Team:UIUC Illinois/Notebook
From 2014.igem.org
(Difference between revisions)
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<li>100uM Theobromine (10mL)</li> | <li>100uM Theobromine (10mL)</li> | ||
<li>250uM Caffeine + 250uM Theobromine (10mL)</li> | <li>250uM Caffeine + 250uM Theobromine (10mL)</li> | ||
- | <ul><br><br> | + | </ul><br><br> |
(page 169 on bottom, can’t read XW’s part) | (page 169 on bottom, can’t read XW’s part) | ||
+ | <ul style="text-indent:30px;"> | ||
<li>Take 1mL of I4/I5 LB cultures and spin for 2 minutes at 8000 rpm</li> | <li>Take 1mL of I4/I5 LB cultures and spin for 2 minutes at 8000 rpm</li> | ||
<li>Removed supernatant</li> | <li>Removed supernatant</li> |
Revision as of 20:53, 17 October 2014
-
PROJECT NOTES
- NOTES BY MONTH
Monday 9th June
ASDF Made LB broth using 10 grams of bacto agar + 12 grams HiVeg LB broth + 600 mL ddH2OAutoclaved 1.5 mL Eppendorf tubes as well as LB
Poured plates of LB and chloramphenicol (CAM)
Streaked 2 plates with E. coli DguaB (pDCAF3)
Incubated in 37 degrees celsius
Aliquoted kanamycin (KAN) in four 1mL tubes
Tuesday 10th June
ASDF Autoclaved at 1:30pm- 0.8 grams of YNB + 156 mL H2O
- 28 grams of salts + 490 mL H2O
Used sterile filter for 1M MgSO4 and 1M CaCl2
Suspended 5 uL of CM34 (antibiotic) + 5 mL of LB + 1 colony of pDCAF3 E. coli
Added .5 grams of caffeine + 400 uL of 1M MgSO4 + 20 uL 1M CaCl2 + 40 mL M95x salts + H2O to YNB + H2O mixture
- Labeled this "M9 media"
Inoculated frozen stock of E. coli guaB pDCAF3 in 5 mL of M9 media
Placed sample in 30 degree celsius shaker for culturing
Wednesday 11th June
ASDF Inoculated CBB1 frozen stock in 5 mL of M9 mediaPlaced sample in 30 degree celsius shaker
Purified pDCAF plasmid using DNA mini kit
- Plasmid concentration was 132.9 ng/uL
Friday 13th June
ASDF Added 10 uL deionized H2O into the J23114 promoter plasmid (Ampᴿ)Followed bacterial transformation protocol to prepare/grow culture overnight
Inoculated 5 mL of M9 with CBB1 and placed it in 30 degree celsius shaker for 3 days
- Previous CBB1 culture did not grow, showed slight growth
- pDCAF3 strain in M9 did grow in the 30 degree celsius shaker
Monday 16th June
ASDF No growth in M9 by CBB1To grow the promoter plasmid:
- 5 mL of LB + 1 uL Amp
- Label tubes
- Grow in 30 degree celsius shaker overnight
- 2 tubes of 1 mL M9 + 2 tubes of 1 mL LB each with 10 uL of sample
Purify genomic DNA plasmid following the Wizard Protocol
- Added lysis buffer before centrifuging. So we separated (translate) sample into 2 tubes and will (translate) accordingly
- We put our 2 promoter plasmid plates in the 4 degree celsius shelf
Tuesday 17th June
ASDF Quantified gDNA with TECAN- Result: 5.4 ng/uL
Made 2 plates of M9 culture and 2 plates of CBB1 culture (100 uL used) then placed them in 37 degree celsius shaker
Wednesday 18th June
ASDF Autoclaved 50% glycerolMade four 25% glycerol stock solutions (stored in the -80 degree celsius freezer):
- CBB1 in M9 (x2 1.5 mL tubes)
- Promoter 1
- Promoter 2 (both promoter plasmids are J23114 Ampᴿ)
- Stored in the -20 degree celsius freezer in the DNA box
Thursday 19th June
ASDF Quantified promoter plasmid (J23114 #1 and #2)-
#1: 342.9 ng/ul with a ratio of 1.9
