Team:SDU-Denmark/labnotes2

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(Transformation of TOP 10 e. coli with ninaB gene in pOT2:chlor vector)
(Transformation of cells with gene in plasmid)
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Notes: Filterpaper was washed with 50ul TE buffer for 2 seconds. Paper punch was then transfered to a sterile eppendorff tube, and transformation protocol TR1.1 was followed from here. The usual positive control was used.<br><br>
Notes: Filterpaper was washed with 50ul TE buffer for 2 seconds. Paper punch was then transfered to a sterile eppendorff tube, and transformation protocol TR1.1 was followed from here. The usual positive control was used.<br><br>
Plates were dried for ca. 12 minutes, showed no sign of cracking.<br><br>
Plates were dried for ca. 12 minutes, showed no sign of cracking.<br><br>
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The gene is inserted into a pOT2 plasmid. A plasmid map can be found [http://www.fruitfly.org/about/methods/pOT2vector.html here]:
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The gene is inserted into a pOT2 plasmid. A plasmid map can be found [http://www.fruitfly.org/about/methods/pOT2vector.html here]:<br><br>
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Two of the chlor plates were damaged (one very slightly) and one ampicilin plate was torn up, again. (good thing two were dried). Plates were incubated ON at 37°.<BR><BR>
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Revision as of 11:18, 21 July 2010