Team:EPF-Lausanne/Notebook/July2011

From 2011.igem.org

(Difference between revisions)
(Thursday, 21 July 2011)
(Thursday, 21 July 2011)
Line 323: Line 323:
== Thursday, 21 July 2011 ==
== Thursday, 21 July 2011 ==
-
Douglas and Alessandro inoculated the colonies transformed with the repressilator plasmid to make minipreps the following day.
+
Douglas and Alessandro inoculated the colonies transformed with the repressilator plasmid to make minipreps the following day. Alessandro also made the LB broth (because one bottle got contaminated) and distilled water.
-
 
+
-
Alessandro made the LB broth (because one bottle got contaminated) and distilled water.
+
[[File:EPFL-2011-07-21_Gibson_detector_fragments_PCR.jpg|thumb|right|Gel from our first attempt to replicate Nadine's PCR, to create fragments for the J61002-based reporter plasmid. None of the expected products show up: they should all be between 700 b and 2.4 kb]]
[[File:EPFL-2011-07-21_Gibson_detector_fragments_PCR.jpg|thumb|right|Gel from our first attempt to replicate Nadine's PCR, to create fragments for the J61002-based reporter plasmid. None of the expected products show up: they should all be between 700 b and 2.4 kb]]
Douglas and Alessandro repeated Nadine's unsuccessful PCR, to make the fragments for Gibson assembly of the 'reporter plasmid' (pTet-lacI-pLac-RFP/Lysis). The PCR was just as unsuccessful, showing no trace of the expected products, as shown on the figure to the right. We found two similarly labelled tubes containing J61002-pTet-RFP, so we used both for our PCRs. The 'bis' reactions used the plasmid miniprepped by Allesandro, labelled in green writing. The 'non-bis' reactions used the other plasmid, of mysterious origin (miniprepped by Vincent perhaps?).
Douglas and Alessandro repeated Nadine's unsuccessful PCR, to make the fragments for Gibson assembly of the 'reporter plasmid' (pTet-lacI-pLac-RFP/Lysis). The PCR was just as unsuccessful, showing no trace of the expected products, as shown on the figure to the right. We found two similarly labelled tubes containing J61002-pTet-RFP, so we used both for our PCRs. The 'bis' reactions used the plasmid miniprepped by Allesandro, labelled in green writing. The 'non-bis' reactions used the other plasmid, of mysterious origin (miniprepped by Vincent perhaps?).
 +
 +
New reagents were prepared to repeat the PCR, using this time the optimal concentrations recommended by Bio-Rad for the iProof polymerase, i.e. primer concentrations of 0.5 uM and DNA template quantities between 1 pg and 10 ng for 50 ul. Specifically, we prepared a set with 1:1000 diluted template (resulting in a mass between 25 and 100 pg) and 1:100 diluted template (resulting in a mass between 0.25 and 1 ng). They have been frozen with no polymerase, to attempt a touchdown PCR tomorrow.
{{:Team:EPF-Lausanne/Templates/Footer}}
{{:Team:EPF-Lausanne/Templates/Footer}}

Revision as of 16:01, 21 July 2011