Genetically encoded system to track histone modification in vivo

Yuko Sato; Masanori Mukai; Jun Ueda; Michiko Muraki; Timothy J. Stasevich; Naoki Horikoshi; Tomoya Kujirai; Hiroaki Kita; Taisuke Kimura; Seiji Hira; Yasushi Okada; Yoko Hayashi-Takanaka; Chikashi Obuse; Hitoshi Kurumizaka; Atsuo Kawahara; Kazuo Yamagata; Naohito Nozaki; Hiroshi Kimura

doi:10.1038/srep02436

Genetically encoded system to track histone modification in vivo

Yuko Sato, Masanori Mukai, Jun Ueda, Michiko Muraki, Timothy J. Stasevich, Naoki Horikoshi, Tomoya Kujirai, Hiroaki Kita, Taisuke Kimura, Seiji Hira, Yasushi Okada, Yoko Hayashi-Takanaka, Chikashi Obuse, Hitoshi Kurumizaka, Atsuo Kawahara, Kazuo Yamagata, Naohito Nozaki, Hiroshi Kimura^*

^*この研究の対応する著者

理工学術院総合研究所

研究成果: Article › 査読

72 被引用数 (Scopus)

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Post-translational histone modifications play key roles in gene regulation, development, and differentiation, but their dynamics in living organisms remain almost completely unknown. To address this problem, we developed a genetically encoded system for tracking histone modifications by generating fluorescent modification-specific intracellular antibodies (mintbodies) that can be expressed in vivo. To demonstrate, an H3 lysine 9 acetylation specific mintbody (H3K9ac-mintbody) was engineered and stably expressed in human cells. In good agreement with the localization of its target acetylation, H3K9ac-mintbody was enriched in euchromatin, and its kinetics measurably changed upon treatment with a histone deacetylase inhibitor. We also generated transgenic fruit fly and zebrafish stably expressing H3K9ac-mintbody for in vivo tracking. Dramatic changes in H3K9ac-mintbody localization during Drosophila embryogenesis could highlight enhanced acetylation at the start of zygotic transcription around mitotic cycle 7. Together, this work demonstrates the broad potential of mintbody and lays the foundation for epigenetic analysis in vivo.

本文言語	English
論文番号	2436
ジャーナル	Scientific Reports
巻	3
DOI	https://doi.org/10.1038/srep02436
出版ステータス	Published - 2013

ASJC Scopus subject areas

一般

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10.1038/srep02436

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Sato, Y., Mukai, M., Ueda, J., Muraki, M., Stasevich, T. J., Horikoshi, N., Kujirai, T., Kita, H., Kimura, T., Hira, S., Okada, Y., Hayashi-Takanaka, Y., Obuse, C., Kurumizaka, H., Kawahara, A., Yamagata, K., Nozaki, N., & Kimura, H. (2013). Genetically encoded system to track histone modification in vivo. Scientific Reports, 3, [2436]. https://doi.org/10.1038/srep02436

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title = "Genetically encoded system to track histone modification in vivo",

abstract = "Post-translational histone modifications play key roles in gene regulation, development, and differentiation, but their dynamics in living organisms remain almost completely unknown. To address this problem, we developed a genetically encoded system for tracking histone modifications by generating fluorescent modification-specific intracellular antibodies (mintbodies) that can be expressed in vivo. To demonstrate, an H3 lysine 9 acetylation specific mintbody (H3K9ac-mintbody) was engineered and stably expressed in human cells. In good agreement with the localization of its target acetylation, H3K9ac-mintbody was enriched in euchromatin, and its kinetics measurably changed upon treatment with a histone deacetylase inhibitor. We also generated transgenic fruit fly and zebrafish stably expressing H3K9ac-mintbody for in vivo tracking. Dramatic changes in H3K9ac-mintbody localization during Drosophila embryogenesis could highlight enhanced acetylation at the start of zygotic transcription around mitotic cycle 7. Together, this work demonstrates the broad potential of mintbody and lays the foundation for epigenetic analysis in vivo.",

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T1 - Genetically encoded system to track histone modification in vivo

AU - Sato, Yuko

AU - Mukai, Masanori

AU - Ueda, Jun

AU - Muraki, Michiko

AU - Stasevich, Timothy J.

AU - Horikoshi, Naoki

AU - Kujirai, Tomoya

AU - Kita, Hiroaki

AU - Kimura, Taisuke

AU - Hira, Seiji

AU - Okada, Yasushi

AU - Hayashi-Takanaka, Yoko

AU - Obuse, Chikashi

AU - Kurumizaka, Hitoshi

AU - Kawahara, Atsuo

AU - Yamagata, Kazuo

AU - Nozaki, Naohito

AU - Kimura, Hiroshi

PY - 2013

Y1 - 2013

N2 - Post-translational histone modifications play key roles in gene regulation, development, and differentiation, but their dynamics in living organisms remain almost completely unknown. To address this problem, we developed a genetically encoded system for tracking histone modifications by generating fluorescent modification-specific intracellular antibodies (mintbodies) that can be expressed in vivo. To demonstrate, an H3 lysine 9 acetylation specific mintbody (H3K9ac-mintbody) was engineered and stably expressed in human cells. In good agreement with the localization of its target acetylation, H3K9ac-mintbody was enriched in euchromatin, and its kinetics measurably changed upon treatment with a histone deacetylase inhibitor. We also generated transgenic fruit fly and zebrafish stably expressing H3K9ac-mintbody for in vivo tracking. Dramatic changes in H3K9ac-mintbody localization during Drosophila embryogenesis could highlight enhanced acetylation at the start of zygotic transcription around mitotic cycle 7. Together, this work demonstrates the broad potential of mintbody and lays the foundation for epigenetic analysis in vivo.

AB - Post-translational histone modifications play key roles in gene regulation, development, and differentiation, but their dynamics in living organisms remain almost completely unknown. To address this problem, we developed a genetically encoded system for tracking histone modifications by generating fluorescent modification-specific intracellular antibodies (mintbodies) that can be expressed in vivo. To demonstrate, an H3 lysine 9 acetylation specific mintbody (H3K9ac-mintbody) was engineered and stably expressed in human cells. In good agreement with the localization of its target acetylation, H3K9ac-mintbody was enriched in euchromatin, and its kinetics measurably changed upon treatment with a histone deacetylase inhibitor. We also generated transgenic fruit fly and zebrafish stably expressing H3K9ac-mintbody for in vivo tracking. Dramatic changes in H3K9ac-mintbody localization during Drosophila embryogenesis could highlight enhanced acetylation at the start of zygotic transcription around mitotic cycle 7. Together, this work demonstrates the broad potential of mintbody and lays the foundation for epigenetic analysis in vivo.

KW - Chromatin Analysis

KW - Fluorescent Proteins

KW - Histone Posttranslational

KW - Modifications

KW - Subject Areas

KW - Time-Lapse Imaging

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Genetically encoded system to track histone modification in vivo

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