Literature DB >> 19637390

Development of a high throughput protein a well-plate purification method for monoclonal antibodies.

Jennifer Hopp1, Ross Pritchett, Maria Darlucio, Junfen Ma, Judy H Chou.   

Abstract

We have developed a new high throughput method for the purification of monoclonal antibodies from harvested cell culture fluid for analytical characterization. This method uses Protein A resin in a 96 well-plate format with protein loading sufficient to perform multiple analyses per well. Resin and buffer conditions were optimized to obtain aggregate and charge variant comparability with three preparative Protein A purified monoclonal antibodies. We are able to successfully demonstrate comparability for aggregate within 0.25% based upon size-exclusion chromatography. Acidic species were found to be within 2% from the preparative purified control based upon cation-exchange chromatography, 5% based upon capillary zone electrophoresis, and 3% based upon imaged capillary isoelectric focusing. Glycan distribution was analyzed and was within 1% of the preparative purified controls. A tryptic digest was performed and all peaks in the preparative purified control were found in the first elution from the well-plate format. 2009 American Institute of Chemical Engineers Biotechnol.

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Year:  2009        PMID: 19637390     DOI: 10.1002/btpr.247

Source DB:  PubMed          Journal:  Biotechnol Prog        ISSN: 1520-6033


  2 in total

1.  Advanced microscale bioreactor system: a representative scale-down model for bench-top bioreactors.

Authors:  Wei-Ting Hsu; Rigzen P S Aulakh; Donald L Traul; Inn H Yuk
Journal:  Cytotechnology       Date:  2012-03-27       Impact factor: 2.058

2.  Cross-interaction chromatography: a rapid method to identify highly soluble monoclonal antibody candidates.

Authors:  Steven A Jacobs; Sheng-Jiun Wu; Yiqing Feng; Deidra Bethea; Karyn T O'Neil
Journal:  Pharm Res       Date:  2009-11-13       Impact factor: 4.200

  2 in total

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