DNA synthesis–based cell proliferation assay
In this assay the modified thymidine analogue EdU (5-ethynyl-2′-deoxyuridine, a nucleoside analog of thymidine) is efficiently incorporated into newly synthesized DNA and fluorescently labeled with a bright, photostable Alexa Fluor® dye in a fast, highly specific, mild click reaction.
This protocol can be used for:
- Detecting DNA synthesis using a fluorescence microscope
This protocol should not be used for:
- Flow cytometry; for a flow cytometry protocol, see Click-iT® EdU Protocol for Flow Cytometry
You will need the following for this protocol:
- Click-iT® Plus EdU Imaging Kit (Cat. Nos. C10637, C10638, C10639, C10640)
- PBS (Cat. No. 10010-023)
- Fixative (e.g., 3.7% Formaldehyde in PBS, Cat. No. R37602)
- Permeabilization reagent (e.g., 0.5% Triton® X-100 in PBS, Cat. No. R37602)
- 3% bovine serum albumin (BSA) in PBS (3% BSA in PBS), pH 7.4
- Deionized water
- 18 x 18-mm coverslips
- Optional: 6-well microplate
Protocol
Prepare stock solutions
- Allow vials to warm to room temperature
- Add 2 mL DMSO (Component C) or an aqueous solution to Component A to make a 10 mM EdU stock solution. Store at –20°C
- Make 1X Click-iT® EdU reaction buffer by transferring the solution (4 mL) in the Component D bottle to 36 mL of deionized water. Store any remaining solution at 2–8˚C
- Make 10X Click-iT® EdU buffer additive by adding 2 mL deionized water to Component F and mixing until fully dissolved. Store at –20°C
- Dilute Hoechst® 33342 (Component G) 1:2,000 in PBS to obtain a 1X solution
Label cells with EdU
- Plate cells on coverslips and incubate overnight
- Dilute 10 µL of 10 mM EdU stock solution in 5 mL of prewarmed tissue culture medium to make a 20 µM EdU labeling solution (enough for 10 coverslips)
- Remove half of the medium from cells
- Replace with an equal volume of EdU labeling solution (final concentration of 10 µM)
- Incubate cells under appropriate growth conditions for two hours. NOTE: the choice of incubation time depends on the cell growth rate; thus optimization may be required
- Proceed immediately to fixation and permeabilization
Fix and permeabilize cells
- Transfer each coverslip into one well of a 6-well plate
- Add 1 mL of 3.7% formaldehyde in PBS to each well
- Incubate for 15 minutes at room temperature
- Remove formaldehyde and wash twice with 1 mL of 3% BSA in PBS
- Remove wash solution and add 1 mL of 0.5% Triton® X-100 in PBS to each well
- Incubate for 20 minutes at room temperature
ERK2 A375 GFP expressing cells labeled with Click-iT® Plus EdU Alexa Fluor® 647 Imaging Kit (pink), Proliferating cells have pink nuclei. Non-proliferating cells have blue nuclei.
Detect EdU
- Make 1X Click-iT® EdU buffer additive by diluting the 10X solution created above 1:10 in deionized water. Prepare this solution fresh and use the solution on the same day.
- Prepare Click-iT® Plus reaction cocktail according to the table below. IMPORTANT: add the ingredients in the order listed in the table.
- Remove permeabilization buffer from cells and wash twice with 1 mL of 3% BSA in PBS
- Remove the wash solution
- Add 0.5 mL of Click-iT® Plus reaction cocktail to each well. Rock the plate briefly to ensure even distribution of reaction cocktail
- Incubate the plate for 30 minutes at room temperature, protected from light
- Remove the reaction cocktail and wash each well once with 1 mL of 3% BSA in PBS
| Reaction components* |
Number of coverslips
| ||||||
|---|---|---|---|---|---|---|---|
| 1 | 2 | 4 | 5 | 10 | 25 | 50 | |
| 1X Click-iT® reaction buffer | 440 µL | 880 µL | 1.84 mL | 2.25 mL | 4.4 mL | 10.9 mL | 21.9 mL |
| Copper protectant | 10 µL | 20 µL | 40 µL | 50 µL | 100 µL | 250 µL | 500 µL |
| Alexa Fluor® picolyl azide (Component B) | 1.2 µL | 2.5 µL | 5 µL | 6 µL | 12.5 µL | 31 µL | 62 µL |
| 1X Click-iT® EdU buffer additive | 50 µL | 100 µL | 200 µL | 250 µL | 500 µL | 1.25 mL | 2.5 mL |
| Total volume | 500 µL | 1 mL | 2 mL | 2.5 mL | 5 mL | 12.5 mL | 25 mL |
| *Note: Add the ingredients in the order listed in the table. | |||||||
Stain DNA
- Wash each well with 1 mL of PBS. Remove the wash solution
- Add 1 mL of 1X Hoechst® 33342 solution per well
- Incubate for 30 minutes at room temperature, protected from light
- Remove the Hoechst® 33342 solution
- Wash each well twice with 1 mL of PBS
- Remove the wash solution
- OPTIONAL: Perform antibody labeling of the samples at this time, following the recommendations from the manufacturer of the primary and secondary antibody. Note: protected samples from light during these incubations.
Image
- Cells labeled with Click-iT® Plus EdU are compatible with all methods of slide preparation including wet mount or prepared mounting media
- Image cells with appropriate filters listed below
| Hoechst® 33342 | Alexa Fluor® 488 | Alexa Fluor® 555 | Alexa Fluor® 594 | Alexa Fluor® 647 | |
|---|---|---|---|---|---|
| Excitation/Emission (in nm) | 350/461 | 495/519 | 555/565 | 590/615 | 650/670 |
| Standard filter set | DAPI | FITC | RFP | TRITC | Cy®5 |