BIOTEC Dresden/Notepad/9 August 2010

From 2010.igem.org

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Check gradient PCR with Taq polymerase from 08.08.2010 on agarose gel on plasmids:
Check gradient PCR with Taq polymerase from 08.08.2010 on agarose gel on plasmids:
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  6e, 4a, 13e, 9b, 15e, 14f, 20f, 21f  
  6e, 4a, 13e, 9b, 15e, 14f, 20f, 21f  
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The plasmid backbone used was pSB1C3. Two ligations were performed - one based on the standard protocol and the other samples were left for overnight ligation. The ligated parts were transformed by electroporation method and plated.
The plasmid backbone used was pSB1C3. Two ligations were performed - one based on the standard protocol and the other samples were left for overnight ligation. The ligated parts were transformed by electroporation method and plated.
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[[Category:BIOTEC Dresden/Notepad/August|August]]
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Latest revision as of 21:53, 27 October 2010

Check gradient PCR with Taq polymerase from 08.08.2010 on agarose gel on plasmids:

23e, 25a, 27e

Gradient PCR using Fusion polymerase on plasmids:

23e, 25a, 27e

Assembly of the following parts were commenced with restriction digest and ligation:

6e, 4a, 13e, 9b, 15e, 14f, 20f, 21f 


The plasmid backbone used was pSB1C3. Two ligations were performed - one based on the standard protocol and the other samples were left for overnight ligation. The ligated parts were transformed by electroporation method and plated.




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