Team:Colombia/Notebook
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Revision as of 21:12, 26 September 2011
Template:Https://2011.igem.org/User:Tabima
Contents |
Colombia @ iGem Notebook
Here you can find our daily work in the Lab!
June
June 30:
- Biobricks 1, 2, 3, 4 and 5 were resuspended
- Miniprep Solutions (I, II and III) were prepared.
July
July 1
- Biobricks 1, 2, 3, 4 and 5 were resuspended.
July 5
- Biobrick 2 presented no colonies.
- Colonies from bricks 1, 3, 4 and 5 were stinged.
- Task:
- To make LB medium (15x25mL)
July 6
- Biobricks 1, 3 and 4 were twice plated.
- Brick 5 didn't grow up.
- We've added Ampiciline (3.75mL) and Kanamicine (1.875mL) to the boxed from the previous day.
- LB medium was prepared (15x25mL).
- Liquid LB was prepared (400mL).
- Task:
- To add ampiciline and tetracicline to the boxes.
- Claim the liquid LB
- Scrape ....
- Sting biobricks 2 and 5 (no clons)
- Pick up the tubes with Merceditas
July 7
- Clons 2 and 5 didn't work out.
- Clons 1, 3 and 4 were planted in LB liquid.
- E. Coli inoculation in Coffee
- Kanamicine resistence plasmid: 0.2 optic density.
- Direct inoculation x 2 and C(-) MgCl2.
- Task:
- Print electroporation protocol.
- Ask Juan D. Olarte about the inoculation in coffee.
- Minipreps for confirmation of 1, 3 and 4.
- Competent cells for clons 2 and 5.
July 8
- Minipreps for 1, 3 and 4 were made.
- Plant sheets of coffee into different plates: Each sheet was cut in the middle and they were incubated at 25°C and 37°C LB+Kan.
- Task:
- To finish the minipreps from the addition of RNAsa.
- Check the E. Coli growth in coffee.
July 11
- Minipreps have been finished. They've been planted in gel: Low concentration (25 ng/uL).
- Transformation protocol in chemical cells.
- Task:
- Prepare 250 mL of SOC medium
- Print the Transformation protocol for chemical cells.
July 12
- Strains 1 and 4 have been conserved.
- LB liquid culture was prepared again for brick 3.
- E. Coli growth results.
- Task:
- Print the Transformation protocol for chemical cells.
- Competent cells for clons 2 and 5.
- Preserve brick 3.
- Confirm bricks 1, 3 and 4 (Digestion)
- Resuspend all Biobricks.
- Check the E. Coli growth in coffee.
July 14
- E. Coli didn't grow up on the sheets.
- Chemical competent cells were made (DH5α).
- Brick 3 was left to grow in liquid medium.
- Bricks 2, 5, 6,7, 8, 9 and 10 were transformed and plated.
- Task:
- Print the Transformation protocol for chemical cells.
- Preserve brick 3.
- Confirm all biobricks (Digestion)
- Sting the transformed bricks.
- Add antibiotic to the mediums made today.
July 15
- Brick 3 was preserved in Revco.
- Bricks 2, 5 and 8 were stinged.
- 25 LB+Kan boxes x 25 mL.
- No colonies in brick 6.
- Bricks 7, 9 and 10 were contaminated.
- Task:
- Print the chemical cells protocol.
- Confirm all biobricks (Digestion).
July 19
- Pass strain of Vibrio fischeri to blood agar base.
- Check the growth of the isolates
- Pass the transformed bricks 6, 7, 9 and 10.
- Pass the isolates the solid media to liquid media (2,4,5 and 8)
July 21
- Digestion to confirm No. 1, 3 and 4
Reactives | 1X | 6X |
H2O | 29,4µL | 160,4 µL |
Buffer N. 3 | 4 µL | 24 µL |
EcoRI | 0,3 µL | 1,8 µL |
PstI | 0,3 µL | 1,8 µL |
DNA | 7 µL | 40 µL |
July 22
- Minipreps
- Electrophoresis of the digestions
- Task:
- Confirm minipreps
- Re-suspend primers
July 27
- To prepare LB and SOC medium and autoclaved
- The bricks 7, 9 and 10 were again transformed and plated
- Plate the brick 6.
July 30
- Minipreps with RNase.
- Agarose gel Electrophoresis—Results were not obtained. REPEAT!!
August
August 3
- PCR 16S to DNA Vibrio fischeri U. Nacional
- To expected a band of 1400 bp.
