Team:Penn/Notebook/DrugDelivery

From 2012.igem.org

(Difference between revisions)

Revision as of 20:35, 26 June 2012

Week 1

6/07/2012

Wet Lab

Today we transformed both versions of cph8 from 2012 Distribution.

Dry Lab

We also placed order for the following new BioBricks:

BBa_K207001 - PhyB-DBD Fusion
BBa_K422012 - Pif3 (Aar1 C part)
BBa_K422013 - PhyB (Aar1 C part)
BBa_K592006 - pFixK2
BBa_K592004 - YF1
BBa_K592005 - FixJ
BBa_K592000 - Cph8
BBa_K365000 - Pif3

In addition, we brainstormed and developed a new idea to use the PYP/GCN system to activate a gene.

6/08/2012

Wet Lab

No colonies appeared in the transformation of both cph8 a/b. We suspect that the failure of the transformatiosns were due to bad sequences.

Week 2

6/11/2012

Wet Lab

We performed PCR to obtain mCherry from the NAS 151 plasmid. Following this we ran a 1% gel and purified the product which resulted in a 30ns/λ yield.

6/12/2012

Wet Lab

We digested mCherry PCR product with restriction enzymes BamHI and NotI. Then we column purified mCherry and ligated into NAS152 backbone. Afterwards we transformed NAS152-mCherry into DH5alpha cell lines. This was then poured 25 LB-Kan plates.

6/13/2012

Wet Lab

Unknown. Must consult lab notebook.

6/14/2012

Wet Lab

Same as above.

6/15/2012

Wet Lab

Once again.

Dry Lab

Met with Mark Goulian to develop the project. Also obtained pDawn and pDusk plasmids.

@@ Line 39: / Line 39: @@
 We digested mCherry PCR product with restriction enzymes BamHI and NotI. Then we column purified mCherry and ligated into NAS152 backbone. Afterwards we transformed NAS152-mCherry into DH5alpha cell lines. This was then poured 25 LB-Kan plates.
+'''6/13/2012'''
+'''Wet Lab'''
+Unknown. Must consult lab notebook.
+'''6/14/2012'''
+'''Wet Lab'''
+Same as above.
+'''6/15/2012'''
+'''Wet Lab'''
+Once again.
+'''Dry Lab'''
+Met with Mark Goulian to develop the project. Also obtained pDawn and pDusk plasmids.