NoteBook
Day 1, Monday 04/06
People In Lab: Amalia, Carla, Daniel, Jasmeen, Nina
Agenda:
LB media
LB + agar plates
Aliquoted autoclaved SOC
70% EtOH
Equipment used:
Autoclave
Bunsen burner
Protocol: iGEM protocols used for LB, LB+agar, SOC (altered to accommodate MgCl2·6H2O because we didn't have anhydrous version, thus, for 1L solution, 2.17g was needed).
Next Steps:
Get MG1655ΔlacI cells from Christian and streak onto LB plate
Transform arg1 and pSB1C3+RFP (iGEM competence test plasmid) into DH10β
Make MG1655ΔlacI glycerol stocks
Make LB+CAM and LB+KAN plates
Day 2, Tuesday 05/06
People In Lab: Carla
Agenda:
KAN plates
CAM plates
Equipment used:
Autoclave
Bunsen burner
Protocol: iGEM protocol used for LB+agar.
Calculation for antibiotics to be added to LB media for plating
Chloramphenicol
C1V1= C2V2
C1= stock concentration = 25mg/mL
C2 = working concentration = 25μg/mL
(25000μg/mL)(V1) = (25μg/mL)(500mL)
V1= 0.5mL
Kanamycin
C1V1= C2V2
C1= stock concentration = 10mg/mL
C2 = working concentration = 50μg/mL
(10000μg/mL)(V1)
= (50μg/mL)(500mL)
V1=
2.5mL
Next Steps:
Obtain overnight culture of MG1655ΔlacI in the morning left for us in the shaker in room 318
Day 3, Wednesday 06/06
People In Lab:Amalia, Carla, Daniel, Jasmeen, Monica, Nina, Tashi
Agenda:
Transform pET28a+arg1 and pSB1C3+RFP (iGEM competence test plasmid) into DH10β
Streak MG1655ΔlacI onto LB plate
Equipment used:
ThermoMixer
Bunsen Burner
37°C incubator in room 301
Protocol: iGEM protocols used for transformation.
Transformation
Transformation 1: pSB1C3+RFP(10pg/μL) in DH10β: 100μL plated on LB+CAM
Transformation 2: pSB1C3+RFP (10pg/μL)in DH10β: 100μL plated on LB+CAM
Transformation 3: pET28a+arg1 in DH10β: 100μL plated on LB+KAN
Transformation 4: pET28a+arg1 in DH10β: 100μL plated on LB+CAM
Negative control: 100μL DH10β plated on LB+CAM and LB+KAN
For each transformation, 50μL of cells and 2μL of plasmid, and 250μL of SOC were used
Next Steps:
Start interlab
Day 4, Thursday 07/06
People In Lab: Ahmed, Amalia, Daniel, Jasmeen, Nina
Agenda:
Observed transformed cells
pSB1C3+RFP (10pg/μL) in DH10β
pET28a+arg1 in DH10β
Observe streaked plate (LB+MG1655ΔlacI)
Make overnight cultures from transformed cells (37°C)
3 LB+CAM+DH10β+pSB1C3+RFP
3 LB+KAN+DH10β+pET28a+arg1
1 LB (negative control)
Transform interlab plasmids into DH5α
10 nuclease-free water aliquots
Equipment used:
Thermomixer
Bunsen Burner
37°C incubator in room 301
Protocol:Interlab protocols used for interlab transformation.
Interlab transformation
resuspend plasmids from plate 7 to a concentration of 200-300pg/μL
1μl plasmid used: 2B, 2D, 2F, 2H, 2J, 2L, 2N, 2P
50μL of competent cells used (DH5α)
50μL of cells plated on LB+CAM
2J was not incubated, has to be transformed again
Observations:
Picture of plates are shown below.
100μl
transformation pET28a+arg1 in DH10β on LB+KAN
100μl transformation pSB1C3+RFP in DH10β on LB+KAN
100μl negative control (DH10β no plasmid) on LB+KAN and LB+CAM
Streaked MG1655ΔlacI on LB
Next Steps:
Miniprep pSB1C3+RFP and pET28a+arg1 from overnight cultures
Interlab calibration #1: OD600 Reference point - LUDOX Protocol
Day 5, Friday 08/06
People In Lab:Ahmed, Amalia, Daniel, Jasmeen, Nina, Tashi
Agenda:
Observe interlab transformations
Miniprep pSB1C3+RFP and pET28a+arg1 from overnight cultures
Nanodrop
Send miniprepped pSB1C3+RFP and pET28a+arg1 to Ranomics to add UNS2 and UNS3 to pSB1C3+RFP and fix illegal cut sites in pET28a+arg1
Interlab calibration #1: OD600 Reference point - LUDOX Protocol
Equipment used:
Thermomixer
Bunsen burner
37°C Incubator in room 301
Centrifuge
Nanodrop
Plate reader
Protocol: Protocol from miniprep kit used for miniprep. Interlab protocol used for Interlab calibration #1: OD600 Reference point - LUDOX Protocol.
Miniprep of pSB1C3+RFP and pET28a+arg1
10mL of each overnight culture used
60μL of nuclease-free water used for each elution
Sending miniprepped pSB1C3+RFP and pET28a+arg1 to Ranomics
(Concentration after nanodrop)(Volume sent) = (mass sent)
pSB1C3+RFP: (39.3ng/μL)(51μL) = 2004.3ng
pET28a+arg1: (142.0ng/μL)(21μL) = 2982ng
Observations:
Interlab Transformation of 2F, 2H, 2N on LB+CAM
Interlab Transformation of 2B, 2D, 2L, 2P on LB+CAM
Interlab calibration #1: OD600 Reference point - LUDOX Protocol absorbance values
*Refer to interlab page on wiki*
Next Steps:
Transform 2J plasmid into DH5α
Make LB+KAN+CAM plates
Make PBS (dilute from stock in fridge or make from scratch)
Transform pET28a+arg1and pSB1C3+RFP into MG1655ΔlacI
Interlab calibration #2: Particle Standard Curve - Microsphere Protocol
Day 1, Monday 11/06
People In Lab:Amalia, Carla, Daniel, Jasmeen, Nina, Tashi
Agenda:
Transform 2J interlab plasmid into DH5α and plate on LB+CAM
LB+CAM plates
Interlab calibration #2: Particle Standard Curve - Microsphere Protocol
Electroporate MG1655ΔlacI
Transform pSB1C3+RFP and pET28a+arg1 into MG1655ΔlacI
Make and autoclave PBS for interlab calibration #3
Autoclave double distilled water
Equipment used:
Autoclave
Bunsen burner
Plate reader
Thermomixer
37°C incubator in room 301
Electroporator
Protocol: iGEM protocols used for transformation, electroporation, LB+agar. Interlab protocol used for Interlab calibration #2: Particle Standard Curve - Microsphere Protocol.
Transformation of 2J plasmid
1μLof 2J plasmid used, 50μLof cells plated
Interlab calibration #2
200μLbead stock in wells A1, B1, C1, D1
100μLdouble distilled water in wells A2-A12, B2-B12, C2-C12, D2-D12
performed serial dilution by transferring 100μLeach time, until well A11, B11, C11, D11
used the plate reader to shake the plate at an amplitude of 3.5 for 7 seconds, and measure the absorbance at wavelength 600nm
Double transformation of pSB1C3+RFP and pET28a+arg1 into MG1655ΔlacI
2μLof pSB1C3+RFP(10pg/μL)
1μLofpET28a+arg1
plated 100μLon LB+CAM+KAN
plated 200μLon LB+CAM+KAN
plated 300μLon LB+CAM+KAN
plated negative control (100μLof untransformed MG1655ΔlacI)
Next Steps:
Interlab calibration #3: Fluorescence standard curve - Fluorescein Protocol
Interlab cell measurement protocol
Day 2, Tuesday 12/06
People In Lab: Amalia, Carla, Daniel, Nina
Agenda:
Second attempt at pSB1C3+RFP and pET28a+arg1 double transformation in MG1655ΔlacI, testing for incompatibility
Interlab calibration #3: Fluorescence standard curve - Fluorescein Protocol
Make overnight cultures from interlab transformation plates
Equipment used:
Bunsen burner
Plate reader
Electroporator
Shaker in room 315
37°C incubator in room 301
Protocol: iGEM protocols used for transformation by electroporation. Interlab protocol used for for Interlab calibration #3: Fluorescence standard curve - Fluorescein Protocol
Double transformation of pSB1C3+RFP and pET28a+arg1 into MG1655ΔlacI (electroporation)
Hypothesis: If we get growth on the positive control, LB+KAN, and LB+CAM plates with transformed cells, but not the double antibiotic plate, we can say that either the plasmids are incompatible, or the double antibiotic plate concentration is too high.
