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Titlebook: CRISPR Guide RNA Design; Methods and Protocol Tudor A. Fulga,David J. H. F. Knapp,Quentin R. V. Book 2021 Springer Science+Business Media,

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發(fā)表于 2025-3-21 20:05:19 | 只看該作者 |倒序瀏覽 |閱讀模式
書目名稱CRISPR Guide RNA Design
副標題Methods and Protocol
編輯Tudor A. Fulga,David J. H. F. Knapp,Quentin R. V.
視頻videohttp://file.papertrans.cn/221/220556/220556.mp4
概述Includes cutting-edge techniques.Provides step-by-step detail essential for reproducible results.Contains key implementation advice from the experts
叢書名稱Methods in Molecular Biology
圖書封面Titlebook: CRISPR Guide RNA Design; Methods and Protocol Tudor A. Fulga,David J. H. F. Knapp,Quentin R. V.  Book 2021 Springer Science+Business Media,
描述This detailed volume focuses on the CRISPR-associated guide RNA and how it can be designed, modified, and validated for a broad repertoire of purposes. Beginning with a section on computational design of target-specific guide RNAs, the book continues by covering chemical modifications to alter guide RNA stability, specificity, and efficiency, as well as to create inducible guide RNAs, append additional functional domains, and express guide RNAs in a conditional manner. It concludes with methods for measuring off-target guide RNA activity. Written for the highly successful .Methods in Molecular Biology. series, chapters include introductions to their respective topics, lists of the necessary materials and reagents, step-by-step, readily reproducible protocols, and tips on troubleshooting and avoiding known pitfalls.?.Authoritative and essential, .CRISPR Guide RNA Design: Methods and Protocols. provides a comprehensive pipeline for guide RNA design and aims to be an invaluable resource in applying this powerful technology to basic research and therapeutic applications..
出版日期Book 2021
關鍵詞CRISPR/Cas9; Guide RNA design; Inducible guide RNAs; Transcriptional activity; DNA modification; Genomic
版次1
doihttps://doi.org/10.1007/978-1-0716-0687-2
isbn_softcover978-1-0716-0689-6
isbn_ebook978-1-0716-0687-2Series ISSN 1064-3745 Series E-ISSN 1940-6029
issn_series 1064-3745
copyrightSpringer Science+Business Media, LLC, part of Springer Nature 2021
The information of publication is updating

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978-1-0716-0689-6Springer Science+Business Media, LLC, part of Springer Nature 2021
地板
發(fā)表于 2025-3-22 05:30:58 | 只看該作者
Tudor A. Fulga,David J. H. F. Knapp,Quentin R. V. Includes cutting-edge techniques.Provides step-by-step detail essential for reproducible results.Contains key implementation advice from the experts
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https://doi.org/10.1057/9780230245099onsiderations for the design of short guide (sg) RNAs include the assessment of possible off-target activities, the prediction of on-target efficacies and mutational outcome. Manual design of sgRNAs taking into account these parameters, however, remains a difficult task. Thus, computational tools to
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https://doi.org/10.1057/9780230245099ine, and gene therapy. However, CRISPR nucleases can cleave off-target sites as well as on-target sites, causing unwanted mutations. Furthermore, after CRISPR treatments are delivered into cells or organisms, it is important to estimate the resulting mutation rates and to determine the patterns of m
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The Thin Filament in Insect Flight Muscleing promise as a therapeutic for patients with genetic diseases. Multiple different CRISPR systems have been identified, each with its own target DNA recognition sequence, expanding the editable mammalian genome. It is also now appreciated that chemically modified nucleic acids can substitute for un
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The Thin Filament in Insect Flight Muscleby enzymatic reactions, however the process becomes time-consuming as the number of sgRNAs increases and does not allow the incorporation of chemical modifications that can improve or expand the functionality of CRISPR. Solid-phase RNA synthesis can overcome these issues, but highly pure full-length
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