Team:TUDelft/18 August 2009
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='''18 August 2009'''= | ='''18 August 2009'''= | ||
+ | |||
+ | ===Sriram=== | ||
+ | Checking the yesterday's gel (shown below) I found that since the ladder didn't run well we couldn't interpret the size properly. hence I decided to do the whole assembly again. Or else we need to follow the back up plan for negative cascade alone created by Daniel. So today to start everything again I made cultures for all the primary biobricks to start the assembly all over again. We also have one problem the restriction enzyme SpeI is getting over. So it was ordered today. | ||
===Calin=== | ===Calin=== | ||
Line 9: | Line 12: | ||
Yesterdays 20 well 1% gel: | Yesterdays 20 well 1% gel: | ||
- | [[Image:Gel17082009-20well-1pc-sd-c.png| | + | [[Image:Gel17082009-20well-1pc-sd-c.png|550px]] |
Line 42: | Line 45: | ||
Yesterdays 26 well 2% gel: | Yesterdays 26 well 2% gel: | ||
- | [[Image:Gel17082009-26well-2pc-dela.png| | + | [[Image:Gel17082009-26well-2pc-dela.png|550px]] |
{| border="1" align="center" | {| border="1" align="center" | ||
| Well || Part || Expected Plasmid Size || Status | | Well || Part || Expected Plasmid Size || Status | ||
|- align="center" | |- align="center" | ||
- | | 1 || | + | | 1 || pTet || || |
|- align="center" | |- align="center" | ||
- | | 2 || | + | | 2 || RBS-cI-RBS || || |
|- align="center" | |- align="center" | ||
- | | 3 || | + | | 3 || pSB1C3 || || |
|- align="center" | |- align="center" | ||
- | | 4 || | + | | 4 || pLacI || || |
|- align="center" | |- align="center" | ||
- | | 5 || | + | | 5 || RBS || || |
|- align="center" | |- align="center" | ||
- | | 6 || | + | | 6 || pSB1C3 || || |
|- align="center" | |- align="center" | ||
- | | 7 || | + | | 7 || pTet || || |
|- align="center" | |- align="center" | ||
- | | 8 || | + | | 8 || lock3c || || |
|- align="center" | |- align="center" | ||
- | | 9 || | + | | 9 || pSB1C3 (not loaded well) || || |
|- align="center" | |- align="center" | ||
- | | 10 || | + | | 10 || pSB1C3 || || |
|- align="center" | |- align="center" | ||
- | | 11 || | + | | 11 || [http://www.eurogentec.com/EGT/Images/RESALES/Electrophoresis/Regular%20DNA%20Ladder/7-SmartLadder.jpg DNA Ladder] || || <font color=red>✖</font> |
|- align="center" | |- align="center" | ||
- | | 12 || | + | | 12 || cI || || |
|- align="center" | |- align="center" | ||
- | | 13 || | + | | 13 || Double Terminator || || |
|- align="center" | |- align="center" | ||
- | | 14 || | + | | 14 || pSB1C3 || || |
|- align="center" | |- align="center" | ||
- | | 15 || | + | | 15 || λp-in || || |
|- align="center" | |- align="center" | ||
- | | 16 || | + | | 16 || RBS-GFP-Double Term || || |
|- align="center" | |- align="center" | ||
- | | 17 || | + | | 17 || pSB1C3 || || |
|- align="center" | |- align="center" | ||
- | | 18 || | + | | 18 || [http://www.eurogentec.com/EGT/Images/RESALES/Electrophoresis/Regular%20DNA%20Ladder/7-SmartLadder.jpg DNA Ladder] || || <font color=red>✖</font> |
|- align="center" | |- align="center" | ||
- | | 19 || | + | | 19 || pLacI || || |
|- align="center" | |- align="center" | ||
- | | 20 || | + | | 20 || key3c || || |
|- align="center" | |- align="center" | ||
- | | 21 || | + | | 21 || pSB1AK3 || || |
|- align="center" | |- align="center" | ||
| 22 || Colony PCR 1A - R751ΔtrbK || 1616 || <font color=red>✖</font> | | 22 || Colony PCR 1A - R751ΔtrbK || 1616 || <font color=red>✖</font> | ||
Line 312: | Line 315: | ||
* *S3 (F) Is not BBa_K142205, but in fact BBa_K142203 | * *S3 (F) Is not BBa_K142205, but in fact BBa_K142203 | ||
* *S3 (R) Is not BBa_K142205, but in fact BBa_K142203 | * *S3 (R) Is not BBa_K142205, but in fact BBa_K142203 | ||
+ | |||
+ | ===Daniel=== | ||
+ | |||
+ | Growth, miniprep: | ||
+ | |||
+ | {| border="1" align="center" | ||
+ | | Biobrick || [DNA] ng/uL | ||
+ | |- align="center" | ||
+ | | C0051 || 45 | ||
+ | |- align="center" | ||
+ | | P0440 || 48.2 | ||
+ | |- align="center" | ||
+ | | R0051 || 22.8 | ||
+ | |- align="center" | ||
+ | | I13504 || 70.1 | ||
+ | |- align="center" | ||
+ | | Ca || 28.1 | ||
+ | |} | ||
+ | |||
{{Template:TUDelftiGEM2009_end}} | {{Template:TUDelftiGEM2009_end}} |
Latest revision as of 09:57, 20 October 2009
Lab Notebook
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18 August 2009
Sriram
Checking the yesterday's gel (shown below) I found that since the ladder didn't run well we couldn't interpret the size properly. hence I decided to do the whole assembly again. Or else we need to follow the back up plan for negative cascade alone created by Daniel. So today to start everything again I made cultures for all the primary biobricks to start the assembly all over again. We also have one problem the restriction enzyme SpeI is getting over. So it was ordered today.
