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        Acid Phosphatase for Glycol Methacrylate Sections Procedure

        互联网

        1008

         

        1. Incubate sections in the incubating medium at 37°C for 5 - 12 hours. Long incubation periods are needed to get significantly visible reaction product.
        2. Wash in distilled water for 2 minutes.
        3. Counterstain with Methyl Green for 5 minutes.
        4. Wash in distilled water for 2 minutes.
        5. Air dry and coverslip.
        Results:
        Nuclei - dark green
        Cytoplasm - light green
        Sites of enzyme activity - red

        Solutions:

        Incubating Medium
        • Combine 20 ml of buffer solution, 48 ml of distilled water and 4 ml. of substrate solution.
        • Combine 3.2 ml of pararosaniline solution with 3.2 ml of sodium nitrite solution. Mix for 1 minute.
        • Add the second solution to the first
        • Adjust pH to 5.
        Buffer Solution
        • Anhydrous sodium acetate - 5.9 g
        • Sodium barbiturate - 14.7 g
        • Distilled water (boiled) - 500 ml
        Do not adjust the pH of the buffer and store at 4°C.
        Substrate Solution
        • Naphtol AS-BI phosphatease, sodium salt (Sigma) - 40 mg
        • N.N-dimethylformamide - 4 ml
        Pararosaniline Solution
        • Pararosaniline (C.I.# 42500) - 2 g
        • 2N HCl - 50 ml
        Use heat to dissolve, filter when cool and store at 4°C.
        Sodium Nitrite Solution
        • Sodium Nitrite - 1 gm
        • Distilled Water - 25 ml
        Prepare fresh and store at 4°C.
        Methyl Green
        • Methyl Green (C.I.# 42585) - 1 g
        • Phosphate/citrate buffer 0.1M pH 4.0 - 100 ml

        Citation:

        Gerrits, P. O. and Smid, L., "Staining Procedures for Tissues Embedded in 2-Hydroxyethyl Methacrylate", Heraeus Kulzer.

         

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