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Absence of protein G-Fc interaction in ficin-derived mouse IgG1 digests.

Journal of immunoassay & immunochemistry (2003-09-05)
Alexander S Belenky, Elzbieta Wask-Rotter, Michael J Sommer
RESUMEN

Typical procedure for IgG fragmentation is based on proteolytic cleavage at the hinge region and usually involves a post-digestion purification step. In mice, IgG1 has been found to bind poorly to protein A. As a result, protein G chromatography could be considered as an alternative for Fc removal. Protein G is generally expected to bind specifically to the Fc region of IgG, but applying protein G for the purification of Fab2 fragment of mouse monoclonal IgG1 under standard physiological conditions, we obtained reproducible clone-independent negligible protein G-Fc reactivity and strong protein G-Fab2 interaction.

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Sigma-Aldrich
Ficin from fig tree latex, lyophilized powder
Sigma-Aldrich
Ficin from fig tree latex, powder, ≥0.1 unit/mg solid
Sigma-Aldrich
Ficin from fig tree latex, saline suspension, ≥1.0 units/mg protein (biuret)