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一种用于量化脱靶碱基编辑的集成酶促和计算流程。

An integrated enzymatic and computational pipeline for quantifying off-target base-editing.

作者信息

McFarland Alexander G, Ooi Soon-Keat, Tafuri Davin, Kamali Elahe, Cooper Natalie, Cook Emma J, Reddy Shantan, Jarocha Danuta, Wellhausen Nils, Gill Saar I, Roche Aoife M, Fraietta Joseph A, Bushman Frederic D, Herbst Friederike

出版信息

bioRxiv. 2025 Aug 26:2025.08.26.667396. doi: 10.1101/2025.08.26.667396.

Abstract

DNA base editing is increasingly used for human genetic modification, but methods for monitoring off-target editing are nascent. Here we present a simple model-independent workflow for identifying sites of off-target base-editing in relevant cell types on a genome-wide level. We report that sites of off-target editing by the ABE8e editor could be identified using an ABE8e derivative with restored DSB cleavage activity. This allows marking of enzyme-generated double-stranded (ds) DNA breaks by incorporation of dsDNA oligonucleotides that are transfected into primary target cells. DNA sequencing at sites of oligonucleotide incorporation reported both the genomic location of off-target cleavage and the extent of base-editing nearby. We present a platform combining this cellular (BEiGUIDE-Seq) and computational workflow (CRISPRito) to generate optimized amplicon panels for convenient monitoring of off-target base editing. This work introduces a generalizable strategy to evaluate off-target edits in patient-derived cells, addressing a critical safety gap for clinical base editing.

摘要

DNA碱基编辑越来越多地用于人类基因改造,但监测脱靶编辑的方法尚处于起步阶段。在此,我们提出了一种简单的、与模型无关的工作流程,用于在全基因组水平上识别相关细胞类型中的脱靶碱基编辑位点。我们报告称,使用具有恢复的双链断裂(DSB)切割活性的ABE8e衍生物,可以识别ABE8e编辑器的脱靶编辑位点。这允许通过掺入转染到原代靶细胞中的双链DNA寡核苷酸来标记酶产生的双链(ds)DNA断裂。在寡核苷酸掺入位点进行DNA测序,既报告了脱靶切割的基因组位置,也报告了附近碱基编辑的程度。我们提出了一个结合这种细胞方法(BEiGUIDE-Seq)和计算工作流程(CRISPRito)的平台,以生成优化的扩增子面板,便于监测脱靶碱基编辑。这项工作引入了一种可推广的策略,用于评估患者来源细胞中的脱靶编辑,解决了临床碱基编辑的一个关键安全缺口。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/912e/12407836/593b74423fab/nihpp-2025.08.26.667396v1-f0001.jpg

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