042-6822(90)90353-S

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title = "Mapping of two immunodominant antigenic epitopes conserved among the major inner capsid protein, VP7 of five bluetongue viruses",

abstract = "A combination of polyclonal, monoclonal, and oligoclonal antibodies was used in Western blot to analyze intact VP7 proteins and their proteolytic peptide fragments of five bluetongue viruses found in the United States. Two linear immunodominant antigenic determinants were located and identified on this major inner capsid protein. One of the antigenic epitopes, which consisted of 11 residues (LTRAIARAAYV), was mapped by polyclonal antibody to the carboxyl terminus of the viral protein (residues 339 through 349). The second epitope (ARQPYGFFLETEEVYQPG) was located by both monoclonal and oligoclonal antibodies and mapped between residues 122 through 139. The exact locations of these two linear and continuous epitopes were also confirmed by competition with sequence-specific synthetic peptides. These epitopes were highly conserved among the VP7 proteins of all five U.S. bluetongue viruses.",

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AB - A combination of polyclonal, monoclonal, and oligoclonal antibodies was used in Western blot to analyze intact VP7 proteins and their proteolytic peptide fragments of five bluetongue viruses found in the United States. Two linear immunodominant antigenic determinants were located and identified on this major inner capsid protein. One of the antigenic epitopes, which consisted of 11 residues (LTRAIARAAYV), was mapped by polyclonal antibody to the carboxyl terminus of the viral protein (residues 339 through 349). The second epitope (ARQPYGFFLETEEVYQPG) was located by both monoclonal and oligoclonal antibodies and mapped between residues 122 through 139. The exact locations of these two linear and continuous epitopes were also confirmed by competition with sequence-specific synthetic peptides. These epitopes were highly conserved among the VP7 proteins of all five U.S. bluetongue viruses.

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Mapping of two immunodominant antigenic epitopes conserved among the major inner capsid protein, VP7 of five bluetongue viruses

Abstract

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UN SDGs

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