Calin
Yesterdays 20 well 1% gel:
Well | Part | Expected Plasmid Size | Status |
1 | |||
2 | |||
3 | |||
4 | |||
5 | |||
6 | [http://www.eurogentec.com/EGT/Images/RESALES/Electrophoresis/Regular%20DNA%20Ladder/7-SmartLadder.jpg DNA Ladder] | ✔ | |
7 | Colony PCR 1A - R751ΔtrbK | 1616 | ✖ |
8 | Colony PCR 1A - R751ΔtrbK | 1616 | ✖ |
9 | Colony PCR R751 + pKD46 + trbK_KO_mod_S | 348 | ✔ |
10 | Colony PCR R751ΔoriTR -L-ara +PCR control | ? | |
11 | Colony PCR R751 + pKD46 + oriTR_KO_mod_S | 398 | ✔ |
12 | [http://www.eurogentec.com/EGT/Images/RESALES/Electrophoresis/Regular%20DNA%20Ladder/7-SmartLadder.jpg DNA Ladder] | ✔ |
Yesterdays 26 well 2% gel:
Well | Part | Expected Plasmid Size | Status |
1 | pTet | ||
2 | RBS-cI-RBS | ||
3 | pSB1C3 | ||
4 | pLacI | ||
5 | RBS | ||
6 | pSB1C3 | ||
7 | pTet | ||
8 | lock3c | ||
9 | pSB1C3 (not loaded well) | ||
10 | pSB1C3 | ||
11 | [http://www.eurogentec.com/EGT/Images/RESALES/Electrophoresis/Regular%20DNA%20Ladder/7-SmartLadder.jpg DNA Ladder] | ✖ | |
12 | cI | ||
13 | Double Terminator | ||
14 | pSB1C3 | ||
15 | λp-in | ||
16 | RBS-GFP-Double Term | ||
17 | pSB1C3 | ||
18 | [http://www.eurogentec.com/EGT/Images/RESALES/Electrophoresis/Regular%20DNA%20Ladder/7-SmartLadder.jpg DNA Ladder] | ✖ | |
19 | pLacI | ||
20 | key3c | ||
21 | pSB1AK3 | ||
22 | Colony PCR 1A - R751ΔtrbK | 1616 | ✖ |
23 | Colony PCR 1A - R751ΔtrbK | 1616 | ✖ |
24 | Colony PCR R751 + pKD46 + trbK_KO_mod_S | 348 | ✔ |
25 | Colony PCR R751ΔoriTR -L-ara +PCR control | ? | |
26 | Colony PCR R751 + pKD46 + oriTR_KO_mod_S | 398 | ✔ |
For the trbK conjugation test 24 plates were made:
Set 1 | |||
Plate ID | Antibiotics | Dilution | |
D1tr | TRI | 100 | |
D2tr | TRI | 10-1 | |
D3tr | TRI | 10-2 | |
D4tr | TRI | 10-3 | |
D5tr | TRI | 10-4 | |
T1tr | TRI + CAM | 100 | |
T2tr | TRI + CAM | 10-1 | |
T3tr | TRI + CAM | 10-2 | |
T4tr | TRI + CAM | 10-3 | |
T5tr | TRI + CAM | 10-4 | |
R1tr | CAM | 100 | |
R2tr | CAM | 10-1 |
Set 2 | |||
Plate ID | Antibiotics | Dilution | |
D6tr | TRI | 100 | |
D7tr | TRI | 10-1 | |
D8tr | TRI | 10-2 | |
D9tr | TRI | 10-3 | |
D10tr | TRI | 10-4 | |
T6tr | TRI + CAM | 100 | |
T7tr | TRI + CAM | 10-1 | |
T8tr | TRI + CAM | 10-2 | |
T9tr | TRI + CAM | 10-3 | |
T10tr | TRI + CAM | 10-4 | |
R3tr | CAM | 100 | |
R4tr | CAM | 10-1 |
For the oriTR conjugation test 51 plates were made:
