Revision as of 07:31, 31 May 2012

Wageningen UR

week 2: 7 may - 11 may

7 may

E. coli in liquid LB

3 plates per strain were picked and grown in 25 ml LB. all plates grown well accept for amp plates, due to drying effects.

8 may

10:00 Continue growth. All 3 strains in shaker, 180 RPM, 30 degree celcius.

4 x 1 L SOB is made

16:55 culture mach1 and DH5X are plated 10x and 1000x diluted on LB plates. Dilutions are done with demi water.

Plates were placed in 37 degree Celcius stove

9 may

9:15 10x dilution was to low, overgrown 1000x was nearly overrown, but still acceptable.

picked 1 MACH1 and 1 DH5X colony and grown in 10 ml SOB medium, 37 degree Celcius, 180 RPM

10 may

MACH1 competent cells followin pinky's protocol. with the following diviations

OD harvest at: 0.5 -0.45

11 may

CCMV protocol inoculated at 8:45 IPTG at 11:45

centrifugation in greiner tubes

pellet stored at -20 degree Celcius, 50 ml greiner tubes

@@ Line 2: / Line 2: @@
 = week 2: 7 may - 11 may =
+== office work ==
+== lab work ==
+may
+''E. coli'' in liquid LB
+plates per strain were picked and grown in 25 ml LB.
+all plates grown well accept for amp plates, due to drying effects.
+may
+:00
+Continue growth.
+All 3 strains in shaker, 180 RPM, 30 degree celcius.
+x 1 L SOB is made
+:55
+culture mach1 and DH5X are plated 10x and 1000x diluted on LB plates. Dilutions are done with demi water.
+Plates were placed in 37 degree Celcius stove
+may
+:15
+x dilution was to low, overgrown
+x was nearly overrown, but still acceptable.
+picked 1 MACH1 and 1 DH5X colony and grown in 10 ml SOB medium, 37 degree Celcius, 180 RPM
+may
+MACH1 competent cells
+followin pinky's protocol. with the following diviations
+*4x 500 ml SOB
+*SLA 3000 rotor
+OD harvest at: 0.5 -0.45
+may
+CCMV protocol
+inoculated at 8:45 IPTG at 11:45
+centrifugation in greiner tubes
+pellet stored at -20 degree Celcius, 50 ml greiner tubes