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        Cell death detection in Xenopus embryos by ELISA

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        Sample preparation

        Wash embryos 1 x in 25% MMR

        Remove excess buffer

        Add 10 volumes "incubation buffer", i.e. 50 µl for 5 embryos

        Lyse the embryos by gently pipetting up and down using a large blue tip
                Use a negative control, as shearing of genomic DNA may give false positive signals

        Dilute 10 µl lysate with 190 µl "incubation buffer"
                Consider testing other dilutions

        Incubate this sample for 30 min. at 4°C

        Centrifuge at 13,000 rpm (eppendorf) for 10 min. at 4°C

        Remove 160 µl supernatant / embryo, avoiding pellet contamination of the supernatant

        Samples can be stored, if not used the same day, in aliquots at -20°C

        Do ELISA according to manufacturer's instructions.
         

         

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