Team:Calgary/29 June 2009
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*PCR products were visualized on a 1% agarose gel run with 1.0kb+ Generuler DNA Ladder. | *PCR products were visualized on a 1% agarose gel run with 1.0kb+ Generuler DNA Ladder. | ||
*Results: See gel photo below. Lanes 1-4 are colonies 1-4 of LuxOD47E in psB1AC3 cut with EcoRI/ PstI, lanes 5-8 are colonies 1-4 of BBK LuxOD47E in the psB1AC3 vector cut with XbaI/ PstI, lane 9 is a negative contorl and lane 10 is a positive contorl with C4-8 TOPO LuxOD47E DNA as the template. | *Results: See gel photo below. Lanes 1-4 are colonies 1-4 of LuxOD47E in psB1AC3 cut with EcoRI/ PstI, lanes 5-8 are colonies 1-4 of BBK LuxOD47E in the psB1AC3 vector cut with XbaI/ PstI, lane 9 is a negative contorl and lane 10 is a positive contorl with C4-8 TOPO LuxOD47E DNA as the template. | ||
+ | <Br> | ||
+ | [[Image:2009.06.30ColPCRVer.jpg]] | ||
*Analysis: Although the DNA bands are at the expected size (~1.4 kb), the contamination in the negative contorl lane is not a good thing. We will proceed making overnght cultures and by re-doing this colony PCR. | *Analysis: Although the DNA bands are at the expected size (~1.4 kb), the contamination in the negative contorl lane is not a good thing. We will proceed making overnght cultures and by re-doing this colony PCR. | ||
Revision as of 22:59, 13 September 2009
UNIVERSITY OF CALGARY