Team:SDU-Denmark/labnotes3

From 2010.igem.org

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(Incertion of Promoter + RBS in pSB3T5)
(Follow-up colony PCR)
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The Concentrations were quite low, but we pooled them (1P+2P and 3B+4B) and used them for ligation.
The Concentrations were quite low, but we pooled them (1P+2P and 3B+4B) and used them for ligation.
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==== Follow-up colony PCR ====
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=== Follow-up colony PCR ===
Date: 26/7<br>
Date: 26/7<br>
Methods: Colony PCR<br>
Methods: Colony PCR<br>
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Analysis: Since we had so many different lengths, we will cut one from each length, specifically colony: 2, 8, 11, 13, 20, 24, 26.
Analysis: Since we had so many different lengths, we will cut one from each length, specifically colony: 2, 8, 11, 13, 20, 24, 26.
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=== Miniprep of follow-up colony PCR ===
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Date: 27/7<br>
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Methods: ON, Miniprep<br>
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Protocol: MP1.1<br>
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Experiment done by: LC
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Notes: Samples L4, L5, L6, L9, L10, L14, L21 and L26 (L for ligation from the follow-up colony PCR) miniprepped and NinaB samples from the 4 frozen cultures of it. <br><br>
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Results: [[Image:Team-SDU-Denmark-miniprep277.jpg|600px]]<br>
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All ligations were around the same length, just under 2000 BP. Even though the correct length should have been about 1000 BP longer, this is not surprising since uncut plasmids often show 1000 BP less in length. NinaB was also too short and there was a second band showing higher up in the gel (weird!). The concentrations averaged around 80ng/ul for the samples.
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Analysis:  We decided to do a new miniprep where we start with a higher concentrated overnight culture, which we will achieve through boosting the ON before doing the miniprep.
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Revision as of 06:50, 28 July 2010