Edinburgh/Week 16

(Difference between revisions)

Revision as of 19:26, 6 October 2008

Edinburgh iGEM 2008

lac promoter added to glgC and glgC16 biobricks, which were then grown overnight in LB and LB+40mM glucose.
- Cells were subsequently resuspended in iodine reagent to test glycogen levels - results are quite promising. See Results section. (CF)

xylE and lacZ reporter genes added to cstA promoter, then grown overnight in LB and LB+40mM glucose.
- xylE assays performed - results are very promising. See Results section. (CF)

cenA (M237~238) and cex (M233~235) biobricks confirmed. Ribosome binding sites are now being added. (CF)
bglX clones (M240, 247) were all wrong. Troubleshooting in progress. (CF)
ISA1 (M229) and ISA2 (M231) clones correct but contained messed-up suffixes. Other clones which, by digestion, seem to have intact XbaI and Spe1 sites have been submitted for sequencing. (CF)

Plac-dxs-lims-appY device is ready to test. Hope to do next week if the GC is available. (CF)
Attempts to make crt construct failed for some unexplained reason - apparently no DNA in the ligations. (CF)

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 * ''cenA'' (M237~238) and ''cex'' (M233~235) biobricks confirmed. Ribosome binding sites are now being added. (CF)
 * ''bglX'' clones (M240, 247) were all wrong. Troubleshooting in progress. (CF)
-* '''ISA1''' (M229) and '''ISA2''' (M231) clones correct but contained messed-up suffixes. Other clones which, by digestion, seem to have intact XbaI and Spe1 sites have been submitted for sequencing. (CF)
+* ''ISA1'' (M229) and ''ISA2'' (M231) clones correct but contained messed-up suffixes. Other clones which, by digestion, seem to have intact XbaI and Spe1 sites have been submitted for sequencing. (CF)
 * ''Plac-dxs-lims-appY'' device is ready to test. Hope to do next week if the GC is available. (CF)
 * Attempts to make ''crt'' construct failed for some unexplained reason - apparently no DNA in the ligations. (CF)