Preparation of Collagen-Coated Compartmented Culture Dishes for Neuronal Cell Culture
Published: August 30, 2024
Abstract
Source: Zepecki, J. P., et al. Real-Time monitoring of human glioma cell migration on dorsal root ganglion axon-oligodendrocyte co-cultures. J. Vis. Exp. (2019)
This video demonstrates constructing a three-compartment cell culture system using collagen and non-reactive grease. This system is used to observe interactions between glioma cells and axons in real-time.
Protocol
- Compartmented culture of Rat Dorsal Root Ganglia (DRGs), Oligodendrocytes (OPCs), and hGCs (human glioma cells)
1. Preparation of compartmented culture dishes
NOTE: Perform the following steps the days before the planned harvest of the DRGs.
- Assemble compartmented culture dishes.
- Dilute collagen stock solution to 500 µg/mL in sterile distilled H2O; mix thoroughly.
- With a sterile transfer pipette, fill a 35 mm culture dish with 2 mL of collagen solution; remove the solution, leaving a thin collagen film behind, and place it into the next 35 mm dish. Repeat this process, adding more collagen solution as needed, until all dishes have been coated.
- Once all plates are coated, place the plates in a 245 mm x 245 mm culture tray and lay three 1 mm x 1 mm gauze pads in the center of the tray.
- To polymerize the collagen, wet gauze pads with 1 mL of concentrated ammonium hydroxide and cover the trays for 15 min.
- Remove the gauze pads and allow the 35 mm dishes to dry in the laminar flow hood.
- While dishes are drying, load the barrel of the syringe grease applicator with high vacuum grease. Place the compartmented chambers in a large mouth media bottle filled with distilled water. Sterilize both by autoclaving and allow to cool.
- File off the point of an 18-G needled to make a blunt tip. Sterilize in 70% ethanol. Attach the needle to the grease syringe.
- Sterilize the pin rake by soaking it in 70% ethanol; allow it to air-dry in the laminar flow hood.
- Remove the lid from a dry, collagen-coated 35 mm dish. Hold the dish between the thumb and pointer finger. Hold the pin rake with the other hand. Apply a firm pressure to create even 200 µM wide scratches across the center of the dish.
- Using a pasture pipette, place two drops of Supplemented Neuronal Basal Medium in the center of the scratches.
- Repeat steps 1.1.10-1.1.11 until all dishes have been scratched.
- Dry the compartmented chambers in a laminar flow hood.
- With sterile hemostatic forceps, grasp one compartmented chamber by the center divider. Flip the hemostatic forceps so the bottom of the chamber is facing up.
- Apply silicone grease to the compartmented chamber, starting at the top. Ensure that grease is placed neatly and overlaps at all corners.
- Remove the lid from a 35 mm dish. Invert the dish and place the scratches over the chamber. Tap down on the bottom of the plate gently with a pair of forceps.
- Gently flip the plate over by using the hemostatic forceps. Release the forceps.
- Place a mound of grease at the base of the center compartment. Fill each chamber with Supplemented Neuronal Basal Medium (NB) and check for leaks. Seal leaks with silicone grease as needed.
- Continue assembling all culture dishes and store overnight at 37°C, 5% CO2.
Divulgations
The authors have nothing to disclose.
Materials
| Cell Culture Dish | Corning | 430165 | 35mm X 10mm |
| Hypodermic Needle, 18G | BD | 511097 | |
| Ammonium Hydroxide Solution | Fisher Scientific | A669-500 | Concentrated |
| Cell Culture Dish | Corning | 430165 | |
| Campenot Chamber | Tyler Research | CAMP-10 | |
| Hemostatic Forceps | Roboz | RS-7035 | |
| Cultrex Rat Collagen I | Trevigen | 3440-100-01 | |
| Pin Rake | Tyler Research | CAMP-PR | |
| Neurobasal Medium | Thermo Fisher | 21103049 | |
| silicone grease | |||
| metal file | |||
| Tray | |||
| gauze | |||
| CO2 incubator | |||
| glass pipette |
Citer Cet Article
Preparation of Collagen-Coated Compartmented Culture Dishes for Neuronal Cell Culture. J. Vis. Exp. (Pending Publication), e22536, doi: (2024).