Team:Calgary/6 September 2010

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<u>Emily</u>
<u>Emily</u>
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Today I ran PCR reactions of malE, malE31, malESSdel and malE31SSdel using the appropriate primers and an mgcl2 concentration of 2.5 as well as an annealing temperature of 55.5-57 degrees C.  I got amplification of the expected bands (~1.2 KB) for the malE and malE31, however I once again got no bands for any of the SSdel stuff.  These reactions will have to be further optimized tomorrow.  Today a lot of work was also put into the presentation for aGEM this weekend in Edmonton.
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Today I ran PCR reactions of malE, malE31, malESSdel and malE31SSdel using the appropriate primers and an mgcl2 concentration of 2.5 as well as an annealing temperature of 55.5-57 degrees C.  I got amplification of the expected bands (~1.2 KB) for the malE and malE31, however I once again got no bands for any of the SSdel stuff.  These reactions will have to be further optimized tomorrow.  Today I also induced my I0500-I13504 cultures as well as Himika's cpxR reporter with malE31 circuit construct cultures with varying concentrations of Arabinose.  We will be looking at GFP and RFP output for these tomorrow.  Today a lot of work was also put into the presentation for aGEM this weekend in Edmonton.
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Revision as of 17:51, 7 September 2010

Monday September 6, 2010

Emily

Today I ran PCR reactions of malE, malE31, malESSdel and malE31SSdel using the appropriate primers and an mgcl2 concentration of 2.5 as well as an annealing temperature of 55.5-57 degrees C. I got amplification of the expected bands (~1.2 KB) for the malE and malE31, however I once again got no bands for any of the SSdel stuff. These reactions will have to be further optimized tomorrow. Today I also induced my I0500-I13504 cultures as well as Himika's cpxR reporter with malE31 circuit construct cultures with varying concentrations of Arabinose. We will be looking at GFP and RFP output for these tomorrow. Today a lot of work was also put into the presentation for aGEM this weekend in Edmonton.