TISSUE PREPARATION FOR IN SITU HYBRIDIZATIONJosiah N. Wilcox It is also possible to use fresh frozen tissue for in situ hybridization if the paraformaldehyde/sucrose method is not feasible. Tissues should be rinsed in saline or PBS and frozen in O.C.T. blocks in liquid nitrogen as outlined above. Although not optimal, it is also possible to use snap frozen material tissue without an embedding matrix. The fixation, sucrose, and O.C.T. steps are used primarily to improve the tissue morphology. It is expected that the fixation times outlined above will not result in complete fixation of large pieces of tissue. However, the additional fixation step at the beginning of the in situ hybridization procedure should ensure adequate fixation of such tissues prior to hybridization. This protocol has been used successfully on large (up to 1 cubic cm) and small (1 cubic mm) tissue samples. 200ml 0.5M NaPO4, pH 7.4800ml depcH20Heat to 70°C with stirring on hot plate in fume hoodAdd 40g Paraformaldehyde (EM grade, Polysciences, Cat No. 0380) Once the solution has cleared (it should take 5 minutes or less), filter with a side-arm flask, Buchner funnel and Whatman No. 2 filter paper.Immediately pour the solution into a one liter bottle which has been packed in ice. This cools the solution quickly and prevents breakdown of the paraformaldehyde. Store at 4°C for up to two weeks. Mix above and filter sterilize with a disposable Nalgene filtration unit type S(0.45 micron). Store at 4°C. USE OF FISHERBRAND SUPERFROST/PLUS MICROSCOPE SLIDES FOR IN SITU HYBRIDIZATION We use Fisherbrand SuperFrost/Plus positively-charged microscope slides (Cat. No. 12-550-15) for all of our frozen tissue sectioning and have very good tissue retention on slides after an in situ hybridization experiment. SuperFrost/Plus slides require no preparation time prior to cryosectioning and are competitive in terms of labor cost and reagent expenses. SECTIONING OF FROZEN TISSUES FOR IN SITU HYBRIDIZATION