X-tremeGENE™ HP DNA Transfection Reagent Protocol
Cell Preparation for Transfection
Plate cells approximately 24 hours before transfection, making sure cells are at optimal concentration (70–90 % confluency).
Steps Before Transfection
- Allow X-tremeGENE™ HP DNA Transfection Reagent, DNA and diluent (Opti:MEM®I Reduced Serum Medium or serum-free medium) to warm to +15 °C to +25 °C, and vortex gently.
- Place diluent in a sterile tube.
- Add plasmid DNA. Gently pipette up and down to mix.
- Add X-tremeGENE™ HP DNA Transfection Reagent to the diluted DNA.
- Incubate for 15 minutes at +15 °C to +25 °C.
- Add transfection complex to the cells in a dropwise manner.
- Gently shake or swirl the wells or flasks to ensure even distribution over the entire plate.
- Incubate cells for 18 – 72 hours before measuring protein expression.
Tips for Successful Transfections using the X-tremeGENE™ DNA Transfection Reagent
- Store X-tremeGENE™ 9 DNA Transfection Reagent at +2 to +8 °C and X-tremeGENE™ HP DNA Transfection Reagent at -15 to -25 °C.
- Bring the vial containing X-tremeGENE™ DNA Transfection Reagent to +15 to +25 °C, and vortex for one second, before removing the desired amount.
- Do not aliquot X-tremeGENE™ DNA Transfection Reagent; store remaining transfection reagent in the original glass vials.
- Minimize contact of undiluted transfection reagent with plastic surfaces.
- After removing the amount required, tightly close the lid of the vial immediately after use.
- The minimum amount of X-tremeGENE™ DNA Transfection Reagent: DNA complex for use in a transfection is 100 μL. Complex formation at lower volumes significantly decreases transfection efficiency.
- Do not use tubes or microplates made of polystyrene for X-tremeGENE™ DNA Transfection Reagent: DNA complex preparation. When not able to avoid polystyrene materials, make certain to pipet the transfection reagent directly into the serum-free medium, or a reduced-serum medium (that does not contain any serum).
- Do not use siliconized pipette tips or tubes.
- Make certain that cells are still actively growing at the time of transfection.
- Include appropriate controls when performing transfections, by including wells with:
(1) untransfected cells
(2) cells with transfection reagent alone
(3) cells with DNA alone - The optimal ratio of transfection reagent: DNA, and the optimal total amount of complex, can vary according to cell line, cell density, status of cell growth for the assay, and gene expressed.
Materials
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