|ZFIN ID: ZDB-PUB-160808-5|
A simplified method for identifying early CRISPR-induced indels in zebrafish embryos using High Resolution Melting analysis
Samarut, É., Lissouba, A., Drapeau, P.
|Source:||BMC Genomics 17: 547 (Journal)|
|Registered Authors:||Drapeau, Pierre, Samarut, Eric|
|Keywords:||CRISPR, Genotyping, High-Resolution-Melting, Mutagenesis, Zebrafish|
|PubMed:||27491876 Full text @ BMC Genomics|
Samarut, É., Lissouba, A., Drapeau, P. (2016) A simplified method for identifying early CRISPR-induced indels in zebrafish embryos using High Resolution Melting analysis. BMC Genomics. 17:547.
Background The CRISPR/Cas9 system has become a regularly used tool for editing the genome of many model organisms at specific sites. However, two limiting steps arise in the process of validating guide RNA target sites in larvae and adults: the time required to identify indels and the cost associated with identifying potential mutant animals.
Results Here we have combined and optimized the HotSHOT genomic DNA extraction technique with a two-steps Evagreen PCR, followed by a high-resolution melting (HRM) assay, which facilitates rapid identification of CRISPR-induced indels. With this technique, we were able to genotype adult zebrafish using genomic DNA extracted from fin-clips in less than 2 h. We were also able to obtain a reliable and early read-out of the effectiveness of guide RNAs only 4 h after the embryos were injected with the constructs for the CRISPR/Cas9 mutagenic system. Furthermore, through mutagenesis kinetic assay, we identified that the 2-cell stage is the earliest time point at which indels can be observed.
Conclusions By combining an inexpensive and rapid genomic DNA extraction method with an HRM-based assay, our approach allows for high-throughput genotyping of adult zebrafish and embryos, and is more sensitive than standard PCR approaches, permitting early identification of CRISPR-induced indels and with applications for other model organisms as well.