Team:EPF-Lausanne/Notebook/August2011

From 2011.igem.org

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(Saturday, 20 August)
(Saturday, 20 August)
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As part of Friday's Colony PCR, Alessandro and Vincent had made liquid cultures and made separate, dedicated plates for each colony that was used. Since the Colony PCR had successfully amplified the K1-T7-RFP plasmids, Vincent brought out those liquid cultures, made glycerol stocks of them, mini-preppred them with the new mini-prep kit, and recorded the resulting DNA concentrations. With these DNA tubes, he went ahead and made a transformation of the three plasmids into BL21 cells (which Alessandro had made throughout the past week). Vincent plated these transformed cells on kanamycin plates and incubated them overnight.  
As part of Friday's Colony PCR, Alessandro and Vincent had made liquid cultures and made separate, dedicated plates for each colony that was used. Since the Colony PCR had successfully amplified the K1-T7-RFP plasmids, Vincent brought out those liquid cultures, made glycerol stocks of them, mini-preppred them with the new mini-prep kit, and recorded the resulting DNA concentrations. With these DNA tubes, he went ahead and made a transformation of the three plasmids into BL21 cells (which Alessandro had made throughout the past week). Vincent plated these transformed cells on kanamycin plates and incubated them overnight.  
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Since the previous day's Colony PCR had partly failed due to an extension time for lysis that was too short (1 minute rather than 2 minutes), Vincent made a Colony PCR for K1-T7-Lysis and a Colony PCR for C5-T7-RFP and C5-T7-Lysis. Perhaps because it was almost 9 in the evening, Vincent did not realize that he had successfully amplified both the K1 and the C5 T7 lysis, showing that the Gibson Assembly had in fact worked as expected.  
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Since the previous day's Colony PCR had partly failed due to an extension time for lysis that was too short (1 minute rather than 2 minutes), Vincent made a Colony PCR for K1-T7-Lysis and a Colony PCR for C5-T7-RFP and C5-T7-Lysis. Perhaps because it was almost 9 in the evening, Vincent did not realize that he had successfully amplified both the K1 and the C5 T7 lysis, showing that the Gibson Assembly had in fact worked as expected. He saw the primer dimers at the bottom of the gel and did not think to even look for faint bands at the 2 kb level where the lysis piece would appear. So the Gibson did in fact work, but Vincent only found this out retrospectively on Tuesday of the following week (this wiki post is written with some tardiness).  
[[File:vince_gel_c5rfp.jpg|600px]]
[[File:vince_gel_c5rfp.jpg|600px]]
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== Sunday, 21 August ==
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Vincent took out the plates from the BL21 transformation. The results were spectacular: thousands of colonies. He then picked one colony from each plate to use for liquid cultures. He did not forget the antibiotic (as he usually does). The idea was to have liquid cultures ready for an IPTG platereader experiment on Monday.
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Vincent also ran a miniprep on the C5-T7-RFP cultures, but got a very low yield of DNA (9-10 ng/uL).
== Monday, 22 August 2011 ==
== Monday, 22 August 2011 ==

Revision as of 08:05, 25 August 2011