In vitro selection of GTP-binding proteins by block shuffling of estrogen-receptor fragments

Toru Tsuji; Michiko Onimaru; Nobuhide Doi; Etsuko Miyamoto-Sato; Hideaki Takashima; Hiroshi Yanagawa

doi:10.1016/j.bbrc.2009.10.029

In vitro selection of GTP-binding proteins by block shuffling of estrogen-receptor fragments

Toru Tsuji, Michiko Onimaru, Nobuhide Doi, Etsuko Miyamoto-Sato, Hideaki Takashima, Hiroshi Yanagawa

生命情報学科

研究成果: Article › 査読

7 被引用数 (Scopus)

抄録

To what extent has alternative splicing contributed to the evolution of protein-function diversity? We previously constructed a pool of block-deletion mutants of the human estrogen receptor α ligand binding domain by random multi-recombinant PCR. Here we performed iterative in vitro selection of GTP-binding proteins by using the library of mRNA-displayed proteins and GTP-affinity chromatography combined with quantitative real-time PCR. We obtained a novel GTP-binding protein with moderate affinity and substrate-specificity. The results of our in vitro simulation imply that alternative splicing may have contributed substantially to the diversification of protein function during evolution.

本文言語	English
ページ（範囲）	689-693
ページ数	5
ジャーナル	Biochemical and Biophysical Research Communications
巻	390
号	3
DOI	https://doi.org/10.1016/j.bbrc.2009.10.029
出版ステータス	Published - 2009 12月 18

ASJC Scopus subject areas

生物理学
生化学
分子生物学
細胞生物学

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10.1016/j.bbrc.2009.10.029

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title = "In vitro selection of GTP-binding proteins by block shuffling of estrogen-receptor fragments",

abstract = "To what extent has alternative splicing contributed to the evolution of protein-function diversity? We previously constructed a pool of block-deletion mutants of the human estrogen receptor α ligand binding domain by random multi-recombinant PCR. Here we performed iterative in vitro selection of GTP-binding proteins by using the library of mRNA-displayed proteins and GTP-affinity chromatography combined with quantitative real-time PCR. We obtained a novel GTP-binding protein with moderate affinity and substrate-specificity. The results of our in vitro simulation imply that alternative splicing may have contributed substantially to the diversification of protein function during evolution.",

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note = "Funding Information: We thank Dr. K. Tsuge for helpful discussions. This work was supported in part by a Grant-in-Aid for Scientific Research and a Special Coordination Fund Grant from MEXT , Japan, and a Grant for Practical Application of University R&D Results under the Matching Fund Method from NEDO , Japan.",

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AU - Onimaru, Michiko

AU - Doi, Nobuhide

AU - Miyamoto-Sato, Etsuko

AU - Takashima, Hideaki

AU - Yanagawa, Hiroshi

N1 - Funding Information: We thank Dr. K. Tsuge for helpful discussions. This work was supported in part by a Grant-in-Aid for Scientific Research and a Special Coordination Fund Grant from MEXT , Japan, and a Grant for Practical Application of University R&D Results under the Matching Fund Method from NEDO , Japan.

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N2 - To what extent has alternative splicing contributed to the evolution of protein-function diversity? We previously constructed a pool of block-deletion mutants of the human estrogen receptor α ligand binding domain by random multi-recombinant PCR. Here we performed iterative in vitro selection of GTP-binding proteins by using the library of mRNA-displayed proteins and GTP-affinity chromatography combined with quantitative real-time PCR. We obtained a novel GTP-binding protein with moderate affinity and substrate-specificity. The results of our in vitro simulation imply that alternative splicing may have contributed substantially to the diversification of protein function during evolution.

AB - To what extent has alternative splicing contributed to the evolution of protein-function diversity? We previously constructed a pool of block-deletion mutants of the human estrogen receptor α ligand binding domain by random multi-recombinant PCR. Here we performed iterative in vitro selection of GTP-binding proteins by using the library of mRNA-displayed proteins and GTP-affinity chromatography combined with quantitative real-time PCR. We obtained a novel GTP-binding protein with moderate affinity and substrate-specificity. The results of our in vitro simulation imply that alternative splicing may have contributed substantially to the diversification of protein function during evolution.

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KW - Combinatorial protein library

KW - In vitro selection

KW - Protein evolution

KW - Synthetic biology

KW - mRNA display

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In vitro selection of GTP-binding proteins by block shuffling of estrogen-receptor fragments

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