Team:SDU-Denmark/labwork/Notebook/week6

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<p> <b>06-08-2012 to 12-08-2012</b> </p>
<p> <b>06-08-2012 to 12-08-2012</b> </p>
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<h2>Mutagenesis on sequenced FFT and SST </h2>
 
<p>
<p>
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This week our primers arrived. We did a <a href="https://2012.igem.org/Team:SDU-Denmark/labwork/Protocols/mutagen"><b>mutagenesis</b></a> on SST and FFT to correct some genetic errors which our sequencing results showed us. Next we tranformed bacteria with SST and FFT.</br>
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The primers for mutagenesis arrived. We used the Stratagene quickchange lightning multi site-directed mutagenesis kit to perform the desired changes to our genes. Old templates were digested with DnpI. New colonies with the mutated plasmids were made through transformation of XL10-GOLD cells.<br/><br/>
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The SST plates that had been grown over night showed some colonies that were selected and put into liquid LB. for overnight culture. The FFT plates showed no colonies.</br>
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We tried to run a new mutagenesis on the FFT genes, this time following the protocol that was delivered with the mutagenesis kit. Next we transformed XL10-GOLD e.coli with the mutated genes and plated them out on ampicilin resistand plates, and left them ON. in the incubator.</br></br>
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FFT plates from the day before showed colonies and were transferred to liquid medium and incubated overnight. Plasmid SST DNA from liquid cultures from the day before were purified, digested with EcoRI, SpeI, XbaI and PstI, then run on a gel(picture not included). Results were awesome.</br>
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EcoRI+PstI: 1-8</br>
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Ladders: 9-10</br>
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XbaI+SpeI: 11-18</br>
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Colony 1 and 2 were most awesome. Will be shipped for sequencing later on.</br></br>
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<h2>Digestion of our genes to check mutagenesis</h2>
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<p>The plasmid DNA from the liquid cultures of FFT from the day before were purified, digested with EcoRI, SpeI, XbaI and PstI, then run on a gel. While the gel was running, appropriate values of expected lengths were calculated:</br>
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EcoRI+SpeI: 2000bp+3000bp  WRONG:200bp+1800bp+3000bp  or  1length </br>XbaI+PstI: 2000bp+400+2600bp WRONG: 1200bp+800bp+400bp+2600bp  or  1length  or  800bp+400bp+3800bp</br>
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The 1-SST plates showed colonies, but none for 1-FFT. Another mutagenesis and transformation, with slightly altered settings to fit the primers better, was performed on 1-FFT while liquid cultures were made from the SST colonies.<br/><br/>
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The following day 1-FFT showed colonies, these were transferred to liquid cultures.<br/><br/>
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The results from the gel:</br>
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The day after miniprepps were made for both 1-SST and 1-FFT, check digest was performed. While the gel was running, expected lengths were calculated based on the expected bands for both correct sequences and sequences still containing the undesired restriction sites.<br/><br/>
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The conclusion from the gel is that the illegal XbaI site is removed, the desired XbaI site is present, and unfortunately almost all the plasmids still contain the illegal EcoRI site except either of colony 3 and 4, which were mixed by accident the day before. Beforehand, we expected trouble with the Primer designed to remove the EcoRI site, because it had a lot of problematic alignments.</br>
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Following, another two batches of liquid colony was prepared (from the remains of colony 3 and 4) and incubated overnight, also another two plates were prepared as a safety backup with the mixed liquid medium of the two colonies.</br></br>
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We had alot of succesful 1-SST colonies with none of the undesired restriction sites. Colony 1 and 2 were most awesome. Will be shipped for sequencing later on.<br/><br/>
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The conclusion from the gel on 1-FFT was that the illegal XbaI restriction site was removed, the desired XbaI site was present, but unfortunately almost all the plasmids still contain the illegal EcoRI site except either of colony 3 and 4, which were mixed by accident the day before. Beforehand, we expected trouble with the Primer designed to remove the EcoRI site, because it had a lot of problematic alignments.<br/><br/>
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Following, another two batches of liquid colony was prepared (from the remains of colony 3 and 4) and incubated overnight, another two plates were prepared as a safety backup with the mixed liquid medium of the two colonies.<br/><br/>
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The liquid cultures of FFT colonies 3 and 4 from the day before were purified, and digested with EcoRI+SpeI and XbaI+PstI, then run on a gel.<br/>
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In conclusion from the gel: though faint, colony 4 shows signs of the illegal EcoRI restriction site.<br/>
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Meanwhile, colony 3 was awesome. It will be prepared and sent for sequencing monday.<br/><br/>
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The backup plates showed immense growth. They will be kept at 4˚C and saved for later use, if the liquid cultures fail.
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The concentration of the FFT plasmid was low. Too low to be sent for sequencing, so a liquid culture was prepared for overnight incubation in the hopes of obtaining a higher concentration.<br/><br/>
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The liquid cultures of FFT colonies 3 and 4 from the day before were purified, and digested with EcoRI+SpeI and XbaI+PstI, then run on a gel.</br>
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The results of the gel:</br>
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From nanodrop the following day:<br/>
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In conclusion: though faint, colony 4 shows signs of the illegal EcoRI restriction site.</br>
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SST 1: 116g/µL<br/>
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Meanwhile, colony 3 is awesome. It will be prepared and sent for sequencing monday.</br>
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SST 2: 135g/µL<br/>
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FFT 3: 57g/µL<br/>
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FFT 3: 41g/µL<br/><br/>
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The concentrations from 1-FFT was too low for sequencing. New liquid cultures were prepared for overnight incubation.<br/>
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</p>