1.5μLof RFP (50pg/μL)
1.5μLof pET28a+arg1
plated 150μLof transformed cells on LB+CAM+KAN
plated 100μLof transformed cells on LB+CAM
plated 100μLof transformed cells on LB+KAN
plated 10μLof untransformed cells on LB+KAN (negative control)
plated 10μLof untransformed cells on LB (positive control)
Interlab calibration #3
serial dilution was performed and the plate was read
shaken 5s at amplitude = 2
excitation = 485nm
emission = 525nm
optimal gain used = 75
read from bottom of plate
The graph obtained from this experiment indicated an error, will repeat tomorrow
Interlab transformation overnight cultures
16 tubes with 5mL of LB and 5μLCAM
2 colonies were taken from each of the 8 plates (2B, 2D, 2F, 2H, 2J, 2L, 2N, 2P)
tubes placed in the shaker overnight at 37° at 250rpm
Observations:
Double transformation of pSB1C3+RFP and pET28a+arg1 into MG1655ΔlacI
no colonies on negative control plate
no colonies on 100μL, 200μL, or 300μLplates
100μL double transformation of pSB1C3+RFP (10pg/μL) and pET28a+arg1 in MG1655ΔlacI (negative control) on LB+CAM+KAN
100μL double transformation of pSB1C3+RFP (10pg/μL) and pET28a+arg1 in MG1655ΔlacI on LB+CAM+KAN
200μL double transformation of pSB1C3+RFP (10pg/μL) and pET28a+arg1 in MG1655ΔlacI on LB+CAM+KAN
300μL double transformation of pSB1C3+RFP (10pg/μL) and pET28a+arg1 in MG1655ΔlacI on LB+CAM+KAN
Potential reasons for results:
antibiotic concentration too high (50μL/mL KAN + 25μL/mL CAM)
MG1655ΔlacIcells may no longer be competent
left MG1655ΔlacIcells thawing in the ice for too long
electroporation might have failed
plasmids may not have been compatible
we could try sequential transformation (still have to consider antibiotic concentration of LB+KAN+CAM plate)
Next Steps:
Finish Interlab calibration #3: Fluorescence standard curve - Fluorescein Protocol
Cell growth, sampling, assay (interlab cell measurement)
Day 3, Wednesday 13/06
People In Lab:Amalia, Carla, Daniel, Nina
Agenda:
Redo Interlab calibration #3: Fluorescence standard curve - Fluorescein Protocol
Autoclave glass bottles, beads, tips, eppendorf tubes
Reculture the overnight cultures from the interlab transformation
Equipment used:
Autoclave
Bunsen burner
Plate reader
37°C shaker in room 315
Protocol: Used interlab protocol for interlab calibration.
Second attempt at Interlab calibration #3: Fluorescence standard curve - Fluorescein Protocol
serial dilution was performed and the plate was read
excitation = 485nm
emission = 525nm
optimal gain used = 90
read from bottom of plate
Reculturing the overnight cultures from the interlab transformation
16 tubes with 5mL of LB and 5μLCAM
100μLfrom each previous overnight culture placed in respective new tube (DH5α)
tubes slightly unscrewed and tape placed on lid for aeration in shaker
tubes placed in the shaker overnight at 37°C at 250rpm
Observations:
Second double transformation pSB1C3+RFP and pET28a+arg1in MG1655ΔlacI
LB+CAM+pSB1C3+RFP and pET28a+arg1
sparsely populated pink colonies
presence of some colonies
LB+KAN+pSB1C3+RFP and pET28a+arg1
no visible colonies
LB+KAN+CAM+pSB1C3+RFP and pET28a+arg1
no visible colonies
LB+KAN+nontrasformed cells (negative control)
no visible colonies
LB+nontransformed cells (positive control)
growth on entire plate
Second double transformation pSB1C3+RFP and pET28a+arg1 in MG1655ΔlacI
Potential reasons for these results:
colonies on LB+CAM+pSB1C3+RFP+pET28a+arg1) because the cells are still competent and were transformed with pSB1C3+RPF
no colonies on LB+KAN+pSB1C3+RFP and pET28a+arg1not because the cells are not competent, but rather the transformation (pET28a+arg1into MG1655ΔlacI) failed
no colonies on LB+KAN+CAM+pSB1C3+RFP+pET28a+arg1 because the backbones are not compatible
no growth on LB+KAN+non transformed cells (negative control) because there was no antibiotic resistance gene in the cells
we had growth on LB+non transformed cells (positive control) because the cells were viable and there was no selection in the plate against them
pET28a = KAN resistant - incompatible with pSB1C3 by group check
pSB1C3 = CAM resistant - higher copy number than pET28a
Next Steps:
Finish interlab cell measurement protocol
Day 4, Thursday 14/06
People In Lab:Ahmed, Amalia, Daniel, Monica, Nina, Tashi
Agenda:
Interlab cell measurement protocol
Autoclave P1000 tips
LB media
LB+CAM plates
Equipment used:
Autoclave
Plate reader
Shaker in autoclave room
Bunsen burner
37°C incubator in room 301
Protocol: iGEM protocols used for LB, LB+agar. Interlab protocols used for interlab OD and CFU measurements.
Observations:
Next Steps:
Count colonies on CFU cell measurement plates for interlab cell measurement protocol
Transform pET28a+arg1intoMG1655ΔlacI cells
Day 5, Friday 15/06
People In Lab:Ahmed, Amalia, Nina, Tashi
Agenda:
Check overnight plated cultures for interlab CFU count
Transformation of pET28a+arg1 into electrically competent MG1655ΔlacIcells
Observations:
Interlab CFU count
Miniscule colonies on some plates after ~11 hours of incubation at 37°C. Some plates did not have any colonies. Plates were put back in the incubator for a few more hours.
Equipment used:
37°C incubator in room 301
Shaker in room 315
Electroporator
Protocol: iGEM protocols used for transformation by electroporation.
