Team:UC Chile/Cyano/Notepad/week20

From 2012.igem.org

(Difference between revisions)
 
(One intermediate revision not shown)
Line 41: Line 41:
</body>
</body>
</html>
</html>
-
 
-
 
-
 
<br>
<br>
<p><font size="5">July 16 - July 22</font></p>
<p><font size="5">July 16 - July 22</font></p>
-
 
-
 
<br><br><p align="justify">
<br><br><p align="justify">
Line 85: Line 80:
Parts for our Argentinian advisor are on their way to Cambridge :) hope they make it through customs!<br><br>
Parts for our Argentinian advisor are on their way to Cambridge :) hope they make it through customs!<br><br>
-
Wednesday:<br><br>
+
<b>Wednesday:</b><br><br>
The bacteria with the last ligation didn't grow in kanamycin plates. We believe the digested parts were wrong labeled (or we just didn't understand Simon's label system). Therefore, a PCR colony was run and gave negative results. Decided to digest parts Lux CD and Lux EG + terminator again.<br><br>
The bacteria with the last ligation didn't grow in kanamycin plates. We believe the digested parts were wrong labeled (or we just didn't understand Simon's label system). Therefore, a PCR colony was run and gave negative results. Decided to digest parts Lux CD and Lux EG + terminator again.<br><br>
Line 95: Line 90:
PCR of parts Lux CD and Lux EG could not be distinguised, probably because they are the same size as the backbone. Anyhow the parts will be ligated and then transformed.<br><br>
PCR of parts Lux CD and Lux EG could not be distinguised, probably because they are the same size as the backbone. Anyhow the parts will be ligated and then transformed.<br><br>
-
Thursday:<br><br>
+
<b>Thursday:</b><br><br>
Lux CD and Lux EG were ligated and then transformed. Everything is being settled for tomorrow's synechocystis transformation.<br><br>
Lux CD and Lux EG were ligated and then transformed. Everything is being settled for tomorrow's synechocystis transformation.<br><br>
Line 107: Line 102:
<br><br>
<br><br>
-
Friday:  
+
<b>Friday: </b>
Synechocystis transformed with: psb1A3_Int C with RFP (from Utah State team) and psbAB+GFP. DNA concentration and volume: 1 ug/uL in 10 uL.<br><br>
Synechocystis transformed with: psb1A3_Int C with RFP (from Utah State team) and psbAB+GFP. DNA concentration and volume: 1 ug/uL in 10 uL.<br><br>
Line 113: Line 108:
Multi colony PCR of C4 and Lux CDEG consisting of 10 colonies was run. Another four PCRs for B0014+RS2+KanR and one for psB4K5+sfGFP were also run. Lux resulted in two bands and colony PCRs gave several sizes.<br><br>
Multi colony PCR of C4 and Lux CDEG consisting of 10 colonies was run. Another four PCRs for B0014+RS2+KanR and one for psB4K5+sfGFP were also run. Lux resulted in two bands and colony PCRs gave several sizes.<br><br>
-
Saturday:
+
<b>Saturday:</b>
Terminator B0014 will be replaced for B0015 as we've been having difficulties with the first part.  
Terminator B0014 will be replaced for B0015 as we've been having difficulties with the first part.  
Line 123: Line 118:
New RS2 E + P was obtained and then religated with B0015. E. coli were transformed and plated with the part.<br><br>
New RS2 E + P was obtained and then religated with B0015. E. coli were transformed and plated with the part.<br><br>
-
Sunday:  
+
<b>Sunday: </b>
Yesterday's PCR was run and strange bands appeared (again). New strategy: will purify RS2 and B0014 and B0015, cut an will try again as such.<br><br>
Yesterday's PCR was run and strange bands appeared (again). New strategy: will purify RS2 and B0014 and B0015, cut an will try again as such.<br><br>

Latest revision as of 00:25, 23 September 2012

Project: Luxilla - Pontificia Universidad Católica de Chile, iGEM 2012