Team:UNICAMP-Brazil/Notebooks/September 25

(Difference between revisions)

Latest revision as of 03:44, 22 October 2009

Today was a happy day to five of us! We went to the U.S. Embassy in Sao Paulo and we got our visas! :D

We ran an agarose gel of yesterday's PCRs product.
We couldn't obtain even a single amplified fragment! =(
Why can the transformed cells grew in the media (that means they actually have the AMP resistence), but they haven't our inserts into it's plasmids?
Our advisors suggested us that, since we digested our plasmid vector with XbaI and SpeI (X sticky ends can come together with S sticky ends), it recircularized without the introduction of our inserts.
Therefore, we must perform the dephosphorylation of our digested vector. That may prevent it from recircularizing without the insert introduction.

Marcelo

We decided to search in the plate possible cells with the right DNA insert. We made 15 colony of each plate. Unfortunately we didn’t get it again.

Ane

Considering that we need more vector to perform the ligation reactions, we electroeluted more vector from the ADH1 biobrick previously digested with XbaI and SpeI (Protocol 12).

Taís

@@ Line 34: / Line 34: @@
 ====Biofusion vector - Electroelution====
-*<p style=”text-align:justify;”>Considering that we need more vector to perform the ligation reactions, we electroeluted more vector from  the ADH1 biobrick previously digested with ''Xba''I and ''Spe''I ([https://2009.igem.org/Team:UNICAMP-Brazil/Protocols/Electroelution Protocol 12]).</p>
+*<p style=”text-align:justify;”>Considering that we need more vector to perform the ligation reactions, we electroeluted more vector from  the ''ADH1'' biobrick previously digested with ''Xba''I and ''Spe''I ([https://2009.igem.org/Team:UNICAMP-Brazil/Protocols/Electroelution Protocol 12]).</p>
 ''Taís''
 {{:Team:UNICAMP-Brazil/inc_rodape}}