Transformation of ARG1 in electrically competent MG1655ΔlacIcells
pET28a+arg1diluted from 39.3ng/mL to 1ng/mL
38.3μLnuclease free water + 1μLpET28a+arg1
transformed cells in cuvette placed in shaker at 37°C, 250rpm
3 plates
40μLof untransformed MG1655ΔlacIcells (negative control)
100μLof MG1655ΔlacItransformed with pET28a+arg1
200μLof MG1655ΔlacItransformed with pET28a+arg1
Next Steps:
Redo Calibration #2: Particle Standard Curve - Microsphere Protocol
Overnight culture of 2B (2 colonies) and 2D (2 colonies) in DH5α
If pET28a+arg1 transformation works
2 MG1655ΔlacI overnight cultures (LB+KAN+IPTG)
2 MG1655ΔlacI overnight cultures (LB+KAN)
streak a single MG1655ΔlacIcolony on an LB+KAN plate
Day 1, Monday 18/06
People In Lab: Amalia, Daniel, Jasmeen, Nina, Tashi
Agenda:
- LB+CAM plates
- Overnight culture of 2B (2 colonies) and 2D (2 colonies) (DH5α) for interlab
- 2 overnight cultures of LB+KAN+MG1655ΔlacI+IPTG
- 2 overnight cultures of LB+KAN+MG1655ΔlacI
- Streak plate pET28a+arg1 transformation on LB+KAN to get single colonies (MG1655ΔlacI)
- Autoclave microcentrifuge tubes
Equipment used:
- Autoclave
- Bunsen burner
- Shaker in room 315
Protocol: iGEM protocols used for LB+agar
Overnight cultures of colonies 2B+2D for interlab CFU
-4 LB+CAM tubes each with 5mL LB+5μL CAM
-2 colonies taken from 2B plate and inoculated
-2 colonies taken from 2D plate and inoculated
-all tubes placed in the shaker at 37°C at 250rpm
Serial dilution of IPTG
-dilution 1: 30μL of 1M IPTG stock in 10mL of LB = conc. 3mM
-10μL of dilution 1 in 10mL of LB = conc. 3μM
Overnight cultures of pET28a+arg1
-4 tubes
-2 with 5mL LB+IPTG+25μL KAN
-2 with 5mL LB+25μL KAN
-all tubes placed in the shaker at 37°C at 250rpm
Observations:
pET28a+arg1 transformation into MG1655ΔlacI
-No colonies on negative control plate or 100μL plate of transformed cells
-2 blobs on the 200μL plate of transformed cells
pET28a+arg1 transformation into MG1655ΔlacI negative control - 40μL untransformed cells
pET28a+arg1 transformation into MG1655ΔlacI 100μL transformed cells
pET28a+arg1 transformation into MG1655ΔlacI 200μL transformed cells
CFU colony count
Colony 1 |
Colony 2 |
|||||||
2B |
dilution 3 |
210 |
201 |
224 |
134 |
0 |
300 |
|
dilution 4 |
* |
* |
* |
* |
* |
* |
||
dilution 5 |
* |
* |
* |
* |
* |
* |
||
2D |
dilution 3 |
144 |
174 |
108 |
352 |
273 |
372 |
|
dilution 4 |
31 |
16 |
33 |
20 |
1 |
11 |
||
dilution 5 |
3 |
1 |
3 |
1 |
4 |
3 |
*plates were cracked because they were frozen
Next Steps:
- Redo interlab CFU protocol
- Let overnight cultures settle on bench (LB+KAN+MG1655ΔlacI+pET28a+arg1+IPTG) and (LB+KAN+MG1655ΔlacI+pET28a+arg1)
- Centrifuge pET28a+arg1 overnight cultures at 350g for 4 hours (LB+KAN+MG1655ΔlacI+pET28a+arg1+IPTG) and (LB+KAN+MG1655ΔlacI+pET28a+arg1)
- Streak out a single colony from the MG1655ΔlacI+pET28a+arg1 plate on an LB+KAN plate
Day 2, Tuesday 19/06
People In Lab: Amalia, Daniel, Nina, Tashi
Agenda:
- Continue interlab CFU protocol (up until plating)
- Centrifuge 1 overnight culture (LB+KAN+MG1655ΔlacI+IPTG) and 1 overnight culture (LB+KAN+MG1655ΔlacI) for 4 hours at 350g
- Keep 1 overnight culture (LB+KAN+MG1655ΔlacI+IPTG) and 1 overnight culture (LB+KAN+MG1655ΔlacI) on bench and observe
- Re-streak MG1655ΔlacI+pET28a+arg1 transformation on LB+KAN to get single colonies (was not incubated yesterday)
- Make new overnight culture of MG1655ΔlacI+pET28a+arg1
Equipment used:
- Bunsen burner
- Plate reader
- Shaker in autoclave room
- Centrifuge in room 301
- 37°C incubator in room 301
Protocol: Interlab protocol used for CFU experiement
Overnight culture of LB+KAN+MG1655ΔlacI+pET28a+arg1
-5mL LB+25μL KAN+incoulation from a blob from the LB+KAN+MG1655ΔlacI+pET28a+arg1 transformation plate
-tube placed in shaker at 37°C at 220rpm
Observations:
pET28a+arg1 induction
LB+KAN+MG1655ΔlacI+pET28a+arg1, LB+KAN+MG1655ΔlacI+pET28a+arg1+IPTG in centrifuge - cells pelleted at the bottom
-potential reason - too many gs
LB+KAN+MG1655ΔlacI+pET28a+arg1, LB+KAN+MG1655ΔlacI+pET28a+arg1+IPTG on bench - no separation
-potential reasons -arg1 not induced by IPTG?
-too hard flotation to see because there is no reporter
Centrifuged LB+KAN+MG1655ΔlacI+pET28a+arg1+IPTG (left )and LB+KAN+MG1655ΔlacI+pET28a+arg1 (right)
Next Steps:
- LB media
- LB+KAN plates
- Dilute overnight culture to OD=0.3
- Make IPTG dilution
- Induce LB+KAN+MG1655ΔlacI+pET28a+arg1 culture with 3μM IPTG for 22 hours (2 tubes)
- Make new LB+KAN+MG1655ΔlacI+pET28a+arg1 overnight culture for 22 hours (2 tubes)
- Count colonies for interlab CFU
- Streak out a single colony from the (MG1655ΔlacI) plate on an LB+KAN plate
- Make protocol for growth curve for dry lab
Day 3, Wednesday 20/06
People In Lab: Amalia, Daniel, Jasmeen, Nina, Tashi
Agenda:
- Make LB liquid media
- Make LB+KAN plates
- Count colonies for interlab CFU
- Streak out a single colony from the MG1655ΔlacI+pET28a+arg1 plate on an LB+KAN plate
- Induce LB+KAN+MG1655ΔlacI+pET28a+arg1 culture with 3μM IPTG for 22 hours (2 tubes)
- Make new LB+KAN+MG1655ΔlacI+pET28a+arg1 overnight culture for 22 hours (2 tubes)
Equipment used:
- Autoclave
- Bunsen burner
- Shaker in autoclave room
- 37°C incubator in room 301
- Spectrophotomter
Protocol: iGEM protocols used for LB+agar, interlab protocol used for CFU experiement
IPTG dilution #1 in LB
C1V1 = C2V2
C1 = 1M
C2 = 3mM
V2 = 10mL
V1 = 30μL
= take 30ul of stock and add to 10mL LB+KAN
IPTG dilution #2 in LB
C1V1 = C2V2
C1 = 3mM
C2 = 3uM
V2 = 25mL
V1 = 25μL
= take 25ul of dilution #1 and add to LB+KAN
pET28a+arg1 overnight culture
1:8 dilution, measure OD, OD = 0.25
0.25x8 = 2
C1V1 = C2V2
C1 = 2
C2 = 0.3
V2 = 25mL
V1 = 3.75mL
Total volume = 25mL
25mL - 3.75mL = 21.25mL