Latest revision as of 02:13, 27 September 2012

iGEM TEAM ::: SDU-DENMARK

Laboratory Notebook

1st week 2nd week 3th week 4th week
5th week 6th week 7th week 8th week
9th week 10th week 11th week 12th week

06-08-2012 to 12-08-2012

The primers for mutagenesis arrived. We used the Stratagene quickchange lightning multi site-directed mutagenesis kit to perform the desired changes to our genes. Old templates were digested with DnpI. New colonies with the mutated plasmids were made through transformation of XL10-GOLD cells.

The 1-SST plates showed colonies, but none for 1-FFT. Another mutagenesis and transformation, with slightly altered settings to fit the primers better, was performed on 1-FFT while liquid cultures were made from the SST colonies.

The following day 1-FFT showed colonies, these were transferred to liquid cultures.

The day after miniprepps were made for both 1-SST and 1-FFT, check digest was performed. While the gel was running, expected lengths were calculated based on the expected bands for both correct sequences and sequences still containing the undesired restriction sites.

We had alot of succesful 1-SST colonies with none of the undesired restriction sites. Colony 1 and 2 were most awesome. Will be shipped for sequencing later on.

The conclusion from the gel on 1-FFT was that the illegal XbaI restriction site was removed, the desired XbaI site was present, but unfortunately almost all the plasmids still contain the illegal EcoRI site except either of colony 3 and 4, which were mixed by accident the day before. Beforehand, we expected trouble with the Primer designed to remove the EcoRI site, because it had a lot of problematic alignments.

Following, another two batches of liquid colony was prepared (from the remains of colony 3 and 4) and incubated overnight, another two plates were prepared as a safety backup with the mixed liquid medium of the two colonies.

The liquid cultures of FFT colonies 3 and 4 from the day before were purified, and digested with EcoRI+SpeI and XbaI+PstI, then run on a gel.
In conclusion from the gel: though faint, colony 4 shows signs of the illegal EcoRI restriction site.
Meanwhile, colony 3 was awesome. It will be prepared and sent for sequencing monday.

The concentration of the FFT plasmid was low. Too low to be sent for sequencing, so a liquid culture was prepared for overnight incubation in the hopes of obtaining a higher concentration.

From nanodrop the following day:
SST 1: 116g/µL
SST 2: 135g/µL
FFT 3: 57g/µL
FFT 3: 41g/µL

The concentrations from 1-FFT was too low for sequencing. New liquid cultures were prepared for overnight incubation.