Issue 58, 2016

Monoclonal antibody capture from cell culture supernatants using epitope imprinted macroporous membranes

Abstract

Epitope-imprinted membranes targeting the C-terminal fragment of the immunoglobuline G (IgG) heavy chain was developed and used for the purification of a commercial monoclonal antibody. The membranes exhibited strongly enhanced IgG affinity when compared with non-imprinted or IgG imprinted membranes reflected in binding selectivities in a protein mixture (IgG/HSA 1 : 10 w/w) of up to 40, and the elution of 95 to 100% pure IgG after washing. The dynamic binding capacity amounted to 3.9 mg mL−1 membrane volume with minor loss in performance upon repeated cleaning with alkali. The depletion of host cell proteins from a cell culture broth after production of anti-IL8 antibody using the best performing imprinted membrane under low-salt conditions reached 88% (0.7–1.2 log units) implying an effective removal of impurities from the cell culture supernatant.

Graphical abstract: Monoclonal antibody capture from cell culture supernatants using epitope imprinted macroporous membranes

Article information

Article type
Paper
Submitted
12 Mar 2016
Accepted
22 May 2016
First published
24 May 2016
This article is Open Access
Creative Commons BY license

RSC Adv., 2016,6, 53162-53169

Author version available

Monoclonal antibody capture from cell culture supernatants using epitope imprinted macroporous membranes

S. Schwark, W. Sun, J. Stute, D. Lütkemeyer, M. Ulbricht and B. Sellergren, RSC Adv., 2016, 6, 53162 DOI: 10.1039/C6RA06632A

This article is licensed under a Creative Commons Attribution 3.0 Unported Licence. You can use material from this article in other publications without requesting further permissions from the RSC, provided that the correct acknowledgement is given.

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