Team:Grenoble/Biology/Notebook/June/week 28
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We also planned to realise the gibson assemblies for the first constructions. | We also planned to realise the gibson assemblies for the first constructions. | ||
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<h2> Monday, July 09<span class="exposant">th</span>:</h2> | <h2> Monday, July 09<span class="exposant">th</span>:</h2> | ||
Precultured cells are prepared: | Precultured cells are prepared: |
Revision as of 14:29, 6 August 2012
Week 27: July 02nd to July 08th
Goal of the week
we wanted to recover and amplify the biobricks involved in our genetic networks:- pAra/Bad_RBS_GFP (1300bp)
- RBS_Cya (2600bp)
- pLAC (100bp)
- fha (80bp)
- eCFP (800bp)
- pLAC_RBS (120bp)
- RsmA (200bp)
- rsmY (170bp)
- pSB1A3 (2400bp)
- pSB4K5 (2400bp)
- pSB3C5 (2400bp)
Monday, July 09th:
Precultured cells are prepared:- Strains = BW25113 WT and BW25113 cya- pAra/Bad
- Conditions = LB liquid medium, 37°C, 200rpm, overnight
Tuesday, July A0th:
For the PCRs, we changed the enzyme from GoTaq to High Fidelity (HF) Phusion.We did some colony PCR with a HF Phusion enzyme (protocol) to amplify:
- fha1, RsmA, rsmY and pSB1A3 from iGEM Grenoble 2011 glycerol stock.
- pAra/Bad_RBS_GFP from BW25113 cya- pAra/Bad precultured cells.
- RBS_Cya from BW25113 WT precultured cells.
To separate the PCR products, we prepared two gels:
- a 1.3% TAE agarose gel, for the small fragments: RsmA, fha1 and rsmY (length < 1000bp)
- a 0.8% TAE agarose gel, for the big fragments: pSB1A3, RBS_Cya, and pAra/Bad_RBS_GFP (length > 1000bp)
Migration conditions = 50V during 1h15.
We used EtBr to reveal the DNA fragments.