Team:NRP-UEA-Norwich/Notebook
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- Started tweeting from the UEA iGEM Twitter account. | - Started tweeting from the UEA iGEM Twitter account. | ||
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- | - Created the UEA iGEM 2014 Facebook page.</p> | + | - Created the UEA iGEM 2014 Facebook page. |
- | <p> | + | </p><p> |
- Emailed MustardTV regarding exposure for our project (local to Norwich).</p> | - Emailed MustardTV regarding exposure for our project (local to Norwich).</p> | ||
<h2>Wednesday</h2> | <h2>Wednesday</h2> |
Revision as of 17:02, 13 October 2014
Lab Notebook
Week One 16/06/2014
Monday
- Contacted by email UEA based organisations UEA:TV, Concrete and Livewire regarding possible exposure for our project.- Emailed Sam Fountain (UEA) regarding possible sources of funding and who to approach from the University of East Anglia.
Tuesday
- Started tweeting from the UEA iGEM Twitter account.- Created the UEA iGEM 2014 Facebook page.
- Emailed MustardTV regarding exposure for our project (local to Norwich).
Wednesday
- Created a poster design for the Oxford SynBio meet up held at Oxford University. - Poster printedThursday
- Attended Synthetic Biology 'Meet up' hosted by Oxford for iGEM teams across the country.Friday
- Submitted 'About our lab' form for iGEM before deadline.Week Two 23/06/2014
Monday
- Completed The Sainsbury Laboratory (TSL) safety induction.- Collected synthesised samples from DNA 2.0 and transformed DNA into E.coli using electrocompetent cells and electroporation. Added 500 μl of Soc broth and incubated for 40 minutes at 37 °C. Spreadplated onto agar plates containing Kanamycin and incubated O/N at 37 °C.
Tuesday
- Selected a single colony from each of the eleven plates and the colonies were grown in TY broth with Kanamycin O/N.- Transformation of pSB1C3 plasmid containing RFP into E.coli using electroporation. Incubated with 50 μl of Soc broth at 37 °C for 1 hour.
- Spreadplated E.coli cells which have been transformed with the pSB1C3 + RFP plasmid.
- Completed calculations for Dig-Lig experiments (Size and conc. of DNA parts calculated,size of acceptor calculated, order of constructs for each reaction determined, dilution and DNA conc. for each reaction determined) Ratio of 2:1, constructs:acceptor (plasmid).
Wednesday
- Midi prep following the Qiagen protocol of the 9 constructs previously synthesised by DNA 2.0 and transformed on Day 2 and DNA conc. of each constrcut determined using the nanodrop. Dig-Lig calculation spread sheet completed using these concentrations.- Set up the first 11 Dig-Lig experiments, placed into PCR block on the slow protocol.
- Carbenicillin plates made and spreadplated with 40 μl of XGAL and 100 μl of IPTG. Plates left to dry upside down in 37°C incubator.
- Transformation of GG DNA into electrocompetent E.coli cells, PROTOCOL:
• Cells removed from -80°C freezer and allowed to thaw.
• A 5 µl sample of DNA was added to a 50 µl aliquot of cells.
• Transfered each 55 µl sample into a cuvette.
• Electroporation pulse on setting ECR1.
• A 500 µl of SOC broth was added to the cuvette.
• A 555 µl cuvette sample was transferred to an eppendorf tube and incubated for 40 min at 37°C.
• A 100 µl sample was spreadplated onto agar plates containing carbenicillin and incubated O/N at 37°C.
- A 20 µl PCR reaction was set up using a GG level 1 acceptor as template DNA containing the primers P1: 0349(PRO+5U) and 0353 (3U+TER) and P2: 0350 (PRO+5U) and 0354 (3U+TER).
- A TBE buffer 1% agarose gel was poured for diagnostic purposes to check the amplification of the PCR products.
- PCR product purification
• Pre-percipitation to remove TAQ polymerase and protein was completed followed by phenolchloroform extraction (x2). Aqueous layer is removed and discarded leaving DNA.
• Precipitation to remove buffer was carried out by adding Na acetate (10%) and ethanol causing the DNA to come out of solution. Aspirator was used to remove buffer, salt and ethanol.
