ICLAMP: a novel technique to explore adenosine deamination via inosine chemical labeling and affinity molecular purification

Yuxi Yang; Koki Nakayama; Shunpei Okada; Kazuki Sato; Takeshi Wada; Yuriko Sakaguchi; Ayaka Murayama; Tsutomu Suzuki; Masayuki Sakurai

doi:10.1002/1873-3468.14854

ICLAMP: a novel technique to explore adenosine deamination via inosine chemical labeling and affinity molecular purification

Yuxi Yang, Koki Nakayama, Shunpei Okada, Kazuki Sato, Takeshi Wada, Yuriko Sakaguchi, Ayaka Murayama, Tsutomu Suzuki, Masayuki Sakurai

研究成果: Article › 査読

抄録

Recent developments in sequencing and bioinformatics have advanced our understanding of adenosine-to-inosine (A-to-I) RNA editing. Surprisingly, recent analyses have revealed the capability of adenosine deaminase acting on RNA (ADAR) to edit DNA:RNA hybrid strands. However, edited inosines in DNA remain largely unexplored. A precise biochemical method could help uncover these potentially rare DNA editing sites. We explore maleimide as a scaffold for inosine labeling. With fluorophore-conjugated maleimide, we were able to label inosine in RNA or DNA. Moreover, with biotin-conjugated maleimide, we purified RNA and DNA containing inosine. Our novel technique of inosine chemical labeling and affinity molecular purification offers substantial advantages and provides a versatile platform for further discovery of A-to-I editing sites in RNA and DNA.

本文言語	English
ページ（範囲）	1080-1093
ページ数	14
ジャーナル	FEBS Letters
巻	598
号	9
DOI	https://doi.org/10.1002/1873-3468.14854
出版ステータス	Published - 5月 2024

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10.1002/1873-3468.14854

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title = "ICLAMP: a novel technique to explore adenosine deamination via inosine chemical labeling and affinity molecular purification",

abstract = "Recent developments in sequencing and bioinformatics have advanced our understanding of adenosine-to-inosine (A-to-I) RNA editing. Surprisingly, recent analyses have revealed the capability of adenosine deaminase acting on RNA (ADAR) to edit DNA:RNA hybrid strands. However, edited inosines in DNA remain largely unexplored. A precise biochemical method could help uncover these potentially rare DNA editing sites. We explore maleimide as a scaffold for inosine labeling. With fluorophore-conjugated maleimide, we were able to label inosine in RNA or DNA. Moreover, with biotin-conjugated maleimide, we purified RNA and DNA containing inosine. Our novel technique of inosine chemical labeling and affinity molecular purification offers substantial advantages and provides a versatile platform for further discovery of A-to-I editing sites in RNA and DNA.",

keywords = "A-to-I RNA editing, adenosine deamination, chemical labeling, inosine, maleimide",

author = "Yuxi Yang and Koki Nakayama and Shunpei Okada and Kazuki Sato and Takeshi Wada and Yuriko Sakaguchi and Ayaka Murayama and Tsutomu Suzuki and Masayuki Sakurai",

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AU - Yang, Yuxi

AU - Nakayama, Koki

AU - Okada, Shunpei

AU - Sato, Kazuki

AU - Wada, Takeshi

AU - Sakaguchi, Yuriko

AU - Murayama, Ayaka

AU - Suzuki, Tsutomu

AU - Sakurai, Masayuki

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AB - Recent developments in sequencing and bioinformatics have advanced our understanding of adenosine-to-inosine (A-to-I) RNA editing. Surprisingly, recent analyses have revealed the capability of adenosine deaminase acting on RNA (ADAR) to edit DNA:RNA hybrid strands. However, edited inosines in DNA remain largely unexplored. A precise biochemical method could help uncover these potentially rare DNA editing sites. We explore maleimide as a scaffold for inosine labeling. With fluorophore-conjugated maleimide, we were able to label inosine in RNA or DNA. Moreover, with biotin-conjugated maleimide, we purified RNA and DNA containing inosine. Our novel technique of inosine chemical labeling and affinity molecular purification offers substantial advantages and provides a versatile platform for further discovery of A-to-I editing sites in RNA and DNA.

KW - A-to-I RNA editing

KW - adenosine deamination

KW - chemical labeling

KW - inosine

KW - maleimide

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