Mammalian Cell Culture Homogenization Using the Bullet Blender

Materials

• Bullet Blender^® for 50 mL tubes
• Homogenization Buffer
• FoamBlocker (Optional)
• Lysis Beads
  • 0.15 mm Zirconium Oxide Beads in HIPPO tubes
• Sample — up to 3500 mg

Procedure

1. Prepare a tube with the recommended volume of bead choices from the table above.
2. If the sample has been grown on a plate or other solid surface, detach it by flooding the surface with PBS and scraping the material into a microcentrifuge tube. Centrifuge to obtain a cell pellet and resuspend in the specified volume of lysis buffer. Liquid cultures may be placed directly in the lysis tube as long as they are of sufficient density.
3. (Optional) To avoid excess foaming, add FoamBlocker up to 1-2% of the total volume of the homogenization buffer.
4. Close the tubes tightly and place into the Bullet Blender sample chamber. If using the Gold or Gold⁺ models, pre-cool the chamber before adding sample tubes.
5. Set the controls to speed 8, time 12 minutes then press Start.
   
6. After the run, remove the tubes from the instrument and visually inspect the samples. If homogenization is incomplete, homogenize for an additional 30 seconds, or repeat the homogenization step with a higher speed.
7. Using a pipette, transfer the homogenized samples into new tubes.
8. Proceed with downstream application.