L445P mutation on heavy chain stabilizes IgG4under acidic conditions

Autor: Xu, Chang-Ai, Feng, Andrew Z., Ramineni, Charan K., Wallace, Matthew R., Culyba, Elizabeth K., Guay, Kevin P., Mehta, Kinjal, Mabry, Robert, Farrand, Stephen, Xu, Jin, Feng, Jianwen
Zdroj: mAbs; October 2019, Vol. 11 Issue: 7 p1289-1299, 11p
Abstrakt: ABSTRACTIgG4, a common type of therapeutic antibody, is less stable during manufacturing processes compared with IgG1. Aggregation and fragmentation are the two main challenges. Here, we report instability of the heavy chain (HC) C-terminal region under acidic conditions, which leads to cleavage and aggregation. Leu445, at the C-terminal region of the HC in IgG4,plays a critical role in its acid-induced fragmentation and subsequent aggregation. We found that mutating HC C-terminal Leu445to Pro (the corresponding residue in IgG1) in IgG4_CDR-X significantly reduces fragmentation and aggregation, while mutating Pro445to Leu in IgG1_CDR-X promotes fragmentation and aggregation. HC C-terminal Gly446cleavage was observed in low pH citrate buffer and resulted in further fragmentation and aggregation, whereas, glycine buffer can completely inhibit the cleavage and aggregation. It is proposed that cleavages occur through acid-induced hydrolysis under acidic conditions and glycine stabilizes IgG4via two main mechanisms: 1) product feedback inhibition of the hydrolysis reaction, and 2) stabilization of protein conformation by direct interaction with the peptide backbone and charged side chains. Experiments using IgG4molecules IgG4_CDR-Y and IgG4_CDR-Z with the same CH domains as IgG4_CDR-X, but different complementarity-determining regions (CDRs), indicate that the stability of the HC C-terminal region is also closely related to the sequence of the CDRs. The stability of IgG4_CDR-X is significantly improved when binding to its target. Both observations suggest that there are potential interactions between Fab and CH2-CH3 domains, which could be the key factor affecting the stability of IgG antibodies.
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