Team:Cambridge/LabBook/Week4
From 2010.igem.org
Monday
7. Experiment: Transformation of TOP10 cc (Ben, Emily, Bill, Hannah, Will & Anja)
Top10 cc taken out of -80°C freezer and tawed on ice. 1ml pipette tip cut with scissors sterilised with ethanol and flamed. Using cut pipette tip ~50μl of TOP10cc were transferred to 1.5ml Eppendorf tubes (3x)
- 2μl of resuspended (in 10μl deionised water) BBa_J13002 (plasmiid with TetR represed PoPs/RIPs generator) was added.
- 2μl of resuspended (in 10μl deionised water) BBa_I712019 (plasmid with firefly luciferase) was added
- 1.5μl of pHK724 (plasmid containing lux4 gene) was addded
Ce]]s were held on ice for 30min. Heat shocked for 60s at 42°C (waterbath). As a control TOP10cc that had not been transformed with anything (no plasmid DNA added) were subjected to same treatment (as cells to be transformed). Put on ice for ~2min. Added 250μl pre-wardmed (in 37°C) SOC. Incubated at 37°C for Ph with rotation (Eppendorf tubes---> 12ml falcon tubes, tape over top). Plated 50micorl on pre-warmed (in 37°C incubator) LB agar plates with Amp (with blue L-shaped spreader). Grow colonies overnight at 37°2.
8.Experiment: Set up overnight culture of E.coli/pHK555 (Will & Anja)
Inoculated single bacterial colony (E.coli/pHK555) in 5ml LB in a 12ml falcon tube. Incubated at 37°C with rotation overnight. (Since it was difficult to see the colony sent from Jim Slock, we picked twice from where we anticipated colony to be and set up 2x5ml LB overnight cultures)
9.Experiment: Set up overnight cultures of W3110 hns 93-1, BW25113 Δhns::kan, W3110 hns-205::Tn10 TetR, GM230 hns-205::Tn10 TetR (Ben & Anja)
Inoculated single bacterial colonies in 5ml SOB (i.e. 4 different cultures), incubated at RT with shaking overnight.
Tuesday
10. Experiment: Preparing chemically competent cells (W3110 hns 93-1, BW25113 Δhns::kan,W3110 hns-205::Tn10 TetR, GM230 hns-205::Tn10 TetR (Ben, Will, Paul, Bill, Emily, Hannah & Anja)
(followed protocol for 'TOP10 chemically competent cells cells' from OpenWetWare) Inoculated 0.5ml of the 4 bacterial strains (overnight cultures) in 85ml SOB each. Incubated at 37°C with shaking (180rpm). put on at 11:55am
Bacterial Strains:
ID | Type |
---|---|
(1) | GM230 hns-205::Tn10 TetR |
(2) | BW25113 Δhns::kan |
(3) | W3110 hns 93-1 |
(4) | W3110 hns-205::Tn10 TetR |
OD600 measurements:
Time | OD600 (1) | OD600 (2) | OD600 (3) | OD600 (4) |
---|---|---|---|---|
1:00pm | 0.019 | -0.008 | -0.020 | 0.049 |
2:00pm | 0.034 | 0.027 | 0.001 | 0.124 |
3:00pm | 0.059 | 0.114 | 0.049 | 0.268 |
3:25pm | 0.092 | 0.235 | 0.116 | - |
3:40pm | - | 0.297 | - | - |
4:00pm | 0.159 | - | 0.267 | - |
4:25pm | 0.203 | - | - | - |
4:40pm | 0.256 | - | - | - |
Cooled cells and (newly prepared) CCMB80 Buffer in ice bath for ~20 minutes. (4) was on ice for over an hour. (2) was on ice for ~40 minutes. (3) was on ice for ~40 minutes.
2 x 30-35ml of each of the four 85ml cultures were poured into 50ml falcon tubes. Centrifuged at 3000g at 4°C for 10 min. Discarded supernatant. Resuspended cell pellet in 20ml tube CCMB80 buffer (ice cold). On ice for 20 min. Centrifuged at 3000g at 4°C for 10 min. Discarded supernatant. Resuspended cell pellet in 5ml tube CCMB80 buffer. Incubated on ice for 20 min. Aliquoted 200μl portions into Eppendorf tubes colour-coded according to the above listed colour labels. Stored at -80°C
11. Experiment: Streaking out of bacterial cultures (E. coli/pHK555) (Paul & Anja)
On LB agar plates with Chloranphenicol: E. coli/pHK555 (from both overnight cultures) on two individual plates incubated at 37°C overnight.
12. Experiment: Set up overnight cultures (TOP10 with BBa-J13002, TOP10 with BBa_I712019) (Ben & Anja)
Results from transformations on 02/08/10
- Colonies grew for TOP10 cells transformed with BBa_J13002 (promoter + rbs) and those transformed with BBa_I712019 (firefly luciferase) :-)
- no cells grew for untransformed TOP10 cells plated on LB agar + Amp plates (neg control)
- small (but plenty) colonies grew for TOP10 cells transformed with pHK724, these were left in the incubator for another 24h, and then put at 4°C
Inoculated single bacterial (TOP10 with BBa-J13002 and TOP10 with BBa_I712019 individually) colony in 5ml LB, incubated at 37°C with shaking (180rpm) overnight
Wednesday
13. Experiment: Measuring competency (W3110 hns 93-1, BW25113 Δhns::kan, W3110 hns-205::Tn10 TetR, GM230 hns-205::Tn10 TetR) (Theo & Hannah)
Followed protocol under 'TOP10 chemically competent cells' from OpenWetware
Competent cells from all 4 different strains taken out of -80°C freezer and thawed on ice. 1ml pipette tips cut with scissors dipped in ethanol and flamed. For each strain 50μl of cells were transferred to a separate 1.5ml Eppendorf tube. 1μl pUC19 (standard plasmid) was added to each 50μl of cells. Held on ice for 30 min. Heat shocked at 42°C for 60s (water bath). On ice for ~2min. 250μl SOC was added to each of 4 tubes. Each Eppendorf tube was put in a 12ml falcon with tape over the top and incubated at 37°C for 1h with rotation. 20μl of each of the 4 different transformed strains were plated on LB agar plages with Amp. Colonies were grown overnight at 37°C.
14. Experiment: Making competent and transforming E. coli/pHK555 (Peter & Paul)
50μl EZ Comp buffer transferred to Eppendorf tube and placed on ice. Single E. coli/pHK555 colony resuspended in EZ Comp buffer(2x single colony in 50μl EZ each, 1 streak of colonies in another 50μl EZ). Vortex if needed to suspend clumps. 3μl of pHK724 plasmid added to solution, mixed and incubated on ice for 20 min.
Heaat shocked at 42°C for 90s (water bath). Incubated at RT for 5 min. 1ml LB added. Eppendorf tubes put in 12ml falcon tubes with tape over top. Incubated at 37°C for 1h with rotation. Plated 100μl on LB agar plates with Cm and Amp. Incubated at 30°C for 48h.
15. Experiment BioBrick Standard Assembly (Emily & Bill, Paul & Anja)
Took overnight cultures of
- TOP10 with BBa_J13002 (plasmid with promoter + rbs)
- TOP10 with BBa_I712019 (plasmid with firefly luciferase)
Plasmid DNA Purification
following the "QIAprrep Spin Miniprep Kit using a Microcentrifuge" protocol.
Restriction enzyme digest
Prepared at RT in the listed order:
promoter + rbs | luciferase | |
---|---|---|
nuclease-free H2O | 15μl | 14μl |
10x Fast Digest Buffer | 2μl | 2μl |
Plasmid DNA | 2μl | 2μl |
FD enxyme SpeI | 1μl | 1μl |
FD enzyme XbaI | - | 1μl |
It was checked (Nanodrop!) that 2μl of plasmid DNA would not contain more than 1μg of DNA. The reaction mixtures were mixed gently (flick tube) and spun in the microcentrifuge for 15s (13,000 rpm). It was then incubated at 37°C (water bath) for 30 min.
Gel Electrophoresis
An E-gel EX Agarose 1% was mounted on the transilluminator. Nanodrop readings were taken for both restriction enzyme digests:
- Plasmid with promoter + rbs: 21.4 ng/μl => 5μl gives 100ng
- Plasmid with luciferase: 19.7ng/μl => 5μl gives 100ng
For each digest the following mixture was made up
- 3μl 6X orange loading Dye
- 5μl plasmid DNA (restriction digest)
- 12μl deionised H2O
Gel was loaded according to the scheme below:
Easyladder II | promoter + rbs | promoter + rbs | luciferase | luciferase |
10μl | 20μl | 20μl | 20μl | 20μl |
Empty wells were filled with 20μl deionised H2O. Gel was run and DNA gragments of appropriate sizes were observed:
- plasmid with promoter andd rbs => 2153b
- plasmid without luciferase => 3426b
- firefly luciferase => 1653b
The plasmid with promoter + rbs as well as te firefly luciferase bands were cut out of the gel (gel cut pipette tips) and DNA was extracted separately from the two gel pieces by following the QIAquick Gel Extraction Kit protocol.
Ligation
Fermentas 5X Rapid ligation buffer was taken out of -20°C fridge, thawed and mixed thoroughly prior to use. Nanodrop measurements of the linearised vector DNA as well as the insert DNA were taken:
- plasmid with promoter + rbs: 56.8ng/μl
- firefly luciferase: 29.6ng/μl
10-100ng of linearised vector DNA should be added to the ligation mix=>1μl. 3:1 molar exess of insert DNA should be added to the ligation mix.
(56.8ng.2153b) * 1653b * 3 = 131ng => 4.5μl
Added to a mirocentrifuge tube:
Plasmid with promoter and rbs | 1μl |
Firefly luciferase | 4.5μl |
5X Rapid ligation buffer | 4μl |
T4 DNA ligase | 1μl |
nuclease-free H2O | 9.5μl |
20μl |
The mix was vortexed and spun for 15s in the microcentrifuge (13,000 rpm). It was incubated at 22°C (RT) for 30 min and stored at 4°C.
16. Experiment: Set up new overnight cultures (TOP10 with BBa_J13002, TOP10 with Ba_I712019) (Peter & Anja)
Thursday
17. Experiment: Measuring competency (W3110 hns 93-1, BW25113 Δhns: kan, W3110 hns-205::Tn10 TetR, GB 230 hns-205::Tn10 TetR) (Theo & Peter)
After 24h the pUC19 transfmration from 04/08/10 had yielded:
W3110 hns 93-1 | 0 colonies/plate |
BW25113 Δhns::kan | 13 colonies/plate |
W3110 hns-205::Tn10 TetR | 1 colony/plate |
GM230 hns-205::Tn10 TetR | 10 colonies/plate (many v small ones-> prob result of degraded Amp) |
pUC19 transformations were repeated following the protocl outlined on 03/08/10, with the exeption that not 20μl but 100μl of the transfomrd strains were plated on LB agar plates with Amp. As a control 100μl of the transformed strains were plated on LB agar plates without anti-biotics.
18. Experiment: Standard BioBrick Assembly (Emily, Bill & Anja)
Took oversight cultures of:
- TOP10 with BBa_J13002 (plasmid with promoter + rbs)
- TOP10 with BBa_I712019 (plasmid with firefly luciferase)
Plasmid DNA purification
following the "QIAprep Spin Miniprep Kit using a Microcentrifuge" protocol
Restriction enzyme digest
Prepared at RT in the listed order:
promoter + rbs | luciferase | |
---|---|---|
nuclease-free H2O | 15μl | 14μl |
10x Fast Digest Buffer | 2μl | 2μl |
Plasmid DNA | 2μl | 2μl |
FD enxyme SpeI | 1μl | - |
FD enzyme PstI | 1μl | 1μl |
FD enzyme XbaI | - | 1μl |
20μl | 20μl |
It was checked (Nanodrop!) that 2μl of plasmid DNA would not contain more than 1μg of DNA. The reaction was mixed gentlyy, spun down and incubated at 37°C for 30 min
Gel electrophoresis
E-gel EX Agarose 1% was mounted on the transilluminator. Nanodrop readings were taken for both reaction enzyme digests
- plasmid with promoter + rbs 27.7ng/μl => 4μl give 100ng
- plasmid with luciferase 29.1ng/μl => 4μl give 100ng
Prepared following mixture for both digests
- 3μl 6X orange loading Dye
- 5μl plasmid DNA (restriction digest)
- 12μl deionised H2O
Gel was loaded according to the scheme below:
Easyladder II | promoter + rbs | promoter + rbs | luciferase | luciferase |
10μl | 20μl | 20μl | 20μl | 20μl |
Empty wells were filled with 20μl deionised H2O. Gel was run and DNA bands of length corresponding to plasmid with promoter + rbs (2153b) as well as firefly luciferase (16553b) were cut out the gel. DNA was extracted separately from the two gel pieces by following the QIAquick Gel Extraction Kit Protocol
Ligation
Fermentas 5X Rapid ligation buffer was taken out the -20°C freezer, thawed on ice and mixed thoroughly.
Nanodrop measurements
Plasmid with promoter + rbs | 2.0ng/μl |
Firefly luciferase | 3.1ng/μl |
10-100ng of linearised vector DNA should be used in ligation mix => 10μl (20ng). 3:1 molar excess of insert DNA should be added to ligation mix.
(20ng/2153b) * 1653b * 3 = 46ng => 15μl (46.5ng)
Added to a microcentrifuge tube:
Plasmid with promoter + rbs | 10μl |
Firefly luciferase | 15μl |
5X Rapid ligation buffer | 8μl |
T4 DNA ligase | 2μl |
Nuclease-free H2O | 5μl |
40μl |
Vortexed, spun briefly and incubated at 22°C (RT) fr 30 min
Transformation
TOP10 cc taken out of -80°C freezer and thawed on ice, 1ml pipette tip cut with scissors sterilised with ethanol and flamed. 50μl of TOP10cc were transferred to 1.5ml Eppendorf tube. 2μl of ligation reaction were added. Cells were held on ice for 30 min. Heat shocked for 60s at 42°C (water bath). Put on ice for ~2min. Added 250μl SOC. Incubated at 37°C for 1h with rotation. Plated 100μl on LB agar plates with Amp. Incubated overnight at 37°C.