N-BANDING PROTOCOL

The following protocol describes the standard N-banding protocol routinely used in our laboratory for chromosome identification in wheat and wheat relatives and will give satisfactory results even in the hands of an inexperiencesd worker.

1. Germinate seeds in petri dishes on moist filter paper for 3–4 days.
2. Collect root tips when 1.5–2.5-cm long and pretreat for 24 h in an ice-water bath.
3. Fix in Carnoy's I at room temperature for 1–3 days and then freeze or refrigerate until use.
4. Stain root tips in 1% acetocarmine for 1–2 h at room temperature, or overnight in at 4°C.
5. Make squash preparations in 45% acetic acid.
6. Remove cover slips by either the dry ice method, dipping slides into liquid nitrogen for about 10 sec, or placing slides into a freezer (-70°C) for 3 min.
7. Incubate slides in hot 45% acetic acid for 3 min in a water bath at 50°C.
8. Transfer slides to 95% ethanol at room temperature for 10 min.
9. Air dry slides overnight.
10. Incubate slides in phosphate buffer (120 g NaH₂PO₄ / L distilled water) for 2 min at 94°C in a water bath.
11. Rinse in tap water and air dry.
12. Stain with Leishman's stain (BDH #R03087) in Soerensen's phosphate buffer for about 20 min. The staining solution is diluted 5 X with water and Leishman's stain added to a final concentration of 15%).

Soerensen's buffer

		Stock	Stain
Part A	sodium phosphate dibasic (Na2HOP4)	9.47 g / L H2O	58 mL
Part B	potassium dihydrogen phosphate (KH2PO4)	9.07 g / L H2O	42 mL

1. Rinse briefly in tap water and air dry.
2. For recording of N-bands, a cover slip can be mounted using a drop of xylene or preparations can be observed without a cover slip using the appropriate lenses.