Team:WashU/Week5
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We have also decided to use PCR to amplify our DNA, as we are getting extremely low yields from our gel extractions. Thus, we designed the primers today. | We have also decided to use PCR to amplify our DNA, as we are getting extremely low yields from our gel extractions. Thus, we designed the primers today. | ||
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We digested the BB-plasmids with using the familiar BioBrick Assembly protocol for the plasmid part and digested a tube of J23119 with SpeI and PstI using the same procedure but different these enzymes. We then used the BioBrick Assembly to ligate together J23119 cut with SpeI and Pst1 with a sample of gel purified Construct #9 and mRFP1 since mRFP1 had the best gel purification result. The other gel purified DNA samples were ligated to plasmids and digested promoter using a new vial of ligase for fear that the previous were hindered by expired ligase. | We digested the BB-plasmids with using the familiar BioBrick Assembly protocol for the plasmid part and digested a tube of J23119 with SpeI and PstI using the same procedure but different these enzymes. We then used the BioBrick Assembly to ligate together J23119 cut with SpeI and Pst1 with a sample of gel purified Construct #9 and mRFP1 since mRFP1 had the best gel purification result. The other gel purified DNA samples were ligated to plasmids and digested promoter using a new vial of ligase for fear that the previous were hindered by expired ligase. | ||
The constructs were all cloned in GC5 competent cells from sigma using the transformation protocol. The J23119 cut with SpeI and PstI constructs were plated onto Amp. The Kan and C plasmid constructs were plated onto their respective resistance plate. The plates were incubated overnight at 37°C. | The constructs were all cloned in GC5 competent cells from sigma using the transformation protocol. The J23119 cut with SpeI and PstI constructs were plated onto Amp. The Kan and C plasmid constructs were plated onto their respective resistance plate. The plates were incubated overnight at 37°C. | ||
- | + | Today, we began a culture of <i>E. coli</i> transformed with plasmid PSL2131. | |
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+ | ==Saffron in a Kan== | ||
+ | We finally received our gene from DNA 2.0!! We streaked out some of the gene, still in its plasmid onto plates with ampicillin. | ||
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+ | In addition, we transformed <i>Synechocystis</i> with the plasmid PSL2131 obtained from one of our mentors, Burt. | ||
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+ | We picked the <i>E. coli</i> colonies transformed with plasmid PSL2131 today. We miniprepped these colonies and then put them into 6803. | ||
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+ | We have started a third wild type liquid culture of <i>Synechocystis</i>. | ||
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+ | ==YLC== | ||
+ | In the interest of time, we will use existing biobrick constructs with the necessary fluorescent proteins to show to the YLC students, and then we will complete our own constructs at a later date. Thus, today, we plated several biobrick constructs (RFP: I13521, | ||
+ | GFP: I13522, | ||
+ | YFP: 13604, and | ||
+ | CFP: S03475) and will pick colonies to prep. | ||
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+ | ==Saffron in a Kan== | ||
+ | We continued to work with our gene construct today. <br> | ||
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+ | We made glycerol stocks of GFP, RFP, plasmid 2131, and then three of our construct, CS42S. | ||
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+ | We performed a miniprep to extract the DNA PSL2131.<br> | ||
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+ | We performed two digestions - see the gel below for results.<br> | ||
+ | [[File:629122gel.jpg]] | ||
+ | [[File:6292012322.jpg]] | ||
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+ | <u>Saturday, June 30</u> | ||
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+ | ==Several Small Projects== | ||
+ | We miniprepped the potential constructs. We will need to digest them to check if they worked. They will hopefully be the plasmid that we want to place into Synechocystis. | ||
+ | <br> | ||
+ | More Amp and Kan LB plates were made. | ||
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+ | Four more glycerol stocks of the construct that we ordered were made. 2 mL of the remaining cells were miniprepped. The rest (.25 mL) were used to continue the line of cells in liquid culture with 3 mL of LB+Amp. | ||
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+ | Two glycerol stocks one of an RFP plasmid and one of our functioning GFP were made and frozen at -80°C. (For the glycerol stocks done today, no dry ice was used to flash freeze as a the stock room is closed on Saturdays.) | ||
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Latest revision as of 16:43, 17 August 2012