Team:Warsaw/Calendar-Stage1/12 July 2010

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(Difference between revisions)

Latest revision as of 16:35, 31 July 2010

Example Tabs

Monday, 12 June 2010; summarised by Milena

Cloning GFP+terminator behind Anderson's RBSes

1. Finish the alkaline lysis from Saturday 10.07, samples: 2.1, 3.1, 4.1, 5.1, 6.1
2. Digest samples 2.1, 3.1, 4.1, 5.1, 6.1 (Anderson's RBSes+GFPterminator) with EcoRI + PstI to examine the correctness of obtained constructs.
3. Gel electrophoresis.[Gel 1]
4. All constructs are of the expected size.

Cloning Community RBSes+GFP+terminator behind J23100

1. Digest sample 12.1 J23100[synthetic promoter] with SpeI(Bcu)+ PstI,
2. Gel electrophoresis [Gel 3]
3. Digest community RBSes-GFP-terminator, samples: 7.2 G, 8.1 E, 9.1 A, 11.1 P, 10.1 F with XbaI + PstI
4. Gel electrophoresis [Gel 2, Gel 3]
5. Ligation of sample 12.1 J23100 [promoter] with the community RBSes-GFP-terminator samples: 7.2 G, 8.1 E, 9.1 A, 11.1 P, 10.1 F
______________________________________________
Electrophoresis (opis zdjęć wg kolejności naniesionych próbek):
Gel 1: 2.1, 3.1, 4.1, 5.1, 6.1 [Anderson RBSes+GFPterminator]
Gel 2: 7.2, 8.1, 9.1, 10.1 [Connumity RBSes+GFPterminator]
Gel 3: 11.1, 12.1 [Community RBS+GFPterminator and J23100]
______________________________________________
Digest conditions, used for all reactions:
8 μl DNA
2 μl BamHI buffer
10 μl H2O
0,3 μl enzymów
20 μl final volume
digest for 3h
______________________________________________
Ligation conditions, used for all reactions:
25ul insert DNA
2ul vector DNA
3ul ligase buffer
30 ul final volume
overnight ligation

GEL 2

Samples: 7.2, 8.1, 9.1, 10.1 [Community RBSes+GFPterminator]
RBSes+GFPterminator at expected size, vectors at expected size;

@@ Line 11: / Line 11: @@
 <!-- do not edit above me! -->
-<div class="note">blablabla temat1</div>
+Monday, 12 June 2010; summarised by Milena
-<br>1. A co to?
+<br><br><div class="note">Cloning GFP+terminator behind Anderson's RBSes </div>
-<br>
-<img src="https://static.igem.org/mediawiki/igem.org/d/de/12_07_communityRBS_Xba_Pst.JPG"/>
-<br><div class="note">blablabla temat2</div>
-<br><img src="https://static.igem.org/mediawiki/igem.org/8/8e/12_07_FluoProteinsXbaPstandVectorSpePst3_1.JPG"/>
+. Finish the alkaline lysis from Saturday 10.07, samples: 2.1, 3.1, 4.1, 5.1, 6.1
+<br>2. Digest samples 2.1, 3.1, 4.1, 5.1, 6.1 (Anderson's RBSes+GFPterminator)	with EcoRI + PstI to examine the correctness of obtained constructs.
+<br>3. Gel electrophoresis.[Gel 1]
+<br>4. All constructs are of the expected size.
+<br><br><div class="note">Cloning Community RBSes+GFP+terminator behind J23100 </div>
+. Digest sample 12.1 J23100[synthetic promoter] with SpeI(Bcu)+ PstI,
+<br>2. Gel electrophoresis [Gel 3]
+<br>3. Digest community RBSes-GFP-terminator, samples: 7.2 G, 8.1 E, 9.1 A, 11.1 P, 10.1 F with XbaI + PstI
+<br>4. Gel electrophoresis [Gel 2, Gel 3]
+<br>5.  Ligation of sample 12.1 J23100 [promoter] with the community RBSes-GFP-terminator samples: 7.2 G, 8.1 E, 9.1 A, 11.1 P, 10.1 F
+<br>______________________________________________
+<br>Electrophoresis (opis zdjęć wg kolejności naniesionych próbek):
+<br>Gel 1: 2.1, 3.1, 4.1, 5.1, 6.1 [Anderson RBSes+GFPterminator]
+<br>Gel 2: 7.2, 8.1, 9.1, 10.1 [Connumity RBSes+GFPterminator]
+<br>Gel 3: 11.1, 12.1 [Community RBS+GFPterminator and J23100]
+<br>______________________________________________
+<br>Digest conditions, used for all reactions:
+<br>8 μl DNA
+<br>2 μl BamHI buffer
+<br>10 μl H2O
+<br>0,3 μl enzymów
+<br>20 μl final volume
+<br>digest for 3h
+<br>______________________________________________
+<br>Ligation conditions, used for all reactions:
+<br>25ul insert DNA
+<br>2ul vector DNA
+<br>3ul ligase buffer
+<br>30 ul final volume
+<br>overnight ligation
+<br>
+<br>
+<div class="note"> GEL 2</div>
+Samples: 7.2, 8.1, 9.1, 10.1 [Community RBSes+GFPterminator]
+<br>RBSes+GFPterminator at expected size, vectors at expected size;
+<img src="https://static.igem.org/mediawiki/igem.org/d/de/12_07_communityRBS_Xba_Pst.JPG"/>