PUBLICATION

CRISPR Guide RNA Validation In Vitro

Authors

Grainger, S., Lonquich, B., Oon, C.H., Nguyen, N., Willert, K., Traver, D.

ID

ZDB-PUB-161110-1

Date

2017

Source

Zebrafish 14(4): 383-386 (Journal)

Registered Authors

Grainger, Stephanie, Traver, David

Keywords

CRISPR, Cas9, in vitro, knock in, validation, zebrafish

MeSH Terms

Animals
CRISPR-Cas Systems*
Endonucleases/metabolism
Gene Editing*
Gene Targeting
In Vitro Techniques
Monophenol Monooxygenase/antagonists & inhibitors
Monophenol Monooxygenase/genetics
RNA, Guide, Kinetoplastida/genetics*
Zebrafish/genetics*

PubMed

27829120 Full text @ Zebrafish

Abstract

Clustered regularly interspaced short palindromic repeats (CRISPR)/Cas9 has been applied to edit genomes in a wide variety of model systems. Although this process can be quite efficient, editing at precise locations in the genome remains difficult without a suitable single guide RNA (sgRNA). We have developed a method for screening sgRNA function in vitro, using reagents that most zebrafish laboratories are already using. The results from our in vitro assay correlate with function in vivo in every sgRNA that we have examined so far. When combined with endonucleases with alternative protospacer adjacent motif site specificities and alternative sgRNAs, this method will streamline genome editing at almost any locus.

Genes / Markers

Figures

Expression

Phenotype

Mutations / Transgenics

Human Disease / Model

Sequence Targeting Reagents

Fish

Antibodies

Orthology

Engineered Foreign Genes

Mapping

Grainger et al., 2017 ZDB-PUB-161110-1 PMID:27829120

CRISPR Guide RNA Validation In Vitro

Grainger et al., 2017

ZDB-PUB-161110-1
PMID:27829120