Melbourne/Lab Notebook
From 2007.igem.org
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**Used 100mg/ml Ampicillin stock from Gooley Lab - In bag in left freezer near our lab bench. | **Used 100mg/ml Ampicillin stock from Gooley Lab - In bag in left freezer near our lab bench. | ||
| - | <font color="red"><b>Transformation</b></font> | + | <font color="red"><b>Transformation</b></font> <BR> |
[[Melbourne/Transformation Protocol|Transformed]] the following and grew on new ampicillin plates | [[Melbourne/Transformation Protocol|Transformed]] the following and grew on new ampicillin plates | ||
*[[Melbourne/BBa_E0040|'''P1 5H''']] | *[[Melbourne/BBa_E0040|'''P1 5H''']] | ||
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**[[Melbourne/BBa_E0040|'''P1 5H 2''']] | **[[Melbourne/BBa_E0040|'''P1 5H 2''']] | ||
**suspected contaminating colony from [[Melbourne/BBa_J61035|'''P4 8J''']] | **suspected contaminating colony from [[Melbourne/BBa_J61035|'''P4 8J''']] | ||
| - | + | <BR> | |
| - | <font color="red"><b>Digest</b></font> | + | <font color="red"><b>Digest</b></font> <BR> |
| - | Performed the following [[Melbourne/Diagnostic Digest|digests]] on DNA from the above miniprep <BR> | + | Performed the following [[Melbourne/Diagnostic Digest|digests]] on DNA from the above miniprep <BR><BR> |
<font color="green"><b>EcoR1/Pst1 with buffer 3</b></font> | <font color="green"><b>EcoR1/Pst1 with buffer 3</b></font> | ||
*[[Melbourne/BBa_I15010|'''I15010 1''']] | *[[Melbourne/BBa_I15010|'''I15010 1''']] | ||
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*[[Melbourne/BBa_E0241|'''P2 15L 2''']] | *[[Melbourne/BBa_E0241|'''P2 15L 2''']] | ||
| - | = | + | <font size=3><b>6 July 2007 |
| + | </b> | ||
| + | </font> | ||
<font color="red"><b>Digest Gel</b></font> | <font color="red"><b>Digest Gel</b></font> | ||
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Also placed Kan plate in the incubator to test antibiotic efficiency - no growth on 8/7 | Also placed Kan plate in the incubator to test antibiotic efficiency - no growth on 8/7 | ||
| - | = | + | <font size=3><b>7 July 2007 |
| + | </b> | ||
| + | </font> | ||
*Made 10x TAE buffer | *Made 10x TAE buffer | ||
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*Added 5uL 6x loading dye and stored at -20 | *Added 5uL 6x loading dye and stored at -20 | ||
| - | = | + | <font size=3><b>8 July 2007 |
| + | </b> | ||
| + | </font> | ||
<font color="red"><b>Transformation</b></font> | <font color="red"><b>Transformation</b></font> | ||
Revision as of 14:16, 29 September 2007
Contents |
Week 1
- 25 June 2007: Prepared LB agar plates Amp & Kana.
- 25 June 2007: Resuspended the following from Registry plates & Transformed (shorter protocol) into competent DH5alpha cells.
- 26 June 2007: Resuspended the following from Registry plates & Transformed into Joe's competent DH5alpha cells.
- 26 June 2007: Streaked the following cells:
- pJS010 (from solid agar, Amp)
- Fusion protein (from glycerol stock, Amp?)
- BBa_I15010 (from solid agar, Kan)
- 27 June 2007: Transformed into Joe's competent DH5alpha cells.
Liquid culture
- Prepared 30mL of Amp LB (100ug/mL). Prepared 5mL Kan LB (50mg/mL).
- Aliquoted 5mL Amp LB into 6 50mL falcon tubes
- To the Amp LB aliquots single transformed colonies from plates of the following were introduced:
- To the Kan LB a single colony from the transformation plate of BBa_I15010 was introduced.
- Cells incubated at 37degrees with shaking overnight.
28 June 2007
Miniprep
- Minipreped the cultures grown overnight after putting aside 1mL(sterile) for glycerol stocks:
- Stored in -20 freezer
Liquid culture
- Cultured the following cells from transformed plates:
29 June 2007 Miniprep
- Minipreped the cultures grown overnight after putting aside 1mL(sterile) for glycerol stocks:
- Stored in -20 freezer
Week 2
- 2 July 2007: Resuspended the following from Registry plates & Transformed into Joe's competent DH5alpha cells.