Set 1 | |||
Plate ID | Antibiotics | Dilution | |
D1ori | TRI + CAM | 100 | |
D2ori | TRI + CAM | 10-1 | |
D3ori | TRI + CAM | 10-2 | |
D4ori | TRI + CAM | 10-3 | |
D5ori | TRI + CAM | 10-4 | |
Ts1ori | AMP + CAM | 100 | |
Ts2ori | AMP + CAM | 10-1 | |
Ts3ori | AMP + CAM | 10-2 | |
Ts4ori | AMP + CAM | 10-3 | |
Ts5ori | AMP + CAM | 10-4 | |
TL1ori | TRI + AMP | 100 | |
TL2ori | TRI + AMP | 10-1 | |
TL3ori | TRI + AMP | 10-2 | |
TL4ori | TRI + AMP | 10-3 | |
TL5ori | TRI + AMP | 10-4 | |
R1ori | AMP | 100 | |
R2ori | AMP | 10-1 |
Set 2 | |||
Plate ID | Antibiotics | Dilution | |
D6ori | TRI + CAM | 100 | |
D7ori | TRI + CAM | 10-1 | |
D8ori | TRI + CAM | 10-2 | |
D9ori | TRI + CAM | 10-3 | |
D10ori | TRI + CAM | 10-4 | |
Ts6ori | AMP + CAM | 100 | |
Ts7ori | AMP + CAM | 10-1 | |
Ts8ori | AMP + CAM | 10-2 | |
Ts9ori | AMP + CAM | 10-3 | |
Ts10ori | AMP + CAM | 10-4 | |
TL6ori | TRI + AMP | 100 | |
TL7ori | TRI + AMP | 10-1 | |
TL8ori | TRI + AMP | 10-2 | |
TL9ori | TRI + AMP | 10-3 | |
TL10ori | TRI + AMP | 10-4 | |
R3ori | AMP | 100 | |
R4ori | AMP | 10-1 |
Set 3 | |||
Plate ID | Antibiotics | Dilution | |
D11ori | TRI + CAM | 100 | |
D12ori | TRI + CAM | 10-1 | |
D13ori | TRI + CAM | 10-2 | |
D14ori | TRI + CAM | 10-3 | |
D15ori | TRI + CAM | 10-4 | |
Ts11ori | AMP + CAM | 100 | |
Ts12ori | AMP + CAM | 10-1 | |
Ts13ori | AMP + CAM | 10-2 | |
Ts14ori | AMP + CAM | 10-3 | |
Ts15ori | AMP + CAM | 10-4 | |
TL11ori | TRI + AMP | 100 | |
TL12ori | TRI + AMP | 10-1 | |
TL13ori | TRI + AMP | 10-2 | |
TL14ori | TRI + AMP | 10-3 | |
TL15ori | TRI + AMP | 10-4 | |
R5ori | AMP | 100 | |
R6ori | AMP | 10-1 |
Tim Weenink
Results of the 24h sequencing are in:
- !BPEA1 (R) correct in reliable part of sequencing file
- !BCEC1 (R) correct in reliable part of sequencing file
- !CCEA1 (F) perfect
- !CCEC2 (F) perfect
- !SPEA1 (F) Assebly with !A and BBa_K142202. !A is not supposed to be there
- !SPEA1 (R) Assebly with !A and BBa_K142202. !A is not supposed to be there
- !SPEC1 (F) Failed (as expected)
- !SPEC1 (R) Failed (as expected)
- *I6F (F) Perfect
- *S3 (F) Is not BBa_K142205, but in fact BBa_K142203
- *S3 (R) Is not BBa_K142205, but in fact BBa_K142203
Daniel
Growth, miniprep:
Biobrick | [DNA] ng/uL |
C0051 | 45 |
P0440 | 48.2 |
R0051 | 22.8 |
I13504 | 70.1 |
Ca | 28.1 |