Precise and efficient C-to-U RNA base editing with SNAP-CDAR-S

被引:8
|
作者
Latifi, Ngadhnjim [1 ]
Mack, Aline Maria [1 ]
Tellioglu, Irem [2 ,3 ]
Di Giorgio, Salvatore [2 ]
Stafforst, Thorsten [1 ,4 ]
机构
[1] Univ Tubingen, Interfac Inst Biochem, Morgenstelle 15, D-72076 Tubingen, Germany
[2] German Canc Res Ctr, Div Immune Divers D150, D-69120 Heidelberg, Germany
[3] Heidelberg Univ, Fac Engn, D-69120 Heidelberg, Germany
[4] Univ Tubingen, Gene & RNA Therapy Ctr GRTC, Fac Med, Tubingen, Germany
基金
欧洲研究理事会; 欧盟地平线“2020”;
关键词
MOLECULAR-CLONING; SITE; MUTATIONS; PROTEINS;
D O I
10.1093/nar/gkad598
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Site-directed RNA base editing enables the transient and dosable change of genetic information and represents a recent strategy to manipulate cellular processes, paving ways to novel therapeutic modalities. While tools to introduce adenosine-to-inosine changes have been explored quite intensively, the engineering of precise and programmable tools for cytidine-to-uridine editing is somewhat lacking behind. Here we demonstrate that the cytidine deaminase domain evolved from the ADAR2 adenosine deaminase, taken from the RESCUE-S tool, provides very efficient and highly programmable editing when changing the RNA targeting mechanism from Cas13-based to SNAP-tag-based. Optimization of the guide RNA chemistry further allowed to dramatically improve editing yields in the difficult-to-edit 5 & PRIME;-CCN sequence context thus improving the substrate scope of the tool. Regarding editing efficiency, SNAP-CDAR-S outcompeted the RESCUE-S tool clearly on all tested targets, and was highly superior in perturbing the & beta;-catenin pathway. NGS analysis showed similar, moderate global off-target A-to-I and C-to-U editing for both tools.
引用
收藏
页码:E84 / E84
页数:12
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