-21.25mL LB + KAN + 3.75mL overnight culture
-21.25mL LB + KAN + IPTG + 3.75mL overnight culture
Abs600 blank (LB+KAN+IPTG) = 0.00 (tared)
Abs600 (LB+KAN+IPTG+ARG1) = 0.127
Both tubes placed in shaker at 37°C at 220 rpm (one with IPTG and one without)
Observations:
CFU colony count #2
Colony 1 |
Colony 2 |
|||||||
2B |
dilution 3 |
180 |
138 |
40 |
77 |
78 |
91 |
|
dilution 4 |
6 |
16 |
8 |
10 |
8 |
4 |
||
dilution 5 |
2 |
3 |
2 |
1 |
0 |
1 |
||
2D |
dilution 3 |
215 |
150 |
149 |
83 |
115 |
274 |
|
dilution 4 |
45 |
28 |
28 |
30 |
14 |
28 |
||
dilution 5 |
2 |
2 |
2 |
0 |
4 |
4 |
Colony forming unit calculation (using Dilution 3 data)
Calculated for Interlab Form IV
(# of colonies) x (Final Dilution Factor) = CFU/mL
Final Dilution Factor = 8 x 104
Colony 1 |
Colony 2 |
- |
Colony 1 |
Colony 2 |
||
2B |
8.64 x 10^6 |
6.16 x 10^6 |
- |
2D |
1.72 x 10^7 |
6.64 x 10^6 |
1.104 x 10^7 |
6.24 x 10^6 |
- |
1.2 x 10^7 |
9.20 x 10^6 |
||
3.20 x10^6 |
7.28 x 10^6 |
- |
1.192 x 10^7 |
2.192 x 10^7 |
MG1655ΔlacI+pET28a+arg1 streak to get single colonies
Next Steps:
- LB+KAN plates
- Make KAN dilutions
- Order primers
- Order blue protein
Day 4, Thursday 21/06
People In Lab: Amalia, Daniel, Jasmeen, Nina
Agenda:
- Make LB + KAN plates
- Make KAN dilutions
- Make overnight culture of LB+KAN+MG1655ΔlacI+pET28a+arg1 for dry lab growth curve
- Order primers for pET28a+arg1
- Order blue protein
Equipment used:
- Bunsen burner
- Shaker in room 315
Protocol:
KAN dilutions
(800μL of nuclease-free water+200μL 50mg/mL KAN = 1mL 10mg/mL KAN) x3
Overnight culture of LB+KAN+MG1655ΔlacI+pET28a+arg1 for growth curve
-(15mL LB + 75μL KAN + incoulation from colony on newest MG1655ΔlacI+pET28a+arg1 plate) x3
-tube placed in shaker at 37°C at 220rpm
Observations:
MG1655ΔlacI+pET28a+arg1 streak to get clonal colonies
Next Steps:
- LB+KAN plates
- Make KAN dilutions
- Do digest and run gel
- Dry lab growth curve
- Order amilCP
Day 5, Friday 22/06
People In Lab: Amalia, Nina, Daniel, Tashi
Agenda:
- Make LB + KAN plates
- Make KAN dilutions
- LB+KAN+MG1655ΔlacI+pET28a+arg1 growth curve
- Order amilCP
Equipment used:
- Bunsen burner
- Shaker in autoclave room
- Plate reader
- Autoclave
Protocol: iGEM protocols for LB+agar and KAN dilutions
KAN dilutions
-80mL of 10mg/mL were made
-50 microcentrifuge tubes were filled with 1mL each and 30mL remains in a falcon tube in the fridge
LB+KAN+MG1655ΔlacI+pET28a+arg1 growth curve
-1:8 dilution made from each overnight culture (175mL LB+KAN and 25mL culture in well)
-200μl LB+KAN pipetted in well (blank)
-measure OD600
-subtract blank value, multiply by 8 to get original concentration (OD)
-dilute each overnight culture to get an OD of 0.1
-take OD again (0h timepoint)
-place the three replicates back in the shaker and measure again every hour (200μL)
Observations:
Volumes for LB+KAN+MG1655ΔlacI+pET28a+arg1 in growth curve cultures based on OD values of 1:8 dilutions-blank value multiplied by 8
Overnight culture 1 1:8 dilution OD without blank = 0.2209
Overnight culture 1 original OD = 1.3576
Replicate 1 LB+KAN = 23.158mL
Replicate 1 overnight culture = 1.841mL
Overnight culture 2 1:8 dilution OD without blank = 0.2167
Overnight culture 2 original OD = 1.324
Replicate 2 LB+KAN = 23.111mL
Replicate 2 overnight culture = 1.888mL
Overnight culture 3 1:8 dilution OD without blank = 0.2235
Overnight culture 3 original OD = 1.3784
Replicate 3 LB+KAN = 23.186mL
Replicate 3 overnight culture = 1.814mL
LB+KAN+MG1655ΔlacI+pET28a+arg1 in growth curve data
0 |
0.094 |
0.0942 |
0.1022 |
*0.0512 |
1 |
0.1808 |
0.1757 |
0.1713 |
|
2 |
0.255 |
0.2538 |
*0.4448 |
|
3 |
0.3391 |
0.3247 |
0.3332 |
|
4 |
0.3937 |
0.4075 |
0.4032 |
|
5 |
0.4539 |
0.4688 |
0.4326 |
|
6 |
0.4652 |
0.4797 |
0.4705 |
*Replicate 3 OD at 2h has an incorrect measurement. All 2h replicates were retested an hour later and they all had very similar values.
*All measurements shown already have the blank value subtracted from the raw value
Next Steps:
- PCR pET28a+arg1 with new primers
- Give Scott LB plate to streak with BL21
- LB+AMP plates (for gibson positive control)
- Order gibson
- Order amilCP
Day 1, Monday 25/06
People In Lab: Daniel, Nina, Tashi
Agenda:
- Make LB+AMP plates
- Autocleave tips (p200)
- Run practice PCR with pSB1C3
- pSB1C3_UNS3_REV Primer
- pSB1C3_UNS2_FWD Primer
Equipment used:
- Autoclave
- Thermocycler
- Bunsen Burner
Protocol:
6 x 50μL reactions for amplifying pSB1C3
-Primers 2.5 ul * 6 = 15 ul * 2 (rev&fwd)
5x buffer (HF or GC) of Phusion ---> 10ul * 6 = 60ul
10mM of dNTPs ---> 1ul * 6 = 6ul
DMSO(100%) ---> 6*50*3% = 9ul
Phusion polymerase ---> 0.5*6 = 3ul
Nuclease free water ----> 300ul - (60ul + 9ul + 3ul + 30 ul + 0.07ul) = 197.93 ul (forgot to add 6ul dNTPs, solution more dilute)
pSB1c3 (142ng/ul)-----> 0.07ul (0.1ul used)
UNS3 _rev : CGACCTTGATGTTTCCAGTCCGATTGAGGACCTTCAGTGCCTCTAGAAGCGGCCGCG
uns2_FWD: GCTGGGAGTTCGTAGACGGAAACAAACGCAGAATCCAAGCTACTAGTAGCGGCCGCT
NEB temp: 72°C
LB+AMP plates:
Accoding to the protocol found in iGEM binder.
C1= 50mg/μL
C2=50ug/mL
V2=500mL
V1=0.5mL
Next steps:
- Run practice PCR with protocol on thermocycler
- Run gel for PCR product
- Overnight culture for growth curve
- Innoculation for growth curve (3x50mL falcon tubes)
Day 2, Tuesday 26/06
People In Lab: Amalia, Daniel, Nina, Jasmeen, Tashi
Agenda:
- Run practice PCR with protocol on thermocycler
- Run gel for PCR product
- Overnight culture for growth curve
- Innoculation for growth curve (3x50ml falcon tubes)
Equipment used:
- Thermalcycler
- Shaker
- Electrophoresis machine
- UV light for gel visualization
Protocol:
Used protocols from iGEM binder for casting and loading gel for gel electrophoresis. Used protocol from Phusion for PCR reaction.
