AI Article Synopsis

  • A new isoform of the human monoclonal antibody panitumumab was created through in vitro aging, primarily due to isomerization of the aspartate 92 residue, which negatively affected its binding ability to EGFR.
  • The rate of isomerization was influenced by temperature and pH, with the modified antibodies showing reduced effectiveness in inhibiting EGFR-mediated cell proliferation when one or both Asp-92 residues were isomerized.
  • Both panitumumab and cetuximab demonstrated that intact antibodies with two functioning antigen-binding regions were significantly more potent in suppressing cell proliferation compared to their individual fragments, highlighting the importance of avidity in their efficacy against the human EGFR.

Article Abstract

A new isoform of the light chain of a fully human monoclonal immunoglobulin gamma2 (IgG2) antibody panitumumab against human epidermal growth factor receptor (EGFR) was generated by in vitro aging. The isoform was attributed to the isomerization of aspartate 92 located between phenylalanine 91 and histidine 93 residues in the antigen-binding region. The isomerization rate increased with increased temperature and decreased pH. A size-exclusion chromatography binding assay was used to show that one antibody molecule was able to bind two soluble extracellular EGFR molecules in solution, and isomerization of one or both Asp-92 residues deactivated one or both antigen-binding regions, respectively. In addition, isomerization of Asp-92 showed a decrease in in vitro potency as measured by a cell proliferation assay with a 32D cell line that expressed the full-length human EGFR. The data indicate that antibodies containing either one or two isomerized residues were not effective in inhibiting EGFR-mediated cell proliferation, and that two unmodified antigen binding regions were needed to achieve full efficacy. For comparison, the potency of an intact IgG1 antibody cetuximab against the same receptor was correlated with the bioactivity of its individual antigen-binding fragments. The intact IgG1 antibody with two antigen-binding fragments was also much more active in suppressing cell proliferation than the individual fragments, similar to the IgG2 results. These results indicated that avidity played a key role in the inhibition of cell proliferation by these antibodies against the human EGFR, suggesting that their mechanisms of action are similar.

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http://dx.doi.org/10.1021/bi7018223DOI Listing

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