- Q04510
- E0241
- E0040
- B0014
- J61035
- 3 July 2007: Re Transformed into Joe's competent DH5alpha cells. Each Plate had additional 40uL of 50mg/ml Ampicillan spread on surface.
- 4 July 2007:
Ampicillin Plates
- Made up 25 Ampicillin plates using 400mL LB agar prepared on the 25th of June.
- Used 100mg/ml Ampicillin stock from Gooley Lab - In bag in left freezer near our lab bench.
Transformation
Transformed the following and grew on new ampicillin plates
- P1 5H
- P4 8J
- P2 15L
- Also Plated an untransformed control (subjected to transformation protocol in absense of DNA) and a blank plate control (no cells)
Liquid Culture
- Cultured 2 colonies from each of the following transformed plates and labelled as follows
5 July 2007
Miniprep
- 1mL culture from the 4th of Julyput aside for glycerol stocks under sterile conditions. Labelled with todays date 5/7
- miniprepped the following overnight cultures set up on the 4th of July. Final elution was performed with TE buffer prepared on 25/06/07 rather than nuclease free water. Labelled with todays date 5/7.
- the following liquid cultures were not miniprepped due to failure (no growth)
Digest
Performed the following digests on DNA from the above miniprep
EcoR1/Pst1 with buffer 3
EcoR1/HaeII in buffer 2
XbaI/SpeI in buffer 2
Incubated for 2hours at 37 degrees, before addition of loading dye and storage at -20
Transformation
- Transformed P1 11H from resuspended DNA.
Liquid Culture
6 July 2007
Digest Gel
- Prepared 20 lane 100mL agarose gel with 0.5xTBE buffer.
- Loaded 20uL of digest samples in the following lane order
- Ran for 1.5hours at 95V
Miniprep
- Put aside 1mL of liquid cultures set up on the 5th for glycerol stocks and labelled with todays date 6/7
- Miniprepped the remains of the cultures and labelled with todays date 6/7. Samples were eluted with TE buffer.
- P1 5H 1
- P1 5H 2
- P4 8J 1
- P4 8J 2
- P2 15L 1
- P2 15L 2
Digest
- Digested 5uL of each of the above miniprep DNA with EcoRI and PstI in buffer 3.
- Incubated for 2hours 25min at 37degrees
- Added 5uL 6x loading dye and stored at -20
Glycerol Stocks The following glycerol stocks were made:
- Put aside from cultures 5/7 (labelled with this date)
- Put aside from cultures 6/7 (labelled with this date)
Stored at -80
Liquid Culture Cultured the following in 5mL LB
Also placed Kan plate in the incubator to test antibiotic efficiency - no growth on 8/7
7 July 2007
- Made 10x TAE buffer
Digest Gel
- Prepared 8 lane 60mL agarose gel with 1xTAE buffer.
- Loaded 20uL of digest samples from 6/7 in the following lane order.
Glycerol Stocks The following glycerol stocks were made and dated 7/7:
Stored at -80
Miniprep
- Miniprepped the remains of the cultures and labelled with todays date 7/7. Samples were eluted with TE buffer.
Digest
- Digested 5uL of each of the above miniprep DNA
- Incubated for 3hours at 37degrees
- Added 5uL 6x loading dye and stored at -20
8 July 2007
Transformation Resuspended and transformed the following
- P1 15P(BBa_R0082, Omp R+, Amp)
- P1 17H(BBa_R0083, truncated BBa_R0082 Omp R+, Amp)
- P1 11A(BBa_E0430, EYFP(RBS+,LVA-,term) Amp)
- P1 16E(BBa_E0430; RBS,GFP,term; Amp)
The following was also retransformed due to colonies on previous plate appearing to be contaminants and failure of plasmid isolation from these colonies.
