Team:UC Chile/Labook/march

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Revision as of 21:02, 23 September 2012

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

March

Constructs and primers design

First constructs (link to constructs)

Primer sequences

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Strategy for integration construct: Part K292003 is not in the kit. It will be assembled from P1003+B0012+B0014

Getting parts ready

Plates prepared Broad host plasmid transformation Batch of new competent bacteria ready Primer alicuoting (primers asked for in late January).

Amplification of parts from 2011 kit: P1003, B0014 and others (specify) are needed for constructs.
Standard Biobrick assembly.

                                                                                                              Transformation.

Plated, only one surviving colony.
Conclusion: psB1C3 was already CUT

                                                                                                                   PCR’s. By electrophoresis we have:

Unsuccessful attempts: psbAB,psbAB2, Kanr, RS1.
Success: RFP, RS2, backbone.
Comment: seems as primers for expression plasmid are problematic.
Kanr new PCR attempts. Unsuccessful results.
PCR for pPMQAK1, psbAB, RFP.

Work plan

Labour division: Bactomithril {Max, Emilia,Ulises, Claudia, Bryon}
Cyano {Simón, Carla, Tamara, Isaac, Sebastián}

Meetings with Dr. Gutiérrez every two weeks to check work done.

@@ Line 60: / Line 60: @@
 Primer alicuoting (primers asked for in late January).
-Amplification of parts from 2011 kit: P1003, B0014 and others (specify) are needed for constructs.
+Amplification of parts from 2011 kit: P1003, B0014 and others (specify) are needed for constructs.<br>
-Standard Biobrick assembly.
+Standard Biobrick assembly.<br>
                                                                                                                 Transformation.<br>
 Plated, only one surviving colony.<br>
 Conclusion: psB1C3 was already CUT<br>
-                                                                                                                     PCR’s. By electrophoresis we have:
+                                                                                                                     PCR’s. By electrophoresis we have:<br>
-Unsuccessful attempts: psbAB,psbAB2, Kanr, RS1.
+Unsuccessful attempts: psbAB,psbAB2, Kanr, RS1.<br>
-Success: RFP, RS2,  backbone.
+Success: RFP, RS2,  backbone.<br>
-Comment: seems as primers for expression plasmid are problematic.
+Comment: seems as primers for expression plasmid are problematic.<br>
-Kanr new PCR attempts. Unsuccessful results.
+Kanr new PCR attempts. Unsuccessful results.<br>
-PCR for pPMQAK1, psbAB, RFP.
+PCR for pPMQAK1, psbAB, RFP.<br>
 <font size="4">Work plan</font>