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        Procedure for Transfection of Mammalian Cells

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        926

         

        Materials:

        bullet Lipofectamine
        bullet IMDM containing 10% fetal bovine serum, 1% glutamine, 1% aa
        bullet IMDM containing 1% glutamine
        bullet IMDM containing 20% fetal bovine serum, 1% glutamine, 1% aa
        1. In a six-well or 35 mm tissue culture plate, seed ~2x 105 cells per well in 2 ml IMDM containing 10% FBS and nonessential amino acids.
        2. Incubate the cells at 37E C in a CO2 incubator until the cells are 70-80% confluent. This will usually take 18-24 h.
        3. Prepare the following solutions in 12 x 75 mm sterile tubes:
          Solution A: For each transfection, dilute 2 μg DNA (plasmid) in 375 μl serum-free IMDM (containing nonessential amino acids).
          Solution B: For each transfection, dilute 12 μl LIPOFECTAMINE Reagent in 375 μl serum-free IMDM.
        4. Combine the two solutions, mix gently, and incubate at room temperature for 15-45 min. The solution may appear cloudy, however this will not impede the transfection.
        5. Wash the cells once with 2 ml serum-free IMDM.
        6. For each transfection, add 750 μl serum-free IMDM to each tube containing the lipid-DNA complexes. Do not add antibacterial agents to media during transfection. Mix gently and overlay the diluted complex solution onto the washed cells.
        7. Incubate the cells for 5 h at 37E C in a CO2 incubator.
        8. Add 1.5 ml IMDM with 20% FBS without removing the transfection mixture. If toxicity is a problem, remove the transfection mixture and replace with normal growth medium.
        9. Replace medium at 18-24 h following start of transfection.
        10. Assay cell extracts for gene activity 24-72 h after the start of transfection, depending on cell type and promoter activity.

         

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