Team:NYU Gallatin/Notebook
From 2012.igem.org
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Note </th> | Note </th> | ||
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<p>During this time, we purified the DNA digested yesterday. We will ligate tomorrow using this DNA if today’s transformation is unsuccessful.</p> | <p>During this time, we purified the DNA digested yesterday. We will ligate tomorrow using this DNA if today’s transformation is unsuccessful.</p> | ||
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<p>The correct pieces of DNA (circled) were cut out and put in the freezer, to be purified later</p> | <p>The correct pieces of DNA (circled) were cut out and put in the freezer, to be purified later</p> | ||
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<p><img src="https://lh5.googleusercontent.com/KWT3nbON6dizYP9U-YK0G_m632oXEToYX6OmHnuOpz6aUAzNYyTJM5FUnkaqlGCE8MiIpyl-Shw" width="300" /></p> | <p><img src="https://lh5.googleusercontent.com/KWT3nbON6dizYP9U-YK0G_m632oXEToYX6OmHnuOpz6aUAzNYyTJM5FUnkaqlGCE8MiIpyl-Shw" width="300" /></p> | ||
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<p>PCR with A gene is running.</p> | <p>PCR with A gene is running.</p> | ||
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<p>Cannot see 4kb insert in any lanes, and can see 2kb backbone in lanes 13, 14, 15.</p> | <p>Cannot see 4kb insert in any lanes, and can see 2kb backbone in lanes 13, 14, 15.</p> | ||
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<p><img src="https://lh4.googleusercontent.com/670iJQwtl-PeFv8hqr8LYZfDRMvZFywoRgI6BtiBNzNWGlJwyNep3WufWNRYx0ywytOrymg1WZ8" width="300" /></p> | <p><img src="https://lh4.googleusercontent.com/670iJQwtl-PeFv8hqr8LYZfDRMvZFywoRgI6BtiBNzNWGlJwyNep3WufWNRYx0ywytOrymg1WZ8" width="300" /></p> | ||
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All in incubator at 37*C overnight.</p> | All in incubator at 37*C overnight.</p> | ||
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<p>Transformed E. coli with Gibson construct were plated onto two plates (see Ellen re: dilution)</p> | <p>Transformed E. coli with Gibson construct were plated onto two plates (see Ellen re: dilution)</p> | ||
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<p>*PCR (version 1 and version 2) is in PCR machine</p> | <p>*PCR (version 1 and version 2) is in PCR machine</p> | ||
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<p>The lab strains look the same. Ph same as well as temp</p> | <p>The lab strains look the same. Ph same as well as temp</p> | ||
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Temp. 23.5 degrees.</p> | Temp. 23.5 degrees.</p> | ||
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<p>Wild kombucha is growing best but still weakly. Ph 4. 5</p> | <p>Wild kombucha is growing best but still weakly. Ph 4. 5</p> | ||
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Ten smaller beakers were also inoculated with the mycelia and were originally in the fan space (fan off).</p> | Ten smaller beakers were also inoculated with the mycelia and were originally in the fan space (fan off).</p> | ||
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<p>Kombucha. Made three with lab strain scoby, two with aceto food, one with blueberry juice</p> | <p>Kombucha. Made three with lab strain scoby, two with aceto food, one with blueberry juice</p> | ||
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<p>Came into lab today, 7 out of 16 molds were contaminated. It seems like the tapes used to seal up cracks are the culprits as most of the mold growing seemed to originate at the tapes. There needs to be a better way to seal things up. what was done: we merely cleaned out the contaminated trays and are leaving the rest for tomorrow.</p> | <p>Came into lab today, 7 out of 16 molds were contaminated. It seems like the tapes used to seal up cracks are the culprits as most of the mold growing seemed to originate at the tapes. There needs to be a better way to seal things up. what was done: we merely cleaned out the contaminated trays and are leaving the rest for tomorrow.</p> | ||
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<p>Pellet for 8.4rcf</p> | <p>Pellet for 8.4rcf</p> | ||
