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Amplite® Fluorimetric Alkaline Phosphatase Assay Kit *Near Infrared Fluorescence*
Example protocol
AT A GLANCE
Protocol summary
- Prepare Alkaline Phosphatase working solution (50 µL)
- Add Alkaline Phosphatase standards and/or test samples (50 µL)
- Incubate at RT or 37°C for 30 to 120 minutes
- Monitor fluorescence intensity at Ex/Em = 620/660 nm (Cutoff = 630 nm)
Important notes
Thaw all the kit components at room temperature before starting the experiment.
PREPARATION OF STOCK SOLUTION
1. SunRed™ Substrate stock solution (250X):
Add 100 µL of double sterile H2O into the vial of SunRed™ Substrate (Component A) to make 250X SunRedTM Substrate stock solution. The stock solution should be used promptly.
2. Alkaline Phosphatase standard solution (100 U/mL):
Add 100 µL of distilled H2O with 0.1% BSA (H2O - 0.1% BSA) to Alkaline Phosphatase Standard (Component C, 10 units) to generate a 100 units/mL Alkaline Phosphatase standard solution. Note: The Alkaline Phosphatase standard solution is not stable.
PREPARATION OF STANDARD SOLUTION
For convenience, use the Serial Dilution Planner: https://www.aatbio.com/tools/serial-dilution/11954
Add 10 µL of 100 units/mL Alkaline Phosphatase standard solution to 990 µL of H2O - 0.1% BSA to generate a 1,000 mU/mL Alkaline Phosphatase standard solution. Take 1,000 mU/mL Alkaline Phosphatase standard solution and perform 1:3 serial dilutions to get serially diluted Alkaline Phosphatase standards (AS7 - AS1) with H2O - 0.1% BSA.
PREPARATION OF WORKING SOLUTION
For one 96-well plate, add 20 μL of 250X SunRed™ Substrate stock solution to 5 mL of Assay Buffer (Component B) and mix well to prepare Alkaline Phosphatase working solution . Note: Keep from light and prepare fresh reaction mixture for each experiment.
For guidelines on cell sample preparation, please visit
https://www.aatbio.com/resources/guides/cell-sample-preparation.html
SAMPLE EXPERIMENTAL PROTOCOL
Table 1. Layout of Alkaline Phosphatase Standards and test samples in a solid black 96-well microplate. AS = Alkaline Phosphatase Standards (AS1 - AS7, 0.3 to 300 mU/mL); BL=Blank Control; TS=Test Samples.
| BL | BL | TS | TS |
| AS1 | AS1 | ... | ... |
| AS2 | AS2 | ... | ... |
| AS3 | AS3 | ||
| AS4 | AS4 | ||
| AS5 | AS5 | ||
| AS6 | AS6 | ||
| AS7 | AS7 |
Table 2. Reagent composition for each well.
| Well | Volume | Reagent |
| AS1 - AS7 | 50 µL | Serial Dilution (0.3 to 300 mU/mL) |
| BL | 50 µL | H2O - 0.1% BSA |
| TS | 50 µL | test sample |
Run Alkaline Phosphatase assay in supernatants:
- Prepare Alkaline Phosphatase standards (AS), blank controls (BL), and test samples (TS) according to the layout provided in Tables 1 and 2. For a 384-well plate, use 25 µL of reagent per well instead of 50 µL.
- Add 50 µL of Alkaline Phosphatase working solution to each well of Alkaline Phosphatase standard, blank control, and test samples to make the total Alkaline Phosphatase assay volume of 100 µL/well. For a 384-well plate, add 25 µL of Alkaline Phosphatase working solution into each well instead, for a total volume of 50 µL/well.
- Incubate the reaction at for 30 to 120 minutes at the desired temperature, protected from light.
- Monitor the fluorescence increase with a fluorescence plate reader at Ex/Em = 620/660 nm (Cutoff = 630 nm).
Run Alkaline Phosphatase assay in cells:
- Treat the cells as desired.
- Remove the growth medium completely from the cell plate. Note: It is important to remove the growth medium completely from the cell plate due to the interference of the growth medium with the SunRed™ Substrate.
- Make 1:1 dilution of the 5 mL Alkaline Phosphatase working solution with 5 mL distilled H2O.
- Add 100 µL (96-well plate) or 50 uL (384-well plate) of 1:1 diluted Alkaline Phosphatase working solution into each cell well.
- Incubate the reaction for 30 to 60 minutes at the desired temperature, protected from light.
- Monitor the fluorescence increase with a fluorescence plate reader at Ex/Em = 620/660 nm (Cutoff = 630 nm).
Spectrum
Product family
| Name | Excitation (nm) | Emission (nm) | Extinction coefficient (cm -1 M -1) | Quantum yield | Correction Factor (260 nm) | Correction Factor (280 nm) |
| Amplite® Fluorimetric Alkaline Phosphatase Assay Kit *Blue Fluorescence* | 360 | 448 | - | - | - | - |
| Amplite® Fluorimetric Alkaline Phosphatase Assay Kit *Green Fluorescence* | 498 | 517 | 800001 | 0.79001, 0.952 | 0.32 | 0.35 |
Citations
Authors: Eweida, Ahmad and Schulte, Matthias and Frisch, Oliver and Kneser, Ulrich and Harhaus, Leila
Journal: Journal of Cranio-Maxillofacial Surgery (2017)
Authors: Xu, Bing and Zheng, Pengbin and Gao, Fei and Wang, Wei and Zhang, Hongtao and Zhang, Xuran and Feng, Xuequan and Liu, Wenguang
Journal: Advanced Functional Materials (2016)
Authors: Kaselis, Andrius and Treinys, Rimantas and Vosyliute, Ruta and Satkauskas, Saulius
Journal: Cellular and molecular neurobiology (2014): 289--296
Authors: Yu, Jin and Chung, Hea-Eun and Choi, Soo-Jin
Journal: Journal of Nanomaterials (2013): 12
Authors: El-Khawaga, OY and El-Waseef, A and Ellazec, YO and El-Naggar, MM and Alla, Abd M
Journal: International Journal of Genomics and Proteomics (2013): 60
References
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Journal: Cell Biol Toxicol (2006): 39
Authors: Ali AT, Penny CB, Paiker JE, Psaras G, Ikram F, Crowther NJ.
Journal: Ann Clin Biochem (2006): 207
Authors: Ali AT, Penny CB, Paiker JE, van Niekerk C, Smit A, Ferris WF, Crowther NJ.
Journal: Clin Chim Acta (2005): 101
Authors: Rieu JP, Ronzon F, Place C, Dekkiche F, Cross B, Roux B.
Journal: Acta Biochim Pol (2004): 189
Certificate of origin