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PCR purification of OmpA and Gel Extraction
Project: Surface Display
Date: Wed, 04 May 2011 00:00:00 GMT
Author: Sukdong Lee (leex4462)
Access: Public
Revision History:
- Mon, 22 Aug 2011 10:46:03 GMT (leex4462): entry created in project'Surface Display' by leex4462 (id=3)
- Tue, 27 Sep 2011 17:07:48 GMT (admin): entry data updated by admin (id=1)
Purpose:
To ensure the Digestion worked and no DNA degradation occurred.
Procedure:
-PCR purify ompA (30uL)
-Run an ompA insert (digested), ompA insert (undigesed, pBAD-plasmid (digested), pBad (undigested)
Lanes
1=Ladder
2-4=pBad digest (40 uL rxn)
5= pBad miniprep
6=ompA digest (5 uL)
7-12= PCR of OmpA PCR Amplification (200ul rxn)
Results:
All suspended in 30 uL:
-pBAD plasmid= 9.7 ng/ul
-OmpA PCR product= 9.0
-OmpA digested=20.8
Revision: Updated 9/27/2011 to include images.
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