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dc.contributor.authorShinoda, Koukien
dc.contributor.authorTsuji, Shogoen
dc.contributor.authorFutaki, Shirohen
dc.contributor.authorImanishi, Mikien
dc.contributor.alternative篠田, 昂樹ja
dc.contributor.alternative辻, 将吾ja
dc.contributor.alternative二木, 史朗ja
dc.contributor.alternative今西, 未来ja
dc.date.accessioned2022-07-08T02:22:54Z-
dc.date.available2022-07-08T02:22:54Z-
dc.date.issued2018-01-18-
dc.identifier.urihttp://hdl.handle.net/2433/274820-
dc.description.abstractRNA-binding proteins recognizing unique sequences within large transcriptomes serve as a powerful tool to control RNA metabolism. Pumilio and fem-3 mRNA-binding factor (PUF) proteins are considered good candidates for such tools, because they are typically composed of eight highly homologous repeat segments and can be designed to recognize arbitrary 8 nt RNA sequences. However, a specific 8 nt RNA sequence is found at multiple sites in various RNAs in the transcriptome, making it difficult to specifically target a single RNA. Designer PUF proteins recognizing longer RNA sequences should achieve more selective binding. Here, we propose an approach for creating 16-repeat PUFs capable of targeting a single, unique mRNA in the transcriptome. Our design is simple and involves either the tandem alignment of two PUF segments or the nesting of one PUF segment within another. Designed 16-repeat PUFs bound to the target RNA sequence without partial recognition derived from the original 8-repeat PUF. Furthermore, based on our strategy, expression of an endogenous mRNA was selectively and effectively modulated, demonstrating the applicability of 16-repeat PUF proteins for regulating endogenous RNA metabolism.en
dc.language.isoeng-
dc.publisherWileyen
dc.rightsThis is the peer reviewed version of the following article: [K. Shinoda, S. Tsuji, S. Futaki, M. Imanishi, ChemBioChem 2018, 19, 171.], which has been published in final form at https://doi.org/10.1002/cbic.201700458. This article may be used for non-commercial purposes in accordance with Wiley Terms and Conditions for Use of Self-Archived Versions. This article may not be enhanced, enriched or otherwise transformed into a derivative work, without express permission from Wiley or by statutory rights under applicable legislation. Copyright notices must not be removed, obscured or modified. The article must be linked to Wiley’s version of record on Wiley Online Library and any embedding, framing or otherwise making available the article or pages thereof by third parties from platforms, services and websites other than Wiley Online Library must be prohibited.en
dc.rightsThe full-text file will be made open to the public on 18 December 2018 in accordance with publisher's 'Terms and Conditions for Self-Archiving'.en
dc.rightsThis is not the published version. Please cite only the published version. この論文は出版社版でありません。引用の際には出版社版をご確認ご利用ください。en
dc.subjectGene expressionen
dc.subjectGene technologyen
dc.subjectProtein engineeringen
dc.subjectRNA recognitionen
dc.titleNested PUF Proteins: Extending Target RNA Elements for Gene Regulationen
dc.typejournal article-
dc.type.niitypeJournal Article-
dc.identifier.jtitleChemBioChemen
dc.identifier.volume19-
dc.identifier.issue2-
dc.identifier.spage171-
dc.identifier.epage176-
dc.relation.doi10.1002/cbic.201700458-
dc.textversionauthor-
dc.identifier.pmid29110405-
dcterms.accessRightsopen access-
datacite.date.available2018-12-18-
datacite.awardNumber16H03281-
datacite.awardNumber.urihttps://kaken.nii.ac.jp/grant/KAKENHI-PROJECT-16H03281/-
dc.identifier.pissn1439-4227-
dc.identifier.eissn1439-7633-
jpcoar.funderName日本学術振興会ja
jpcoar.awardTitle生細胞内での部位特異的なエピゲノム操作法の確立ja
出現コレクション:学術雑誌掲載論文等

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