Project description:Directed Evolution of an Adenine Base Editor with Increased Activity and Context Compatibility

Project description:Directed Evolution of an Adenine Base Editor withIncreased Activity and Context Compatibility [sgRNA-target library]

Project description:Directed Evolution of an Adenine Base Editor with Increased Activity and Context Compatibility [RNA-seq data]

Project description:Engineering of adenine base editor with improved editing activity across NNN PAMs

Project description:Directed Evolution of Adenine Base Editors with Increased Activity and Therapeutic Application

Project description:Structure-guided engineering of adenine base editor with minimized RNA off-targeting activity

Project description:Adenine base editors (ABEs) are precise gene-editing agents that convert A:T pairs into G:C through a deoxyinosine intermediate. ABEs function most effectively when the target A is in a TA context. Deficient ABE processing of RA (R = A or G) is most evident when the target A is outside the comfortable editing window or when delivery is suboptimal. In the current study, we report directed evolution of TadA8r, a new variant of the Escherichia coli tRNA-specific adenosine deaminase (TadA) with ultra-fast deoxyadenosine deamination and no context bias.

Project description:Adenine and cytosine base editors (ABEs and CBEs) represent a new genome editing technology that allows the programmable installation of A-to-G or C-to-T alterations on DNA. We engineered Streptococcus pyogenes Cas9-based adenine and cytosine base editor (SpACE) that enables efficient simultaneous introduction of A-to-G and C-to-T substitutions in the same base editing window on DNA.

Project description:High-throughput profiling of base editor activity

Project description:Engineering RsDddA as mitochondria base editor with wide target compatibility and enhanced activity