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Highly Efficient Knockout of a Squid Pigmentation Gene.

Current biology : CB (2020-08-01)
Karen Crawford, Juan F Diaz Quiroz, Kristen M Koenig, Namrata Ahuja, Caroline B Albertin, Joshua J C Rosenthal
ABSTRACT

Seminal studies using squid as a model led to breakthroughs in neurobiology. The squid giant axon and synapse, for example, laid the foundation for our current understanding of the action potential [1], ionic gradients across cells [2], voltage-dependent ion channels [3], molecular motors [4-7], and synaptic transmission [8-11]. Despite their anatomical advantages, the use of squid as a model receded over the past several decades as investigators turned to genetically tractable systems. Recently, however, two key advances have made it possible to develop techniques for the genetic manipulation of squid. The first is the CRISPR-Cas9 system for targeted gene disruption, a largely species-agnostic method [12, 13]. The second is the sequencing of genomes for several cephalopod species [14-16]. If made genetically tractable, squid and other cephalopods offer a wealth of biological novelties that could spur discovery. Within invertebrates, not only do they possess by far the largest brains, they also express the most sophisticated behaviors [17]. In this paper, we demonstrate efficient gene knockout in the squid Doryteuthis pealeii using CRISPR-Cas9. Ommochromes, the pigments found in squid retinas and chromatophores, are derivatives of tryptophan, and the first committed step in their synthesis is normally catalyzed by Tryptophan 2,3 Dioxygenase (TDO [18-20]). Knocking out TDO in squid embryos efficiently eliminated pigmentation. By precisely timing CRISPR-Cas9 delivery during early development, the degree of pigmentation could be finely controlled. Genotyping revealed knockout efficiencies routinely greater than 90%. This study represents a critical advancement toward making squid genetically tractable.

MATERIALS
Product Number
Brand
Product Description

Roche
DIG RNA Labeling Mix, sufficient for 20 reactions, solution
Roche
DIG Wash and Block Buffer Set, storage temp.:2-8°C
Roche
RNA from yeast, dry powder, pkg of 100 g
Sigma-Aldrich
Diethyl pyrocarbonate, 96% (NT)
Sigma-Aldrich
Dimethyl sulfoxide, for molecular biology
Sigma-Aldrich
680C91, ≥98% (HPLC)
Roche
Anti-Digoxigenin-POD, Fab fragments, from sheep