A study in glycation of a therapeutic recombinant humanized monoclonal antibody: Where it is, how it got there, and how it affects charge-based behavior

糖基化 化学 色谱法 亲和层析 重组DNA 单克隆抗体 阿玛多利重排 糖基化 抗体 质谱法 赖氨酸 生物化学 氨基酸 受体 免疫学 基因 生物
作者
Cynthia Quan,Emily W. Alcala,Irena Petkovska,Domenic Matthews,Eleanor Canova‐Davis,Ron Taticek,Stacey Ma
出处
期刊:Analytical Biochemistry [Elsevier]
卷期号:373 (2): 179-191 被引量:194
标识
DOI:10.1016/j.ab.2007.09.027
摘要

The glycated form of a basic recombinant humanized monoclonal antibody (rhuMAb) was separated and quantitated by boronate affinity chromatography using optimized shielding reagents. Characterization on the isolated glycated material by peptide mapping analysis, using liquid chromatography–mass spectrometry (LC–MS) and tandem mass spectrometry (MS/MS) sequencing techniques, identified eight reactive lysine primary amine sites. The glycation reaction extent was similar among the various reactive sites, ranging from approximately 1 to 12%, and a single histidine residue separated the most and least reactive sites. Boronate chromatography run in a linear gradient mode separated monoglycated rhuMAb from higher order glycated species and indicated that the majority (∼ 90%) of glycated rhuMAb is monoglycated. Low-level glycation on a heavy chain lysine located within a complementarity-determining region (CDR) did not significantly affect binding activity in potency measurements. The glycated forms also behaved as slightly more acidic than the nonglycated antibody in charge-based separation techniques, observable by capillary isoelectric focusing (cIEF) and ion exchange chromatography (IEC). The boronate column has significantly increased retention of aggregated rhuMAb material under separation conditions optimized for the monomer form. Recombinant protein glycation initially occurred during production in mammalian cell culture, where feed sugar and protein concentrations contribute to the total overall glycation on this antibody product.
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