EPF-Lausanne/20 August 2009

From 2009.igem.org

(Difference between revisions)
(New page: {{EPF-Lausanne09}} <div CLASS="epfltrick">__TOC__ </div><div CLASS="epfl09"> <html> <body> <form action="input_button.htm"> <p align="right"> <input type="button" name="lien" value="19 Au...)
(People in the lab)
 
(2 intermediate revisions not shown)
Line 27: Line 27:
==Wet Lab==
==Wet Lab==
 +
Long day.......
 +
Miniprep of the LovTap-Term clones we'd put in liquid culture. Then we tried to do the whole protocol to obtain our BioBrick LacI-RBS-LovTap-Term by 2 strategies:
 +
 +
- classic iGEM protocol: amplify LacI-RBS by PCR, purify, then digest it with E/S and digest the LovTap-Term vector with E/X , dephosphorylate the vector, purify again, then do the ligations of the various LacI-RBS with the LovTap-Terms in random combinations
 +
 +
- the "dirty" technique: digest both the LovTap-Term and LacI-RBS plasmids, dephosphorylate the LovTap-Term vector, purify, then do the ligation by just "mixing" the 2 solutions (so containing pieces of both vectors). The point is that since the LovTap-Term vector has a kanamycin resistance and the LacI-RBS is ampicilin, only the correct combination should manage to grow
 +
 +
We then did the transformations with the resulting ligation products. Plates were left to incubate overnight at 37°C.
 +
 +
Also, we obtained 2 clones from the previous day transformations with readout system 1. Did a colony PCR and a gel to check the insert, but the result of the gel showed some bands which we couldn't seem to identify. Did liquid cultures of the 2 clones so that we can do more tests tomorrow.
==People in the lab==
==People in the lab==
-
Nath, Basile, Gab, Christian
+
Basile, Gab, Christian, Heidi

Latest revision as of 13:56, 21 August 2009



Contents

20 August 2009




Wet Lab

Long day.......

Miniprep of the LovTap-Term clones we'd put in liquid culture. Then we tried to do the whole protocol to obtain our BioBrick LacI-RBS-LovTap-Term by 2 strategies:

- classic iGEM protocol: amplify LacI-RBS by PCR, purify, then digest it with E/S and digest the LovTap-Term vector with E/X , dephosphorylate the vector, purify again, then do the ligations of the various LacI-RBS with the LovTap-Terms in random combinations

- the "dirty" technique: digest both the LovTap-Term and LacI-RBS plasmids, dephosphorylate the LovTap-Term vector, purify, then do the ligation by just "mixing" the 2 solutions (so containing pieces of both vectors). The point is that since the LovTap-Term vector has a kanamycin resistance and the LacI-RBS is ampicilin, only the correct combination should manage to grow

We then did the transformations with the resulting ligation products. Plates were left to incubate overnight at 37°C.

Also, we obtained 2 clones from the previous day transformations with readout system 1. Did a colony PCR and a gel to check the insert, but the result of the gel showed some bands which we couldn't seem to identify. Did liquid cultures of the 2 clones so that we can do more tests tomorrow.

People in the lab

Basile, Gab, Christian, Heidi



Retrieved from "http://2009.igem.org/EPF-Lausanne/20_August_2009"