An Acetic Acid Dissociation, Air-Drying Technique for Insect Chromosomes, With Aceto-Lactic Orcein Staining

Abstract

The method differs from mammalian techniques for somatic chromosomes in that it uses very small amounts of material. Drosopmla melanogaster and an ant, Dorymyrmex sp., are used as examples. Pretreatment with 0.05% Colcemid in insect Ringer solution is applied to mature Drosophlla larvae for 5 hr., by feeding, but Dorymyrmex prepupae require puncture and a 15 hr. exposure of the puncture to the solution. Organs are removed under 1% sodium citrate, transferred to fresh citrate for 10-20 min., than fixed in acetic-methanol, 13, for 30 min. Transfer to a drop of 60% acetic acid on a clean warmed slide dissociates the cells, which are spread by adding a small drop of fixative and tilting the slide in all directions. After immersion in acetic ethanol 1:3, for 4 hr., rinsing in the stain solvent and draining the slides then have 2-3 drops of aceto-lactic orcein placed on each, coverslips added, and warmed (at about 50[degree]C) for about 12 hr. or until staining is sufficient. They can then either be treated as semipermanent or made permanent by allowing the cover-slips to slide off in acetic-ethanol, dehydrating, and mounting in Euparal, or a synthetic resin.