Revision as of 18:47, 15 July 2013

13 July 2013

208 lab

Main purpose today

Make gel purifications to enable USER-reactions and to make PCR of the fragments missing.

Who was in the lab

Kristian

Procedure

Purification gel 1,2 and 3

1kb ladder
Nir
Nir
Nir
Nir
Nir
Nir
Nir
Nir
HAO

1kb ladder, NEB
cycAX
cycAX
cycAX
cycAX
AMO
AMO
AMO
AMO
HAO
HAO
HAO

100 bp ladder, NEB
RFP
RFP
RFP

PCR of AMO

Did PCR on AMO on two programs: 1-3 on 54°C 4-6 on 52°C Both with the annealing time 3 min.

USER-reactions

There was made USER-reactions with all fragments after purification. AMO was purified even though it was only one very faint band; the others were bright band. The following plates where made:

RFP USER - RFP inside pZA21
AMO USER - AMO inside pZA21
HAO USER - HAO inside pZA21
cycAX USER - cycAX inside pZA21
Nir USER - Nir inside pZA21
Neg. USER - pZA21 linearized only

Conclusion

PCR of AMO with USER-primers was not a success we will see if the new PCR have done better. We will evaluate the transformants on Monday with colony-PCR.

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Team:DTU-Denmark/Notebook/13 July 2013

From 2013.igem.org