A rapid and effective method for screening, sequencing and reporter verification of engineered frameshift mutations in zebrafish

A rapid and effective method for screening, sequencing and reporter verification of engineered frameshift mutations in zebrafish

Clustered regularly interspaced palindromic repeats (CRISPR)/Cas-based adaptive immunity against pathogens in bacteria has been adapted for genome editing and applied in zebrafish ( ) to generate frameshift mutations in protein-coding genes. Although there are methods to detect, quantify and sequenc...

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Veröffentlicht in:Disease models & mechanisms 2017-06, Vol.10 (6), p.811-822
Hauptverfasser: Prykhozhij, Sergey V, Steele, Shelby L, Razaghi, Babak, Berman, Jason N
Format: Artikel
Sprache:eng
Schlagworte:
Animals
Base Sequence
Cas9
Cloning
Cloning, Molecular
CRISPR
Exons - genetics
Fluorescence
Frameshift Mutation - genetics
Genes
Genes, Reporter
Genetic Engineering
Genetic Testing - methods
Genome editing
Genomes
Mutation
Phenotype
Proteins
Reading
Reporter
Reproducibility of Results
Resource
RNA Splicing - genetics
Sequence Analysis, DNA
SgRNA
Site selection
Zebra
Zebrafish
Zebrafish - genetics
Zebrafish Proteins - genetics
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Zusammenfassung:Clustered regularly interspaced palindromic repeats (CRISPR)/Cas-based adaptive immunity against pathogens in bacteria has been adapted for genome editing and applied in zebrafish ( ) to generate frameshift mutations in protein-coding genes. Although there are methods to detect, quantify and sequence CRISPR/Cas9-induced mutations, identifying mutations in F1 heterozygous fish remains challenging. Additionally, sequencing a mutation and assuming that it causes a frameshift does not prove causality because of possible alternative translation start sites and potential effects of mutations on splicing. This problem is compounded by the relatively few antibodies available for zebrafish proteins, limiting validation at the protein level. To address these issues, we developed a detailed protocol to screen F1 mutation carriers, and clone and sequence identified mutations. In order to verify that mutations actually cause frameshifts, we created a fluorescent reporter system that can detect frameshift efficiency based on the cloning of wild-type and mutant cDNA fragments and their expression levels. As proof of principle, we applied this strategy to three CRISPR/Cas9-induced mutations in , and genes. An insertion of seven nucleotides in resulted in the first reported observation of exon skipping by CRISPR/Cas9-induced mutations in zebrafish. However, of these three mutant genes, the fluorescent reporter revealed effective frameshifting exclusively in the case of a two-nucleotide deletion in , suggesting activity of alternative translation sites in the other two mutants even though exon-skipping deletion is likely to be deleterious. This article provides a protocol for characterizing frameshift mutations in zebrafish, and highlights the importance of checking mutations at the mRNA level and verifying their effects on translation by fluorescent reporters when antibody detection of protein loss is not possible.
ISSN:1754-8403
1754-8411
DOI:10.1242/dmm.026765