Team:UNIPV-Pavia/Notebook/Week8

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Notebook

Week 1	Week 2	Week 3	Week 4	Week 5	Week 6	Week 7
Week 8	Week 9	Week 10	Week 11	Week 12	Week 13	Week 14

Week 8: 07/7/08 - 07/12/08

07/7/08

Colony PCR (5 colonies for each plate) for:
- BBa_J23100-BBa_B0030-BBa_C0012 (for the second time, we hoped to find true positive colonies)
- BBa_J23100-BBa_B0030-BBa_I15010 (for the second time, we hoped to find true positive colonies)
- BBa_B0030-BBa_E0040-BBa_B1006
- BBa_B0030-BBa_C0051-BBa_B0030
- BBa_B0030-BBa_E1010-BBa_B1006

Colony PCR: Marker (1), empty (2) BBa_J23100-BBa_B0030-BBa_C0012, BBa_J23100-BBa_B0030-BBa_I15010, BBa_B0030-BBa_E0040-BBa_B1006, BBa_B0030-BBa_C0051-BBa_B0030, BBa_B0030-BBa_E1010-BBa_B1006, blank

Gel results:
- No true positives for BBa_J23100-BBa_B0030-BBa_C0012
- No true positives for BBa_J23100-BBa_B0030-BBa_I15010
- Non pure true positives for BBa_B0030-BBa_E0040-BBa_B1006
- Pure true positives for BBa_B0030-BBa_C0051-BBa_B0030
- Non pure true positives for BBa_B0030-BBa_E1010-BBa_B1006

We chose to keep the first colony for all the 3 working ligation plates.

NOTE: BBa_B0030-BBa_E0040-BBa_B1006 and BBa_B0030-BBa_E1010-BBa_B1006 are final parts; we decided to sequence these 2 parts even if gel showed a weak contamination: sequencing results will tell us if there are false positive plasmids in those colonies or if the contamination was only a PCR contamination.

We infected 9 ml LB + suitable antibiotic with 30 µl of these glycerol stocks:

BBa_B0030	BBa_I15010	BBa_B0030-BBa_E0040-BBa_B1006 (1)	BBa_B0030-BBa_E1010-BBa_B1006 (1)
BBa_C0012	BBa_R0062	BBa_B0030-BBa_C0051-BBa_B0030	BBa_J23100-BBa_B0030

We incubated the 8 cultures at 37°C, 220 rpm overnight.

Tomorrow we will be ready to perform NINE LIGATIONS...(@_@!)

07/8/08

We received sequencing results for BBa_B0030-BBa_C0078: sequence showed an extra DNA fragment between BBa_C0078 and Suffix...We decided to ignore it because there was a stop codon before that fragment.

Glycerol stocks for:

BBa_B0030	BBa_I15010	BBa_B0030-BBa_E0040-BBa_B1006 (1)	BBa_B0030-BBa_E1010-BBa_B1006 (1)
BBa_C0012	BBa_R0062	BBa_B0030-BBa_C0051-BBa_B0030	BBa_J23100-BBa_B0030

Miniprep for these parts.

Plasmid digestion for:

BBa_B0030 (S-P)	BBa_I15010 (X-P)	BBa_B0030-BBa_E0040-BBa_B1006 (1) (E-X)	BBa_B0030-BBa_E1010-BBa_B1006 (1) (E-X)
BBa_C0012 (X-P)	BBa_R0062 (E-X)	BBa_B0030-BBa_C0051-BBa_B0030 (S-P)	BBa_J23100-BBa_B0030 (E-S)
BBa_J23100-BBa_B0030-BBa_C0040 (E-S)	BBa_R0051-BBa_B0030-BBa_C0062 (E-S)	BBa_B0030-BBa_C0061-BBa_B1006 (E-S)

Gel run/cut.

Gel extraction for these 11 parts.

(We already had BBa_I15009(X-P) and BBa_B1006(E-X))

Ligations:

BBa_B0030-BBa_I15009
BBa_J23100-BBa_B0030-BBa_C0040-BBa_B1006
BBa_R0051-BBa_B0030-BBa_C0062-BBa_B1006
BBa_B0030-BBa_C0051-BBa_B0030-BBa_C0079
BBa_B0030-BBa_C0061-BBa_B1006-BBa_R0062
BBa_J23100-BBa_B0030-BBa_C0012 (again)
BBa_J23100-BBa_B0030-BBa_I15010 (again)
BBa_J23100-BBa_B0030-BBa_E0040-BBa_B1006 (to test the part)
BBa_J23100-BBa_B0030-BBa_E1010-BBa_B1006 (to test the part)

We incubated ligations at 16°C overnight.

We infected 9 ml LB + Amp with 30 µl of BBa_B1006 and BBa_B0030-BBa_C0078 glycerol stocks. We incubated the 2 cultures at 37°C, 220 rpm ovenight.

07/9/08

@@ Line 81: / Line 81: @@
 |}
-*Tomorrow we will be ready to perform NINE LIGATIONS...!;)
+*We incubated the 8 cultures at 37°C, 220 rpm overnight.
+*Tomorrow we will be ready to perform NINE LIGATIONS...(@_@!)
 <br><br>
@@ Line 136: / Line 138: @@
 #BBa_J23100-BBa_B0030-BBa_E0040-'''BBa_B1006''' (to test the part)
 #BBa_J23100-BBa_B0030-BBa_E1010-'''BBa_B1006''' (to test the part)
+*We incubated ligations at 16°C overnight.
+*We infected 9 ml LB + Amp with 30 µl of BBa_B1006 and '''BBa_B0030'''-BBa_C0078 glycerol stocks. We incubated the 2 cultures at 37°C, 220 rpm ovenight.
+<br><br>
+'''07/9/08'''
+<br>