Abstract

A majority of antibodies raised against p-azophenylarsonate (Ars)-protein conjugates in A/J mice share a heritable cross-reactive idiotype, as they are encoded by a single combination of variable region germline gene segments termed """"""""canonical."""""""" The dominance of the canonically-encoded structure is due to the favorable intrinsic Ars affinity of the V region germline gene combination and its ability to sustain somatic mutations conferring higher affinity leading to preferred antigen-driven selection of B cells expressing canonical V regions. The Ars systems is an important model for defining combining site structural changes occurring temporally in immune responses (affinity maturation), as functional differences among these antibodies can be related structurally by comparison to unmutated precursors. The goals of this project include: 1) To access the differentiative capacity of the germline canonical structure to generate increased affinity and to change specificity for structurally-related analogues as compared to that of a higher-affinity somatically mutated canonical antibody of known crystal structure. 2) To engineer changes in specificity and affinity ex vivo that may not be possible in vivo owing to biases inherent in the germline sequence and the somatic mutation process. A """"""""selective"""""""" approach will be used primarily, in which libraries of mutant Fabs derived from germline (unmutated) canonical anti-Ars antibodies and high-affinity (somatically mutated) canonical anti-Ars antibodies are displayed on filamentous bacteriophage and sorted by affinity, and specificity of these mutants for Ars analogues are determined and the results interpreted in the context of the crystal structures of anti-Ars Fabs. In addition to saturation mutagenesis of different CDRs, """"""""random"""""""" mutagenesis of entire V regions, combinatorial mutagenesis of CDRs and regions from both chains, as well as site-directed mutagenesis, will be carried out. Novel mutants will be crystallized and their structures determined. The feasibility of antibody combining site engineering to design antibodies with altered function, and in particular to increase specificity, is critical for the success of clinical immunotherapy.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA024432-37
Application #
2894503
Study Section
Special Emphasis Panel (ZRG2-ALY (01))
Program Officer
Mccarthy, Susan A
Project Start
1986-09-01
Project End
2001-04-30
Budget Start
1999-05-01
Budget End
2000-04-30
Support Year
37
Fiscal Year
1999
Total Cost
Indirect Cost

  Institution

Name
Massachusetts General Hospital
Department
Type
DUNS #
City
Boston
State
MA
Country
United States
Zip Code
02199

  Publications

Parhami-Seren, Behnaz; Krudysz, Jolanta; Tsantili, Panayota (2002) Affinity panning of peptide libraries using anti-streptokinase monoclonal antibodies: selection of an inhibitor of plasmin(ogen) active site. J Immunol Methods 267:185-98
Krykbaev, Rustem A; Tsantili, Panayota; Jeffrey, Philip D et al. (2002) Modifying specificity of antidigoxin antibodies using insertional mutagenesis. Protein Sci 11:2899-908
Parhami-Seren, Behnaz; Viswanathan, Malini; Margolies, Michael N (2002) Selection of high affinity p-azophenyarsonate Fabs from heavy-chain CDR2 insertion libraries. J Immunol Methods 259:43-53
Parhami-Seren, Behnaz; Haberly, Richard; Margolies, Michael N et al. (2002) Ouabain-binding protein(s) from human plasma. Hypertension 40:220-8
Parhami-Seren, B; Viswanathan, M; Strong, R K et al. (2001) Structural analysis of mutants of high-affinity and low-affinity p-azophenylarsonate-specific antibodies generated by alanine scanning of heavy chain complementarity-determining region 2. J Immunol 167:5129-35
Parhami-Seren, B; Bell, C; Margolies, M N et al. (1999) Monoclonal antibodies that distinguish between two related digitalis glycosides, ouabain and digoxin. J Immunol 163:4360-6
Wong, Y W; Gill, D S; Parhami-Seren, B et al. (1998) Structural requirements for a specificity switch and for maintenance of affinity using mutational analysis of a phage-displayed anti-arsonate antibody of Fab heavy chain first complementarity-determining region. J Immunol 160:5990-7
Parhami-Seren, B; Keel, T; Reed, G L (1997) Sequences of antigenic epitopes of streptokinase identified via random peptide libraries displayed on phage. J Mol Biol 271:333-41
Gill, D S; Wong, Y W; Margolies, M N (1997) Differences in sequence-specific expression of two anti-arsonate Fabs in E. coli. Biotechnol Prog 13:692-4
Parhami-Seren, B; Margolies, M N (1996) Contribution of heavy chain junctional amino acid diversity to antibody affinity among p-azophenylarsonate-specific antibodies. J Immunol 157:2066-72

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