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Applications for an engineered Protein-G variant with a pH controllable affinity to antibody fragments.

J Immunol Methods.. 2014-10; 
LJ Bailey, KM Sheehy, RJ Hoey, ZP Schaefer, M Ura, A A Kossiakoff. Department of Biochemistry and Molecular Biology, University of Chicago, Chicago, IL, 60637, USA.
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摘要

Immunoglobulin binding proteins (IBPs) are broadly used as reagents for the purification and detection of antibodies. Among the IBPs, the most widely used are Protein-A and Protein-G. The C2 domain of Protein-G from Streptococcus is a multi-specific protein domain; it possesses a high affinity (KD ~ 10 nM) for the Fc region of the IgG, but a much lower affinity (KD ~ low μM) for the constant domain of the antibody fragment (Fab), which limits some of its applications. Here, we describe the engineering of the Protein-G interface using phage display to create Protein-G-A1, a variant with 8 point mutations and an approximately 100-fold improved affinity over the parent domain for the 4D5 Fab scaffold. Protein-G... More

关键词

Immunoglobulin binding protein; Antibody fragment purification; Protein-G; Affinity reagent; Affinity maturation; Phage display
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