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Integrating SpyCatcher/SpyTag covalent fusion technology into phage display workflows for rapid antibody discovery.

Sci Rep. 2019; 
Fierle Julie K,Abram-Saliba Johan,Brioschi Matteo,deTiani Mariastella,Coukos George,Dunn Stev
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Mammalian Expression System Ligands were diluted to 2 μg/ml in PBST+1% BSA and incubated for 1h at RT. Afer washing, bound Fc-fusions and bound Muc16 were detected with goat anti-human IgG Fc polyclonal HRP conjugate (Sino Biologicals, #SSA001; 1:5000 dilution) or anti-His tag HRP conjugate (Genscript, #A00612; 1:1000 dilution) using TMB as substrate. Get A Quote

摘要

An early bottleneck in the rapid isolation of new antibody fragment binders using in vitro library approaches is the inertia encountered in acquiring and preparing soluble antigen fragments. In this report, we describe a simple, yet powerful strategy that exploits the properties of the SpyCatcher/SpyTag (SpyC/SpyT) covalent interaction to improve substantially the speed and efficiency in obtaining functional antibody clones of interest. We demonstrate that SpyC has broad utility as a protein-fusion tag partner in a eukaryotic expression/secretion context, retaining its functionality and permitting the direct, selective capture and immobilization of soluble antigen fusions using solid phase media coated ... More

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