Revision as of 12:37, 10 September 2015

Ferment It Yourself

iGEM Paris-Bettencourt 2O15

Analytical digestion protocol

Prepare the following mix:
- 2µL 10X Digestion buffer
- 0.5µL Eco31I
- 0.5µL BbsI
- 2µL of DNA (200ng)
- 15µL water
incubate 1h at 37°C

Annealing Protocol

Phosphorylation of the oligos

5.6μL DNAse/RNAse free water
6.0μL oligo 1 (10µM)
6.0μL oligo 2 (10µM)
2.0μL 10X T4 DNA ligase buffer
0.4μL T4 PolyNucleotide Kinase

Total: 20μL

incubate 30min at 37°C
add 1μL of 1M NaCl
incube 5min at 95°C
let the mix cool down
use 2μL of the mix as a 10X solution

Chemical test for competent cells

20-30 sec at 8-10 krpm for the DNA tube (from the kit).
Thow cell competent on ice. Label 2 ml eppendorf µtube for each concentration and put it on ice.
Add 1µl of DNA into each µtube.
Add 50µl of competent cell into each tube. Flick gently to mix. Incubate in ice for 30 minutes. Pre-heat waterbath at 42°C.
Heat-shock cell by placing in waterbath 1 minute. CAUTION : The top need to be close to the water level, but not immerge in.
Keep back the tube to ice for 5 minutes.
Add 200µl of SOC media, incubate 37°C for 2h. Prepare agar plate of the media that you want, and label it (3 plate for each concentration).
Add 20µl of each tube n the appropriate plate. Incubate 37°C for OVN (12-16h).

Analytical digestion

Annealing

Chemical test for competent cell

Electroporation

Electrocompetent Cells Preparation

Digestion

Electrocompetent Cells Preparation for Lactobacillus plantarum

Heat Shock transformation

Titration protocols for vitamin A

Titration protocols for vitamin A with HPLC

Yeast lysis with NaOH

Heat shock transformation for yeast

Ligation

Titration protocols for vitamin B2 with HPLC

Idli recipe

Miniprep protocol

PCR purification

PCR

Gel purification

Yeast DNA extraction

Titration of phytic acid

Gel Electrophoresis with SYBR safe

@@ Line 41: / Line 41: @@
 </div>
+<div class="textBox" id="ChemicalTestCompetentCells">
+  <h3>Chemical test for competent cells</h3>
+  <ul>
+    <li>20-30 sec at 8-10 krpm for the DNA tube (from the kit).</li>
+    <li>Thow cell competent on ice. Label 2 ml eppendorf µtube for each concentration and put it on ice.</li>
+    <li>Add 1µl of DNA into each µtube.</li>
+    <li>Add 50µl of competent cell into each tube. Flick gently to mix. Incubate in ice for 30 minutes. Pre-heat waterbath at 42°C.</li>
+    <li>Heat-shock cell by placing in waterbath 1 minute. CAUTION : The top need to be close to the water level, but not immerge in.</li>
+    <li>Keep back the tube to ice for 5 minutes.</li>
+    <li>Add 200µl of SOC media, incubate 37°C for 2h. Prepare agar plate of the media that you want, and label it (3 plate for each concentration).</li>
+    <li>Add 20µl of each tube n  the appropriate plate. Incubate 37°C for OVN (12-16h).</li>
+  </ul>
+</div>
 <div id="protocolsGallerie">
@@ Line 62: / Line 74: @@
    <div class="box">
      <div class="innerBox magenta">
-       <a href="https://2015.igem.org/Team:Paris_Bettencourt/Protocols/Chemical test competent cell ">
+       <a href="https://2015.igem.org/Team:Paris_Bettencourt/Protocols#ChemicalTestCompetentCells">
          <p>Chemical test for competent cell</p>
-         <img src="https://static.igem.org/mediawiki/2015/2/24/ParisBettencourt_protocolsCentrifuge.JPG">
+         <img src="https://static.igem.org/mediawiki/2015/e/ec/ParisBettencourt_protocolsHeatBlock.JPG">
        </a>
      </div>

Difference between revisions of "Team:Paris Bettencourt/Protocols"