The culture dish is sealed and placed in a humid chamber, where the embryo is cultured for up to 24 hrs

The culture dish is sealed and placed in a humid chamber, where the embryo is cultured for up to 24 hrs. to 24 hrs. Finally, the embryo is removed from the ring, fixed and processed for further applications. A troubleshooting guide is also presented. Download video stream. == Protocol == == Part 1: Bench set up == A humid chamber is prepared by placing Kimwipe/ddH2O in plastic chamber. A Falcon tube to collect albumin, dishes for culture, rings, watchglass and Igf1r waste disposal are placed on bench. Pyrex dish is filled Pirinixil with 1.4 l saline (see notes [a]). == Part 2: Embryo is explanted in saline == Eggs are removed from the incubator after 16 hrs (stage 4). The egg is opene by tapping the shell with forceps. Shell pieces are removed. The thin albumin is collected in Falcon tube. The thick albumin is removed with forceps. The embryo is placed in a plastic dish inside the saline dish. The remaining albumin is removed with forceps. == Part 3: Embryo is centered on ring == The yolk sac is tilted with forceps so that embryo faces upwards. The yolk sac Pirinixil is cut Pirinixil at the level of the equator or below. Using fine forceps, the vitelline membrane is swiftly peeled. The vitelline membrane is oriented so that its granular side (non shinny) faces upwards. Using fine forceps, the vitelline membrane is placed on the watch glass. Using fine forceps, a glass ring is applied on top of vitelline membrane and the embryo is centered. The vitelline membrane is lifted around edges of the glass ring. The assembly is removed from the saline dish. == Part 4: The culture is set up under microscope == The vitelline membrane is lifted over the glass ring using fine forceps under microscope. Using Pasteur pipette, the saline is removed from the outer edge of the ring. Using fine scissors, excess vitelline membrane is removed from the inner edge of the glass ring. Care is taken not to pierce the membrane with pipette or forceps. The embryo is gently rinsed with saline to remove loose membranes and yolk cells. 200 l saline is added to outer edge of the ring (this will facilitate later transfer). The assembly is covered with an inverted plastic dish. == Part 5: The culture is transferred to incubator == A Falcon culture dish is labelled. 2.5ml of thin albumin is added to the bottom of the Falcon dish. 200l of thin albumin is added to the inner edge of the lid of the Falcon dish. The inverted dish is removed from the assembly. Using fine forceps, the glass ring is slided along the edge of the watch glass, and transfered to the Falcon dish. All remaining saline is removed from inner surface of the ring. The Falcon dish is covered with lid and sealed. The assembly is placed in humid chamber and then in the incubator. The embryos are cultured for up to 24 hrs at 38C. == Part 6: Following culture, the embryo is fixed; culture is transferred to incubator == A fixation dish is filled with Pirinixil ice-cold PBS (or depc-PBS if embryos are to be processed forin situhybridization). The culture is removed from the incubator and immediately placed on ice. The culture dish is immediately filled with ice-cold PBS/depc-PBS. The embryo is detached from the vitelline membrane. The embryo is transferred to the fixation dish, using the blunt end of a Pasteur pipette. The embryo is pinned down using blunt-ended fine forceps. The PBS covering the fixation dish is removed. Fixative is added (see notes [b]). Depending on application, the embryo is fixed for 6-8 hr at 4C (cryostat), O/N at 4C (in situs), or 1 hr at RT for whole mount immunohistochemistry. The fixative is removed and replaced with ice-cold PBS/depc PBS. For downstream applications such asin situhybridization or immantibody staining: the nervous system and the heart are perforated using a blunt end microcapillary needle or a microdissection knife; this will prevent trapping of probe/antibody in later steps.Notes: [a] Saline consists of: solution A (for 1 l): 121.0 g NaCl, 15.5 g KCl, 10.4 g CaCl2.2H2O, 12.7 g MgCl2.6H2O; solution B (for 1 l): 2.4 g Na2HPO4.2H2O, 0.2 g NaH2PO4.2H2O; Autoclave; Prior to.