Team:Warsaw/Calendar-Stage1/6 July 2010
From 2010.igem.org
(Difference between revisions)
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<br>2. Alkaline lysis of part of liquid culture used to prepare stocks. Undigested plasmids run on the gel. Results seem to be correct. | <br>2. Alkaline lysis of part of liquid culture used to prepare stocks. Undigested plasmids run on the gel. Results seem to be correct. | ||
<br> | <br> | ||
- | <br><div class="note">Cloning | + | <br><div class="note">Cloning GFP-terminator behind RBSes - approach 2 </div> |
- | <br>1. Digest GFP-terminator in psb1A2 plazmid. [16 μl DNA, 6 μl buforu, 16 μl H2O, 0,5 μl Xba/ Pst] | + | <br>1. Digest of GFP-terminator in psb1A2 plazmid. [16 μl DNA, 6 μl buforu, 16 μl H2O, 0,5 μl Xba/ Pst] |
- | <br>2. | + | <br>2. GFP-terminator gel extraction. |
- | <br>3. | + | <br>3. GFPterminator ligation with |
<a href="http://partsregistry.org/Part:BBa_B0030">B0030,</a> | <a href="http://partsregistry.org/Part:BBa_B0030">B0030,</a> | ||
<a href="http://partsregistry.org/Part:BBa_B0031">B0031,</a> | <a href="http://partsregistry.org/Part:BBa_B0031">B0031,</a> | ||
Line 43: | Line 43: | ||
<br>4. Transformation with 20 μl ligation mixture | <br>4. Transformation with 20 μl ligation mixture | ||
<br> | <br> | ||
- | <br><div class="note">Cloning | + | <br><div class="note">Cloning GFP-terminator behind RBSes - approach 1 </div> |
<br>7. 05.07.2010 transformation results: contamination with ampicillin susceptible bacteria. | <br>7. 05.07.2010 transformation results: contamination with ampicillin susceptible bacteria. | ||
- | <br>8. Set up one liquiquid culture | + | <br>8. Set up one liquiquid culture from each plate. Cultures inocculated with mix of all clones obtained on the plate. |
<br> | <br> |
Revision as of 22:44, 9 July 2010
Preparation of glycerol stocks
1.Glycerol stocks of following biobricks: J61100, J61101, J61107, J61117, J61127 [Anderson's RBSes], B0030, B0031, B0032, B0033, B0034 [community RBSes], J23100 [synthetic promoter].
2. Alkaline lysis of part of liquid culture used to prepare stocks. Undigested plasmids run on the gel. Results seem to be correct.
Cloning GFP-terminator behind RBSes - approach 2
1. Digest of GFP-terminator in psb1A2 plazmid. [16 μl DNA, 6 μl buforu, 16 μl H2O, 0,5 μl Xba/ Pst]
2. GFP-terminator gel extraction.
3. GFPterminator ligation with B0030, B0031, B0032, B0033, B0034 [community RBSes], [1 μl vector-RBSes, 10 μl < insert-GFPterminator, 2 μl buffer, 7 μl water]
4. Transformation with 20 μl ligation mixture
Cloning GFP-terminator behind RBSes - approach 1
7. 05.07.2010 transformation results: contamination with ampicillin susceptible bacteria.
8. Set up one liquiquid culture from each plate. Cultures inocculated with mix of all clones obtained on the plate.
Summarised by Milena.