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Screen Quest™ Live Cell Chemokine (CC) receptor CCR2B cAMP Assay Service Pack
Product key features
- Real-Time cAMP detection: Enables precise, live-cell measurement of intracellular cAMP changes in response to CCR2B activation without requiring cell lysis.
- Convenient: Provides all necessary components for precise measurement of CCR2B-mediated cAMP changes.
- High-Throughput: Optimized for use with FLIPR, FDSS, and other fluorescence microplate readers, making it ideal for large-scale screening of CCR2B-targeting compounds.
- Simple workflow: Utilizes wash-free calcium sensitive dyes reducing assay complexity and time.
Product description
CCR2B or Chemokine (CC) receptor type 2B, a key member of the GPCR family, is implicated in a variety of inflammatory, autoimmune diseases, cancer, fibrosis, and other pathological conditions, making it a vital therapeutic target. Traditional methods for studying GPCRs often fail to address the signaling mechanisms of specific GPCRs like CCR2B, which couple to adenylyl cyclase activity and intracellular cAMP production.
The Screen Quest™ Live Cell Chemokine (CC) Receptor CCR2B cAMP Assay Service Pack is specifically designed for real-time, high-throughput monitoring of intracellular cAMP changes associated with CCR2B activation using transfected cell lines and Calbryte™ 520 wash-free calcium fluorescence detection methods. Unlike conventional assays requiring cell lysis, this assay preserves cellular integrity, enabling both temporal and spatial resolution of specific signaling events associated with CCR2B. This assay employs cell lines transfected to express CCR2B along with a promiscuous G-protein Gα16. The Gα16 protein allows CCR2B, which primarily signals through the cAMP pathway, to also couple to Gq signal transduction and mobilize intracellular calcium. Activation of CCR2B by specific ligands, such as CCL2 (MCP-1), can be detected using calcium-sensitive dyes like Calbryte™ 520 AM, Cal-520™ AM, Fluo-8™ AM, Fluo-4™ AM, or corresponding no-wash calcium kits. The inclusion of CCR2B and Gα16 co-expression ensures robust calcium signaling for reliable assay performance.
This service pack provides all necessary components for precise measurement of CCR2B-mediated cAMP changes using FLIPR, FDSS, or equivalent fluorescence microplate readers. It is an ideal tool for studying CCR2B activity, enabling researchers to explore CCR2B signaling pathways and evaluate potential therapeutic compounds targeting this receptor.
Example protocol
AT A GLANCE
Prepare cells for transfection
Prepare Transfectamine™ 5000-DNA mixture
Add Transfectamine™ 5000-DNA mixture to the cell culture, incubate overnight
Transfer the transfected cells to a 96-well plate 24-30 hours after transfection, and incubate the culture overnight
Add Calbryte™ 520 NW dye-loading solution
Incubate at room temperature or 37 °C for 30-60 minutes
Monitor the fluorescence intensity at Ex/Em = 490/525 nm
Thaw the kit components at room temperature before starting the experiment.
CELL PREPARATION
Seed the cells such that they will be ~60-70% confluent at the time of transfection.
Replace with fresh growth medium before transfection. 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
Add 20 µL of DMSO (Component F) into the vial of Calbryte™ 520NW (Component C), and mix them well.
Note: 20 µL of Calbryte™ 520NW stock solution is enough for one plate. Unused Calbryte™ 520NW stock solution can be aliquoted and stored at < -20 °C for more than one month, provided the tubes are tightly sealed. Protect from light and avoid repeated freeze-thaw cycles.
PREPARATION OF WORKING SOLUTION
- Combine 9 mL of HHBS (Component E) with 1 mL of 10X Pluronic® F127 Plus (Component D), and mix thoroughly.
Add 20 µL of Calbryte™ 520 NW stock solution to 10 mL of 1X Assay Buffer, and mix well.
Note: The working solution is stable for at least 2 hours at room temperature.
Add 15 µL of ddH2O to the vial of Ga16 DNA (Component A) and CCR2B DNA (Component G), to get the final concentration of 1 µg/µL for both DNAs.
Mix 3 µg of DNA [for example, 1.5 µg of Ga16 DNA (Component A) and 1.5 µg of CCR2B DNA (Component G)] with 200 µL of serum-free medium.
Add 9 µL of Transfectamine™ 5000 (Component B) to the mixture from Step 2.
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, the ratio for Transfectamine™ 5000 Transfection Reagent (µL) to DNA (µg) should be 3-5 µL : 1 µg.
Table 1. Sample protocols 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 | 10~15 µg |
| Serum-free medium | 200 µL | 600 µL |
| Transfectamine™ 5000 Transfection Reagent | ~9 µL | ~30-45 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 post transfection and incubate overnight.
- For adherent cells: Plate cells overnight in the growth medium at 40,000 to 80,000 cells/well/100 µL for a 96-well plate.
- For non-adherent cells: Centrifuge the cells from the culture medium and then suspend the cell pellet in cell growth medium or HHBS at 125,000 to 250,000 cells/well/100 µL for a 96-well poly-D lysine plate. Centrifuge the plate at 800 rpm for 2 minutes with brake off prior to the experiments.
Note: Each cell line should be evaluated on the individual basis to determine the optimal cell density for the intracellular calcium mobilization.
Add 100 µL/well (96-well plate) of Calbryte™ 520NW working solution into the cell plate.
Incubate the dye-loaded plate in a cell incubator for 30 minutes, and then incubate the plate at room temperature for another 15-30 minutes.
Note: If the assay requires 37 °C, perform the experiment immediately without further room temperature incubation.
Note: If the cells can function well at room temperature for longer time, incubate the cell plate at room temperature for 1 hour (It is recommended that the incubation time be no longer than 2 hours.)
Prepare the compound plate with HHBS or your desired buffer.
Run the calcium flux assay by monitoring the fluorescence intensity at Ex/Em = 490/525 nm.
References
Authors: Feigl, Frederik Fabian and Stahringer, Anika and Peindl, Matthias and Dandekar, Gudrun and Koehl, Ulrike and Fricke, Stephan and Schmiedel, Dominik
Journal: International journal of molecular sciences (2023)
Authors: Wang, Yanan and Wang, Jing and Yang, Xinyi and Yang, Jinlong and Lu, Panpan and Zhao, Lin and Li, Bokang and Pan, Hanyu and Jiang, Zhengtao and Shen, Xiaoting and Liang, Zhiming and Liang, Yue and Zhu, Huanzhang
Journal: Frontiers in immunology (2021): 628906
Authors: Li, Guangchao and Zhang, Qing and Han, Zeping and Zhu, Yangmin and Shen, Huijuan and Liu, Zhi and Zhou, Zhao and Ding, Wen and Han, Siqi and He, Jinhua and Yin, Zhao and Zhou, Jie and Ou, Ruiming and Luo, Min and Liu, Shuang
Journal: Frontiers in oncology (2021): 734593
Authors: Markx, Daniel and Schuhholz, Julia and Abadier, Michael and Beier, Sandra and Lang, Mariana and Moepps, Barbara
Journal: Cellular signalling (2019): 170-183
Authors: Kozireva, Svetlana and Rudevica, Zhanna and Baryshev, Mikhail and Leonciks, Ainars and Kashuba, Elena and Kholodnyuk, Irina
Journal: Viruses (2018)
Safety data sheet