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<p>PCR products (tubes A, B, C, D) are in the hot pink “Cloning Materials” box and labeled “Genes N/U RE & PCR Products 8/23”</p> | <p>PCR products (tubes A, B, C, D) are in the hot pink “Cloning Materials” box and labeled “Genes N/U RE & PCR Products 8/23”</p> | ||
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<p><img src="http://farm9.staticflickr.com/8456/8049368751_497bdfabb9_m.jpg" /></p> | <p><img src="http://farm9.staticflickr.com/8456/8049368751_497bdfabb9_m.jpg" /></p> | ||
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<p><img src="http://farm9.staticflickr.com/8030/8049366364_94191cecc0_m.jpg" /></p> | <p><img src="http://farm9.staticflickr.com/8030/8049366364_94191cecc0_m.jpg" /></p> | ||
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<p>(I may be off. I didn't take notes here. If I'm wrong and you remember, please let me know.)</p> | <p>(I may be off. I didn't take notes here. If I'm wrong and you remember, please let me know.)</p> | ||
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UAP1 - clone 3</p> | UAP1 - clone 3</p> | ||
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<p>The digests were run on a 1% agarose gel. I've attached the picture (gel annotated.png) that shows the inserts with the correct sized bands (the samples with the asterisks). These were sent for sequencing using the VF and VR (verify forward and verify reverse) primers.</p> | <p>The digests were run on a 1% agarose gel. I've attached the picture (gel annotated.png) that shows the inserts with the correct sized bands (the samples with the asterisks). These were sent for sequencing using the VF and VR (verify forward and verify reverse) primers.</p> | ||
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<p>The next day we had lots of colonies (I don't have the pictures of the plates, but maybe someone else does). Many of these were red, indicating they were transformed due to residual RFP plasmid (as had happened previously). We circled several white colonies as prospective positive transformants. For each construct, we chose 5 clones and inoculated 4 ml of LB-chlor to grow these overnight at 37 deg C.</p> | <p>The next day we had lots of colonies (I don't have the pictures of the plates, but maybe someone else does). Many of these were red, indicating they were transformed due to residual RFP plasmid (as had happened previously). We circled several white colonies as prospective positive transformants. For each construct, we chose 5 clones and inoculated 4 ml of LB-chlor to grow these overnight at 37 deg C.</p> | ||
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<p>We incubated these for 1 hr at 50 deg C and then immediately transformed the commercial competent cells.</p> | <p>We incubated these for 1 hr at 50 deg C and then immediately transformed the commercial competent cells.</p> | ||
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20.0 µL</p> | 20.0 µL</p> | ||
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<p><img src="http://farm9.staticflickr.com/8174/8048768673_d51ef329a3.jpg" /></p> | <p><img src="http://farm9.staticflickr.com/8174/8048768673_d51ef329a3.jpg" /></p> | ||
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3) overall total conc of DNA in the rxn mix could be upped.</p> | 3) overall total conc of DNA in the rxn mix could be upped.</p> | ||
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= 20 μL</p> | = 20 μL</p> | ||
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<p>G-blocks arrived</p> | <p>G-blocks arrived</p> | ||
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<p><img src="http://farm9.staticflickr.com/8451/8048765553_1ffd507e36.jpg" /><br /><img src="http://farm9.staticflickr.com/8172/8048770556_2604c4a9b2.jpg" /><br /><img src="http://farm9.staticflickr.com/8316/8048765169_52ca13cda9_n.jpg" /></p> | <p><img src="http://farm9.staticflickr.com/8451/8048765553_1ffd507e36.jpg" /><br /><img src="http://farm9.staticflickr.com/8172/8048770556_2604c4a9b2.jpg" /><br /><img src="http://farm9.staticflickr.com/8316/8048765169_52ca13cda9_n.jpg" /></p> | ||
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<li>Almost entirely cellulose, very little liquid left.</li> | <li>Almost entirely cellulose, very little liquid left.</li> | ||
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Revision as of 04:58, 3 October 2012