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− | <li> </li> | + | <li> Designed new WRKY primer</li> |
− | <li> </li> | + | <li> Can’t do anything else until level0 plasmids are done to perform minipreps.</li> |
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− | <li> </li> | + | <li> Performed a mini prep on the one colony that grew successfully (QLAprep Spin Miniprep Kit).</li> |
− | <li> </li> | + | <li> Performed PCR on the mini prep, GFP plasmid, and level 0 colonies </li> |
− | <li> </li> | + | <li> Ran a gel using the PCR products and the hyperladder 4 </li> |
− | <li> </li> | + | <li> Helen: Grew bacterial cultures using chloramphenicol and kanamycin antibiotics. 5ml LB broth and 5 ul of antibiotics. Left overnight on 200 RPM at 37 degrees. </li> |
− | <li> </li> | + | <li> Grew colonies from plate A (4), B (1), C (4), Rob’s colonies. </li> |
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− | <li> </li> | + | <li> Re-incubated the agrobacterium overnight as they were not spinning so could not grow.</li> |
− | <li> | + | <li> Made some more competent E.coli using previously made competent E.coli as a starting point.</li> |
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− | <li> </li> | + | <li> Performed minipreps on samples A1 and A2, C1 and C4. Isolated the DNA and measured concentrations of samples A1-A4 and C1-C4 against EB as a blank.</li> |
− | <li> </li> | + | <li> Performed restriction digest on P19, Luc, PDF1, PR2 and GST6, according to long protocol in ligase buffer. Put in PCR machine for the process.</li> |
− | <li> </li> | + | <li> Performed ligation and gel analysis to see whether the plasid cut and incorporated the recombinant DNA.</li> |
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− | <li> </li> | + | <li> Minipreps on plates A (level 0) and C (level 1). </li> |
− | <li> </li> | + | <li> Digest process and then used PCR using long protocol.</li> |
− | <li> </li> | + | <li> Tested level 0 plasmids.</li> |
− | <li> </li> | + | <li> Also completed 2 minipreps of GBA2 using QIAprep protocol</li> |
− | <li> </li> | + | <li> Did a digest of the plasmid in the water bath at 37 degrees using BsmB1 </li> |
+ | <li> Ran a gel comparing the undigested plasmid and the ones digested with BsmB1 </li> | ||
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− | <li> | + | <li> Ran a transformation to compare the newly made competent cells with the competent cells made on 12/07/17.</li> |
− | + | <li> The agrobacterium that were grown overnight were used to infiltrate the leaves of tobacco (to be harvested in two days time), by suspending the cells in induction buffer.</li> | |
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Revision as of 12:22, 20 July 2017
Project Diary
10/07/2017
- Meet up
- Safety and risk assessment forms
- Review to do lists
- Helen = safety
- Sequencing = Niall
- Plants = Jade and Sarah
- Stockroom = Emily, Ryan, and Thomas
- Arranged lab and workspaces
- Sorted pipette tips into boxes and autoclaved.
- Made medium using 25 g/l LB broth. Made medium using 10g/L agar granulated (made up to 400ml water). Then autoclaved. Pyrex class will not smash, cools down quickly/till hand-hot.
- Chloramphenicol + kanamycin resistance antibiotics: One medium had 100mg/ml kanamycin added (400microlitres to 400ml), the other had 34mg/ml chloramphenicol added (400microlitres to 400ml). Plated 19 plates of each.
- Transferred tobacco plants (grown on 19/6) into new pots to prevent overcrowding.
- Organised ourselves into 3 'teams':
- Team_PlantP = Niall and Ryan
- Team_TSH = Helen, Emily, and Sarah
- Team_Luc = Jade and Tom
11/07/2017
Team_PlantP | Team_TSH | Team_Luc |
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12/07/2017
Team_PlantP | Team_TSH | Team_Luc |
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13/07/2017
Team_PlantP | Team_TSH | Team_Luc |
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14/07/2017
Team_PlantP | Team_TSH | Team_Luc |
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17/07/2017
Team_PlantP | Team_TSH | Team_Luc |
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18/07/2017
Team_PlantP | Team_TSH | Team_Luc |
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19/07/2017
Team_PlantP | Team_TSH | Team_Luc |
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