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Single-Nucleotide Microbial Genome Editing Using CRISPR-Cas12a

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dc.contributor.authorLee, Ho Joung-
dc.contributor.authorLee, Sang Jun-
dc.date.accessioned2024-04-04T01:00:27Z-
dc.date.available2024-04-04T01:00:27Z-
dc.date.issued2024-03-
dc.identifier.issn1940-6029-
dc.identifier.urihttps://scholarworks.bwise.kr/cau/handle/2019.sw.cau/73132-
dc.description.abstractMicrobial genome editing can be achieved by donor DNA-directed mutagenesis and CRISPR-Cas12a-mediated negative selection. Single-nucleotide-level genome editing enables the manipulation of microbial cells exactly as designed. Here, we describe single-nucleotide substitutions/indels in the target DNA of E. coli genome using a mutagenic DNA oligonucleotide donor and truncated crRNA/Cas12a system. The maximal truncation of nucleotides at the 3'-end of the crRNA enables Cas12a-mediated single-nucleotide-level precise editing at galK targets in the genome of E. coli. © 2024. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.-
dc.format.extent9-
dc.language영어-
dc.language.isoENG-
dc.publisherHumana Press Inc.-
dc.titleSingle-Nucleotide Microbial Genome Editing Using CRISPR-Cas12a-
dc.typeArticle-
dc.identifier.doi10.1007/978-1-0716-3658-9_9-
dc.identifier.bibliographicCitationMethods in molecular biology (Clifton, N.J.), v.2760, pp 147 - 155-
dc.description.isOpenAccessN-
dc.identifier.scopusid2-s2.0-85187780845-
dc.citation.endPage155-
dc.citation.startPage147-
dc.citation.titleMethods in molecular biology (Clifton, N.J.)-
dc.citation.volume2760-
dc.type.docTypeArticle-
dc.publisher.location미국-
dc.subject.keywordAuthor3′-truncated crRNA-
dc.subject.keywordAuthorPrecise genome editing-
dc.subject.keywordAuthorSingle-base-
dc.subject.keywordAuthorCas12a-
dc.description.journalRegisteredClassscopus-
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생명공학대학 (시스템생명공학과)
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