Growth Curve
-add 25mL LB+KAN to 3 50mL falcon tubes
-run blank readings
-innoculate 3 tubes with clonal ARG1 plasmid in MG1655deltalacI and take OD readings every 30 mins for 10 hours
PCR mastermix
FWD PSB1C3 UNS2 505.7 ng/ul (nanodrop)
REV PSB1C3 UNS 3 894.1 ng/ul (nanodrop)
4 x 50ul reactions
-5x buffer 10ul x 4 = 40ul
-10mM dNTPs 1ul x 4 = 3ul (wrong)
-DMSO 1.5ul x 4 = 6ul
-phusion polymerase 0.5ul x 4 = 2ul
-RFP plasmid (142 ng/ul)
-dilute to 1ng/ul
-141ul UP water + 1ul RFP plasmid
-10ng x 4 = 10ul x 4 = 40ul
-FWD primer
-dilute to 1ng/ul
-504.7 UP water + 1ul primer
-2.5ul x 4 = 10ul
-REV primer
-dilute to 1ng/ul
-893.1 UP water + 1ul primer
-2.5ul x 4 = 10ul
-UP water 50ul x 4 - (40ul + 3ul + 6ul + 2ul + 40ul + 10ul + 10ul) = 89ul
-add 50ul of mastermix to 3 PCR tubes
Thermocycler settings
Hot start: 98 degrees
Denaturing: 98 degrees - 30s
Annealing: 98 degrees - 10s
72 degrees - 30s
72 degrees - 90s
Extension: 72 degrees - 10min
Hold: 4 degrees
Gel electrophoresis:
-nanodrop of product concentrations
PCR 1 |
600.2 ng/ul |
PCR 2 |
341 ng/ul |
PCR 3 |
398 ng/ul |
PCR 4 |
403.4 ng/ul |
PCR 5 |
313 ng/ul |
PCR 1.1 |
269 ng/ul |
PCR 1.2 |
280 ng/ul |
PCR 1.3 |
323 ng/ul |
PCR 1-5 = PCR products from 06/25/18
PCR 1.1-1.3 = PCR products from 06/26/18
-make dilutions usch that each PCR product has a concentration of 10ng/ul
-take 1ul of product and dilute in UP water
-eg. 1ul PCR 1 + 59ul UP water
-take 10ul of dilution and mix with 2ul loading dye
-load 12ul into wells
-V = 100
-A = 3.00 max
-W = 300 max
Observations:
DNA wells in gel
DNA ladder (0.1-10kb) |
PCR 1 |
PCR 2 |
PCR 3 |
PCR 4 |
PCR 5 |
PCR 1.1 |
PCR 1.2 |
PCR 1.3 |
Next steps:
- Finish dry lab growth curve for MG1655deltalacI in LB+KAN
Day 3, Wednesday 27/06
People In Lab: Amalia, Jasmeen, Nina, Tashi
Agenda:
- Finish dry lab growth curve for MG1655deltalacI in LB+KAN
- Run PCR with undiluted DNA
- Autoclave beakers and jars
- Streak out BL21 on an LB plate
Equipment used:
- Autoclave
- Electrophoresis machine
- Gel doc in room 319
- Bunsen burner
Protocol:
Used protocols from iGEM binder for casting and loading gel for gel electrophoresis.
Gel electrophoresis:
-load wells
-V = 100
-A = 3.00 max
-W = 300 max
Observations:
Dry lab growth curve for MG1655deltalacI in LB+KAN data
Blank |
0.0465 |
0.0469 |
0.0475 |
0 |
0.0009 |
0 |
0.0012 |
0.5 |
0.0006 |
0.0002 |
-0.0006 |
1 |
0.0004 |
0.007 |
0 |
1.5 |
0.0015 |
-0.0017 |
-0.002 |
2 |
0.0008 |
0.005 |
0.0006 |
2.5 |
0.0026 |
-0.0024 |
0.0021 |
3 |
0.0125 |
0.0112 |
0.0073 |
3.5 |
0.0052 |
0.0099 |
0.0135 |
4 |
0.0182 |
0.0218 |
0.0301 |
4.5 |
0.0026 |
0.0475 |
0.0569 |
5 |
0.0675 |
0.1095 |
0.1241 |
5.5 |
0.105 |
0.1352 |
0.1496 |
6 |
0.1894 |
0.2295 |
0.2437 |
6.5 |
0.2181 |
0.2469 |
0.2506 |
7 |
0.2452 |
0.2818 |
0.2734 |
7.5 |
0.2649 |
0.3103 |
0.2781 |
8* |
0.3018 |
0.3585 |
0.3656 |
8.5 |
0.3376 |
0.364 |
0.3548 |
9 |
0.358 |
0.3953 |
0.3864 |
9.5 |
0.3888 |
0.4057 |
0.404 |
10 |
0.4101 |
0.4305 |
0.4261 |
10.5 |
0.4494 |
0.4483 |
0.4571 |
11.5 |
0.468 |
0.4638 |
0.4764 |
23 |
0.8631 |
0.9021 |
0.963 |
*this measurement was taken after being out of the shaker for 30 mins
All measurements shown already have the blank value subtracted from the raw value
Gel electrophoresis for PCR
DNA ladder |
PCR 1 |
PCR 2 |
PCR 3 |
PCR 4 |
PCR 5 |
PCR 1.1 |
PCR 1.2 |
PCR 1.3 |
PCR 1 |
PCR 1-5 = PCR products from 06/25/18
PCR 1.1-1.3 = PCR products from 06/26/18
Gel from PCR.jpg
Potential reasons for this result:
-PCR did not work
-the annealing temperature was wrong because it was calculated using the whole primer, instead of only the binding sequence
-the primers don't work
-the primers were suspended in water instead of TE buffer and could therefore be degraded
-nanodrop had inaccurate measurement for primer concentrations since they were old and small
-the primers were diluted to a concentration that would make them the limiting reagent for the reaction
Next steps:
- Make LB
- Overnight culture of BL21
- PCR ARG1 + UNSs
- Transform ARG1 into BL21
Day 4, Thursday 28/06
People In Lab: Ahmed, Amalia, Daniel, Jasmeen, Nina, Tashi
Agenda:
- Make LB
- PCR ARG1 + UNSs
- Transform ARG1 into BL21
- RFP digest
Equipment used:
- Autoclave
- Shaker in autoclave room
- Benchtop incubator with shaker
- Bunsen burner
- Thermocycler
- Electrophoresis machine
- Gel doc
Protocol:
Used protocols from NEB for PCR and digestion
PCR mastermix
6 x 20ul reactions
UNS3 FWD
UNS2 REV
-5x HF buffer 4ul x 6 = 24ul
-10mM dNTPs 0.4ul x 6 = 2.4ul
-10uM FWD primer 1ul x 6 = 6ul
-we have 100uM so we will dilute 2ul primer + 18ul UP water = 20ul 10uM FWD primer
-10uM REV primer 1ul x 6 = 6ul
-we have 100uM so we will dilute 2ul primer + 18ul UP water = 20ul 10uM REV primer
-ARG 1 - dilute to 1ng/ul (original 39.3ng/ul)
-1ul ARG1 + 38.3ul UP water
-1ul x 6 = 6ul
-phusion DNA polymerase 0.2ul x 6 = 1.2ul
-DMSO 0.6ul x 6 = 3.6ul
-UP water 20ul x 6 - (24ul + 2.4u + 6ul + 6ul + 6ul + 1.2ul + 3.6ul) = 89ul
-add 20ul of mastermix to 5 PCR tubes
-annealing temperature = 60 degrees
Thermocycler settings
Denaturing: 98 degrees - 30s
Annealing x30: 98 degrees - 10s
60 degrees - 30s
72 degrees - 363s
Extension: 72 degrees - 10min
Hold: 4 degrees
RFP digest
-1ul SPeI
-1ul EcoRI-HF
-7ul RFP plasmid
-5ul 10x cutsmart
-36ul UP water
Observations:
Gel for ARG1 PCR
DNA ladder 1kb |
1 |
2 |
3 |
4 |
NTC |
Table 5 - concentration of template is too high because the plasmid was not diluted, proper concentrations in gel represented by table 6
Gel for ARG 1 PCR with correct concentrations
DNA ladder 1kb |
1.1 |
1.2 |
1.3 |
1.4 |
NTC |
Digest |
Next steps:
- Run gels with a different ladder
- Rerun gels with fresh TAE buffer
- Do a PCR using the thermocycler in room 303 of PSB1C3 + RFP and colony PCR primers using thermo DNA polymerase (temperature gradient)
- Do a PCR using the thermocycler in room 403 of PSB1C3 + RFP and colony PCR primers
- Make competent BL21 cells
Day 5, Friday 29/06
People In Lab: Ahmed, Amalia, Daniel, Nina, Tashi
Agenda:
- Run gels with a different ladder
- Rerun gels with fresh TAE buffer
- Do a PCR using the thermocycler in room 303 of pSB1C3+RFP and colony PCR primers using thermo DNA polymerase (temperature gradient)
- Do a PCR using the thermocycler in room 403 of pSB1C3+RFP and colony PCR primers
- Make competent BL21 cells
- Autoclave baffel flasks
Equipment used:
- Thermocycler in 303
- Thermocycler in 403
- Electrophoresis machine
- Gel doc
- Autoclave
Protocol:
PCR mastermix
pSB1C3+RFP with pSB1C3 colony primers
6 x 20ul reactions
-5x HF buffer 4ul x 6 = 24ul
-10mM dNTPs 0.4ul x 6 = 2.4ul
-10uM FWD primer 1ul x 6 = 6ul
-we have 100uM so we will dilute 10ul primer + 90ul UP water = 100ul 10uM FWD primer
-10uM REV primer 1ul x 6 = 6ul
-we have 100uM so we will dilute 10ul primer + 90ul UP water = 100ul 10uM REV primer
-RFP - dilute to 1ng/ul (original 142ng/ul)
-1ul RFP + 141ul UP water
-1ul x 6 = 6ul - 1 (NTC) = 5ul
-phusion DNA polymerase 0.2ul x 6 = 1.2ul
-DMSO 0.6ul x 6 = 3.6ul
-total in mastermix without water or template = 24ul + 2.4u + 6ul + 6ul + 6ul + 1.2ul + 3.6ul = 43.2ul = 7.2ul per reaction
-for NTC: 7.2ul mastermix + 12.8ul UP water
-for remaining mastermix: 100ul - (43.2ul - 7.2ul NTC) - 5ul RFP = 59ul UP water
-add 20ul of mastermix to 5 PCR tubes
-temperature gradient:
1: 55 degrees
2: 59.3 degrees
3: 61 degrees
4: 65 degrees
NTC: 61 degrees
Thermocycler settings
Denaturing: 98 degrees - 30s
Annealing x30: 98 degrees - 10s
55-60 degrees - 30s
72 degrees - 363s
Extension: 72 degrees - 10min
Hold: 4 degrees
Observations:
Jun 29th 2018 Thermo Phusion Arg1 UNS2 FWD and UNS3 REV at 60C room 303.jpg
Jun 29th 2018 Thermo Phusion Arg1 (1ng) UNS2 FWD and UNS3 REV and digest at 60C room 303.jpg
Next steps:
- Temperature gradient PCR without DMSO
- Find Susie to do a biowaste disposal and autoclaving
- Redesign primers for arg1
Day 1, Tuesday 03/07
People In Lab: Daniel, Tashi, Jasmeen
Agenda:
- Growth curve for BL21 + Arg1 -> innoculation
Protocol:
- Growth Curve(BL-21 cells + arg1 plasmid)
- We started from innoculation.
