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Protocol for Malanga Root Tuber
                  Homogenization in the Bullet Blender™
The protocol described in this document is for the use of the Bullet Blender™ for the
homogenization of malanga (Xanthosoma sagittifolium) root tubers. This protocol does not
specify a particular buffer - you may choose which is most appropriate for your
downstream application (nucleic acid isolation, protein extraction, etc.).

Materials Required:      Malanga tuber, Bullet Blender™, homogenization buffer,
                         pipettor, microcentrifuge tubes, and 0.9-2.0mm stainless steel
                         bead blend or 1.0mm zirconium oxide beads (SSB14B or
                         ZROB10)
Instructions
  1. OPTIONAL: Wash malanga 3x with ~1mL PBS to remove soil and other surface
      contaminants and debris.
  2. Cut malanga into long, thin slices of 200mg or less and place each slice into a
      microcentrifuge tube.
  3. Add a mass of the stainless steel bead blend equal to 3x the mass of malanga, or a
      mass of 1.0mm zirconium oxide beads equal to 2x the mass of malanga.
  4. Close the microcentrifuge tubes and place them into the Bullet Blender™. NOTE:
      There should be no buffer in the tubes at this point.
  5. Set controls for SPEED 8 and TIME 4.
  6. Remove the samples from the Bullet Blender. The malanga should be finely
      pulverized into a thick paste. If not, run for another three minutes at speed 10.
  7. Add 2 volumes of buffer to the tube for every mass of sample (ex. for 100 mg
      malanga add 200µL buffer).
  8. Close the microcentrifuge tubes and place them back into the Bullet Blender™.
  9. Set controls for SPEED 8 and TIME 3 minutes. Press Start.
  10. After the run, remove tubes from the instrument.
  11. Visually inspect samples. If homogenization is unsatisfactory, run for another three
      minutes at speed 10.
  12. Proceed with your downstream application.

                                 SAFETY NOTE!!!
      When using a centrifuge to separate your homogenate from the
         debris and beads, make sure your tubes are balanced.




          Before                     Pulverized                            After
Date 11/23/2009                                                          Next Advance, Inc.
                                                      24 Prospect Avenue, Averill Park, NY 12018 USA
                                    Phone (518) 674-3510 Fax (518) 674-0189 www.nextadvance.com

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Bullet_Blender_Homogenizer_Protocol_Homogenization_Malanga_Root_Tuber_Xanthosoma_sagittifolium

  • 1. Protocol for Malanga Root Tuber Homogenization in the Bullet Blender™ The protocol described in this document is for the use of the Bullet Blender™ for the homogenization of malanga (Xanthosoma sagittifolium) root tubers. This protocol does not specify a particular buffer - you may choose which is most appropriate for your downstream application (nucleic acid isolation, protein extraction, etc.). Materials Required: Malanga tuber, Bullet Blender™, homogenization buffer, pipettor, microcentrifuge tubes, and 0.9-2.0mm stainless steel bead blend or 1.0mm zirconium oxide beads (SSB14B or ZROB10) Instructions 1. OPTIONAL: Wash malanga 3x with ~1mL PBS to remove soil and other surface contaminants and debris. 2. Cut malanga into long, thin slices of 200mg or less and place each slice into a microcentrifuge tube. 3. Add a mass of the stainless steel bead blend equal to 3x the mass of malanga, or a mass of 1.0mm zirconium oxide beads equal to 2x the mass of malanga. 4. Close the microcentrifuge tubes and place them into the Bullet Blender™. NOTE: There should be no buffer in the tubes at this point. 5. Set controls for SPEED 8 and TIME 4. 6. Remove the samples from the Bullet Blender. The malanga should be finely pulverized into a thick paste. If not, run for another three minutes at speed 10. 7. Add 2 volumes of buffer to the tube for every mass of sample (ex. for 100 mg malanga add 200µL buffer). 8. Close the microcentrifuge tubes and place them back into the Bullet Blender™. 9. Set controls for SPEED 8 and TIME 3 minutes. Press Start. 10. After the run, remove tubes from the instrument. 11. Visually inspect samples. If homogenization is unsatisfactory, run for another three minutes at speed 10. 12. Proceed with your downstream application. SAFETY NOTE!!! When using a centrifuge to separate your homogenate from the debris and beads, make sure your tubes are balanced. Before Pulverized After Date 11/23/2009 Next Advance, Inc. 24 Prospect Avenue, Averill Park, NY 12018 USA Phone (518) 674-3510 Fax (518) 674-0189 www.nextadvance.com