A comprehensive search of functional sequence space using large mammalian display libraries created by gene editing
Authors: Kothai Parthiban*, Rajika L. Perera *†, Maheen Sattar, Yanchao Huang‡, Sophie Mayle § , Edward Masters,Daniel Griffiths , Sachin Surade , Rachael Leah, Michael R. Dyson , and John McCafferty

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Summary
The construction of large libraries in mammalian cells allows the direct screening of millions of molecular variants for binding properties in a cell type relevant for screening or production. We have created mammalian cell libraries of up to 10 million clones displaying a repertoire of IgG-formatted antibodies on the cell surface.
TALE nucleases or CRISPR/Cas9 were used to direct the integration of the antibody genes into a single genomic locus, thereby rapidly achieving stable expression and transcriptional normalization.
The utility of the system is illustrated by the affinity maturation of a PD-1-blockingantibody through the systematic mutation and functional survey of 4-mer variants within a 16 amino acid paratope region.
Mutating VH CDR3 only, we identified a dominant “solution” involving substitution of a central tyrosine to histidine. This appears to be a local affinity maximum, and this variant was surpassed by a lysine substitution when light chain variants were introduced.
We achieve this comprehensive and quantitative interrogation of sequence space by combining high-throughput oligonucleotide synthesis with mammalian display and flow cytometry operating at the multi-million scale.
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