IGEM:MIT/2006/Notebook/2006-8-29

to do

 * 1) analyze sequencing results mid-morning - done
 * 2) *then miniprep/sequence all new rbs.pchBA.term LCs that could still possibly have R0011 attached and throw out bad - all failed to attach an rbs, so are starting over assembly from pchBA.Term-mut glycerol that we think is correct
 * 3) *check for which osmY-Q-J.xxx structures look good and throw out bad - incomplete sequencing results, but O-Q-119B is good and potentially O-Q-199A is too
 * 4) glycerol pE3/pE3R (plus miniprep) and YYC912 IK strain - done, but pE3 had a low miniprep concentration
 * 5) glycerol with nice labels, miniprep, sequence final bb-construct parts (6) to doublecheck their integrity - done, but realized that the J45396 is not a mutagenized construct - made a new correct LC
 * 6) make iGEM yeast LC (one big for pelleting/baking and one small for miniprepping/digesting/ligating) - done, and bread machine has arrived
 * 7) 3-part assemble/transform B0015 with the 2 correctly mutagenized/ES digested 30.Bat2.30.THI3 - done
 * 8) add methyl salicylate to pseudomonas cells (if grown-up enough) and see if it is readily degraded - done

today's time line

 * 1) first: remove all LCs
 * 2) second: analyze sequencing
 * 3) third: minipreps and glycerols
 * 4) fourth: sequencing
 * 5) fifth: ligations/transformations