• A salt wash was completed to remove the acetate and ethanol.
• Sample was incubated at 65°C for 2 min to evaporate the ethanol.
Thursday
- Checked Dig-Lig tranformation plates grown O/N and poor blue white selection observed with many blue colonies.- Selected 2 white colonies from each plated and colony PCR performed.
- Following colony PCR, amplified fragments ran on gel to determine size and therefore whether they contained the construct.
- Decided to repeat the 11 Dig-Lig experiments
- Ran digested PCR product from 25.06.2014 on a diagnostic 1% agarose gel in TBE buffer and determined that LacZ had internal restriction enzyme cut sites and product was split into two bands.
Friday
- Found poor blue/white selection on dig-ligs from 26.06.14. Suspected to be due to either the enzyme used or PCR block.- Set up a new set of dig-ligs to test the source of this problem.
Week Three 30/06/2014
Monday
- Set up 10 Dig-Lig reactions with new BSA1 enzyme provided by TSL.- DNA was transformed into E.coli using electroporation method previously discussed.
- Transformed bacteria was spreadplated onto canamycin plates containing XGAL and IPTG and incubated O/N at 37°C.
- Mini-prep of DNA obtained from Week 2's successful Dig-Lig experiments according to Qiagen protocol. However, DNA eluted in 25 µl of eluting buffer rather than 50 µl as protocol suggests.
- DNA conc. of each sample quanitifed using the Nanodrop.
- DNA diluted to obtain 5 ng in each 5 µl sample.
- Sense and Antisense primers to each 5 µl DNA (+H20) to achieve 20 µl sample in total and sent for sequencing to verify construct sequence.
Tuesday
- Selection of 2 white colonies from 30.06.14 Dig-Lig transformed plates for a colony PCR reaction. The same 2 colonies were grown in 5 ml of SOC broth O/N at 37°C.- Poured a 1% agarose gel using TBE buffer with a 1:20,000 dilution of ethidium bromide.
- Gel run with Dig-Lig PCR products.
Wednesday
- Transformed 5 constructs into Argobacterium tumefacians- Mini prep of 5 constructs from colonies picked 1.7.14
- Electroporated to transform into agro
- Incubated at 28 °C for 1 hour
- Spread plated transformed agro
Thursday
- Set up a 20 µl PCR reaction using primers synthesized from Sigma and a level 1 acceptor as the template DNA• Pro + 5UTR
• CDS
• Ter + 3UTR
- Ran PCR product on a gel to check amplification
- PCR product purification using phenol chloroform
Friday
- Digest of PCR samples from 3.7.14- Gel purification and quantification of digested fragments (now ready to ligate into PSB1C3 backbone)
- Digest of PSB1C3 plasmid with EcoR1 and PST1 (removes blunt ends)
- Dephosphorylation of plasmid backbone
- Colony PCR of colonies picked from agro plates (transformed 10.7.14)
Week Four 07/07/2014
Monday
- Colonies picked from agrobacterium plates from 2.7.14- Overnight culture in 5 ml of broth containing Carbenicillin, Gentamicin, Rifampicin
Tuesday
- No wet lab work completed- Team meeting to discuss human practices events we would like to organise
Wednesday
- Safety induction in UEA labs for all team members- Human Practices meeting. Ideas included: Food security event, surveys, School events and possible speed debate.
Thursday
- Agrobacterium-mediated transient expression in leaves of N. benthamiana PROTOCOL:1. Single colony of each constructs 2,3,4,10,11 grown overnight at 28 °C in 5 ml media containing chloramphenicol.
2. Pellet by centrifugation at 4000 rpm for 15 min.
3. Resuspend in 10 mM MES, 10 mM MgCl2 and 150 μM Acetosyringone.
4. 1:100 dilution to give a final OD of 0.1-0.5
5. Incubate at RT for 4 hours.
6. Create a small puncture using a needle on the underside of N. benthamiana leaves of plants 6-8 weeks old. Using a blunt syringe infiltrate the agro constructs into the leaf puncture. Each construct is infiltrated into 4 sections on one leaf. 2 constructs per plant.
7. Store plants in controlled environment at 19-23 °C for 3 days.
-Ligation reaction to join PSB1C3 and GG compatible ends.
