Team:WashU/Week12
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<h1>Saffron in a Kan</h1> | <h1>Saffron in a Kan</h1> | ||
We also PCR'd the Z construct in the submission plasmid, Psb1c3. We then digested the results with both EcoRI and PstI, as shown below, and saw that the PCR had indeed succeded.<br> | We also PCR'd the Z construct in the submission plasmid, Psb1c3. We then digested the results with both EcoRI and PstI, as shown below, and saw that the PCR had indeed succeded.<br> | ||
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Finally, we ran an SDS-PAGE gel of our Z construct with a histidine tag in order to see the proteins produced using an extraction protocol from Sigma found here [INSERT PROTOCOL]. | Finally, we ran an SDS-PAGE gel of our Z construct with a histidine tag in order to see the proteins produced using an extraction protocol from Sigma found here [INSERT PROTOCOL]. | ||
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We started with a transformation of the ligation yesterday using GC10s and 5 microliters of ligation mixture. Then, we plated the transformed cells in 100 microliter aliquots. | We started with a transformation of the ligation yesterday using GC10s and 5 microliters of ligation mixture. Then, we plated the transformed cells in 100 microliter aliquots. | ||
- | Next, we ran a PCR of Z + Thiofusion using KlenTaq at three different temperatures (45, 50, and 55 degrees) in order to figure out why the PCR isn't working. | + | Next, we ran a PCR of Z + Thiofusion using KlenTaq at three different temperatures (45, 50, and 55 degrees) in order to figure out why the PCR isn't working. <html> |
+ | <img src="https://static.igem.org/mediawiki/2012/0/05/0.png"> | ||
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- | We also attempted to perform a zeaxanthin extraction using our culture of the <i>Synechocystis</i> PAL mutant. | + | We also attempted to perform a zeaxanthin extraction using our culture of the <i>Synechocystis</i> PAL mutant. |
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+ | <table style="width:auto;"><tr><td><a href="http://picasaweb.google.com/lh/photo/2iExq1RPSgh9PGJVACqNsT5bkQKfZwcjUCwEKVIJGfc?feat=embedwebsite"><img src="http://lh4.googleusercontent.com/-5UrHwTMRPiM/UCvyrIlsayI/AAAAAAAAAhc/CKYZHdMvoFo/s640/P1060127.JPG" height="428" width="640" /></a></td></tr><tr><td style="font-family:arial,sans-serif; font-size:11px; text-align:right">From <a href="http://picasaweb.google.com/100308169786596215568/August152012?authuser=0&authkey=Gv1sRgCK2xxviFoP6ySA&feat=embedwebsite">August 15, 2012</a></td></tr></table> | ||
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+ | Since <i>Synechocystis</i> is a photoautotroph, it produces chlorophyll, resulting in the green color. The cyanobacterium also produces beta carotene, the precursor to zeaxanthin, which is the precursor to the crocin we are trying to produce. The peaks for beta carotene and zeaxanthin overlap, so resolving the difference may be difficult. | ||
SDS-PAGE gel of ZCD and UGTCS2 <i>E. coli</i> cultures (both induced at 20 degrees and non-induced) in order to see how much protein is produced from our cultures. TO do this, had to sonicate cultures. Potential issue: used LB to sonicate instead of proper sonication buffer. | SDS-PAGE gel of ZCD and UGTCS2 <i>E. coli</i> cultures (both induced at 20 degrees and non-induced) in order to see how much protein is produced from our cultures. TO do this, had to sonicate cultures. Potential issue: used LB to sonicate instead of proper sonication buffer. | ||
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KlenTaq PCR of Z construct with TOPO in order to eventually submit this part, regular Taq PCR of U construct with TOPO because we are running low on KlenTaq | KlenTaq PCR of Z construct with TOPO in order to eventually submit this part, regular Taq PCR of U construct with TOPO because we are running low on KlenTaq | ||
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+ | Trypsin digestion of ZCD, UGTCS2, Z-construct, and a control<br> | ||
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+ | <img src="http://lh6.googleusercontent.com/-9EHSF2-bvAo/UC54AJNrE4I/AAAAAAAAAhw/kDoPb-XA_h0/s640/induced%2520SDS.png"><br> | ||
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+ | We performed a digest of Z-TOPO and U-TOPO from yesterday, followed by ligation of Z + TOPO, U + TOPO, and our main construct CS42S for submission. | ||
+ | We then transformed our cells with ligation results and plated them. | ||
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+ | Finally, we cleaned up our lab and moved items into storage. :( | ||
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+ | On our last day, we spent time working on the dry lab stuff and getting our DNA ready for submission and sequencing. | ||
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[https://2012.igem.org/Team:WashU/WeeklyLog Back to Weekly Log] | [https://2012.igem.org/Team:WashU/WeeklyLog Back to Weekly Log] |
Latest revision as of 02:26, 15 September 2012