Team:EPF-Lausanne/Notebook/July2011

From 2011.igem.org

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Also, we have some light smaller bands in colonies 1 and 4, indicating that the miniprep is perhaps not so pure.
Also, we have some light smaller bands in colonies 1 and 4, indicating that the miniprep is perhaps not so pure.
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Vincent and Alessandro transformed the J61002 original plasmid, since we were running out of DNA with which to compare to the Gibson assembly. In addition, they transformed the results of the previous day's registry search for convenient substitute plasmids (for p23019) using Alina's cells. These were plated appropriately and put in the incubator overnight.  
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Vincent and Alessandro transformed the J61002 original plasmid, since we were running out of DNA with which to compare to the Gibson assembly. In addition, they transformed the results of the previous day's registry search for convenient substitute plasmids (for p23019) using Alina's cells using 50 ng/microL concentration (Chloramphenicol Chl-SB3C5 70.6 ng/microL, K-SB3K1 67.7 ng/microL). These were plated appropriately and put in the incubator overnight.  
== Friday, 8th of July 2011 ==
== Friday, 8th of July 2011 ==
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The fluorescence traces are insufficiently clear for accurate conclusions, therefore the PCR and gel will be repeated with different concentrations on Monday.
The fluorescence traces are insufficiently clear for accurate conclusions, therefore the PCR and gel will be repeated with different concentrations on Monday.
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== Saturday, 9th of July 2011 ==
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Vincent came in to pick up the J61002, pSB3C5, and pSB3K1 cultures from the incubator. He found that all the J61002 cultures were pink (as expected since they have the RFP gene). Both kanamycin cultures were pink, and two of the three chloramphenicol cultures were pink (though not as strong a pink as that of the J61002 plasmid). He went ahead and mini-prepped all the cultures, using hot water (55 C) instead of warm TE buffer during the elution step. He then made glycerol stocks (50% cell, 50% glycerol) and placed them in the -80 freezer. Finally, he measured the concentration of the resulting DNA after the mini-prep:
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pSB3C5, colony 1: 35.2 ng/microL (accidentally used 2 microL, vs. 1 microL so more diluted)
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pSB3C5, colony 2: 78.4 ng/microL
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pSB3C5, colony 3: 70.2 ng/microL
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pSB3K1, colony 1: 15.5 ng/microL
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pSB3K1, colony 2: 14.3 ng/microL
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J61002, colony 1: 54.2 ng/microL
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J61002, colony 2: 74.3 ng/microL
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J61002, colony 3: 45.9 ng/microL
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Revision as of 18:22, 9 July 2011