Friday
- Analysis of infiltrations using light microscope and UV light.- Colonies picked from ligation on 10.7.14 (GG compatible PSB1C3 for accepting Pro, CDS, Ter level 0 parts) and grown in 5 ml of LB broth, incubated in shaker O/N at 37 °C
- Attended the UEA BIO Research Colloquium from 9am - 3.30pm
Week Five 14/07/2014
Monday
- Mini prep of Mo Flipper Modules DNA- Quantification of DNA (Nanodrop)
PRO 1 - 78.5 ng/µl
PRO 2 - 93.5 ng/µl
PRO 3 - 73.8 ng/µl
CDS 1 - 77.7 ng/µl
CDS 2 - 71.1 ng/µl
CDS 3 - 66.8 ng/µl
TER 1 - 91.8 ng/µl
TER 2 - 89.2 ng/µl
TER 3 - 89.2 ng/µl
Tuesday
- Visited The CUT venue in Halesworth in preparation for the Food for Thought organised event on the 26th July.Wednesday
- Meeting with Dr Anna Smajdor, a bio-ethicist, to discuss ethical implications of our project.- Discussed the need for ethical approval for data collection for possible ideas such as surveys.
Thursday
- Team meeting to discuss how lab work is progressing and who/when the further lab work will be carried out.Friday
- Preparation of media required: LB, LB agar, LB + Chloramphenicol plates and LB + Kanamycin plates.Week Six 21/07/2014
Monday
- 2 single colonies picked from agro plates grown 02/07/2014.- Colonies added to 5 ml of broth containing Carbenicillin, Gentamicin and Rifampicin
Tuesday
- Transformation of synthesised DNA from DNA 2.0 into E.coli. Tubes 1 to 7.1. AtPR1
2. ArvBS3
3. NbBi1-RNA
4. NbProB-RN
5. AvrXa27 T
6. OsXa27 Pro
7. Control (No DNA)
- Followed heat shock protocol:
- 5 µl DNA added to 50 µl of chemically competent E.coli
- Spreadplated onto agar plates containing KAN
- Incubated O/N at 37°C
Wednesday
- Met with Dr Kay Yeoman, BIO outreach officer (UEA) to discuss activities for school outreach events.- Discussed activities for 'Food for Thought' event at the cut on 26/07 including visual representations of crop losses in cylinders.
Thursday
- DNA preparation of Nevada 2010 biobricks in preparation for characterisation.- O/N culture of single colonies of level 0 constructs (currently in E.coli)
Friday
- Mini-prep of O/N cultures grown on 23/07/14 of DNA synthesised by DNA 2.0.Tubes 1 to 6:
1. AtPR1 Conc: 182.2 ng/µl 260/280: 1.94
2. ArvBS3 Conc: 342.7 ng/µl 260/280: 1.93
3. NbBi1-RNA Conc: 152.2 ng/µl 260/280: 1.95
4. NbProB-RN Conc: 181.6 ng/µl 260/280: 1.90
5. AvrXa27 T Conc: 263.2 ng/µl 260/280: 1.90
6. OsXa27 Pro Conc: 286.5 ng/µl 260/280: 1.90
- DNA quantified using Nanodrop and blanked with EB buffer.
- Further mini prep of O/N cultures grown on 22/07/14 and 23/07/14 from the BioBricks requested from the 2010 Nevada team's (https://2010.igem.org/Team:Nevada) project 5 mL was analysed from an inoculation of 10 mL LB + CAM. Biobricks obtained are: BBa_K414001, BBa_K414003, BBa_K414004 and BBa_K414008
- Run on a 1% agarose gel with TAE buffer.
- Preparation of the 'Food for Thought event at 'The CUT' tomorrow where we will be giving presentations and demonstrations about food security.
- Created business cards for distribution at outreach events
- Collected leaflets for distribution
- Digest of PSB1C3 to drop out RFP and ran on 1% TAE agarose gel to characterise.
Week Seven 28/07/2014
Monday
- Meeting with Tom Shakespeare based at UEA Med to discuss the ethics of 'The Green Canary' Project.Tuesday
- Digest of PRO, CDS and TER with Bsa1- Set up level one dig-ligs 1, 5, 9, 15, 16, 17, 18, 19 and PCR.
