ID | 116611 |
Author |
Osakabe, Keishi
Tokushima University
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Murakami, Emi
Tokushima University
Miyashita, Naoyuki
Kindai University
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Content Type |
Journal Article
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Description | Adoption of CRISPR–Cas systems, such as CRISPR–Cas9 and CRISPR–Cas12a, has revolutionized genome engineering in recent years; however, application of genome editing with CRISPR type I—the most abundant CRISPR system in bacteria—remains less developed. Type I systems, such as type I-E, and I-F, comprise the CRISPR-associated complex for antiviral defense (‘Cascade’: Cas5, Cas6, Cas7, Cas8 and the small subunit) and Cas3, which degrades the target DNA; in contrast, for the sub-type CRISPR–Cas type I-D, which lacks a typical Cas3 nuclease in its CRISPR locus, the mechanism of target DNA degradation remains unknown. Here, we found that Cas10d is a functional nuclease in the type I-D system, performing the role played by Cas3 in other CRISPR–Cas type I systems. The type I-D system can be used for targeted mutagenesis of genomic DNA in human cells, directing both bi-directional long-range deletions and short insertions/deletions. Our findings suggest the CRISPR–Cas type I-D system as a unique effector pathway in CRISPR that can be repurposed for genome engineering in eukaryotic cells.
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Journal Title |
Nucleic Acids Research
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ISSN | 13624962
03051048
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NCID | AA00760269
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Publisher | Oxford University Press
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Volume | 49
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Issue | 11
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Start Page | 6347
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End Page | 6363
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Published Date | 2021-06-02
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Rights | This is an Open Access article distributed under the terms of the Creative Commons Attribution-NonCommercial License (http://creativecommons.org/licenses/by-nc/4.0/), which permits non-commercial re-use, distribution, and reproduction in any medium, provided the original work is properly cited. For commercial re-use, please contact journals.permissions@oup.com
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DOI (Published Version) | |
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language |
eng
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TextVersion |
Publisher
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departments |
Bioscience and Bioindustry
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