Team:TUDelft/SDP Results

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[[Image:BBa_K175044.png|400px|thumb|center| Makeup of <partinfo>BBa_K175044</partinfo>. It consists of the I-SceI homing endonuclease restriction site and an anhydrotetracyclin inducible GFP-LVA generator.]]
[[Image:BBa_K175044.png|400px|thumb|center| Makeup of <partinfo>BBa_K175044</partinfo>. It consists of the I-SceI homing endonuclease restriction site and an anhydrotetracyclin inducible GFP-LVA generator.]]
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This part was successfully sequenced and shown to work. Firstly, aTc fluorescence induction worked, as shown in the following image.
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[[Image:GFP-LVAinduction.png|200px|thumb|center| anhydrotetracyclin induction of GFP fluorescence in centrifuged culture containing <partinfo>BBa_K175044</partinfo>. Left tube is uninduced, right tube is induced.]]
=='''I-SceI homing endonuclease'''==
=='''I-SceI homing endonuclease'''==

Revision as of 20:07, 21 October 2009

Experimental results

The experimental results for the Self Destructive Plasmid are detailed below. In the process of constructing it, we deviated from the cloning strategy after proving that it didn't work as expected.

I-SceI restriction site

Gel electrophoresis of in pSB1AK3 backbone. Lane 1: undigested (supercoiled) plasmid. Lane 2: BglI digested part, expected size = 3219bp. Lane 3: BglI and I-SceI restricted part, expected band lenghts are 2275 and 944bp. Expected lenghts correspond to the bands observed in the gel.

Construction of the I-SceI homing endonuclease restriction site was done by primer synthesis. Primers were annealed and ligated into a pSB1AK3 backbone (3189bp without the insert). Together with the 30bp recognition sequence (shown below) this gave a 3219 bp part. The sites where cleavage of the DNA backbone occurs are indicated with ^.

5' A G T T A C G C T A G G G A T A A^C A G G G T A A T A T A G 3'
3' T C A A T G C G A T C C C^T A T T G T C C C A T T A T A T C 5'

The resulting biobrick () was successfully sequenced and tested for functionality. Sequencing results can be found on the part page. Functionality was assessed using commercially available I-SceI restriciton enzyme. The plasmid was purified and subjected to a digestion with BglI alone and BglI plus I-SceI. The latter would theoretically result in two fragments of 2275 and 944bp.

The results in the adjecent image show that the digestion indeed results in the expected band pattern. This shows that the restriction site works as expected.

As shown in the cloning strategy, the restriction site was cloned inbetween the promoter and the RBS, resulting in , which was expected not to influence transcription. However, when a culture containing this biobrick was induced with anhydrotetracyclin (aTc), no fluorescence was observed. This led to a modification of the cloning strategy.

A simpler part was constructed (), which only contained the restriction site in front of the aTc inducible GFP-LVA generator.

Makeup of . It consists of the I-SceI homing endonuclease restriction site and an anhydrotetracyclin inducible GFP-LVA generator.

This part was successfully sequenced and shown to work. Firstly, aTc fluorescence induction worked, as shown in the following image.

anhydrotetracyclin induction of GFP fluorescence in centrifuged culture containing . Left tube is uninduced, right tube is induced.

I-SceI homing endonuclease

Integration

Experimental results

Experimental results

'Experimental results'

Experimental results

Experimental results

Experimental results

'Experimental results'

Experimental results

Experimental results

Experimental results

'Experimental results'

Experimental results