- Agrobacterium transformation. 2 μl DNA into 50 μl of cells followed by electroporation. Incubation in LB for 2 hours. Spreadplated onto LB containing: 1 μl/ml of Ampicillin (100 mg/mL), 1 μl/ml of Rif (25 mg/mL) and 1 μl/ml of Gentamycin (10 mg/mL). Incubated O/N at 30 °C.
Wednesday
- Made 2 L of LB Agar- Poured 8 agar plates containing Ampicillin (1 µl/ml). Spreadplated IPTG and X-GAL. Spreadplated the 8 dig-lig reactions created on the 28/07/14. Tubes 1,5,9,15,16,17,18,19.
- Picked 1 colony from PRO, CDS and TER plates with Psb1c3 + RFP containing BSA1 sites to make them GG compatible to be grown in an O/N culture (37°C with shaking) in 5 ml of LB.
- Picked 1 colony of the newly transformed DNA from DNA 2.0 to be grown in an O/N culture (37°C with shaking) in 5 ml of LB.
Thursday
- Picked 1 white colony from 29/07/14 transformed dig-lig plates and added to 5 ml LB + 5 μl Ampicillin and incubated at 37 °C also added to 50 μl of PCR Master Mix containing:1 μl DNTPs
2 μl Primer 1
2 μl Primer 2
5 μl Buffer
2 μl MgCl2
0.5 μl BIOTAQ Enzyme
37 μl Water
- PCR programme:
Step 1 : 95 °C 5 min
Step 2 : 95 °C 1 min
Step 3 : 54 °C 1.5 min
Step 4 : 72 °C 1 min
Step 5 : 72 °C 5 min
Steps 2, 3, 4 repeated x 34 times
- Run on a 1 % agarose TAE gel at 100V. Each well loaded with 2 μl of loading dye and 20 μl of DNA. Two 1kb ladders loaded.
- DNA mini prep of cultures from 29/07/14 (DNA 2.0 level 0's and PRO, CDS, TER) (2.5 mls)
- Glycerol stocks made from 1 ml of O/N culture.
- Transformations of DNA iGEM #2-19 and Vectors #1-4 intro E.coli to generate more DNA.
Friday
- Arranged meeting with Mark Wilkinson to discuss University regulation ethics approval for the Green Canary ProjectWeek Eight 04/08/2014
Monday
- Colony PCR of Agrobacterium plates containing constructs 2,3,4,10,11 which had been grown over the weekend at 28 °C.- Colony PCR products run on a 1% agarose TAE gel with a DNA positive control.
- Picked single colonies of Level 1 constructs: 1, 5, 9, 15, 16, 17, 18, 19. Colony PCR of these level 1 constructs.
- 2 Agrobacterium colonies selected from each plate to be grown in 5 ml of LB, 100 µl Ampicillin, 200 µl Gentamycin and 200 µl Rifampicin O/N at 28 °C with shaking.
- 93 agar plates autoclaved and poured for Human Practices school events in September, kept in cold room at 4 °C.
Tuesday
- Added 2g of sucrose and 0.441g of MS salts to 100ml of sterile water + Acetosyringone.- Spun down agrobacterium cultures grown on 4.8.14
- Resuspended pellets in 10ml of prepared solution
- Left to grow on the bench for 3 hours
- Each construct infiltrated into one nicotiana benthamiana plant on two separate leaves
- Mini preps of level 1 dig-ligs (1,5,9,15,16,17,18,19)
- Quantification of DNA required for next level two dig-ligs.
