Team:SDU-Denmark/labnotes3

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(Difference between revisions)
(Coloni PCR of photosensor in pUC19 from transformation 27/7)
(Taq PCR of photosensor in pUC19)
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PCR samples are loaded onto a 1% agarose gel. Gene ruler DNA ladder mix (red) is used as marker.<br><br>
PCR samples are loaded onto a 1% agarose gel. Gene ruler DNA ladder mix (red) is used as marker.<br><br>
''Results:''<br>
''Results:''<br>
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[[Image:Team-SDU-Denmark-PSplasmid PCR.jpg|600px]]<br><br>
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[[Image:Team-SDU-Denmark-PSplasmid PCR.jpg|300px]]<br><br>
''Analysis:''<br>
''Analysis:''<br>
Two weak bands at app. 4500bp and 850bp respectively. The upper band could correspond to the pKJ606 plasmid with insert, and the lower band might indicate VF2-VR without insert, rendering these results rather inconlclusive. Therefore an ON culture for miniprep was made. <br>
Two weak bands at app. 4500bp and 850bp respectively. The upper band could correspond to the pKJ606 plasmid with insert, and the lower band might indicate VF2-VR without insert, rendering these results rather inconlclusive. Therefore an ON culture for miniprep was made. <br>
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3: pOT2 with ''ninaB'' cut with EcoRI and XhoI (EX)<br>
3: pOT2 with ''ninaB'' cut with EcoRI and XhoI (EX)<br>
A 1.5% agarose gel was run:<br>
A 1.5% agarose gel was run:<br>
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[[Image:team-sdu-denmark-NinaB_restriction_E.jpg | 400px]]
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[[Image:team-sdu-denmark-NinaB_restriction_E.jpg | 300px]]
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Nucleic acid concentrations were measured with NanoDrop after gel extraction and purification:  
Nucleic acid concentrations were measured with NanoDrop after gel extraction and purification:  

Revision as of 21:21, 23 October 2010