- P2 13K (BBa_Q04510, c1 inverter, Kan)
Week 3
9 July 2007
- Digested I15010(E/P),P1-11H(E/H),P2-15L 1.5hrs run
- liquid culture P1-11H,I15010,P1-15P,P1-16E,P1-17H,P2-13K
10 July 2007
- Miniprep
- Digest P1-16E,P1-11A,P2-13K,I15010,P1-15P,P1-11H,P1-17H 1.0hrs run
- liquid culture I15010, P2
11 July 2007
- Digest for ligation P1-15P(1)10/7,P1-11H 10/7,P1-17H(1)10/7,P1-16E(2)10/7,P1-11A(1)10/7
- loaded order X/P P1-11A,X/P P1-16E,S/P P1-15P,S/P P1-11H
- Spe1(6uL)/Pst1(7.5uL)/AP(1.5uL), Buffer2 9uL, BSA 9uL, milliQ 27uL into 20uL aliquots with 10uL DNA.
- Xbal1(3uL)/PstI(4uL),Buffer2 6uL,10XBSA 6uL,milliQ 21uL into 20uL aliquots with 10uL DNA
- Excise bands of interest and purify invitrogen
- liquid culture P1-11A,P1-15P 10ml
- Transform P2-21B,P2-23N,P3-20I into DB3.1 heat shock.
- Glycerol stocks P1-11A,P1-16E,P1-11H,P1-15P,P1-17H
12 July 2007
- Ran Gel P1-11A,P1-16E,P1-15P,P1-11H
- miniprepped P1-11A,P1-15P
- Digest
- Ligate control=(2uL ligase buffer,1uL ligase,5uL vector(P1-15P),12uL H20)
- Ligate (2uL ligase buffer,1uL ligase,5uL vector(P1-15P),10uL insert(P1-11A),2uL H20)
- Liquid culture transformants 11/7
13 July 2007
- miniprep cultures from transformants 11/7
- Digestion P1-15P and P1-11A from 12/7/07 37degC 3hours 15 minutes stopped 5uL of 6X loading dye.
- Excise bands 800bp from P1-11A, 2Kbp from P1-15P and purified.
- Glycerol stocks of P3-20I,P2-21B,P2-23N
- Transform DH5a with ligation product
14 July 2007
- Transform using 10uL of ligation reaction
Week 4
16 July 2007
17 July 2007
18 July 2007
- Purchased XbaI,EcoRI,PstI
- Miniprepped cultures 1,3,6 from 16/7
- Digestion with E/P
- Ran Gel:std,ctrl(from PCR reaction 1 earlier),Digest1,3,6,(P2-15P)ages ago,(P1-11A)ages ago?
19 July 2007
20 July 2007
Week 5
23 July 2007
24 July 2007
25 July 2007
26 July 2007
27 July 2007
Week 6
30 July 2007
31 July 2007
1 Aug 2007
2 Aug 2007
3 Aug 2007
4 Aug 2007
Week 7
5 Aug 2007
6 Aug 2007
7 Aug 2007
8 Aug 2007
9 Aug 2007
10 Aug 2007
11 Aug 2007
Week 8
12 Aug 2007
13 Aug 2007
14 Aug 2007
15 Aug 2007
16 Aug 2007
17 Aug 2007
18 Aug 2007
Week 9
19 Aug 2007
20 Aug 2007
21 Aug 2007
22 Aug 2007
23 Aug 2007
24 Aug 2007
25 Aug 2007
Week 10
26 Aug 2007
27 Aug 2007
28 Aug 2007
29 Aug 2007
30 Aug 2007
31 Aug 2007
1 Sept 2007
Week 11
2 Sept 2007
3 Sept 2007
4 Sept 2007
5 Sept 2007
6 Sept 2007
7 Sept 2007
8 Sept 2007
Week 12
9 Sept 2007
10 Sept 2007
11 Sept 2007
12 Sept 2007
13 Sept 2007
14 Sept 2007
15 Sept 2007
Week 13
16 Sept 2007
17 Sept 2007
18 Sept 2007
19 Sept 2007
20 Sept 2007
21 Sept 2007
22 Sept 2007
Week 13
23 Sept 2007
24 Sept 2007
25 Sept 2007
26 Sept 2007
- Miniprepped the following
- TetR-RBS-P2,21A-ter A,B,C and D
- TetR-RBS-ComP-ter A,B,C and D
- GenRBS-ComA-ter A,B,C and D
- cI-L3 A,B,C and D
