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        Yeast Ethanol Lysates for SDS-PAGE and Western Blotting

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        845

        Procedure

         

        1. pick one colony
        2. inoculate in 3 ml of the appropriate media
        3. grow at 30° overnight
        4. pellet the cells (5 min, 5000g)
        5. wash 1X in sterile ddH2O
        6. re- suspend the pellet in 200 µl EthOH (optional: +2 µl PMSF)
        7. add approx. 100 µl glass beads (0.5 µ) in a reaction tube (you can use the cap of a 0.5 ml reaction tube as bucket)
        8. vortex vigorously for 2 min., cold (optimal is an auto- vortex like “vortex turbo-mix”)
        9. collect the supernatant in an fresh reaction tube
        10. add again 200 µl EthOH
        11. vortex
        12. collect the supernatant
        13. add again 200 µl EthOH
        14. vortex for 2 min
        15. (optional: repeat this again)
        16. collect the supernatant
        17. incubate at -20°C for 30 min or longer
        18. centrifuge 16000g, for 15 min at 4°C
        19. remove supernatant and re- suspend pellet in SDS page sample buffer and directly
        20. boil the samples to denature
        21. SDS Page and western blotting

         

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