| Literature DB >> 30010654 |
Ceres Kosuta1, Kate Daniel2, Devon L Johnstone1, Kevin Mongeon1, Kevin Ban1, Sophie LeBlanc2, Stuart MacLeod2, Karim Et-Tahiry3, Marc Ekker3, Alex MacKenzie2, Izabella Pena4.
Abstract
Zebrafish (Danio rerio) possess orthologues for 84% of the genes known to be associated with human diseases. In addition, these animals have a short generation time, are easy to handle, display a high reproductive rate, low cost, and are easily amenable to genetic manipulations by microinjection of DNA in embryos. Recent advances in gene editing tools are enabling precise introduction of mutations and transgenes in zebrafish. Disease modeling in zebrafish often leads to larval phenotypes and early death which can be challenging to interpret if genotypes are unknown. This early identification of genotypes is also needed in experiments requiring sample pooling, such as in gene expression or mass spectrometry studies. However, extensive genotypic screening is limited by traditional methods, which in most labs are performed only on adult zebrafish or in postmortem larvae. We addressed this problem by adapting a method for the isolation of PCR-ready genomic DNA from live zebrafish larvae that can be achieved as early as 72 h post-fertilization (hpf). This time and cost-effective technique, improved from a previously published genotyping protocol, allows the identification of genotypes from microscopic fin biopsies. The fins quickly regenerate as the larvae develop. Researchers are then able to select and raise the desired genotypes to adulthood by utilizing this high-throughput PCR-based genotyping procedure.Entities:
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Year: 2018 PMID: 30010654 PMCID: PMC6102016 DOI: 10.3791/58024
Source DB: PubMed Journal: J Vis Exp ISSN: 1940-087X Impact factor: 1.355