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Reliable CRISPR/Cas9 Genome Engineering in Caenorhabditis elegans Using a Single Efficient sgRNA and an Easily Recognizable Phenotype
Wednesday, 2017/05/10 | 07:48:28
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Sonia El Mouridi, Claire Lecroisey, Philippe Tardy, Marine Mercier, Alice Leclercp-Blondel, Nora Zariohi and Thomas Boulin G3: Genes, Genomes, Genetics May 1, 2017 vol. 7 no. 5 1429-1437; https://doi.org/10.1534/g3.117.040824 AbstractCRISPR/Cas9 genome engineering strategies allow the directed modification of the Caenorhabditis elegans genome to introduce point mutations, generate knock-out mutants, and insert coding sequences for epitope or fluorescent tags. Three practical aspects, however, complicate such experiments. First, the efficiency and specificity of single-guide RNAs (sgRNA) cannot be reliably predicted. Second, the detection of animals carrying genome edits can be challenging in the absence of clearly visible or selectable phenotypes. Third, the sgRNA target site must be inactivated after editing to avoid further double-strand break events. We describe here a strategy that addresses these complications by transplanting the protospacer of a highly efficient sgRNA into a gene of interest to render it amenable to genome engineering. This sgRNA targeting the dpy-10 gene generates genome edits at comparatively high frequency. We demonstrate that the transplanted protospacer is cleaved at the same time as the dpy-10 gene. Our strategy generates scarless genome edits because it no longer requires the introduction of mutations in endogenous sgRNA target sites. Modified progeny can be easily identified in the F1 generation, which drastically reduces the number of animals to be tested by PCR or phenotypic analysis. Using this strategy, we reliably generated precise deletion mutants, transcriptional reporters, and translational fusions with epitope tags and fluorescent reporter genes. In particular, we report here the first use of the new red fluorescent protein mScarlet in a multicellular organism. wrmScarlet, a C. elegans-optimized version, dramatically surpassed TagRFP-T by showing an eightfold increase in fluorescence in a direct comparison.
See: http://www.g3journal.org/content/7/5/1429?etoc=
Figure 1 Generation of d10-entry strains. (A) Insertion of the d10 sequence into sup-9, egl-23b, egl-23 (C-terminus), and twk-18 using a single-strand oligonucleotide repair template compatible with multiple sgRNAs. Genes and their intron/exon structure are displayed in the 5′–3′ orientation. The ssON repair templates are represented by black arrows (containing the d10 sequence in green) above the coding strand and translation of the target gene. Correspondence of homology regions between the ssON repair template and genomic locus is indicated in gray. sgRNA binding sites are indicated by blue open arrows. (B) unc-58 coconversion is used to detect the insertion of d10 sequences into a gene of interest. unc-58(e665) mutants are easily identified in the F1 progeny of injected P0 animals based on their straight body posture, lack of mobility, and characteristic rotation around the antero-posterior body axis. RT, repair template. (C) BanI, BssSI, and BsrBI restriction sites are present in the d10 protospacer sequence and are used for RFLP analysis. The Cas9 double-strand break site is indicated by an arrowhead. (D) R12E2.15 contains the only predicted off-target site of the d10 sgRNA. Four base changes (in pink) distinguish both sites. A BsrBI site follows the Cas9 double-strand break site (indicated by an arrowhead), between the −3 and −4 bases relative to the protospacer adjacent motif (PAM). |
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