EMS26602
Components:
Rhodamine Saturated Solution
Mayer’s Haematoxylin
Sodium Borate 5% Aqueous Solution
Fixation:
10% Buffered Neutral Formalin
Embedding:
Cut paraffin sections at 6 to 10µm. (Thicker sections may stain better)
Staining Procedure:
- Hydrate slides to distilled water.
- Incubate in Rhodanine working solution at 37°C for 18 hours. *To prepare Rhodanine Working Solution mix: Rhodanine Saturated Solution 6ml Distilled water 94ml. Note: Shake stock solution before measuring and mixing solutions and shake working solution when pouring it on slides.
- Wash well in several changes of distilled water.
- Stain in diluted Mayer’s Haematoxylin for 10 minutes. (To prepare diluted Mayer’s Haematoxlin mix - Mayers Haematoxylin 50ml Distilled water 50ml)
- Rinse with distilled water.
- Quickly rinse in Sodium Borate, 5%.
- Rinse well with distilled water.
- Dehydrate through 95% alcohol to absolute alcohol. Clear in Xylene, 2 changes each, and coverslip using a synthetic mounting medium.
Note: The use of chemically clean glassware is necessary. Shake stock solution before measuring and mixing solutions and shake the working solution before pouring it onto the slides.
Results:
Copper – orange/red
Nuclei – light blue
Note: With low copper concentrations in tissue, slight fading may occur after coverslipping and the golden precipitate may be difficult to distinguish from lipofuscin.
References:
Sheehan and Hrapchack, Theory and Practice of Histotechnology. St. Louis, The Mosby Company 1980 p. 230.
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