Team:Wageningen UR/Protocol/RoundupHepB

From 2012.igem.org

Revision as of 13:23, 24 September 2012

• Home
• Team
  • The Team
  • Team Registration
• Project
  • 1. Introduction
  • 2. PnA System
  • 3. Virus-Like Particles
    • CCMV
    • HepB
    • Polerovirus Natural BioBrick
  • 4. Outside Modification
  • 5. Inside Modification
  • 6. Detection of VLPs
  • 7. Applications
  • 8. The Constructor
  • 9. Final Overview
• Human Practices
  • Human Practices Home
  • 1. Mini Symposium
  • 2. Visiting Secondary Schools
  • 3. Discovery Festival
    • Communication Science
  • 4. Stakeholders
  • 5. Munich CAS Conference
• Safety
  • Introduction
  • 1. General safety
  • 2. Virus-related safety
  • 3. Regulations
  • 4. Safety suggestions
  • 5. Safety of applications
• Modeling
  • Human Body Model
  • Tertiary folding prediction
  • VLP assembly model
• Attributions
• Parts
• Notebook
  • Journal
  • Protocols

---

Last year's project: Synchronized Oscillatory System

iGEM Home

Contact Us

Our Sponsors:

Materials:

• Pipettes + Pipette tips
• Eppendorf tubes
• Greiner tubes
• Centrikon or a similar ultracentrifuge + all additional equipment

Procedure

1. Cut the knot of the dialysis tubing and empty the content into a clean 50 mL Greiner tube
2. Prepare a Centrikon T-1055 ultra-centrifugation vessel and use a TFT 65.13 rotor, fill the vails with 4 ml of the sample
3. Gently put 4 mL of a 20% Sucrose in demiwater solution under the 4 mL sample
4. Balance the vails with reassembly buffer
5. Centrifuge at 45000 rpm for 3 h, remember the orientation of the vessel so you know where to look for the pellet
6. Take a sample from the supernatant (for Western blotting) and decant the rest (supernatant also contains single subunits)
7. A transparent pellet should be visible
8. Resuspend/ dissolve the pellet in 200 uL of Formation Buffer