CRISPROne

Design of Base Editing guide RNAs

Base editors (BE) have two principal components that are fused together to form a single protein: (i) a CRISPR protein, bound to a guide RNA, and (ii) a base editing enzyme, such as a deaminase, which carries out the desired chemical modification of the target DNA base. More ....

Advantages:

1) The creation of precise, predictable and efficient genetic outcomes at a targeted sequence; 2) High efficiency editing without need for template-based homology directed repair, and 3) Avoidance of the unwanted consequences of double-stranded DNA breaks.

Note:

The designed sgRNA can enable efficient disruption of genes through induction of STOP Codons and Alternative Splicing (AS).

Input Sequence (Only One Id/Position/Sequence required; Design speed: Id = Position > Fasta Sequence)

An Substitution module is input for pegRNAs Design

ABE (A to G) CBE (C to T) GBE (C to G) ABE + CBE

PAM Type See notes on enzymes in the help

Target Genome: More Information of Genomes Metadata

Customized PAM (Need to select Customized PAM in PAM Type )

Please input a valid PAM DNA Sequence (Only Capital Letter).

sgRNA module of Customized PAM

Spacer length of Customized PAM

Please input a valid Spacer Length (10-50).

Note: For a Customized PAM select Customized PAM: 5'-XXX-3' in PAM Type and then set sgRNA module and Spacer length .

Base editing window:

Design of Base Editing guide RNAs

Mandatory Parameters