- For first 2 hours, we took the OD measurement every 30 minutes.
- The plate reader was pre-set to 1) shake ( 1 mm amplitude, 7 sec) 2) measure ( 600mm wavelength, 5 flashes)
- After 2 hours, we took the OD measuremetn every 15 minutes.
- Since the measurements obtained were seemed to be random flucuation, the time interval for every measurement was switched back to 30mins (after ~5 hours)
Results:
Growth Curve
OD Measurements ( in triplicate) |
||||||
Time (h) |
1 |
2 |
3 |
log 1 |
log 2 |
log 3 |
0 |
0.0128 |
-0.0032 |
-0.009 |
-1.89279 |
/ |
/ |
0.5 |
0.0018 |
-0.0015 |
-0.0045 |
-2.74473 |
/ |
/ |
1 |
0.0013 |
-0.0015 |
-0.0024 |
-2.88606 |
/ |
/ |
1.5 |
-0.0002 |
-0.0013 |
-0.0075 |
/ |
/ |
/ |
2 |
0.0065 |
0.0004 |
-0.0073 |
-2.18709 |
-3.39794 |
/ |
2.25 |
0.0004 |
-0.002 |
-0.0073 |
-3.39794 |
/ |
/ |
2.5 |
0.0012 |
-0.0019 |
-0.0065 |
-2.92082 |
/ |
/ |
2.75 |
0.0007 |
-0.002 |
-0.008 |
-3.1549 |
/ |
/ |
3 |
0.0013 |
0.0006 |
-0.0078 |
-2.88606 |
-3.22185 |
/ |
3.25 |
0.0032 |
0.0052 |
-0.0069 |
-2.49485 |
-2.284 |
/ |
3.5 |
0.0026 |
0 |
-0.0061 |
-2.58503 |
/ |
/ |
3.75 |
0.0014 |
0 |
-0.0073 |
-2.85387 |
/ |
/ |
4 |
0.0011 |
0.0004 |
-0.0053 |
-2.95861 |
-3.39794 |
/ |
4.25 |
0.0056 |
0.0003 |
-0.0057 |
-2.25181 |
-3.52288 |
/ |
4.5 |
0.0076 |
0.0001 |
-0.0061 |
-2.11919 |
-4 |
/ |
4.75 |
0.0008 |
0.0009 |
-0.0073 |
-3.09691 |
-3.04576 |
/ |
5 |
0.0051 |
-0.0002 |
-0.0059 |
-2.29243 |
/ |
/ |
5.25 |
0.0049 |
0.0034 |
-0.0024 |
-2.3098 |
-2.46852 |
/ |
5.75 |
0.007 |
0.0088 |
0.0043 |
-2.1549 |
-2.05552 |
-2.36653 |
6.25 |
0.0156 |
0.0193 |
0.0187 |
-1.80688 |
-1.71444 |
-1.72816 |
6.75 |
0.0293 |
0.0403 |
0.0462 |
-1.53313 |
-1.39469 |
-1.33536 |
7.25 |
0.0681 |
0.0828 |
0.0946 |
-1.16685 |
-1.08197 |
-1.02411 |
7.75 |
0.1115 |
0.1328 |
0.1299 |
-0.95273 |
-0.8768 |
-0.88639 |
8.25 |
0.1629 |
0.2011 |
0.2112 |
-0.78808 |
-0.69659 |
-0.67531 |
image.png
Plan for future:
Redo growth curve and take OD measurements every 30 minutes.
Day 2, Wednesday 04/07
Individual Name: Daniel
People In Lab: Daniel, Tashi, Amalia, Jasmeen
Agenda:
- Inoculate BL21+arg1 and BL21 cells
- IPTG induction
- Make liquid LB medium
Protocol:
- Floatation Assay:
- Inoculate BL21 +arg1 cells and wait the OD reach 0.3 before 22hrs of IPTG induction
- Total of 6 tubes : 3 tubes ( BL21 + IPTG , BL21 + arg1, BL21 + arg1 + IPTG) * 2 treatments ( stand on tabletop and centrifuge under 350g for 4hrs)
- When OD600 = 0.47 we add 30uL of 3mM IPTG to the sample tube to make conc. reach 3uM in the medium.
Day 3, Thursday 05/07
People In Lab: Amalia, Daniel, NIna, Tashi, Jasmeen, Ahmed
Agenda:
- Floatation Assay
- Pick the overnight induction sample and measure the OD
- Inoculate new culture (BL21 +arg1 *2, BL21) and measure OD to reach 0.3
- IPTG induction for newly inoculated culture
- Growth curve with BL21+arg1 cells ( 30mins interval)
Protocol:
1. Floatation Assay:
- Based on Shapiro Lab protocol
- centrifuge the sample tubes under 350g for 4 hrs
- 3 sample tubes were set on the benchtop
Change plan for the floatation assay:
- starting from 5 ml of overnight culture for 16hrs
- 1:100 dilution of the starting culture and let the OD reaches 0.5
- Add IPTG to make conc. of 0.4mM(maybe 0.8mM for cell line we used) in the cell culture and start the induction for 22hrs under 30oC.
- After induction, centrifuge under 350g for 4 hrs
2. Growth curve:
- starting from inoculation
- the cell was grown in shaker( 220RPM & 37oC)
- Take the OD every 30 mins ( add 200ul to the plate reader)
Results:
Flotation observation:
BL21+arg1 Benchtop.jpg
BL21+IPTG Benchtop.jpg
BL21+arg1+IPTG Benchtop.jpg: Floating tissue observed
BL21+arg1 centrifuged.jpg
BL21 + IPTG Centrifuged.jpg: Floating tissue observed why?
