Team:Heidelberg/Templates/MM week8

From 2013.igem.org

(Difference between revisions)

Latest revision as of 03:31, 5 October 2013

2013-06-17

Colony-PCR of BAP1-pKD46 electroporated with PCR amplificate of pLF03 grown on Cm+IPTG. Lanes 1-6: annealing at 66°C; lanes 8-11: touch-down 66->60°C; lane 6: NEB 2-log; lane 1,7: negative control (BAP1-pLF03); lane 2,8: colony-PCR of colony electroporated with gel-extracted PCR product; rest: colony-PCRs of colonies electroporated with PCR-purified PCR product.

repeat colony PCR, use 1 µl of liquid culture from gel-extracted plate, pick colonies from PCR-purified plate (Taq, 25 µl total volume)
2 conditions:

Cycles	temperature [°C]	Time [s]
1	95	600
30	95	240
	64	30
	72	60
1	72	600
1	4	inf

Cycles	temperature [°C]	Time [s]
1	95	600
12	95	240
	66°C ↓0.5°C	30
	72	60
18	95	240
	60°C	30
	72	60
1	72	600
1	4	inf

no positives
plate samples of liquid cultures from 2013-06-15 on Amp, grow at 37°C

2013-06-18

colonies grew on Amp

2013-06-19

Gel electrophoresis of the PCR amplificate. Lane 1: NEB 2-log ladder; lanes 2-5: PCR with Phusion Flash (2 µl of product were put on gel)

prepare for repetition of experiment: run 4 PCRs of 1 ng pLF03 (miniPrep from 2013-06-04) with primers ygfG21C1 and ygfG21C2 using Phusion Flash (performed by Dominik), one reaction = 50 µl total volume

Cycles	temperature [°C]	Time [s]
1	98	10
5	98	1
	45	5
	72	130
25	98	1
	55	5
	72	120
1	72	120
1	4	inf

Gel electrophoresis of the purified PCR amplificate. Lane 1: NEB 2-log ladder; lane 2: purified PCR with Phusion Flash (1 µl of product were put on gel)

pool products, purify (digestion only 3 h)
nanoDrop: 2088 ng/µl -> remeasure: 532 ng/µl
load 1 µl purified PCR product on gel -> very weak band -> nanoDrop wrong
to eliminate error: make fresh electrocompetent cells:
- pick colony from BAP1-pKD46 plate from 2013-06-04
- inoculate 1 ml LB + