Latest revision as of 20:11, 18 September 2015

Week 6

Miniprepped the liquid cultures from lldd_ IDT, 4 tubes.
Resuspended RFP in PCSB1C3 backbone (shipping plasmid) from distribution kit in 10uL nuclease-free water ( Plate 4, well 4B)
Transformed 2 tubes with RFP backbones to amplify, 4uL plasmid per tube.
Plated on 2 plates, 100uL mixture per plate. The plates were plates in the incubator
Also performed the digestion and ligation : Promoter + LLD on AmpR.
4 separate tubes of ligation product, labelled P+LLD ligate 1-4 is in the freezer box
tubes 1 and 2 were ligated to Amna’s AmpRbackbone
tubes 3 and 4 were ligated to Amna’s AmpRbackone 2

Transformed Pro +lldd contruct ( AmpR). The 4 plates are in the incubator
Miniprepped the Pro+ TnaA contruct ( KanR). The 6 tubes are in the freezer box, the average concentration is 20ng/uL

Used tubes 4,5,6, from Pro+TnaA miniprep from 9/09
We halved the volumes of digestion procedure to give total digest volume of 25uL.

Picked the colonies of the tnaA and lldd and inoculated the final construct on AmpR backbone and shipping plasmid

Transformation of shipping constructs lldd and tnaA onto shipping plasmid using previous standard protocol
Created 4 replicates for each

picked the white colonies and inoculated the liquid cultures following standard protocol

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 	<li>We followed the standard digestion and ligation protocol </li>
 	<li>Join Pr +TnaA to TnaB + Ter and put on both pSBC13 and AmpR backbone </li>
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+	<div class="diagram"><img src="https://static.igem.org/mediawiki/2015/5/50/NYUAD-NotebookFigure3.png"></div>
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 	<li>Used tubes 4,5,6, from Pro+TnaA miniprep from 9/09</li>
 	<li>We halved the volumes of digestion procedure to give total digest volume of 25uL. </li>