BL21+arg1+IPTG centrifuged.jpg: Floating tissue observed
Growth Curve:
0-11 hrs
image.png
14.5-25 hrs
image.png
Day 4, Friday 06/07
People In Lab: Amalia, Daniel, NIna, Tashi, Jasmeen, Ahmed
Agenda:
- Streak the plate of BL-21 non-transformed cell onto LB only plate
- Run PCR with Phusion
- Re-design the Arg1-UNS2&uns3 primers
- Take reading for 23/24 hrs OD of growth curve tubes in the morining(results was already added to the growth curve
Protocol:
- PCR MasterMix: Arg1 UNS2 FWD UNS3 REV (temp graident) 58 560C
- HF buffer 5X 8ul
- 10mM dNTPs 0.8ul
- 10um FWD primer 2ul
- 10um REV primer 2ul
- 1ng/ul Arg1 2ul
- phusion DNA polyemrase 0.4ul
Results:
Arg1 UNS2 FWD UNS3 REV (temp graident) 58 56C.jpg: no band observed
Day 1, Tuesday 03/07
People In Lab: Daniel, Tashi, Jasmeen
Agenda:
- Growth curve for BL21 + Arg1 -> innoculation
Protocol:
- Growth Curve(BL-21 cells + arg1 plasmid)
- We started from innoculation.
- For first 2 hours, we took the OD measurement every 30 minutes.
- The plate reader was pre-set to 1) shake ( 1 mm amplitude, 7 sec) 2) measure ( 600mm wavelength, 5 flashes)
- After 2 hours, we took the OD measuremetn every 15 minutes.
- Since the measurements obtained were seemed to be random flucuation, the time interval for every measurement was switched back to 30mins (after ~5 hours)
Results:
Growth Curve
OD Measurements ( in triplicate) |
||||||
Time (h) |
1 |
2 |
3 |
log 1 |
log 2 |
log 3 |
0 |
0.0128 |
-0.0032 |
-0.009 |
-1.89279 |
/ |
/ |
0.5 |
0.0018 |
-0.0015 |
-0.0045 |
-2.74473 |
/ |
/ |
1 |
0.0013 |
-0.0015 |
-0.0024 |
-2.88606 |
/ |
/ |
1.5 |
-0.0002 |
-0.0013 |
-0.0075 |
/ |
/ |
/ |
2 |
0.0065 |
0.0004 |
-0.0073 |
-2.18709 |
-3.39794 |
/ |
2.25 |
0.0004 |
-0.002 |
-0.0073 |
-3.39794 |
/ |
/ |
2.5 |
0.0012 |
-0.0019 |
-0.0065 |
-2.92082 |
/ |
/ |
2.75 |
0.0007 |
-0.002 |
-0.008 |
-3.1549 |
/ |
/ |
3 |
0.0013 |
0.0006 |
-0.0078 |
-2.88606 |
-3.22185 |
/ |
3.25 |
0.0032 |
0.0052 |
-0.0069 |
-2.49485 |
-2.284 |
/ |
3.5 |
0.0026 |
0 |
-0.0061 |
-2.58503 |
/ |
/ |
3.75 |
0.0014 |
0 |
-0.0073 |
-2.85387 |
/ |
/ |
4 |
0.0011 |
0.0004 |
-0.0053 |
-2.95861 |
-3.39794 |
/ |
4.25 |
0.0056 |
0.0003 |
-0.0057 |
-2.25181 |
-3.52288 |
/ |
4.5 |
0.0076 |
0.0001 |
-0.0061 |
-2.11919 |
-4 |
/ |
4.75 |
0.0008 |
0.0009 |
-0.0073 |
-3.09691 |
-3.04576 |
/ |
5 |
0.0051 |
-0.0002 |
-0.0059 |
-2.29243 |
/ |
/ |
5.25 |
0.0049 |
0.0034 |
-0.0024 |
-2.3098 |
-2.46852 |
/ |
5.75 |
0.007 |
0.0088 |
0.0043 |
-2.1549 |
-2.05552 |
-2.36653 |
6.25 |
0.0156 |
0.0193 |
0.0187 |
-1.80688 |
-1.71444 |
-1.72816 |
6.75 |
0.0293 |
0.0403 |
0.0462 |
-1.53313 |
-1.39469 |
-1.33536 |
7.25 |
0.0681 |
0.0828 |
0.0946 |
-1.16685 |
-1.08197 |
-1.02411 |
7.75 |
0.1115 |
0.1328 |
0.1299 |
-0.95273 |
-0.8768 |
-0.88639 |
8.25 |
0.1629 |
0.2011 |
0.2112 |
-0.78808 |
-0.69659 |
-0.67531 |
image.png
Plan for future:
Redo growth curve and take OD measurements every 30 minutes.
Day 2, Wednesday 04/07
Individual Name: Daniel
People In Lab: Daniel, Tashi, Amalia, Jasmeen
Agenda:
- Inoculate BL21+arg1 and BL21 cells
- IPTG induction
- Make liquid LB medium
Protocol:
- Floatation Assay:
- Inoculate BL21 +arg1 cells and wait the OD reach 0.3 before 22hrs of IPTG induction
- Total of 6 tubes : 3 tubes ( BL21 + IPTG , BL21 + arg1, BL21 + arg1 + IPTG) * 2 treatments ( stand on tabletop and centrifuge under 350g for 4hrs)
- When OD600 = 0.47 we add 30uL of 3mM IPTG to the sample tube to make conc. reach 3uM in the medium.
Day 3, Thursday 05/07
People In Lab: Amalia, Daniel, NIna, Tashi, Jasmeen, Ahmed
Agenda:
- Floatation Assay
- Pick the overnight induction sample and measure the OD
- Inoculate new culture (BL21 +arg1 *2, BL21) and measure OD to reach 0.3
- IPTG induction for newly inoculated culture
- Growth curve with BL21+arg1 cells ( 30mins interval)
Protocol:
1. Floatation Assay:
- Based on Shapiro Lab protocol
- centrifuge the sample tubes under 350g for 4 hrs
- 3 sample tubes were set on the benchtop
Change plan for the floatation assay:
- starting from 5 ml of overnight culture for 16hrs
- 1:100 dilution of the starting culture and let the OD reaches 0.5
- Add IPTG to make conc. of 0.4mM(maybe 0.8mM for cell line we used) in the cell culture and start the induction for 22hrs under 30oC.
- After induction, centrifuge under 350g for 4 hrs
2. Growth curve:
- starting from inoculation
- the cell was grown in shaker( 220RPM & 37oC)
- Take the OD every 30 mins ( add 200ul to the plate reader)
Results:
Flotation observation:
BL21+arg1 Benchtop.jpg
BL21+IPTG Benchtop.jpg
BL21+arg1+IPTG Benchtop.jpg: Floating tissue observed
BL21+arg1 centrifuged.jpg
BL21 + IPTG Centrifuged.jpg: Floating tissue observed why?
