Team:Cambridge/Experiments/Initial Exercise Group A
From 2011.igem.org
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+ | 1. Template = B. subtilus genome. Aiming to amplify ftsZ | ||
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+ | Fwd : ccaattaaaggaggaattcaaaATGTTGGAGTTCGAAACAAACAT | ||
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+ | Rev: agtgaacagctcttcgcctttacgGCCGCGTTTATTACGGTTTC | ||
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+ | Fwd primer for plasmid amplication: | ||
+ | AGAAACCGTAATAAACGCGGCcgtaaaggcgaagagctgttcact | ||
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+ | Rev: ATGTTTGTTTCGAACTCCAACATtttgaattcctcctttaattgg | ||
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Revision as of 13:23, 7 July 2011
Initial Exercise: Cat, Jonathan, Haydn and Ai
As a 'warm-up' exercise to acquaint the group with molecular biological laboratory techniques, three mini-teams were tasked with creating an interesting GFP fusion. Group A decided that visualing ftsZ in real time, in vivo would be rather cool.\
Ftsz was first identified in a mutant screen in 1980 <ref>(Lutkenhaus, Wolf-Watz and Donachie)</ref> as a gene recquired for bacterial cytokinesis (cell division).
Notes
Primer Design
The plasmid vector we were supplied with contains a strong promoter upstream of a sfGFP coding sequence. Our fusion design relies on amplifying the ftsZ coding region from Bacillus and creating regions of overlap between this and the GFP coding sequence in the plasmid, in order to create the gene fusion.
ccaattaaaggaggaattcaaaATGTTGGAGTTCGAAACAAACAT-----AGAAACCGTAATAAACGCGGCcgtaaaggcgaagagctgttcact ggttaatttcctccttaagtttTACAACCTCAAGCTTTGTTTGTA-----TCTTTGGCATTATTTGCGCCGgcatttccgcttctcgacaagtga
1. Template = B. subtilus genome. Aiming to amplify ftsZ
Fwd : ccaattaaaggaggaattcaaaATGTTGGAGTTCGAAACAAACAT
Rev: agtgaacagctcttcgcctttacgGCCGCGTTTATTACGGTTTC
Fwd primer for plasmid amplication: AGAAACCGTAATAAACGCGGCcgtaaaggcgaagagctgttcact
Rev: ATGTTTGTTTCGAACTCCAACATtttgaattcctcctttaattgg