Team:SDU-Denmark/project-p

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(UV-Vis determination of beta-carotene and retinal production)
(Motility assay)
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* MG1655 cells with pSB3K3-K343004 have moved farthest of all 5 cultures. These cells and the positive control both look as though they are still swimming. This transformant show similar motility as in the first assay <br>
* MG1655 cells with pSB3K3-K343004 have moved farthest of all 5 cultures. These cells and the positive control both look as though they are still swimming. This transformant show similar motility as in the first assay <br>
The plates were left in the 37 degrees incubator for another 24 hours to see if our assumptions are correct. <br><br>
The plates were left in the 37 degrees incubator for another 24 hours to see if our assumptions are correct. <br><br>
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===Flagella staining===
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When the E.coli strain MG1655 have a constitutive active transcription of the FlhDC operon more flagella’s were expected. The idée was to get a quantities measure of the increase flagella production by comparing the observed number flagellas on the wildtype MG1655 and the hyperflagellated MG1655. We tried to stain the flagella using silver staining and afterwards examined the bacteria under the microscope. We started the staining procedure before we had the mutated FlhDC operon as a composed part because we then had time to optimize the staining protocol and become really good at it. We started with staining DH5α and H10407.  A E-coli strain which do not express flagellas (negative controle) and a hyperflagellated E-coli (positive control), respectively. The bacteria were grown on agar plates ON and stained with this protocol. <br> <br>
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Unfortunately it was not possible to see clear and significant different between the positive and negative control. Though at some placeses it could look like flagellas on the positive control but it was never enough to determine a different. After repeating the protocol four times each time with many samples we decided to give up on the protocol. <br>
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=== Scanning Electron microscopy ===
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After the failed staning of flagellas we fried to visualize the flagellas with scanning electron microscopy (SEM). The bacteria were grown ON in liquid cultures (5 ml LB-media). The bacteria were diluted to approximately 106 cells pr 10 µl solution. At the time being we do not have our FlhDC as a composite part so therefore we only tried SEM with the negative controls DH5alpa and MG1655. We did this as a preliminary work so we were ready to do microscopy on the MG1655 containing the composite part when it is ready. Unfortunately we only had a SEM available at the university and with repeatedly tries to microscopy the controls we were to realize that it was not possible to visualize the bacteria so clearly that we were to see the flagellas expected on MG1655 containing our FlhDC operon with  the magnitude possible with this microscope.
===Stability assay===
===Stability assay===

Revision as of 21:54, 25 October 2010