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Journal article

Pitfalls to avoid when using phage display for snake toxins

In Toxicon 2017, Volume 126, pp. 79-89
From

Network Engineering of Eukaryotic Cell factories, Section for Synthetic Biology, Department of Biotechnology and Biomedicine, Technical University of Denmark1

Department of Biotechnology and Biomedicine, Technical University of Denmark2

University of Costa Rica3

University of Copenhagen4

Antivenoms against bites and stings from snakes, spiders, and scorpions are associated with immunological side effects and high cost of production, since these therapies are still derived from the serum of hyper-immunized production animals. Biotechnological innovations within envenoming therapies are thus warranted, and phage display technology may be a promising avenue for bringing antivenoms into the modern era of biologics.

Although phage display technology represents a robust and high-throughput approach for the discovery of antibody-based antitoxins, several pitfalls may present themselves when animal toxins are used as targets for phage display selection. Here, we report selected critical challenges from our own phage display experiments associated with biotinylation of antigens, clone picking, and the presence of amber codons within antibody fragment structures in some phage display libraries.

These challenges may be detrimental to the outcome of phage display experiments, and we aim to help other researchers avoiding these pitfalls by presenting their solutions.

Language: English
Year: 2017
Pages: 79-89
ISSN: 18793150 , 00410101 and 01905368
Types: Journal article
DOI: 10.1016/j.toxicon.2016.12.010
ORCIDs: 0000-0003-2419-6469 , 0000-0003-0479-8980 , Laustsen, Andreas Hougaard and Andersen, Mikael Rørdam

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