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9EDA

SpCas9 with 17-bp R-loop containing 2 terminal mismatches (State IV - product)

9EDA の概要
エントリーDOI10.2210/pdb9eda/pdb
関連するPDBエントリー9EAK 9EAL 9ED9
EMDBエントリー47942
分子名称sgRNA, PAM-proximal Target Strand, Non-target strand, ... (6 entities in total)
機能のキーワードcrispr-associated endonuclease, dna binding protein, dna binding protein-dna-rna complex, dna binding protein/dna/rna
由来する生物種Streptococcus pyogenes
詳細
タンパク質・核酸の鎖数5
化学式量合計223883.28
構造登録者
Kiernan, K.A.,Taylor, D.W. (登録日: 2024-11-16, 公開日: 2025-06-18, 最終更新日: 2025-07-09)
主引用文献Kiernan, K.A.,Taylor, D.W.
Visualization of a multi-turnover Cas9 after product release.
Nat Commun, 16:5681-5681, 2025
Cited by
PubMed Abstract: While the most widely used CRISPR-Cas enzyme is the Cas9 endonuclease from Streptococcus pyogenes (Cas9), it exhibits single-turnover enzyme kinetics which leads to long residence times on product DNA. This blocks access to DNA repair machinery and acts as a major bottleneck during CRISPR-Cas9 gene editing. Cas9 can eventually be removed from the product by extrinsic factors, such as translocating polymerases, but the mechanisms contributing to Cas9 dissociation following cleavage remain poorly understood. Here, we employ truncated guide RNAs as a strategy to weaken PAM-distal nucleic acid interactions and promote faster enzyme turnover. Using kinetics-guided cryo-EM, we examine the conformational landscape of a multi-turnover Cas9, including the first detailed snapshots of Cas9 dissociating from product DNA. We discovered that while the PAM-distal product dissociates from Cas9 following cleavage, tight binding of the PAM-proximal product directly inhibits re-binding of new targets. Our work provides direct evidence as to why Cas9 acts as a single-turnover enzyme and will guide future Cas9 engineering efforts.
PubMed: 40593576
DOI: 10.1038/s41467-025-60668-7
主引用文献が同じPDBエントリー
実験手法
ELECTRON MICROSCOPY (2.88 Å)
構造検証レポート
Validation report summary of 9eda
検証レポート(詳細版)ダウンロードをダウンロード

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件を2026-01-28に公開中

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