From 2012.igem.org

Keep constantly the cells on ice
Rehydratation of DNA in 10uL H2O 2) Add 1 uL of DNA in 50 uL of T10
Incubate 30 min on ice
Heat shock the cells during 30 sec at 42 degree Celsius in a water-bath without shaking
Put 2 min on ice
Add 500 uL of pre warmed SOC-medium
Incubate 1h at 37 degree Celsius at 225 rpm
Spin at 5000 rpm during 30 sec
Remove 150 uL - 400 uL of supernatant
Resuspend the pellet in the 150 uL left
Spread on appropriate plates
Incubate overnight at 37 degree Celsius

Tuesday, 26th June

Bacterial Transformation:

Petri dish

YFP
GFP
CFP
RFP
pCS2 (+) from 22/06/12

Wednesday, 27th June

MiniPrep- followed by nanodrop: confirmation of DNA presence in transformed bacteria
Agarose gel electrophoresis (samples of 4 fluorescent DNA)
Inoculation of colonies in LB medium- incubation at 37 degrees overnight

Thursday, 28th June

Gel migration 1

Gel preparation: 25mL agarose+TAE (freezer) + 2microL BET
Sample preparation:
- DNA Ladder 1kB: 1microL ladder + 1microL loading buffer + 4microL ddH2O
- Digested RFP, YFP, CFP, GFP, pCS2+ (from 28 june): 10microL sample + 2microL loading buffer
100V, 1h

Result: no DNA detectable, Solution: to redo the step of digestion with more DNA

DNA digestion:

4ul of CFP, GFP, RFP, YFP dosed on 28 june
3ul of pSC2+ dosed on 28 june

Gel migration 2:

Gel preparation: 50mL agarose+TAE (freezer) + 4ul BET
Sample preparation:
- DNA Ladder 1kB: 1ul ladder + 1ul loading buffer + 4ul ddH2O
- Digested RFP, YFP, CFP, GFP, pCS2+ (from 29 june) : 15ul sample + 3ul loading buffer
100V, 1h

Result: no RFP detectable (see picture below):
Friday, 29th June

Retrieved from "http://2012.igem.org/Team:Evry/Notebook/w3"

@@ Line 68: / Line 68: @@
 <h2>Tuesday, 26th June</h2>
+<h3>Bacterial Transformation:</h3>
+Petri dish
+<ul>
+<li>YFP
+<li>GFP
+<li>CFP
+<li>RFP
+<li>pCS2 (+) from 22/06/12
+</ul>
 <h2>Wednesday, 27th June</h2>
+<ol>
+<li>MiniPrep- followed by nanodrop: confirmation of DNA presence in transformed bacteria
+<li>Agarose gel electrophoresis (samples of 4 fluorescent DNA)
+<li>Inoculation of colonies in LB medium- incubation at 37 degrees overnight
+</ol>
 <h2>Thursday, 28th June</h2>
+<h3>Gel migration 1</h3>
+<ul>
+<li>Gel preparation: 25mL agarose+TAE (freezer) + 2microL BET
+<li>Sample preparation:
+<ul>
+<li>DNA Ladder 1kB: 1microL ladder + 1microL loading buffer + 4microL ddH2O
+<li>Digested RFP, YFP, CFP, GFP, pCS2+ (from 28 june): 10microL sample + 2microL loading buffer
+</ul>
+<li>100V, 1h
+</ul>
+<strong>Result:</strong> no DNA detectable, Solution: to redo the step of digestion with more DNA
+<h3>DNA digestion:</h3>
+<ul>
+<li>4ul of CFP, GFP, RFP, YFP dosed on 28 june
+<li>3ul of pSC2+ dosed on 28 june
+</ul>
+<h2>Gel migration 2:</h2>
+<ul>
+<li>Gel preparation: 50mL agarose+TAE (freezer) + 4ul BET
+<li>Sample preparation:
+<ul>
+<li>DNA Ladder 1kB: 1ul ladder + 1ul loading buffer + 4ul ddH2O
+<li>Digested RFP, YFP, CFP, GFP, pCS2+ (from 29 june) : 15ul sample + 3ul loading buffer
+</ul>
+<li>100V, 1h
+</ul>
+<strong>Result:<strong> no RFP detectable (see picture below):
+<img src="https://static.igem.org/mediawiki/2012/8/8d/Photo_GelMigration2906.jpeg" alt:"migration results">
 <h2>Friday, 29th June</h2>