Amplite® Gaussia Luciferase Reporter Gene Assay Kit *Bright Glow*
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Unit Size | |
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Telephone | 1-800-990-8053 |
Fax | 1-800-609-2943 |
sales@aatbio.com | |
Quotation | Request |
International | See distributors |
Shipping | Standard overnight for United States, inquire for international |
Certificate of Origin | Download PDF |
H-phrase | H303, H313, H333 |
Hazard symbol | XN |
Intended use | Research Use Only (RUO) |
R-phrase | R20, R21, R22 |
UNSPSC | 41105331 |
Overview | ![]() ![]() |
Platform
Luminescence microplate reader
Recommended plate | Solid white |
Components
Example protocol
AT A GLANCE
- Prepare samples (50 µL)
- Add 50 µL Gaussia Luciferase working solution
- Incubate at room temperature for 10 - 15 minutes
- Monitor luminescence intensity
CELL PREPARATION
For guidelines on cell sample preparation, please visit https://www.aatbio.com/resources/guides/cell-sample-preparation.html
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
Transfer 50 µL (for Cat#12530), 0.5 mL (for Cat#12531) or 2.5 mL (for Cat#12532) of Reaction Buffer (Component B) into 1 vial of Luciferase Substrate (Component A), and mix well. Note: Prior to addition, centrifuge briefly before opening the vial of Luciferase Substrate (Component A).
PREPARATION OF WORKING SOLUTION
Dilute 100X Gaussia Luciferase assay stock solution using 1:100 dilution factor with Assay Buffer (Component C) to prepare Gaussia Luciferase working solution.
Note The reconstituted Gaussia luciferase working solution is very sensitive to light. It is not stable, should be prepared fresh, kept on ice, and used within 2 hours.
SAMPLE EXPERIMENTAL PROTOCOL
- Treat cells (or samples) with test compounds by adding 10 µL of 10X test compounds (96-well plate) or 5 µL of 5X test compounds (384-well plate) in desired compound buffer. For blank wells (medium without the cells), add the corresponding amount of compound buffer.
Incubate the cell plates in a 37 °C, 5% CO2 incubator for a desired period of time, typically 4 hours to overnight.
- Run Gaussia Luciferase Assay: Pipette 50 µL/well/96-well plate or 12.5 µL/well/384-well plate of the serial diluted Gaussia Luciferase or culture supernatant into a microtiter plate, and then mix with 50 µL/well/96-well plate or 12.5 µL/well/384-well plate of the Gaussia Luciferase working solution.
- Incubate the plate at room temperature for 10 to 15 minutes, protected from light.
- Read luminescence intensity with a luminometer.
Images
Citations
Authors: Wei, Zhengxi and Sakamuru, Srilatha and Zhang, Li and Zhao, Jinghua and Huang, Ruili and Kleinstreuer, Nicole C and Chen, Yanling and Shu, Yan and Knudsen, Thomas B and Xia, Menghang
Journal: Chemical research in toxicology (2019)
References
Authors: Chung E, Yamashita H, Au P, Tannous BA, Fukumura D, Jain RK.
Journal: PLoS One (2009): e8316
Authors: Patel KG, Ng PP, Kuo CC, Levy S, Levy R, Swartz JR.
Journal: Biochem Biophys Res Commun (2009): 971
Authors: Santos EB, Yeh R, Lee J, Nikhamin Y, Punzalan B, La Perle K, Larson SM, Sadelain M, Brentjens RJ.
Journal: Nat Med (2009): 338
Authors: Enjalbert B, Rachini A, Vediyappan G, Pietrella D, Spaccapelo R, Vecchiarelli A, Brown AJ, d'Enfert C.
Journal: Infect Immun (2009): 4847
Authors: Kim SB, Sato M, Tao H.
Journal: Anal Chem (2009): 67
Authors: Tannous BA., undefined
Journal: Nat Protoc (2009): 582
Authors: Maguire CA, Deliolanis NC, Pike L, Niers JM, Tjon-Kon-Fat LA, Sena-Esteves M, Tannous BA.
Journal: Anal Chem (2009): 7102
Authors: Ruecker O, Zillner K, Groebner-Ferreira R, Heitzer M.
Journal: Mol Genet Genomics (2008): 153
Authors: Inouye S, Sahara Y.
Journal: Biochem Biophys Res Commun (2008): 96
Authors: Shao N, Bock R.
Journal: Curr Genet (2008): 381
Application notes
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