Team:BYU Provo/Notebook/Cholera - Detection/Springexp

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Revision as of 16:22, 21 September 2013

Cholera Detection May - June Notebook
Cholera Detection March-April May-June July-August September-October	May 1 - May 12 We attempted to amplify Cro through pcr and cut it out of a gel. Cro will be used to induce the lytic cycle of lambda. We believe that when there is an abundance of cro, there will be an increased lysis of lambda. Daily log
	May 13 - May 26 Moving right along, we cloned the CRO gene from bacteriophage lambda into pIG12, a vector with the arabinose-inducible pBAD promoter. We transformed the ligated plasmid into our target strains, TT9901, TT9907 (which have bacteriophage lambda integrated into their genomes as a prophage) and TT25281 (our control without the lysogen) by electroporation. Daily log
	May 27 - June 9 Add description! Daily log
	June 10 - June 23 With the correct primers, DMSO, and fresh template, we performed a successful PCR reaction of CRO. We continued the cloning process by digesting pIG12 and CRO, ligating them together, and transforming the ligated plasmid into DH5a E.Coli. Daily log
	June 24 - June 30 Add description! Daily log

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+<font size="3" font face="Calibri"> Moving right along, we cloned the CRO gene from bacteriophage lambda into pIG12, a vector with the arabinose-inducible pBAD promoter. We transformed the ligated plasmid into our target strains, TT9901, TT9907 (which have bacteriophage lambda integrated into their genomes as a prophage) and TT25281 (our control without the lysogen) by electroporation. </font>
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