Team:Lyon-INSA/notebook

From 2012.igem.org

(Difference between revisions)
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                       </jour>
                       </jour>
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Friday 24th August  
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<jour nb="24">
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For all :
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                        <date>Friday, August 24th 2012</date>
 +
                        <titre>For all purposes</titre>
 +
<description>
 +
The transformation of the cloned shuttle vectors was successful, so 12 clones are put in liquid culture for further tests.
 +
</description>
 +
                      <titre>Surfactant</titre>
 +
<description>
 +
3A ligation of pBK4 (pUC57 containing the lacI gene) and pBK29 (pSB1A3 containing the sfp and abrB genes) in pBK24 backbone (pSB1C3 containing a RFP gene). The cloned fragment was transformed in the NM522 strain.
 +
</description>
 +
                      <titre>Stick</titre>
 +
<description>
 +
<ul>
 +
<li>After the bad results with xylR, we decided to cut pBK10 plasmid in Sma1 site, and ligate with xylR, doing a blunt ligation. We also decided to ligate xylR with xylR, creating a big polymer, which will be like a “pre-ligation” molecule.</li>
 +
<li>Extraction of pBK24-xylR from 7 clones. Gel electrophoresis is run → ONE CLONE IS GOOD!! meaning that it’s the first time we manage to ligate xylR successfully.</li>
 +
</ul>
 +
</description>
 +
                      </jour>
-
the transformations of the cloned shuttle vectors was successful, so 12 clones are put in liquid culture for further tests;
+
<jour nb="25">
-
Kill:
+
                        <date>Saturday, August 25th 2012</date>
-
Surfactant :
+
                        <titre>For all purposes</titre>
 +
<description>
 +
Miniprep of 12 clones selected from transformed bacteria with the cloned shuttle vectors; we ran out of SpeI enzyme, so we could not digest the extracted plasmids.
 +
</description>
 +
                      </jour>
-
3A ligation of pBK4 (pUC57 containing the lacI gene) and pBK29 (pSB1A3 containing the sfp and abrB genes) in pBK24 backbone (pSB1C3 containing a RFP gene). The cloned fragment was transformed in the NM522 strain;
+
<jour nb="26">
-
 
+
                        <date>Sunday, August 26th 2012</date>
-
Stick :
+
                        <titre>Surfactant</titre>
-
- After the bad results with xylR, we decided to cut pBK10 plasmid in Sma1 site, and ligate with xylR, doing a blunt ligation. We also decided to ligate xylR with xylR, creating a big polymer, which will be like a “pre-ligation” molecule.
+
<description>
-
- Extraction of pBK24-xylR from 7 clones. Gel electrophoresis is run → ONE CLONE IS GOOD!! meaning that it’s the first time we manage to ligate xylR successfully.
+
Miniprep of 6 clones (3A ligation: pBK24, pBK4, pBK29). The electrophoresis showed that none of the tested clones had integrated the right plasmid.
-
------------------------------------------------------------------------------------------------------------------
+
</description>
-
Saturday, 25th August
+
                      </jour>
-
For all :
+
-
 
+
-
miniprep of 12 clones selected from transformed bacteria with the cloned shuttle vectors; we were out of SpeI enzyme, so we could not digest the extracted plasmids.
+
-
Kill:
+
-
Surfactant :
+
-
 
+
-
Stick :
+
-
-
+
-
------------------------------------------------------------------------------------------------------------------
+
-
 
+
-
Sunday, 26th August
+
-
For all :
+
-
Kill:
+
-
Surfactant :
+
-
 
+
-
miniprep of 6 clones (3A ligation: pBK24, pBK4, pBK29). The electrophoresis showed that none of the tested clones had integrated the right plasmid.
+
-
Stick :
+

Revision as of 17:26, 10 September 2012


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