Team:UCL/Labbook
From 2013.igem.org
(Difference between revisions)
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- | <p class="major_title"> | + | <p class="major_title">June</p> |
<p class="minor_title">Week 1-3</p> | <p class="minor_title">Week 1-3</p> | ||
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26th June - We are given safety training in the Advanced Centre for Biochemical Engineering in all relevant laboratories, as well as general procedures in case of emergency. | 26th June - We are given safety training in the Advanced Centre for Biochemical Engineering in all relevant laboratories, as well as general procedures in case of emergency. | ||
</p> | </p> | ||
- | + | <p class="major_title">July</p> | |
<p class="minor_title">Week 5-6</p> | <p class="minor_title">Week 5-6</p> | ||
<p class="body_text"> | <p class="body_text"> | ||
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23rd July - No colony growth was observed on Ampicillin plates [link to ampicillin plate protocol] indicating no plasmid uptake. Transformation was repeated with YB3110. | 23rd July - No colony growth was observed on Ampicillin plates [link to ampicillin plate protocol] indicating no plasmid uptake. Transformation was repeated with YB3110. | ||
</p> | </p> | ||
- | + | <p class="minor_title">Week 9</p> | |
- | + | <p class="body_text"> | |
+ | Bacterial Lab | ||
+ | <p class="major_title">August</p> | ||
Revision as of 11:09, 5 September 2013
June
Week 1-3
No lab work
Week 4
26th June - We are given safety training in the Advanced Centre for Biochemical Engineering in all relevant laboratories, as well as general procedures in case of emergency.
July
Week 5-6
No lab work
Week 7
Bacterial Lab
15th July - The team is introduced to the laboratories which will be used during the summer for both bacterial and mammalian experiments. 16th July - 5X M9 salts [link to protocol], minimal agar [link to protocol], 1.4% molten agar solution [link to protocol] and 0.1M CaCl2/15% glycerol [link to protocol] were prepared for the generation of competent cells. Minimal agar plates were poured and streaked [link to streaking protocol] with W3110 Escherichia coli cells and left overnight to incubate at 37C. 17th July - Very little colony growth was observed from W3110 E.coli streaked plates. Plates were therefore left to incubate for a further 17 hours. 18th July - Sufficient colony growth allowed for the selection of a single colony from each plate. This was then inoculated in 5ul LB media [link to LB recipe] + 100ul 1M MgSO4 and left to incu-shake overnight at 37C. 19th July - Cultures re-suspended in new LB media and 100µl aliquots placed into individual eppendorf tubes for placement at -80C. Mammalian Lab 17th July - Mammalian cell culture and maintenance [link to mammalian protocol] training by Mrs. Ludmilla Ruban. Passaged primary MEF (mouse embryonic fibroblast) cells. Passage 3. 18th July - MEF passage 4 19th July - MEF passage 5Week 8
Bacterial Lab
22nd July -Transformation [link to transformation protocol] of our competent cells with plasmid YB3110 was carried out. 23rd July - No colony growth was observed on Ampicillin plates [link to ampicillin plate protocol] indicating no plasmid uptake. Transformation was repeated with YB3110.Week 9
Bacterial Lab
August