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Figure 7

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ZDB-IMAGE-210113-8
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Figures for England et al., 2020
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Figure 7

Phenotypic and genotypic analysis of embryos from an incross of hmx3aSU42/+ parents injected with hmx2MENTHU CRISPR reagents. (A and B) Lateral views of ear phenotypes at 4 day in live uninjected (A) and hmx2MENTHU CRISPR-injected (B) hmx3aSU42 homozygous mutant embryos. Rostral, left; Dorsal, top. The uninjected hmx3aSU42 homozygous mutant embryo has two normal otoliths in each ear (A). In contrast, the hmx2MENTHU CRISPR-injected hmx3aSU42 homozygous mutant embryo has fused otoliths in both ears. (C and D) Wild-type (top row) and hmx2MENTHU (bottom row) genomic sequences on top. Each colored box represents a specific nucleotide in the hmx2 coding sequence: A, green; C, blue; G, black; T, red. The hmx2MENTHU mutant sequence contains a 5 bp deletion (CGCAG, red line), which introduces a premature stop codon (red dashed box) 14–16 bases after the deletion. Sequencing traces (below) from individual embryos from an incross of hmx3aSU42/+ parents injected with hmx2MENTHU CRISPR reagents. In the injected embryos, hmx2MENTHU mutant sequences (with the 5 bp deletion) comprise ∼60% (C) to 90% (D) of all amplified sequences at this locus. Bar, 50 µm (A and B).

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