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A Protein-Engineered, Enhanced Yeast Display Platform for Rapid Evolution of Challenging Targets

J. Zahradník, D. Dey, S. Marciano, L. Kolářová, CI. Charendoff, A. Subtil, G. Schreiber

Zahradník, Jiří
Author Zahradník, Jiří Weizmann Institute of Science, Herzl St. 234, Rehovot 7610001, Israel
Dey, Debabrata
Author Dey, Debabrata Weizmann Institute of Science, Herzl St. 234, Rehovot 7610001, Israel
Marciano, Shir
Author Marciano, Shir Weizmann Institute of Science, Herzl St. 234, Rehovot 7610001, Israel
Kolářová, Lucie
Author Kolářová, Lucie Institute of Biotechnology, CAS v.v.i., Prumyslova 595, Vestec 252 50 Prague region, Czech Republic
Charendoff, Chloé I
Author Charendoff, Chloé I Institut Pasteur, Unité de Biologie cellulaire de l'infection microbienne, 25 rue du Dr Roux, Paris 75015, France
Subtil, Agathe
Author Subtil, Agathe Institut Pasteur, Unité de Biologie cellulaire de l'infection microbienne, 25 rue du Dr Roux, Paris 75015, France
Schreiber, Gideon
Author Schreiber, Gideon ORCID Weizmann Institute of Science, Herzl St. 234, Rehovot 7610001, Israel

ACS synthetic biology. 2021 ; 10 (12) : 3445-3460. [pub] 20211122

ACS synth. biol.
ISSN 2161-5063
Medvik
Source

Language English Country United States

Document type Journal Article, Research Support, Non-U.S. Gov't

Persistent link https://www.medvik.cz/link/bmc22019599

PubMed 34809429
DOI 10.1021/acssynbio.1c00395
Knihovny.cz E-resources

MeSH
Protein Engineering * methods MeSH
Proteins metabolism MeSH
Saccharomyces cerevisiae * genetics metabolism MeSH
Protein Transport MeSH
Publication type
Journal Article MeSH
Research Support, Non-U.S. Gov't MeSH

Here, we enhanced the popular yeast display method by multiple rounds of DNA and protein engineering. We introduced surface exposure-tailored reporters, eUnaG2 and DnbALFA, creating a new platform of C and N terminal fusion vectors. The optimization of eUnaG2 resulted in five times brighter fluorescence and 10 °C increased thermostability than UnaG. The optimized DnbALFA has 10-fold the level of expression of the starting protein. Following this, different plasmids were developed to create a complex platform allowing a broad range of protein expression organizations and labeling strategies. Our platform showed up to five times better separation between nonexpressing and expressing cells compared with traditional pCTcon2 and c-myc labeling, allowing for fewer rounds of selection and achieving higher binding affinities. Testing 16 different proteins, the enhanced system showed consistently stronger expression signals over c-myc labeling. In addition to gains in simplicity, speed, and cost-effectiveness, new applications were introduced to monitor protein surface exposure and protein retention in the secretion pathway that enabled successful protein engineering of hard-to-express proteins. As an example, we show how we optimized the WD40 domain of the ATG16L1 protein for yeast surface and soluble bacterial expression, starting from a nonexpressing protein. As a second example, we show how using the here-presented enhanced yeast display method we rapidly selected high-affinity binders toward two protein targets, demonstrating the simplicity of generating new protein-protein interactions. While the methodological changes are incremental, it results in a qualitative enhancement in the applicability of yeast display for many applications.

Institut Pasteur Unité de Biologie cellulaire de l'infection microbienne 25 rue du Dr Roux Paris 75015 France

Institute of Biotechnology CAS v v i Prumyslova 595 Vestec 252 50 Prague region Czech Republic

Weizmann Institute of Science Herzl St 234 Rehovot 7610001 Israel

References provided by Crossref.org

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520 9_: $a Here, we enhanced the popular yeast display method by multiple rounds of DNA and protein engineering. We introduced surface exposure-tailored reporters, eUnaG2 and DnbALFA, creating a new platform of C and N terminal fusion vectors. The optimization of eUnaG2 resulted in five times brighter fluorescence and 10 °C increased thermostability than UnaG. The optimized DnbALFA has 10-fold the level of expression of the starting protein. Following this, different plasmids were developed to create a complex platform allowing a broad range of protein expression organizations and labeling strategies. Our platform showed up to five times better separation between nonexpressing and expressing cells compared with traditional pCTcon2 and c-myc labeling, allowing for fewer rounds of selection and achieving higher binding affinities. Testing 16 different proteins, the enhanced system showed consistently stronger expression signals over c-myc labeling. In addition to gains in simplicity, speed, and cost-effectiveness, new applications were introduced to monitor protein surface exposure and protein retention in the secretion pathway that enabled successful protein engineering of hard-to-express proteins. As an example, we show how we optimized the WD40 domain of the ATG16L1 protein for yeast surface and soluble bacterial expression, starting from a nonexpressing protein. As a second example, we show how using the here-presented enhanced yeast display method we rapidly selected high-affinity binders toward two protein targets, demonstrating the simplicity of generating new protein-protein interactions. While the methodological changes are incremental, it results in a qualitative enhancement in the applicability of yeast display for many applications.

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