Team:Lyon-INSA/notebook

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</description>
</description>
                       </jour>
                       </jour>
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<jour nb="5">
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                      <date>Wednesday, September 5th 2012</date>
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                      <titre>Surfactant</titre>
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<description>
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Standard ligation of pBK22 (sfp gene) and pBK39 (abrB-lacI) and transformation into the NM522 <i>E. coli</i> strain.
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</description>
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                      </jour>
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<jour nb="6">
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                      <date>Thursday, September 6th 2012</date>
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                      <titre>For all purposes</titre>
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<description>
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Ampicillin resistances tests had some surprising results : even at 1.3 mg/mL there is bacterial growth. However, the higher Ampicillin concentration is, the lower is the OD of the liquid cultures. Ampicillin resistance test of the two shuttle vectors did not show any significant difference between the two strains (BK37 and BK38). The result is not surprising, given the fact that both plasmids (pBK36 and pBK35) derive from the shuttle vectors pHT315 and pHT304 which have the same origin replication as pUC19. However, the test must be done again, this time with at least two samples for each Ampicillin concentration in order to be able to estimate an error.
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</description>
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                      <titre>Kill</titre>
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<description>
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Transformation of BS 168 : new try ! To improve our protocol, we took periodic OD600 readings in order to stop the cell growth at the best stage (just between the exponential and the stationary phase). The BS 168 strain is transformed by :
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      <ul>
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            <li>pBK 25 (= modified shuttle vector pHT 304);</li>
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            <li>pBK 26 (= modified shuttle vector pHT 315);</li>
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            <li>pBK 28 (= Lysostaphin in the  modified shuttle vector pHT 304);</li>
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            <li>pBK 38 (= Lysostaphin in the modified shuttle vector pHT 315);</li>
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            <li>Dispersin in pBK26.</li>
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      </ul>
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We spread 200 µL of each transformed cells on GL + Erythromycin ([ERY] = 16 µg/mL) plates.
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</description>
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                      <titre>Surfactant</titre>
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<description>
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12 clones transformed with the ligation pBK22 and pBK39 are screened.
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</description>
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                      </jour>
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Friday, 7th September
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Kill :
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- Result of the transformation of BS 168 :
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- all the negative controls plates are empty : the erythromycin concentration is enough high to do a selection.
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- some plates with the transformed bacteria are empty but some have from 1 to 4 clones : these clones are put in liquid cultures in order to make miniprep and analyse their DNA.
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- Transformation of BS 168 : new try by electroporation. As the last transformation, the BS 168 strain is transformed by pBK 25, pBK 26, pBK 28, pBK 38 and dispersine in pBK26.
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Surfactant:
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All the screened clones had the religated vector, so we decided to use commercial competent cells from STLB2 strain to transform the ligation of pBK39 AND pBK22 in order to diminish the number of clones so that the chances of finding the recombinant plasmid containing the 3 genes (sfp, abrB and lacI) would be higher;
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Saturday, 8th September
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Kill :
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- Miniprep of the clones BS 168 transformed by pBK26, pBK28 : we use the same protocol than to extract the DNA of E.coli except that we add Lysosyme with the buffer A1. Electrophoresis to analyse the DNA extracted : there is nothing on the gel => Maybe the DNA isn’t concentrated enough ?
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New clones are put in liquid cultures in order to make other minipreps.
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Surfactant:
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16 clones containing the ligation of pBK22 and pBK39 transformed into STLB2 commercial competent cells are screened;
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Sunday, 9th September
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Kill :
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- Miniprep of the clones BS 168 transformed by pBK25, pBK26, pBK28, and Dispersin in pBK26. Electrophoresis to analyse the DNA extracted :
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- the clone BS 168 transformed by pBK25 has the right plasmid !! =)
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- the clone BS 168 transformed by pBK28 has the right plasmid !! BACILLUS LYSOSTAPHIN IS HERE !! :D :D :D
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- the clones BS 168 transformed by pBK26 and dispersine in pBK26, there is nothing on the gel ...
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- Transformation of BS 168 GFP with the five same plasmids as before. The transformed bacteria are spread on GL + ERY plates, with two different concentrations : [ERY]=10 µg/mL and [ERY]=15 µg/mL.
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- Given the fact that there was nothing on the miniprep for pBK26 and pBK28, we made a new electrophoresis after using the seeDNA method  to concentrate the DNA of the miniprep. We see very light strips on the gel, but the results for pBK26 and dispersine in pBK26 need to be confirm again...
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- Thanks to the good results, we put in storage the transformed Bacillus under the reference :
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- BK41 : BS 168 + pBK25
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- BK42 : BS 168 + pBK28
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- BK43 : BS 168 + pBK26 (to confirm)
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- BK44 : BS 168 + Disp in pBK26 (to confirm)
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Surfactant:
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the electrophoresis of the 16 digested plasmids extracted does not turn out as expected: all clones are in fact the initial plasmid, pBK39!
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</month>
</month>

Revision as of 00:40, 18 September 2012


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