Latest revision as of 18:51, 23 July 2010

13 July 2010

Chemical competence for E.Coli DB3.1 (step : Day 4) -> stored at -80°C
Preparation of GLY Medium / LB Medium / SOC Medium / TAE 1X / TAE 0.5X
Run a gel for the PCR -> failed (mix of two different kits)
Preparation of plates (GLY Agar / LB+Kan Agar / LB+Amp Agar)
Learned to autoclave
Restarted PCR (Asaia ORI + primers)
Plated Asaia (O/N culture)
Choice of Antibiotics Biobricks resistance (Kan / Amp / Tet / Chl) from the iGem Kit and preparation of them (streak out)
Transformation of E.coli DB3.1 with pUC19 to check its competence
Transformation of E.coli DH5 with p1003 (Kan) / p1002 (Amp) / p1004 (Chl) / p1005 (Tet)
E.coli DB3.1 and DH5 were plated on LB+Amp Agar plates (Kan was plated on LB+Kan Agar plate)
Ordered material
Wiki brainstorming
Protocols printing and organization

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 = 13 July 2010 =
-Empty yet but it will be filled soon, don't worry ;)
+*Chemical competence for E.Coli DB3.1 (step : Day 4) -> stored at -80°C
+*Preparation of GLY Medium / LB Medium / SOC Medium / TAE 1X / TAE 0.5X
+*Run a gel for the PCR -> failed (mix of two different kits)
+*Preparation of plates (GLY Agar / LB+Kan Agar / LB+Amp Agar)
+*Learned to autoclave
+*Restarted PCR (Asaia ORI + primers)
+*Plated Asaia (O/N culture)
+*Choice of Antibiotics Biobricks resistance (Kan / Amp / Tet / Chl) from the iGem Kit and preparation of them (streak out)
+*Transformation of E.coli DB3.1 with pUC19 to check its competence
+*Transformation of E.coli DH5 with p1003 (Kan) / p1002 (Amp) / p1004 (Chl) / p1005 (Tet)
+*E.coli DB3.1 and DH5 were plated on LB+Amp Agar plates (Kan was plated on LB+Kan Agar plate)
+*Ordered material
+*Wiki brainstorming
+*Protocols printing and organization
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