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A rational engineering strategy for structural dynamics modulation enables target specificity enhancement of the Cas9 nuclease
DC Field | Value | Language |
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dc.contributor.author | 김형범 | - |
dc.date.accessioned | 2025-10-17T08:13:03Z | - |
dc.date.available | 2025-10-17T08:13:03Z | - |
dc.date.issued | 2025-06 | - |
dc.identifier.issn | 0305-1048 | - |
dc.identifier.uri | https://ir.ymlib.yonsei.ac.kr/handle/22282913/207686 | - |
dc.description.abstract | Structural dynamics of an enzyme plays a crucial role in enzymatic activity and substrate specificity, yet rational engineering of the dynamics for improved enzymatic properties remains a challenge. Here, we present a new biochemical strategy of intermediate state stabilization that modulates the multistep dynamic mechanisms of enzyme reactions to improve substrate specificity. We employ this strategy to enhance CRISPR-Cas9 nuclease specificity. By incorporating positively charged residues into the noncatalytic REC2 domain of Cas9, we stabilize the REC2-DNA interaction that forms exclusively in a catalytically inactive intermediate conformation of the Cas9 complex. This enables off-target trapping in the inactive conformation and thus reduces off-target cleavage in human cells. Furthermore, we combine the REC2 modification with mutations in previous rational variants, leading to the development of a combinational variant named Correct-Cas9, which connotes "combined with rationally engineered REC-Two" Cas9. Assessed by high-throughput analysis at thousands of target sequences, Correct-Cas9 exhibits increased target specificity compared to its parental variants, demonstrating a synergy between our strategy and previous rational approaches. Our method of intermediate state stabilization, either alone or combined with conventional approaches, could be applied to various nucleic acid-processing enzymes that undergo conformational changes upon target binding, to enhance their target specificity effectively. | - |
dc.description.statementOfResponsibility | open | - |
dc.language | English | - |
dc.publisher | Oxford University Press | - |
dc.relation.isPartOf | NUCLEIC ACIDS RESEARCH | - |
dc.rights | CC BY-NC-ND 2.0 KR | - |
dc.subject.MESH | CRISPR-Associated Protein 9* / chemistry | - |
dc.subject.MESH | CRISPR-Associated Protein 9* / genetics | - |
dc.subject.MESH | CRISPR-Associated Protein 9* / metabolism | - |
dc.subject.MESH | CRISPR-Cas Systems* | - |
dc.subject.MESH | DNA / chemistry | - |
dc.subject.MESH | DNA / metabolism | - |
dc.subject.MESH | Endonucleases* / chemistry | - |
dc.subject.MESH | Endonucleases* / genetics | - |
dc.subject.MESH | Endonucleases* / metabolism | - |
dc.subject.MESH | Gene Editing | - |
dc.subject.MESH | Humans | - |
dc.subject.MESH | Models, Molecular | - |
dc.subject.MESH | Mutation | - |
dc.subject.MESH | Protein Engineering* / methods | - |
dc.subject.MESH | Substrate Specificity | - |
dc.title | A rational engineering strategy for structural dynamics modulation enables target specificity enhancement of the Cas9 nuclease | - |
dc.type | Article | - |
dc.contributor.college | College of Medicine (의과대학) | - |
dc.contributor.department | Dept. of Pharmacology (약리학교실) | - |
dc.contributor.googleauthor | Keewon Sung | - |
dc.contributor.googleauthor | Youngri Jung | - |
dc.contributor.googleauthor | Nahye Kim | - |
dc.contributor.googleauthor | Yong-Woo Kim | - |
dc.contributor.googleauthor | Hyongbum Henry Kim | - |
dc.contributor.googleauthor | Seong Keun Kim | - |
dc.contributor.googleauthor | Sangsu Bae | - |
dc.identifier.doi | 10.1093/nar/gkaf535 | - |
dc.contributor.localId | A01148 | - |
dc.relation.journalcode | J02387 | - |
dc.identifier.eissn | 1362-4962 | - |
dc.identifier.pmid | 40539512 | - |
dc.contributor.alternativeName | Kim, Hyongbum | - |
dc.contributor.affiliatedAuthor | 김형범 | - |
dc.citation.volume | 53 | - |
dc.citation.number | 12 | - |
dc.citation.startPage | gkaf535 | - |
dc.identifier.bibliographicCitation | NUCLEIC ACIDS RESEARCH, Vol.53(12) : gkaf535, 2025-06 | - |
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