Validation of CRISPR-based Gene Editing
Research using CRISPR/Cas nuclease-based genome editing, such as modeling diseases or identifying potential therapeutics, relies on methods to validate targeting efficiency in vitro and in vivo. NEB offers reagents for in vitro enzymatic indel detection assays and next-generation sequencing of edited nucleic acids.
Cas9 digest and enzymatic mismatch assays
Cas9 digests and enzymatic mismatch cleavage assays are simple and sensitive methods for validating editing efficiency. DNA isolated from editing experiments typically contains a mixture of edited and unedited sequences. PCR amplification followed by re-annealing can produce heteroduplex DNA containing mixtures of edited and unedited strands. Enzymes such as T7 Endonuclease I and Authenticase® can cleave these mismatched indel sequences and provide an estimate of editing efficiency. The Cas9 nuclease itself can be used to estimate editing efficiency as it can digest fully matched unedited sequences, but not most edited sequences.
- Authenticase (NEB #M0689) is a mixture of structure-specific nucleases that outperforms T7 Endo I in detecting CRISPR-induced on-target mutations across a broad range of mutations/wild-types.
- EnGen® Mutation Detection Kit (NEB #E3321) provides optimized reagents for conventional T7 Endonuclease-based mutation detection of genome editing events.
- Cas9 Nuclease, S.pyogenes (NEB #M0386) detects indels with the advantage of assessing locus modification at genome editing targeting efficiency above 50%.
Sequencing to detect CRISPR on- and off-targeting
NEB carries a broad range of next-generation sequencing kits to analyze gene editing events with automation compatibility. Targeted or whole genome CRISPR validation approaches permit accurate genotyping, and large-scale CRISPR screening of genomes, pools and clone analyses. NEB recommends PCR-free NGS library preparation to produce the highest quality, high-yield libraries of whole genomes without PCR bias.
- NEBNext® Ultra™ II DNA Library Prep Kit for Illumina® (NEB #E7645) or NEBNext Ultra™ II DNA Library Prep with Sample Purification Beads (NEB #E7103) are recommended for amplicon sequencing.
- NEBNext Ultra II DNA PCR-free Library Prep Kit for Illumina (NEB #E7410) enables whole genome libraries with sheared DNA.
- NEBNext Ultra II FS DNA PCR-free Library Prep Kit for Illumina (NEB #E7430) enables whole genome libraries with unsheared DNA which fragments, end repairs, and dA-tails DNA, all in a single tube with no cleanups or transfers.
Choose Product:
Choose Type:
- Mismatch Detection Assay (NEB #M0689)
- Supplemental Protocol 1: Generation of DNA fragments by PCR assembly of pooled oligos (NEB #M0689)
- Supplemental Protocol 2: Using colony PCR to identify positive clones (NEB #M0689)
- T7 Endonuclease I-based Mutation Detection with the EnGen® Mutation Detection Kit (NEB #E3321)
- Using recombinant Cas9 nuclease to assess locus modification in genome editing experiments (NEB #M0386)
Interactive Tools
CRISPR Plasmid Repositories
CRISPR-gRNA Design Tools
Online Forums
Organism-specific Resources
Products and content are covered by one or more patents, trademarks and/or copyrights owned or controlled by New England Biolabs, Inc (NEB). The use of trademark symbols does not necessarily indicate that the name is trademarked in the country where it is being read; it indicates where the content was originally developed. All other trademarks are the property of their respective owners. The use of this product may require the buyer to obtain additional third-party intellectual property rights for certain applications. For more information, please email busdev@neb.com.
This product is intended for research purposes only. This product is not intended to be used for therapeutic or diagnostic purposes in humans or animals.
 |
Choose a product for your application |
Learn about Genome Editing with CRISPR/Cas
Explore our genome editing toolbox |
|
|
Choose a product for your application |
Learn about Genome Editing with CRISPR/Cas
Explore our genome editing toolbox |
