Team:BCCS-Bristol/Notebook/Week 8

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BCCS-Bristol
iGEM 2009

Week Zero	Week 1	Week 2	Week 3	Week 4	Week 5	Week 6	Week 7	Week 8	Week 9	Week 10	Week 11	Week 12

Week 8

pQE31-GFP was digested and ligations with digested and purified FhuA were performed.

XL1-Blue competent cells were transformed with the pQE31-GFP+FhuA ligations.

The concentration of the DNA parts that we are going to send for sequencing was determined by spectrophotometry. These parts include: AraC-RBS, AraC-RBS-FhuA/OsmE, GFP-terminator and bioscaffolds-GFP-terminator.

Liquid cultures of the bioscaffolds-GFP-terminator were prepared and minipreps performed to isolated the plasmid DNA. Then the whole bioscaffold-GFP-terminator constructs were purified by gel extraction and ligations with the AraC-RBS-FhuA/OsmE were prepared.

Overnight ligations set-up;

1) AraC-RBS-FhuA-Bioscaffold-GFP-Terminator
2) AraC-RBS-OsmE-Bioscaffold-GFP-Terminator

Prepare liquid cultures for pQE31-GFP-FhuA.

Promoter-RBS-GFP-terminator ligation

This will be used to check that GFP works and also to check if the AraC promoter works by trying to control its level of activity using arabinose.

Restriction digest and gel purify GFP-terminator part and then ligate it to the already cut AraC-RBS on pSB1A2 plasmid.

The figure illustrates the construct AraC-RBS-GFP-TErminator created to assess promoter activity. The ladder is 1kb DNA marker from NEB. Lanes run in triplets with Double Digest (XbaI/Osme), Single Digest(XbaI) and Uncut versions of DNA plasmids carrying the construct. Presence is illustrated by the bands created in the double digest lane (top:plasmid backbone bottom:construct)