Click display: a rapid and efficient in vitro protein display method for directed evolution

Author:

Zeng Yu1,Woolley Michael1ORCID,Chockalingam Karuppiah1,Thomas Benjamin2,Arora Srishtee3,Hook Magnus3,Chen Zhilei12ORCID

Affiliation:

1. Department of Microbial Pathogenesis and Immunology, Texas A&M University Health Science Center , Bryan , TX  77807 , USA

2. Interdisciplinary Graduate Program in Genetics and Genomics, Texas A&M University , Houston, TX 77030, USA

3. Center for Infectious and Inflammatory Diseases, Institute of Biosciences and Technology, Texas A&M University Health Science Center , Houston , TX  77030 , USA

Abstract

Abstract We describe a novel method for in vitro protein display—click display—that does not depend on maintaining RNA integrity during biopanning and yields covalently linked protein–cDNA complexes from double-stranded input DNA within 2 h. The display is achieved in a one-pot format encompassing transcription, translation and reverse transcription reactions in series. Stable linkage between proteins and the encoding cDNA is mediated by a modified DNA linker—ML—generated via a click chemistry reaction between a puromycin-containing oligo and a cDNA synthesis primer. Biopanning of a click-displayed mock library coupled with next-generation sequencing analysis revealed >600-fold enrichment of target binders within a single round of panning. A synthetic library of Designed Ankyrin Repeat Proteins (DARPins) with ∼1012 individual members was generated using click display in a 25-μl reaction and six rounds of library panning against a model protein yielded a panel of nanomolar binders. This study establishes click display as a powerful tool for protein binder discovery/engineering and provides a convenient platform for in vitro biopanning selection even in RNase-rich environments such as on whole cells.

Funder

NIH

TAMU

HSC

Publisher

Oxford University Press (OUP)

Subject

Genetics

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