#2: 373.2 ng/ul with a ratio of 1.91
Checking to see if expired enzymes work: Using the J23114 promoter plasmid, we will see if the 3-year expired SpeI works
- We combined 1 uL of 2.1 buffer, 1 uL of Spe1, and 6 uL of J23114 promoter
- Heat bath at 37 degrees celsius for 1 hour because 2.1 buffer is <100% effective on this enzyme
- Then we will run gel electrophoresis: Concluded that the enzyme works
Cutting the promoter with restriction enzymes
- Combined 24 uL of J23114 promoter + 3 uL of CutSmart buffer + 1 uL of each EcoRI and SpeI
- Heat bath at 37 degrees celsius for 1 hour + 20 minute heat-kill at 80 degrees celsius
Cutting linearized backbone
- Linearized backbone with chloraphenicol marker (12 uL) + 12 uL water + 1 uL of each EcoRI, PstI, and DpnI + 3 uL 2.1 buffer
- Heat bath at 37 degrees celsius for 1 hour + 20 minute heat-kill at 80 degrees celsius
Wednesday 9th July
ASDF Made 400mL of M9 solution- Made 40% glucose solution of 50mL: 2g glucose
- Added the following to 316mL of DI H2O: Na2HPO4: 13.56g Na2HPO4, 2g NH4Cl, 1g NaCl, 6g KH2PO4
- Added 80mL 5x M9 salt solution (20% of 400mL)
- Added 800uL MgSO4 + 40uL CaCl2
- Added 4mL glucose solution using syringe
- Stirred until all dissolved
Removed competent cells from the -80 freezer
Thawed on ice for 30 minutes
Removed CAM agar plate from 4 degree cold room
Mixed 4uL of pDCAF3 plasmid with 30uL competent cells in microcentrifuge tube, placed on ice for 30 minutes
Placed mixture in water bath (42C) for 45 seconds
Placed mixture on ice for 2 minutes
Added 300uL LB to mixture
Placed in 37 degree shaker for 45 minutes
Plated cells on CAM plate, placed in 37 degree drawer overnight
Thursday 10th July
ASDF GuaB/pDCAF suspension in caffeine/theobromine- 0.0975g/10mL caffeine, 0.09g/10mL -> 50 mM
- 2.5mL of M9 (with Glucose) + 2.4875mL of H2O + 12.5uL of caffeine/theobromine
- Use syringe to filter out 10mL of caffeine/theobromine into new conical test tubes
- Take out guaB/pDCAF from -80C freezer, suspend it using 10uL pipette tips
- Place them into 37C inclubator overnight
Wednesday 16th July
ASDF Incubate 4 tubes with LB+CM- Red 1 and 2
- Green 1 and 2
- Placed in shaker at 12:20pm
Thursday 17th July
ASDF Made 1mg/mL Erm of 50mLUsed syringe to filter out
25mL Erm into LB agar
Made 13 places
Erm is in -20C
Friday 18th July
ASDF Streak out Erm-R onto Erm plates (made 2)Put them into incubator (start: 9:35am)
Monday 21th July
ASDF cdh PCR redo: Made 4 master mixes: 5uL gDNA CBB1, 45uL DDH2O Master Mix 1: Regular-
20uL Buffer G
4uL forward primer
4uL reverse primer
0.4uL Q5 polymerase
2uL template
9.6uL H2O
Saturday 26th July
ASDF MRS agar of 200mL- 3g agar (15g/L)
- 10.41g MRS
300mL LB + 3uL CM34 + IG4
300mL LB + 3uL CM34 + IG5
Monday 28th July
ASDF Diluted caffeine and theobromine solutions for HPLC- 500uM Caffeine (10mL)
- 500uM Theobromine (10mL)
- 100uM Caffeine (10mL)
- 100uM Theobromine (10mL)
- 250uM Caffeine + 250uM Theobromine (10mL)
(page 169 on bottom, can’t read XW’s part)
- Take 1mL of I4/I5 LB cultures and spin for 2 minutes at 8000 rpm
- Removed supernatant
- Added 1mL of OH salt, resuspended
- 2 minutes at 8000 rpm
- Removed supernatant
- Resuspended in 1mL of M9 media �