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        70% Ethanol Fixation 70%酒精固定

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        3247

        70% Ethanol Fixation
        for Recovery of DNA, RNA, and Protein

        This method was successful in our lab using prostate tissue and for our specific objectives. Investigators must be aware that they will need to tailor the following protocol for their own research objectives and tissue under study.

        This work was published in the American Journal of Pathology, volume 160, p 449-457, 2002 by Gillespie JW et al . For a synopsis of the results, please go to Summary of Published Results

        1. Materials

        • 70% ethanol, 4°C
        • 70% ethanol, 4°C
      • 2. Method

        TIP: Small biopsy samples can be fixed for shorter time intervals, typically 4-6 hours.

          1. The initial fixation of tissue specimens in 70% ethanol is similar for subsequent embedding in either low-melt polyester or paraffin.
          2. In the surgical suite immediately after resection, place the tissue specimen directly onto wet ice or into 70% ethanol at 4°C.

            TIP: Placement into 70% EtOH may restrict subsequent processing, e.g., inking of surgical markings.

             

          3. Transport to the pathology department for evaluation and further processing.
          4. Grossly process the tissue specimen into thin sections in order to allow quick penetration by the fixative. In general, the specimen should be a maximum of 3 mm thick. If the tissue is a large mass, it should be grossly cut into several slices and/or small pieces.

            TIP: This is particularly important for molecular profiling studies because ethanol does not penetrate tissue as rapidly as formalin and it is critical to minimize the interval between surgical removal and cellular fixation.

             

          5. Place into a sufficiently large container with a 10X volume:volume amount of cold 70% ethanol and fix overnight at 4°C.

        Note: There are many issues to consider when evaluating new fixation and embedding schemes for molecular profiling efforts. These include the effects of the new protocol on subsequent macromolecule stability and recovery, histology, immunohistochemistry, and in-situ hybridization studies. Associated issues include the ease of use of the method and the cost of the required reagents. For more information and research examples, see Prostate Tissue Processing .

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