IGEM:Harvard/2006/Cyanobacteria/Notebook/2006-8-6

  Previous Entry  Current Entry  Next Entry  

To-do

 * 1) Make frozen stocks of the KaiA+bkb and KaiB+bkb transformants that we grew up in liquid culture yesterday
 * 2) Miniprep the above
 * 3) (Maybe) Do an X-P digest of the KaiA+bkb and KaiB+bkb plasmids (though we may want to wait and do this along with the other KaiA+bkb and KaiB+bkb ligation transformants) (Will do later) completed 8/7/06
 * 4) Inoculate the KaiA+bkb and KaiB+bkb transformants from yesterday's ligation
 * 5) Add CIP to the E-S digest of LC vector
 * 6) Run the digests from yesterday on a gel (E-S digest of LC vector, X-P digest of J04450+bkb)
 * 7) Gel-extract and purify the LC vector and J04450 insert if they exist (Will purify tomorrow, along with the high-copy backbone that the J04450 was inserted in)
 * 8) (maybe) Perform a ligation and transformation of the J04450 insert into LC vector (Will do after we gel-purify them) completed 8/7/06
 * 9) Do 12 minipreps for Mingming
 * 10) Check sequencing on the Genewiz website (the orders have not been processed)

KaiA/B + bkb inoculation
We found 10 colonies on the KaiA+bkb plate and 5 colonies on the KaiB+bkb plate. We inoculated all 15 colonies in liquid culture (8 mL LB, 8 uL Amp) and placed them in the 37C shaker around 1830.

Gel images of E-S digest of LC vector and X-P digest of J04450+bkb (high copy)


We extracted the high-copy vector (2kb) and J04450 insert (1kb) from lanes 2 and 4, and the low-copy vector (3.5 kb) from lanes 6 and 8.