IGEM:PennState/Labbook/NoahJohnson/2007-9-5

September 5, 2007
 * Made more 1X TAE buffer
 * Added 40mL of 50X TAE buffer to 4 L flask
 * Added 1960mL dH20 and mixed
 * Restriction digest on crp* and P1010 in psB1A2
 * cut with EcoR1 and SpeI
 * Started incubating at 6:45pm
 * Ran gel on restriction products and gel extracted psB1A2

6-11