Epitope mapping by screening of phage display libraries of a monoclonal antibody directed against the receptor binding domain of human α2‐macroglobulin

摘要

>The human proteinase inhibitor, α2-macroglobulin (α2-M), inhibits a large number of proteinases. α2-M-proteinase complexes are rapidly cleared from the circulation by binding to a cellular receptor (α2-M-R/LRP) via the receptor binding domain (RBD) which is made up of a 20 kDa C-terminal stretch of the 180 kDa monomer of the inhibitor. A monoclonal antibody (mab α-1) has been described which reacts with the receptor-recognizable form of the inhibitor, the so called transformed α2-M (α2-Mt). By screening of a phage display library an epitope in the RBD of the inhibitor was identified that reacts with mab α-1. Out of 25 phage clones a heptapeptide sequence (S-x₁-x₂-D-x₃-x₄-K) was obtained containing identical amino acids in three positions. A consensus peptide (S-R-S-D-P-P-K) was synthesized and found to displace α2-Mt from binding to mab α-1 and to receptor. The specificity of competition was demonstrated by a reversed peptide and a control antibody. By structural comparison it was found that the consensus heptapeptide mimics a discontinuous conformationally constrained epitope present in the RBD of the inhibitor. This is the first report describing the detection of discontinuous epitopes by phage display using a short linear peptide.