Reactives | 1X | 3X |
H2O | 6,8µL | 20,4µL |
Bµffer | 1µL | 3µL |
MgCl2 | 0,8µL | 2,4µL |
dNTPs | 0,2µL | 0,6µL |
Fw7 | 0,2µL | 0,6µL |
Rv49 | 0,2µL | 0,6µL |
Taq | 0,1µL | 0,3µL |
DNA | 1µL | - |
10µL |
PCR Conditions
94 C for 5 min |
95 C for 50 sec |
55 C for 45 sec 35X |
72 C for 1:30 min |
72 C for 12 min |
12 C forever |
August 5
- Re-suspend primers
100µM → 10 µM
Example: igem 1 → 36.1 nm → 361 µL H2O igem 2 → 32.2 nm → 322 µL H2O ➱ Vortex
Vf= 50 µL Ci= 100 µL Cf= 10 µL Vi= ?
Vi= 5 µL
- Diluted DNA Vibrio fischeri
1244.1 ng/ µL
Ci= 1244.1 ng/ µL
Cf= 25 ng/ µL
Vf= 50 µL
Vi= 1 µL + 49 µL H2O
August 6
- Solutions 2 and 3 of miniprep
- Transformations of 2, 5, 7 and 13
- Check primers
Inventory
The petri dishes with bacteria are in Q401
PCR genes (sensor, CBP and chitoporin) of Vibrio fischeri with Pfx
Name | Dir | Gene | TM |
Igem 1 | Fw | sensor | 48,8 C |
Igem 2 | Rv | sensor | 50,8 C |
Igem 3 | Fw | CBP | 48,9 C |
Igem 4 | Rv | CBP | 49,1 C |
Igem 5 | Fw | Chitopor | 49,3 C |
Igem 6 | Rv | Chitopor | 49,4 C |
August 9
- Minipreps:
1 | ✔ |
2 | ✕ |
3 | so-so |
4 | ✔ |
5 | ✕ |
8 | so-so |
9 | so-so |
10 | so-so |
August 11
- PCR chiA of Vibrio fischeri with Pfx
Name | Dir | Gene | Tm | Lenght |
Igem 7 | Fw | ChiA | 55,4 C | 3378 pb |
Igem 8 | Rv | ChiA | 53,3 C | 3378 pb |
PCR Conditions
Denaturation Step | 94 C for 3 min |
Denaturation | 95 C for 45 sec |
Annealing | 53,5 C for 45 sec 35X |
Extension | 68 C for 2:10 min |
Final Elongation | 68 C for 6 min |
12 C forever |
August 16
- Minipreps bricks 5 and 10
- Plate the bricks 8 and receptor plasmid ( purple colonies)
Task:
- Electrophoresis minipreps bricks 5 and 10
- Growth in liquid media LB colonies of the bricks 8 and receptor plasmid -- minipreps
- PCR of Vibrio fischeri: sensor, chitoporin and ChiA
- Digestions of the bricks
August 17
- Brick 8 didn’t grow
- We made Chloramphenicol stock solution.
August 25
Plasmid 1
BACKBONE pSB1C3 1. Cut with NotI and SpeI backbone 2. Phosphate backbone
SENSOR Cut with: 1. Amplification Senor and Adelinate 2. Cloning into pGEM Teasy 3. Cut with NotI and XmaJI Sensor 4. Insert into backbone= backbone 1 (use ligase T4)
Terminator: 1. Miniprep terminator (21) 2. Cut with PstI and SpeI 3. Cut backbone 1 with XbaI 4. Insert terminator into backbone 1 = backbone 2 (use ligase T4)
CBP: (XhoI-FW Sensor)-(XmaJI RVSensor) –(XbaI Terminador-PstI)- (XbaI FW CBP)-(NheI RV CBP) – (XbaI RV Chitoporin)-(PstI FW Chitoporin)
Plasmid 2
7-18-(11/12/19)- 8- (11/12/19)-6 - 21- 1- 18-(11/12/19)-14-(11/12/19)-9-21
Plasmid 3
2-(11/12/19)6-T-1-(11/12/19)-5 -T-1-4-T
7:30 pm
- Vibrio fischeri PCR
- Attempt to achieve the PCR amplification of the ChiA and Chitoporin genes.
- Amplification results are to be visualized on a gel tomorrow.
- The amplification of ChiA and Chitoporin genes didn´t work. : ( REPEAT!!!
- Digestions for Brick 2 and 8A employed the EcoRI and BSA buffer.
Reactives | 1X | 2X |
H2O | 32,2 | 64,4 |
Buffer 10x | 4uL | 8uL |
ADN | 3uL | 3uL |
EcoRI | 0.4uL | 0.8uL |
BcuI(SpeI) | 0.4uL | 0.8uL |
Digestions for 3 hours at 37C and inactivated at 65C for 15 seconds.
Brick 8 ok (750 bp) Brick 2 : (