Team:Paris Liliane Bettencourt/Notebook/2011/08/30/

(Difference between revisions)

Latest revision as of 15:21, 3 September 2011

Team IGEM Paris 2011

S24 + YFP-TetR:

YFP-TetR PstI-- 5re;oving the qdditionnal PstI site

Competent cell preparation of MH1

same protocol as those from the 17th of august:

We are going to extract the ComS gene from the PY79 strain. Oligo has been designed for this purpose.

Prepare 5 sterile tube with 20 µL of H2O for each colony Pick the colony using a pipetman woth a sterile tube. The pipetor is set at 3 µL for mixing

Resuspend the primers adding 10µL of water by nmol of primer. Final concentration at 100 mM. Add 1µL in 2 ml of water to get the 50 µM

60    µL HF phusion buffer
6      µL dNTPs
15    µL of colony mix
6      µL Primer fwd at (50µM)
6      µL Primer rev at (50µM)
157 µL of H2O

Aliquot 49 µL in 5 PCR tubes Add 1 µL of phusion in each tube.

1 - 98°C - 15 min
2 - 98°C - 30 sec
3 - 70°C - gradient +-10  - 1 min
4 - 55°C  - 1 min
5 - 72°C - 1 min
6 - Repeat 2-5 39 times
7 - 7°C forever

result of the gel: (biobricked ComS is about 160bp) ladder 100bp

ladder - col1 - col2 - col3 - col4 - col5 - control no colony

From the overnight culture I did minipreps, and obtained :

I sent them for sequencing.

@@ Line 1: / Line 1: @@
+{{:Team:Paris_Bettencourt/tpl_test}}
 == Cyrille ==
@@ Line 56: / Line 58: @@
 ladder 100bp
 [[File:ComS extraction.jpg|thumb|center|ladder - col1 - col2 - col3 - col4 - col5 - control no colony]]
+==Camille==
+From the overnight culture I did minipreps, and obtained :
+{| border="1" class="wikitable" style="text-align: center;"
+|Strain
+|[DNA] in ng/µL
+|ratio
+|-
+|S38+pHyperspank 1
+|483.1
+|1.76
+|-
+|S38+pHyperspank 2
+|281.9
+|1.67
+|}
+I sent them for sequencing.
+<br><br><br><br><br>