IGEM:MIT/2006/Notebook/2006-9-9

To Do

 * 1) check sequences (dye blob re-runs should be in from 9/1 order) - done (KB)
 * 2) pellet new yeast cells: bake with 1 pellet and resuspend 2nd in milk - done (KB)
 * 3) glycerol any of the LCs in fridge that look good post this second sequence analysis (299A, 319ABC are good) - done (KB)
 * 4) *discard of confirmed bad dna and glycerols! - done (KB)
 * 5) glycerol 3 additional LCs of the 399-1s and glycerol y0078/y0080- done (KB)
 * 6) make LCs from sketchy 400 plates: (1 colonies: ligation 3, 5 colonies: ligation 4, other plates seem to be too contaminated and overgrown) - done (SP)
 * 7) Y0080 and Y0078 yeast vectors - done (SP)
 * 8) *miniprep
 * 9) *digest with XS
 * 10) **pcr clean-up