Difference between revisions of "Template:Team:Groningen/CONTENT/EXPERIMENTS/tasA Ligation in RFP Backbone (t15)"
(Created page with "{{Team:Groningen/TEMPLATES/LOG |title=00:00, 21 May 2015 - 00:00, 21 May 2015 |executor=Harm Ruesink |content=<html><div class="text">The RFP backbone DNA was extracted fro...") |
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Latest revision as of 00:28, 18 September 2015
00:00, 21 May 2015 - 00:00, 21 May 2015
The RFP backbone DNA was extracted from the gel with the PCR purification kit. For this binding buffer was added to the cut out gel in the ratio 2:1 binding buffer:gel weight. It was stored as BB1, purified backbone (50 µL elution buffer). Afterwards the ligation of tasA in BB1 was carried out. For that the following components were combined.
15 µL BB1
2 µL 10x buffer (2.1)
1 µL tasA DNA (4.2)
2 µL T4 ligase
The mixture was incubated at room temperature for 2 hours. During this time ampicillin plates were poured (100 µg/mL).