Latest revision as of 21:00, 16 September 2013

12 June 2013

Navigate to the Previous or the Next Entry

New PCR amplification of USER fragments

MasterMix x 17 was made to each tube 3ul of Fw and 3 ul of rv primer was added as well as 1ul DNA template

every fragment was run 2 min 98 C followed by 35 cycles of

10 sec 98 C

1 sec 65 C ramp by 0.1C/s down to

10 sec of 55C

3 min 72C

after repetitions, 5 min of 72 C

1l of 10x TBE
200ml of 2% agarose solution and added 10 ul EtBr
casting 3x 2% gels and 1x1% gel
200ml EDTA stock solution 0.5 M from powder, dissolved at pH 8 and later equilibrated to pH 7
200ml LB medium w. agar and kanamycin
autoclaved 1.5l of LB medium
new batch of competent cells
glycerol stock from I14032

got SFGFP for TAT and SFGFP for Sec

Navigate to the Previous or the Next Entry

@@ Line 1: / Line 1: @@
-{{:Team:DTU-Denmark/Templates/StartPage}}
+{{:Team:DTU-Denmark/Templates/StartPage|12 June 2013}}
+Navigate to the [[Team:DTU-Denmark/Notebook/11_June_2013|Previous]] or the [[Team:DTU-Denmark/Notebook/13_June_2013|Next]] Entry
+=208=
+<hr/>
+==Main purposes today==
+<hr/>
+New PCR amplification of USER fragments
+==Procedure==
+<hr/>
+===PCR===
+MasterMix x 17 was made
+to each tube 3ul of Fw and 3 ul of rv primer was added as well as 1ul DNA template
+every fragment was run 2 min 98 C followed by 35 cycles of
+sec 98 C
+sec 65 C ramp by 0.1C/s down to
+sec of 55C
+min 72C
+after repetitions, 5 min of 72 C
+===prepared===
+*1l of 10x TBE
+*200ml of 2% agarose solution and added 10 ul EtBr
+* casting 3x 2% gels and 1x1% gel
+* 200ml EDTA stock solution 0.5 M from powder, dissolved at pH 8 and later equilibrated to pH 7
+* 200ml LB medium w. agar and kanamycin
+*autoclaved 1.5l of LB medium
+*new batch of competent cells
+* glycerol stock from I14032
+===run gel of todays PCR===
+got SFGFP for TAT and SFGFP for Sec
 Navigate to the [[Team:DTU-Denmark/Notebook/11_June_2013|Previous]] or the [[Team:DTU-Denmark/Notebook/13_June_2013|Next]] Entry
 {{:Team:DTU-Denmark/Templates/EndPage}}