Obtaining Wildtype and Transgenic Zebrafish Larvae and WildType Whole Larvae Dissociation

Begin by obtaining the wildtype and transgenic zebrafish eggs from the respective breeding setup. Take a 15-centimeter Petri dish containing HEPES-buffered E3 medium or E3.And collect the appropriate amount of fertilized eggs from the desired zebrafish breeding setup. Incubate the fertilized eggs in E3 at 28 degrees Celsius with an appropriate light and dark cycle.

At one days post fertilization or dpf, remove any unfertilized eggs and let the fertilized ones develop until five dpf. Select the transgenic zebrafish larvae at one dpf. Before proceeding for whole larvae dissociation, anesthetize the five dpf wildtype larvae using 0.016%Tricaine, and transfer 30 anesthetized larvae into a Petri dish containing one milliliter of 10x trypsin-EDTA solution.

Then, using a razor blade, chop the larvae into small pieces in the Petri dish. Transfer the chopped larvae into a micro centrifuge tube with two milliliters of 10x trypsin-EDTA solution, and leave the tube on ice for three hours. Pipette the contents up and down with a P1000 pipette every hour to stimulate dissociation.