BL21+arg1+IPTG centrifuged.jpg: Floating tissue observed
Growth Curve:
0-11 hrs
image.png
14.5-25 hrs
image.png
Day 4, Friday 06/07
People In Lab: Amalia, Daniel, NIna, Tashi, Jasmeen, Ahmed
Agenda:
- Streak the plate of BL-21 non-transformed cell onto LB only plate
- Run PCR with Phusion
- Re-design the Arg1-UNS2&uns3 primers
- Take reading for 23/24 hrs OD of growth curve tubes in the morining(results was already added to the growth curve
Protocol:
- PCR MasterMix: Arg1 UNS2 FWD UNS3 REV (temp graident) 58 560C
- HF buffer 5X 8ul
- 10mM dNTPs 0.8ul
- 10um FWD primer 2ul
- 10um REV primer 2ul
- 1ng/ul Arg1 2ul
- phusion DNA polyemrase 0.4ul
Results:
Arg1 UNS2 FWD UNS3 REV (temp graident) 58 56C.jpg: no band observed
Day 1, Monday 16/07
People In Lab: Daniel, Nina, Tashi, Jasmeen
Agenda:
- Making AMP stock solution
- Make LB+ AMP plates
- Overnight cultures of BL21 and BL21+ Arg1
Running very low on AMP powder
Day 2, Tuesday 17/07
People In Lab: Daniel, Nina, Tashi, Jasmeen
Agenda:
- PCR of ARG1 plasmid using new IDT primers (UNS3 REV & UNS 2 FWD)
- 1:100 dilution BL21 +ARG 1 in baffle flask, BL21 in baffle flask
Protocol:
1. ARG1 new primer gradient PCR [64.5°C-67°C (extra rxn at 66°C)]:
- 7 RXNs 20ul each (One without a template)
- annealing temp: 660C
- Reagent used:
- Q5 Buffer (4μl x 7) 28ul
- 10mM FWD primer (1μ x 7) 7ul
- 10mM REV Primer (1μ x 7) 7ul
- 10mM dNTPs (0.4μl x 7) 2.8ul
- Q5 ploymerase (0.2μl x 7) 1.4ul
- 1μg/μl Template DNA (6μ x 6) 6ul
- Nuc Water Total mix with template for each rxn = 7.6μl
- (20μl each rxn - 7.6μl = 12.5μl ) x 6 = 74.4ul H20 for mastermix
- Total mix without template for each rxn = 6.6μl
- 20μl each rxn - 6.6μl = 13.5μl H2O for NTC
2. OD readings of BL21+ARG1 and BL21 for induction.
- 1ml was taken out of each culture every hour and placed in a cuvette
- OD was measured using a spectrophotometer
3. Cultures were induced with IPTG at 2:40pm. replicate 1 of BL21+ARG1 was induced with 0.4mM of IPTG. Replicate 2 of BL21+ARG1 was induced with 0.8mM IPTG. BL21 cells were not induced with IPTG.
Results
1. ARG1 PCR with new primers results
37291721_2649158358642891_3010098950041501696_n.jpg
2. OD readings
Time |
BL21+ Arg1 rep1 |
BL21+Arg2 rep2 |
BL21 rep1 |
1:16pm |
0.086 |
0.097 |
0.323 |
2:30pm |
0.353 |
0.359 |
1.081 |
Day 3, Wednesday 18/07
People In Lab: Amalia, Nina, Tashi
Agenda
- Dpn1 digest of PCR1 product
- PCR purification of PCR1 products
- Nanodrop of PCR1 products after digest and purification
- Overnight culture LB+BL21
- Overnight culture of DH10B Arg1 and pSB1C3
- place tubes in centrifuge 1hr
Dpn1 Digest
We have 10ul of PCR product per tube [4 tubes]
- 8ul of PCR product
- 1 ul of Dpn1
- 1 ul of cutsmart (10x)
10 ul of rxn (total)
PCR Purification (16,000 g/ 13,000 rpm)
- 30 ul sample
- 2:1 ratio binding buffer sample = 60ul
- Load sample onto column
- spin 1 min and discard flow through
- reinsert column, add 200ul repeat DNA wash buffer
- Transfer column to 1.5ml centrifuge tube
- add 6ul nuclease free water
- wait 1 min, spin 1 min
Completed nanodrop of 1ul of PCR purified product
concentration: 100.1 ug/ul
Day 4, Thursday 19/07
People In Lab: Amalia, Tashi, Ahmed, Daniel, Jasmeen
Agenda
- PCR on new primers Arg1+UNS2FWD&UNS3REV (anneailing temp 66°C)
- Nanodrop
- Purification of PCR products
- PCR product digest
- Cell competency for BL21
- Gibson assembly (blue protein and Arg1+UNS1&UNS3
- Miniprep: Arg1+cor, RFP + UNS
- Transform gibson into DH5⍺ cell from the kit
- transform RFP from competency cell kit into BL21 cells
Protocols
PCR Calculation (7 reactions planned) 50 ul
- Master Mix for 8 reactions
- Reagent used:
- Q5 master mix (25μl x 8) 200ul
- 10mM FWD primer (2.5μl x 7) 20ul
- 10mM REV Primer (2.5μl x 7) 20ul
- 1μg/μl Template DNA (2.5μl x 7) 17.5ul
- Nuc Water Total mix with template for each rxn = 17.5μl
20μl for NTC
OD readings 1:100 dilution of BL21 for competency
Time |
BL21 rep1 |
BL21 rep2 |
12:13pm |
0.132 |
0.133 |
12.45pm |
0.279 |
0.279 |
1:08pm |
0.459 |
0.466 |
Note: Competency protocol was started after the last OD reading
Nanodrop ARG1 cor and RFP+UNS
Plasmid |
Conc (ng/ul) |
ARG1 cor |
64.7 |
RFP+UNS |
85.3 |
PCR gel for ARG1 and UNS (primers UNS2FWD, UNS3REV)
1kb+ NEB ladder |
1 |
2 |
3 |
4 |
5 |
6 |
NTC |
Gel result
image.png
DPN1 digest protocol
- For a 10μl rxn x 2 = 20μl
- 16μl PCR product (well #1 ARG1 with UNS2FWD UNS3 primers)
- 2μl cutsmart buffer
- 2μl DPNI
DNA cleanup
- 2:1 ratio binding buffer :Digest product
- 40μl buffer:20μl digest product
- For elution step use 20μl nuclease free water
Nanodrop ARG1+UNS after cleanup
Plasmid |
conc(ng/μl) |
260/280 |
260/230 |
ARG1+UNS |
75.4 |
1.96 |
1.65 |
Gibson calculations (note limit for DNA in gibson rxn=0.2 picomoles)
ARG1+UNS
DNA length=12209bp
picomoles we want= 0.0667pmol
DNA Mass we had according to NEB calculator= 503.2ng
503.2ng/75.4ng/μl= 6.67μl --> ARG1+UNS added to gibson rxn
Blue protein (K=BBa_K592009)
DNA length= 764bp
picomoles we want= 0.1333333pmol
DNA mass we had according to NEB calculator=62.95ng
Note: the blue protein was resuspended in 50μl of nuclease free water for a final concentration of 20ng/μl
62.95ng/20ng/μl=3.15μl--> blue protein added to gibson
Transformation of gibson products
Gibson positive control (plated 100μl transformed DH5a (20μl of DH5a cells + 2 μl positive control gibson) onto AMP plate)
Gibson positive control transformation (plated 100μl transormed DH5a (20μl DH5a cells + positive control plasmid) onto AMP plate)
Gibson products (plated 50μl, 100μl, 200μ transformed DH5a (50μl DH5a cells + 2μl of gibson product) onto KAN plates)
Tranformation of RFP plasmid from competency cell kit
plated 100μl of transformed BL21 cells (100μl BL21 cells + 10pg, 50pg, 100pg RFP plasmid) onto CAM plates
Day 5, Friday 20/07
People In Lab: Amalia, Tashi, Ahmed, Nina
Agenda
- Check Gibson and Bl21 competency plates
- re-transform Gibson positive controls and gibson products
Results from Gibson
Both positive control plates (transformation control and gibson control) have colonies
None of the gibson product plates have colonies
image.png: Gibson plates: top left is positive control for transformation, top right is positive control for gibson, bottom 3 plates are plates with our gibson product transformation. Note the fact that only positive controls have colonies.
Troubleshooting
transformation was repeated
6 KAM plates were plated each with 200μl of transformed DH5a cells (50μl of DH5a cells transformed with 2μl of gibson product)
2 positive control plates: positive control for transformation (20μl of DH5a cells transformed with 2μl positive control plasmid)
positive control for gibson (20μl of DH5a cells transformed with 2μl of positive control gibson)
Results competency plates
plate plated with 50pg of plasmid grew 4 colonies
plate plated with 100pg of plasmid grew 3 colonies
plate plated with 10pg of plasmids did not grow colonies
image.png: 10pg
image.png: 50pg
image.png: 100pg
Note: these photos were taken after 4 days of plating but small colonies were observed after incubation overnight