DNA Display of Biologically Active Proteins for In Vitro Protein Selection

Masato Yonezawa; Nobuhide Doi; Toru Higashinakagawa; Hiroshi Yanagawa

doi:10.1093/jb/mvh034

DNA Display of Biologically Active Proteins for In Vitro Protein Selection

Masato Yonezawa, Nobuhide Doi, Toru Higashinakagawa, Hiroshi Yanagawa

Department of Biosciences and Informatics

Research output: Contribution to journal › Article › peer-review

31 Citations (Scopus)

Abstract

In vitro display technologies are powerful tools for screening peptides with desired functions. We previously proposed a DNA display system in which streptavidin-fused peptides are linked with their encoding DNAs via biotin labels in emulsion compartments and successfully applied it to the screening of random peptide libraries. Here we describe its application to functional and folded proteins. By introducing peptide linkers between streptavidin and fused proteins, we achieved highly efficient (>95%) formation of DNA-protein conjugates. Furthermore, we successfully enriched a glutathione-S-transferase gene by a factor of 20-30-fold per round on glutathione-coupled beads. Thus, DNA display should be useful for rapidly screening or evolving proteins based on affinity selection.

Original language	English
Pages (from-to)	285-288
Number of pages	4
Journal	Journal of biochemistry
Volume	135
Issue number	3
DOIs	https://doi.org/10.1093/jb/mvh034
Publication status	Published - 2004 Mar

Keywords

Biotin
DNA display
In vitro translation
Protein engineering
Streptavidin

ASJC Scopus subject areas

Medicine(all)

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10.1093/jb/mvh034

Cite this

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title = "DNA Display of Biologically Active Proteins for In Vitro Protein Selection",

abstract = "In vitro display technologies are powerful tools for screening peptides with desired functions. We previously proposed a DNA display system in which streptavidin-fused peptides are linked with their encoding DNAs via biotin labels in emulsion compartments and successfully applied it to the screening of random peptide libraries. Here we describe its application to functional and folded proteins. By introducing peptide linkers between streptavidin and fused proteins, we achieved highly efficient (>95%) formation of DNA-protein conjugates. Furthermore, we successfully enriched a glutathione-S-transferase gene by a factor of 20-30-fold per round on glutathione-coupled beads. Thus, DNA display should be useful for rapidly screening or evolving proteins based on affinity selection.",

keywords = "Biotin, DNA display, In vitro translation, Protein engineering, Streptavidin",

author = "Masato Yonezawa and Nobuhide Doi and Toru Higashinakagawa and Hiroshi Yanagawa",

note = "Funding Information: We thank N. Matsumura, H. Takashima and Y. Oishi for the discussions, experimental advice and plasmids, respectively. The plasmid carrying Rae28/Mph1 cDNA was a gift from K. Shimada. This work was supported in part by the Special Coordination Fund of the Ministry of Education, Science and Technology of Japan.",

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AU - Yonezawa, Masato

AU - Doi, Nobuhide

AU - Higashinakagawa, Toru

AU - Yanagawa, Hiroshi

N1 - Funding Information: We thank N. Matsumura, H. Takashima and Y. Oishi for the discussions, experimental advice and plasmids, respectively. The plasmid carrying Rae28/Mph1 cDNA was a gift from K. Shimada. This work was supported in part by the Special Coordination Fund of the Ministry of Education, Science and Technology of Japan.

PY - 2004/3

Y1 - 2004/3

N2 - In vitro display technologies are powerful tools for screening peptides with desired functions. We previously proposed a DNA display system in which streptavidin-fused peptides are linked with their encoding DNAs via biotin labels in emulsion compartments and successfully applied it to the screening of random peptide libraries. Here we describe its application to functional and folded proteins. By introducing peptide linkers between streptavidin and fused proteins, we achieved highly efficient (>95%) formation of DNA-protein conjugates. Furthermore, we successfully enriched a glutathione-S-transferase gene by a factor of 20-30-fold per round on glutathione-coupled beads. Thus, DNA display should be useful for rapidly screening or evolving proteins based on affinity selection.

AB - In vitro display technologies are powerful tools for screening peptides with desired functions. We previously proposed a DNA display system in which streptavidin-fused peptides are linked with their encoding DNAs via biotin labels in emulsion compartments and successfully applied it to the screening of random peptide libraries. Here we describe its application to functional and folded proteins. By introducing peptide linkers between streptavidin and fused proteins, we achieved highly efficient (>95%) formation of DNA-protein conjugates. Furthermore, we successfully enriched a glutathione-S-transferase gene by a factor of 20-30-fold per round on glutathione-coupled beads. Thus, DNA display should be useful for rapidly screening or evolving proteins based on affinity selection.

KW - Biotin

KW - DNA display

KW - In vitro translation

KW - Protein engineering

KW - Streptavidin

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DNA Display of Biologically Active Proteins for In Vitro Protein Selection

Abstract

Keywords

ASJC Scopus subject areas

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