| Literature DB >> 25548140 |
Simon Tickle1, Louise Howells2, Victoria O'Dowd2, Dale Starkie2, Kevin Whale2, Mark Saunders2, David Lee2, Daniel Lightwood2.
Abstract
For a therapeutic antibody to succeed, it must meet a range of potency, stability, and specificity criteria. Many of these characteristics are conferred by the amino acid sequence of the heavy and light chain variable regions and, for this reason, can be screened for during antibody selection. However, it is important to consider that antibodies satisfying all these criteria may be of low frequency in an immunized animal; for this reason, it is essential to have a mechanism that allows for efficient sampling of the immune repertoire. UCB's core antibody discovery platform combines high-throughput B cell culture screening and the identification and isolation of single, antigen-specific IgG-secreting B cells through a proprietary technique called the "fluorescent foci" method. Using state-of-the-art automation to facilitate primary screening, extremely efficient interrogation of the natural antibody repertoire is made possible; more than 1 billion immune B cells can now be screened to provide a useful starting point from which to identify the rare therapeutic antibody. This article will describe the design, construction, and commissioning of a bespoke automated screening platform and two examples of how it was used to screen for antibodies against two targets.Keywords: antibody; automation or robotics; database and data management; large molecule therapeutics; liquid handling
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Year: 2014 PMID: 25548140 DOI: 10.1177/1087057114564760
Source DB: PubMed Journal: J Biomol Screen ISSN: 1087-0571