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Cell Meter™ Beta-Arrestin Translocation GPCR Signaling Kit
Example protocol
AT A GLANCE
- Prepare cells for transfection
- Prepare Transfectamine™ 5000-DNA mixture
- Add Transfectamine™ 5000-DNA mixture to cell culture, and incubate overnight
- Transfer the transfected cells to a 96-well plate 24-30 hours after transfection, and incubate the culture overnight
- Analyze translocation induced by GPCR activation under a fluorescence microscope
Thaw all the components at room temperature before starting the experiment.
CELL PREPARATION
- Seed the cells at a density such that they will be ~60-70% confluent at the time of transfection.
Replace with fresh growth medium before transfection.
Note: For example, replace with 2 mL of medium per well for 6-well plates and 6 mL of medium for 10 cm plates.
PREPARATION OF STOCK SOLUTIONS
Unless otherwise noted, all unused stock solutions should be divided into single-use aliquots and stored at -20 °C after preparation. Avoid repeated freeze-thaw cycles
Add 15 µL of ddH2O to the vial of beta-arrestin-GFP DNA (Component A), mix well to have the final concentration of 1 µg/µL.
PREPARATION OF WORKING SOLUTION
- Mix 3 µg of DNA [for example, 1.5 µg of Beta-arrestin-GFP DNA stock solution and 1.5 µg DNA of the GPCR that you are interested] with 200 µL of serum-free medium.
- Add 9 µL of Transfectamine™ 5000 (Component B) to the mixture.
Mix well and incubate at room temperature for 20 minutes.
Note: The ratio of Transfectamine™ 5000 and DNA need to be optimized for different cell lines, in general, in our testings, the ratio for Transfectamine™ 5000 Transfection Reagent (µL) to DNA (µg) Ratio should be 3-5 µL : 1 µg.
Table 1. Sample rprotocols for a 6-well plate and a 10 cm plate
| Component | 6-well plate (per well) | 10 cm plate |
| Fresh culture medium | 2 mL | 6 mL |
| Plasmid | 3 µg | 10 µg |
| Serum-free medium | 200 µL | 600 µL |
| Transfectamine™ 5000 Transfection Reagent | ~9 µL | ~30 µL |
SAMPLE EXPERIMENTAL PROTOCOL
Add Transfectamine™ 5000 -DNA mixture to the culture plate and incubate overnight.
Note: The recombinant protein can start to be detected as early as 16 hours after transfection. The maximal expression level may be observed 72~96 hours after transfection.
- Transfer the transfected cells to a 96-well plate 24-30 hours after transfection and incubate overnight.
- Monitor the beta-arrestin translocation induced by the receptor activation under a fluorescence microscope with the FITC filter (Ex/Em = 488/530 nm).
References
Authors: Logan, David J and Carpenter, Anne E
Journal: Journal of biomolecular screening (2010): 840-6
Authors: Doucette, Christopher and Vedvik, Kevin and Koepnick, Elizabeth and Bergsma, Aaron and Thomson, Brian and Turek-Etienne, Tammy C
Journal: Journal of biomolecular screening (2009): 381-94
Authors: Ross, D A and Lee, S and Reiser, V and Xue, J and Alves, K and Vaidya, S and Kreamer, A and Mull, R and Hudak, E and Hare, T and Detmers, P A and Lingham, R and Ferrer, M and Strulovici, B and Santini, F
Journal: Journal of biomolecular screening (2008): 449-55
Authors: Oakley, Robert H and Hudson, Christine C and Sjaastad, Michael D and Loomis, Carson R
Journal: Methods in enzymology (2006): 50-63
Authors: Hudson, Christine C and Oakley, Robert H and Sjaastad, Michael D and Loomis, Carson R
Journal: Methods in enzymology (2006): 63-78
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