J.Burtonlowe (Talk | contribs) |
J.Burtonlowe (Talk | contribs) |
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<h6 style="padding-left:0;padding-top:20px;">Log entry</h6> | <h6 style="padding-left:0;padding-top:20px;">Log entry</h6> | ||
<p id="pp" style="padding-left:0;padding-right:0;padding-top:0;"> | <p id="pp" style="padding-left:0;padding-right:0;padding-top:0;"> | ||
+ | <p id="pp">Andy and Alan worked in the Physics labs today, measuring the intensity of our light box, and calculating the W/cm^2 that the plates placed inside the light box will be receiving. We need to know this so we can look at how intensity impacts upon the rate at which Killer Red and Killer Orange kill cells.</p> | ||
+ | <p id="pp">Today’s lab team - Eloise, Emily, Hannah and Dan - started using a new method of cloning called Modular Cloning, which we intend to use codon optimised Killer Red and Killer Orange to submit to the registry. They also used an adjusted digestion and ligation method to cut RFP from template backbones, ran on a gel, then transformed for overnight incubation.</p> | ||
</p> | </p> | ||
</div> | </div> | ||
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<h6 style="padding-left:0;padding-top:20px;">Log entry</h6> | <h6 style="padding-left:0;padding-top:20px;">Log entry</h6> | ||
<p id="pp" style="padding-left:0;padding-right:0;padding-top:0;"> | <p id="pp" style="padding-left:0;padding-right:0;padding-top:0;"> | ||
+ | <p id="pp">The ligated Killer Red parts from yesterday were mini prepped, and the successful Cas9 colony was put in overnight incubation. We re-transformed the unsuccessful transformations from yesterday, as only the plasmids with chloramphenicol and tetracycline backbones were successful.</p> | ||
+ | <p id="pp">The successful Killer Red ligations were sent off for sequencing today to check that we made the part in the correct order sequence.</p> | ||
</p> | </p> | ||
</div> | </div> |
Revision as of 21:16, 19 October 2016