How to Prepare GelMA Bioink (Sterile-Solution)
Overview
GelMA is a highly used material in bioprinting due to its mechanical properties and printability. However, methacrylating gelatin in the lab is an inconveniently time-consuming process. In addition, buying lyophilized GelMA to make it into the desired w/v concentration and sterile-filtering it in the lab is extremely cumbersome and inefficient. This protocol provides you with instructions on how to prepare sterile 20% w/v GelMA bioink solution that is ready to be easily mixed with your cell suspension and LAP (or photoinitiator of choice).
Materials
· 1.5 mL 20% w/v GelMA
· 0.05 g LAP (or photoinitiator of choice)
· Allevi Sterile Syringe (5 mL or 10 mL)
· Sterile Syringe coupler
· Amber or Aluminum Foil Wrapped Glass Container
· 0.22 µm filter
· Cell Media
· Centrifuge Tubes
· Micropipettes
· Micropipette Tips
· 70% Ethanol
· Kimwipes
· Stirring Hot Plate
· Water/Bead Bath (37˚C)
Methods: Prepare GelMA Bioink (sterile-solution)
Our recommended GelMA print concentration is 10% w/v (with 0.5% w/v LAP), so you will need to mix your 20% w/v sterile GelMA 1:1 with a photoinitiator-cell solution.
- Place your GelMA syringe in a water bath at 37˚C;
- Note: Our 20% w/v sterile GelMA Solution should only go through only one freeze-thaw cycle before use.
- Aliquot 0.02 g of LAP in a glass container;
- Note: Ensure that your glass container is either amber or tightly wrapped with aluminum to prevent premature photoinitiator activation.
- Add 2 mL of cell media;
- Place a stirrer in your vial and leave it on the hot plate at 60˚C until all LAP is dissolved (15-30 min);
- Note: Ensure that your container is tightly sealed to avoid evaporation.
- Take your LAP solution into a biosafety cabinet, ensuring to spray everything down with 70% ethanol;
- Pull up your solution into a sterile syringe;
- Using the plunger, carefully push the solution up until you see a meniscus form over the tip of the syringe;
- Note: If there are bubbles trapped in the system, tapping the syringe may help make the bubbles surface.
- Attach the sterile filter to the syringe;
- Push the plunger and place you filtered solution into a sterile centrifuge tube;
- Prepare a cell pellet by following this protocol;
- Ensuring that you have enough cells to yield your desired final cell concentration, pipette 2 mL of your LAP solution onto your cell pellet;
- Example: If you wish to use a concentration 2.5 x 106 cells/mL and the final bioink volume will be 3 mL, you will need a total of 7.5 million cells in the 1.5 mL of LAP-cell solution that will be mixed with the GelMA syringe. Since you are preparing 2 mL of LAP-cell solution, you will need a cell pellet containing 10 million cells.
- Pipette this solution up and down to ensure thorough mixing of cells in media;
- Load 1.5 mL of LAP-cell solution into an empty sterile syringe;
- ollow this protocol on Cell-Bioink Mixing to mix your LAP-cell solution with GelMA;
- Follow this protocol on how to load your GelMA for bioprinting, and this protocol on how to bioprint GelMA.