Wednesday
- Set up level 2 dig-lig reactions (Vector, buffer, inserts, ligases)Level 2 Constructs:
A= 35s_AvrBS3 + BS3_GFP
B= 35s_AvrBS3 + BS3_NbHb1
C= BS3_Bax + BS3_Bi1RNAi
D= 35s_AvrBS3 + BS3_Bax +BS3_BiRNAi
E= 35s_Bax1 + 35s_BiRNAi
F= PDF1.2_Bax1 + PDF1.2_BiRNAi
G=PR1_Bax + PR1_Bi1RNAi
- PCR of Level 2 Constructs (cycles: 3 cycles of 10 minutes 37°C, 10 minutes 16°C, followed by 10 minutes 37°C, 20 minutes 65°C , 4°C forever)
- Made 1µl/ml Streptomycin plates. Spread with 100µl IPTG and 80µl of X-gal per plate
- Transformed 5µl of level 2 construct DNA from PCR into 50µl E.coli cells, electroporation of cells, spread (amount?) onto streptomycin plates, incubated overnight at 37°C
Thursday
- Charles Brearley (UEA) demonstrated the use of the epi-fluorescence microscope in the Teaching Lab.- Infiltrations from 5/8/14 did not show GFP fluoresence as expected so will need to be repeated.
- Mischa discussed ethics approval for The Green Canary project with Dr Mark Wilkinson and Dr Micheal Pfiel.
Friday
- Spread the level 2 constructs A-G on spectinomycin plates with IPTG and XGAL for blue white selection as well as plating the transformation of vector pAGM8031.- Plated end linkers 2 and 3 on ampicillin and all plates incubated overnight at 37°C.
- Picked colonies of Agrobacterium tumerfaciens, 2, 3, 4, 10 and 11 and grew in an overnight culture with shaking (28°C) with 400 μL LB and 1μL/mL of ampicillin.
- We invited the Cambridge iGEM team up to meet us and discuss each others projects as well as future collaborations and gave them a tour of the NRP, JIC and UEA. We discussed providing Cambridge with our MoFlipper so they can submit their parts in BioBrick form as well.
- Jack met with Graeme Byrne to prepare for meeting with InCrops on the 28th of August.
Week Nine 11/08/2014
Monday
- Picked 2 colonies of the level 2 dig-lig's transformed on friday. A, B, C, D, E, F, G and the level 2 Vector pAGM8031. Colonies grown in 1 ml of LB containing 1 μL/mL of Spectinomycin O/N.- Colony PCR of agro cultures grown for 2 days. Construct numbers 2, 3, 4, 10, 11. 4 cultures per construct were grown. Run on a 1% TAE gel with a positive control of pure DNA for each construct.
Tuesday
- Mini prep of Level 2 E. coli A-G (2 of each, e.g A1 & A2) and Level 2 vector in preparation for PCR.- Quantified all previously prepared DNA
- Ran 1% TAE agarose gel of Level 2 colony PCR products.
Wednesday
- Transformation of Mo Flipper modules (Pro, CDS, Ter, CGCT) by Calcium Chloride heat shock.- Spreadplated each Flipper module onto LB plates containing Chloramphenicol.
- Glycerol stock made for each transformation.
Thursday
- Collected plants from TSL but unable to infiltrate as positive control was not saturated enough.Friday
- Set up overnight cultures of all Agro. transformations (2.1, 3.1, 4.1, 10.2 and 11.1).- Set up overnight cultures of Mo Flippers, to be incubated over the weekend so they can be minipreped and sent for sequencing.
Week Ten 18/08/2014
Monday
- Transformed Agro for Canary 1 experiments and spreadplated onto LB plates containing Rif, Gen and Amp antibiotics and stored at 28 °C for 2 days.- Infiltration of Agro constructs 2,3,4,10,11 into N. Benthamiana and plants stored in Plant Growth room at UEA O/N.
- Cells from Flipper cultures harvested and frozen at -20 °C O/N.
Tuesday
- Mini prep of all 4 Mo flipper modules (PRO, CDS, TER CGCT)- Nanodrop quantification- concentration of DNA not great enough for sequencing.
- O/N cultures of Mo flippers
- Discussions with head of school regarding authorised absence for iGEM
Wednesday
- O/N cultures of agro level 1s and 2s- Mini prep of O/N cultures of mo flippers, quantification of DNA - acceptable amount to be sequenced
Thursday
- Mo flipper DNA prepared and sent for sequencing- Glycerol stocks of agro level 1 and 2 constructs
- Meeting with Michael Pfeil regarding ethics approval for surveys
- Set up 100 mL cultures for all four Flippers
- Checked infiltrations under UV but no fluorescence observed
Friday
- Midiprep of overnight Mo flipper cultures from wk10 d4.- Quantification of DNA from Mo flipper midiprep.