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Lipofectamine® RNAiMAX is a proprietary formulation specifically developed for the transfection of siRNA and Stealth™ RNAi duplexes into eukaryotic cells. Lipofectamine® RNAiMAX provides the following advantages:
Important Guidelines for Transfection
Use this procedure to forward transfect Stealth™ RNAi or siRNA into mammalian cells in a 24 well format (for other formats, see Scaling Up or Down Transfections, page 4) . In forward transfections, cells are plated in the wells, and the transfection mix is generally prepared and added the next day. Optimize transfections as described in Optimizing Transfections, (page 3), especially if transfecting a mammalian cell line for the first time. All amounts and volumes are given on a per well basis.
Note: For some cell lines (e.g. MCF-7 or HepG2), we recommend reverse transfections.
To qualitatively assess transfection efficiency, we recommend using a KIF11 Stealth™ Select RNAi (available through www.lifetechnologies.com/rnaiexpress; for human cells, oligo HSS105842 is a good choice). Adherent cells in which KIF11/Eg5 is knocked down exhibit a "rounded-up" phenotype after 24 hours due to mitotic arrest (Weil, D. et al. Biotechniques 2002, 33: 1244-1248); slow growing cells may take up to 72 hours. Alternatively, growth inhibition can be assayed after 48-72 hours. Note: The BLOCK-iT™ Fluorescent Oligo (Cat. No 2013) is optimized for use with Lipofectamine® 2000, and is not recommended for Lipofectamine® RNAiMAX.
Optimizing Transfections
To obtain the highest transfection efficiency and low non-specific effects, optimize transfection conditions by varying RNAi duplex and Lipofectamine® RNAiMAX concentrations. Test 0.6-30 pmol RNAi duplex (final concentration 1-50 nM) and 0.5-1.5 µl Lipofectamine® RNAiMAX for 24-well format. For extended time course experiments (> 72 hours), consider a cell density that is 10-20% confluent 24 hours after plating.
Note: The concentration of RNAi duplex required will vary depending on the efficacy of the duplex.
To transfect cells in different tissue culture formats, vary the amounts of Lipofectamine® RNAiMAX, RNAi duplex, cells, and medium used in proportion to the relative surface area, as shown in the table.
Culture vessel | Rel. surf. area1 | Vol. of plating medium | Dilution medium reverse transfection | Dilution medium forward transfection | RNAi (pmol) | RNAi (nM) | Lipofect-amine® RNAiMAX2 |
96-well
|
0.2
|
100 µl
|
20 µl
|
2 x 10 µl
|
0.12-6
|
1-50
|
0.1-0.3 µl
|
48-well
|
0.4
|
200 µl
|
40 µl
|
2 x 20 µl
|
0.24-12
|
1-50
|
0.2-0.6 µl
|
24-well
|
1
|
500 µl
|
100 µl
|
2 x 50 µl
|
0.6-30
|
1-50
|
0.5-1.5 µl
|
6-well
|
5
|
2.5 ml
|
500 µl
|
2 x 250 µl
|
3-150
|
1-50
|
2.5-7.5 µl
|
60 mm
|
10
|
5 ml
|
1 ml
|
2 x 500 µl
|
6-300
|
1-50
|
5-15 µ
|
100 mm
|
30
|
10 ml
|
2 ml
|
2 x 1 ml
|
12-600
|
1-50
|
15-35 µl
|
¹ Surface areas may vary depending on the manufacturer.
² If the volume of Lipofectamine® RNAiMAX is too small to dispense accurately, and you cannot pool dilutions, predilute Lipofectamine® RNAiMAX 10-fold in Opti-MEM® I Reduced Serum Medium, and dispense a 10-fold higher amount (should be at least 1.0 µl per well). Discard any unused diluted Lipofectamine® RNAiMAX.
For cotransfections of plasmid DNA and Stealth™ RNAi or siRNA into mammalian cells, we recommend using Lipofectamine® 2000 (Catalog no. 11668-027), which is superior for plasmid transfections. If you want to use Lipofectamine® RNAiMAX for your cotransfections, perform a reverse transfection as described on page 2 with the following modifications:
1: Add 20 ng (for 24-well format) of plasmid DNA to the diluted RNAi duplex.
2: Add cells such that they will be 80-100% confluent 24 hours after plating.