Changing the Antigen Binding Specificity by Single Point Mutations of an Anti-p24 (HIV-1) Antibody

The murine mAb CB4-1 raised against p24 (HIV-1) recognizes a linear epitope of the HIV-1 capsid protein. Additionally, CB4-1 exhibits cross-reactive binding to epitope-homologous peptides and polyspecific reactions to epitope nonhomologous peptides. Crystal structures demonstrate that the epitope pe...

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Bibliographic Details
Published in:The Journal of immunology (1950) 2000-10, Vol.165 (8), p.4505-4514
Main Authors: Winkler, Karsten, Kramer, Achim, Kuttner, Gabriele, Seifert, Martina, Scholz, Christa, Wessner, Helga, Schneider-Mergener, Jens, Hohne, Wolfgang
Format: Article
Language:English
Subjects:
Alanine - genetics
Amino Acid Sequence
Amino Acid Substitution - genetics
Animals
Antibodies, Monoclonal - genetics
Antibodies, Monoclonal - metabolism
Binding Sites, Antibody - genetics
Binding, Competitive - genetics
Binding, Competitive - immunology
Cloning, Molecular
HIV Antibodies - genetics
HIV Antibodies - metabolism
HIV Core Protein p24 - immunology
HIV-1 - immunology
Human immunodeficiency virus 1
Humans
Immunoglobulin Fragments - biosynthesis
Immunoglobulin Fragments - chemistry
Immunoglobulin Fragments - genetics
Immunoglobulin Fragments - metabolism
Immunoglobulin Variable Region - biosynthesis
Immunoglobulin Variable Region - chemistry
Immunoglobulin Variable Region - genetics
Immunoglobulin Variable Region - metabolism
Mice
Molecular Sequence Data
Mutagenesis, Site-Directed
p24 protein
Peptide Fragments - genetics
Peptide Fragments - metabolism
Phenylalanine - genetics
Point Mutation - immunology
Protein Binding - genetics
Protein Binding - immunology
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Summary:The murine mAb CB4-1 raised against p24 (HIV-1) recognizes a linear epitope of the HIV-1 capsid protein. Additionally, CB4-1 exhibits cross-reactive binding to epitope-homologous peptides and polyspecific reactions to epitope nonhomologous peptides. Crystal structures demonstrate that the epitope peptide (e-pep) and the nonhomologous peptides adopt different conformations within the binding region of CB4-1. Site-directed mutagenesis of the fragment variable (Fv) region was performed using a single-chain (sc)Fv construct of CB4-1 to analyze binding contributions of single amino acid side chains toward the e-pep and toward one epitope nonhomologous peptide. The mutations of Ab amino acid side chains, which are in direct contact with the Ag, show opposite influences on the binding of the two peptides. Whereas the affinity of the e-pep to the CB4-1 scFv mutant heavy chain variable region Tyr(32)Ala is decreased 250-fold, the binding of the nonhomologous peptide remains unchanged. In contrast, the mutation light chain variable region Phe(94)Ala reduces the affinity of the nonhomologous peptide 10-fold more than it does for the e-pep. Thus, substantial changes in the specificity can be observed by single amino acid exchanges. Further characterization of the scFv mutants by substitutional analysis of the peptides demonstrates that the effect of a mutation is not restricted to contact residues. This method also reveals an inverse compensatory amino acid exchange for the nonhomologous peptide which increases the affinity to the scFv mutant light chain variable region Phe(94)Ala up to the level of the e-pep affinity to the wild-type scFv.
ISSN:0022-1767
1550-6606
DOI:10.4049/jimmunol.165.8.4505