Team:Warsaw/Calendar-Main/3 June 2008

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Preparation of T7 constructs

Michał K.:

  1. DNA (PCR products from previous day) gel electrophoresis and isolation of DNA from proper band.
  2. Digest of DNA with HindIII and SalI (2x Tango buffer).
  3. Digest of pMPM-T5 + AID with HindIII and SalI.
  4. Clean-up of reaction products.
  5. Ligation of p.4 products (pMPM-T5 + AID transcription fusion with AID-T7 RNA-polymerase translation fusion).
  6. Transformation of E.coli TOP10 with ligation product.
  7. Plating transformants on LB+tetracycline.
  8. Digest of pMPM-T5 + transcription fusion with EcoRHI and HindIII.
  9. Use of T4 polymerase for blunting.
  10. DNA gel electrophoresis.
  11. Isolation of DNA from proper band.
  12. Ligation of product p.11 (pMPM-T5 + T7 RNA-polymerase).
  13. Transformation of E.coli TOP10 with ligation product.
  14. Plating transformants on LB + tetracycline.