Team:Bielefeld-Germany/Labjournal/week21

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Week 21 (09/17 - 09/23/12)

Monday September 17th

Team Cultivation & Purification:
- Cell disruption of fermentation of E. coli Rosetta-Gami 2 with BBa_K863012 via high-pressure homogenization and purification via Ni-NTA column.

Tuesday September 18th

Team Cellulose Binding Domain:
- Primer arrived:
- Gradient-PCR with the CBDcex(T7)+GFP_His-plasmid and S3N10-CBDcex_RV and S3N10-GFP_FW primer-mix. the right product appeared only at 66,5°C; Lower: wrong product; Higher: no product
  - Following PCR at 66,5°C(50µL) had the wrong product (main product at 2 kbp); could be because of a different template concentration or not exact temperature.
  - Alternativly took the 20 µL-tube with right product and added 0,5 µL DpnI for over-night digestion.
- Gradient-PCR with CBDcex(T7)+GFP_His-template and a CBDcex_Freiburg- + GFP_Freiburg_compl-primer-mix to amplify the whole fusion-protein and get rid of the His-tag.
- Gradient-PCR with CBDclos(T7)+GFP_His-template and a CBDclos_Freiburg- + GFP_Freiburg_compl-primer-mix to amplify the whole fusion-protein and get rid of the His-tag.

Wednesday September 19th

Team Cellulose Binding Domain:
- Stopped over-night-DpnI-digestion of S3N10-clos-GFP_his PCR-product and cleaned up in gel. Ligated the PCR-product with itself via Blunt-end-ligation and transformed it into KRX. Plated on Select-Agar.
- Gradient-PCRs of the CBDcex(T7)+GFP_His-plasmid and a CBDclos(T7)+GFP_His-plasmid (unsequenced) with the CBDcex_Freiburg- and GFP_Freiburg-compl- and the CBDclos_Freiburg- and GFP_Freiburg_compl primers, respectively. The CBDcex-setup showed no correct product, but the CBDclos-setup had the right bands at temperatures from 57°C to 64°C; Merged the correct fractions and cleaned them up through the gel.
- Digested the cleaned-up product with SpeI and XbaI and DpnI.
- Ligated <partinfo>J61101</partinfo> and CBDclos_Freiburg with GFP_Freiburg and transformed it into KRX.

Thursday September 20th

Team Cellulose Binding Domain:
- No Colonies on the S3N10-CBDclos(T7)+GFP_His-transformations-dish with the blunt-end ligation; reason: forgotten to phosphorylate the PCR-product.
- Two colonies on the CBDclos+GFP-dish with the constitutive J23100 + J61101 promoter. But none of them is glowing. And them shouldn't ... used the wrong selection-agar (since J61101 carries pSB1A2-backbone with AMP-resistence.

Friday September 21st

Team Cellulose Binding Domain:
- Transformated <partinfo>J61101</partinfo> with CBDclos+GFP again and plated on the right selection-agar this time!

Saturday September 22nd

Team Cellulose Binding Domain:
- Once again two colonies on the agar-dish: can not say if they have a green glow...
  - picked the colonies and them put into AMP-LB-Medium.
- Also made a flask with 10 mL LM-Medium and Cells with the CBDcex(J61101)+GFP_His-plasmid

Sunday September 23rd

Team Cellulose Binding Domain:
- All cultures did not show any sign of GFP-glow under uv-light.

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Fifteen students from different fields of study from the Bielefeld University aspired to complete a project called TOXIC COMPOUNDS IN NATURAL WATER - A CASE FOR LACCASE. In his Wiki we document our achievements and our approach.

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