Team:UNITN-Trento/Notebook/Labposts/08/06
From 2013.igem.org
{ "date" : "2013-08-05", "author" : "thomas", "title" : "EFE PCR", "content" : "Today I performed a PCR on EFE in pUC57 vector in order to linearize it and eliminate the vector. To do this I used primers BBa_Fwd and BBa_Rev. The reaction was assembled as follow exploting both OneTaq and Phusion polymerase.
5x One Taq Buffer | 10µl |
---|---|
Fwd Primer | 1µl |
Rev Primer | 1µl |
10 mM dNTP's | 1µl |
One Taq | 0.25µl |
Phusion | 0.3µl |
Template DNA | 0.7µl (about 500 ng) |
H2O | 35.75µl |