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Revision as of 00:25, 14 October 2014

Wednesday 3rd September

LabWork

B- Construction of the fusion protein

We made a classic exttraction of plasmids from the liquid cultures.

Check by electrophoresis if it worked and send it for sequencing.

D- Lemon scent

by Mélanie

PCR LS

Electrophoresis of the PCR made Yesterday

well 2-3 = PCR with Dream taq or Vent taq

(well 4-5 = checking of the pps5 Extraction)

The PCR have success so I use the PCR clean up kit to purify it

Electrophoresis after purification

Digestion

In order to clone LS in pPSI, i Digest it by PacI


component	volume
H₂O	3μl
buffer	1μl
PacI	1μl
PCR purify	5μl

Ligation

We already have some pPSI digested and dephosphorelated

So I do a ligation:


component	volume
H₂O	5μl
buffer	2μl
ligase	1μl
pPSI	2μl
LS PCR	10μl

2 hours at room temperature and over night at 4°

pPS5

Plasmid exctraction using the kit (picture is here)

digestion by SalI


component	volume
H₂O	11μl
buffer	5μl
SalI	2μl
pPS5	30μl

Electrophoresis

We saw that we have something strang with our plasmid but we wil check it tomorrow with a good ladder (the ladder here was normally on the well 1)

pPS3 and pPS4

We digest the plasmid by HindIII to direct our insert


component	volume
H₂O	6μl
buffer	1μl
HindIII	1μl
pPS3/4	2μl

well 1 = ladder well 2-3-4 = pPS3 Well 5-6-7 = pPS4

results are very strange

Photo of the Day

[http://iramis.cea.fr/llb/Phocea/Pisp/visu.php?id=35&uid=%20alexei.grinbaum Alexei Grinbaum] , one of those few we have interviewed.

Back to the calendar

@@ Line 140: / Line 140: @@
 ==Photo of the Day==
-[[File:Paris Saclay 3_september.jpg|300px|center]]
+[[File:Paris Saclay 3_september.jpg|250px|center]]
 [http://iramis.cea.fr/llb/Phocea/Pisp/visu.php?id=35&uid=%20alexei.grinbaum Alexei Grinbaum] , one of those few we have interviewed.

Team:Paris Saclay/Notebook/September/3