Team:UNICAMP-Brazil/Notebooks/October 16

(Difference between revisions)

Revision as of 18:47, 21 October 2009

To perform our tests, we digested the following minipreps: pJEN1+YFP, pJEN1+Lys, pDLD+YFP, pDLD+Lys with XbaI and PstI to connect to YEP vector. We also digested the plasmid YEP+Adh1-YFP to confirm the correct insertion of the part into YEP vector. The digestion showed that our new devices are ricght! =) But there is something wrong with the YEP+Adh1-YFP construction, it seams the digestion were incomplete.

We purified one digested fragment of each device: pJEN1+YFP (1781bp), pJEN1+Lys(1567bp), pDLD+YFP (1246bp), pDLD+Lys (1032bp). We ligated the digested fragments with YEP vector and transformed in competent E. coli.

We did miniprep of YEP+Adh1-lysozyme. Later we digested the plasmids to confirm the insertion of the Adh1-Lysozyme construction into YEP. We also digested 10 more plasmids YEP-Adh1-YFP again, this time we digested a little longer to try to avoid the incomplete digestion problem.

We prepares competent S.cerevisiae (protocol 13) and transformed competent yeasts with YEP+Adh1-YFP without confirming the correct ligation.

Raíssa and Taís

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 [[Image:miniprepYEP+.jpg|400px|center]]
-*<p style=”text-align:justify;”>We transformed competent yeasts with YEP+Adh1-YFP without confirming the correct ligation.</p>
+*<p style=”text-align:justify;”>We prepares competent ''S.cerevisiae'' (protocol 13) and transformed competent yeasts with YEP+Adh1-YFP without confirming the correct ligation.</p>
 *<p style=”text-align:justify;”>We did the YNP Ura- solid medium.</p>