We have performed a systematic variability study of polyclonal antibody catalysis by using five rabbits immunized with the same hapten. Important results from this work are the following. (1) Similarities were observed in the catalytic polyclonal antibodies derived from all five rabbits. Four of the five rabbits produced polyclonal samples that were nearly the same in terms of catalytic activity, whereas the fifth rabbit, designated as rabbit 2, displayed a somewhat higher level of catalytic activity. The catalytic activities (as kcat/kuncat) of these polyclonal samples were similar to that from the best murine monoclonal antibody that had been previously elicited by the same hapten. (2) Titre was not an accurate indicator of polyclonal antibody catalytic activity. (3) A mathematical analysis to describe a distribution of Michaelis–Menten catalysts was performed to help interpret our results. (4) Kinetic analysis indicated that the binding parameters of the different samples were remarkably homogeneous, because one or two components were all that were required to fit the on-rate and off-rate data satisfactorily. Interestingly, the most active catalytic polyclonal sample, that from rabbit 2, displayed the slowest off-rate (so slow it could not be measured) and thus the highest overall affinity. (5) Catalytic analysis of eluted fractions of antibody from a substrate column indicated that each polyclonal sample was also relatively homogeneous in terms of catalytic parameters. The main conclusion of our study is that for this hapten–animal system, the overall catalytic immune response is relatively consistent at two levels. Consistent catalytic activity was observed between the polyclonal samples elicited in the different animals, and the elicited hapten-specific polyclonal antibodies were relatively homogeneous in terms of binding and catalytic parameters within each immunized animal. The observed similarities of the catalytic activity in the different animals is surprising, because the immune response is based on specific binding of antibodies to hapten. There is no known selective pressure to maintain consistent levels of catalytic activity. Our results can therefore be interpreted as providing evidence that for this hapten there is a fixed relationship between hapten structure and catalytic activity and/or consistent genetic factors that dominate the catalytic immune response.
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May 1998
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Research Article|
May 15 1998
Polyclonal antibody catalytic variability Available to Purchase
David B. STEPHENS;
David B. STEPHENS
1The Department of Chemistry and Biochemistry, The University of Texas at Austin, Austin, TX 78712, U.S.A.
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Richard E. THOMAS;
Richard E. THOMAS
1The Department of Chemistry and Biochemistry, The University of Texas at Austin, Austin, TX 78712, U.S.A.
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John F. STANTON;
John F. STANTON
1The Department of Chemistry and Biochemistry, The University of Texas at Austin, Austin, TX 78712, U.S.A.
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Brent L. IVERSON
Brent L. IVERSON
1
1The Department of Chemistry and Biochemistry, The University of Texas at Austin, Austin, TX 78712, U.S.A.
1To whom correspondence should be addressed (e-mail [email protected]).
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Publisher: Portland Press Ltd
Received:
January 12 1998
Accepted:
February 11 1998
Online ISSN: 1470-8728
Print ISSN: 0264-6021
The Biochemical Society, London © 1998
1998
Biochem J (1998) 332 (1): 127–134.
Article history
Received:
January 12 1998
Accepted:
February 11 1998
Citation
David B. STEPHENS, Richard E. THOMAS, John F. STANTON, Brent L. IVERSON; Polyclonal antibody catalytic variability. Biochem J 15 May 1998; 332 (1): 127–134. doi: https://doi.org/10.1042/bj3320127
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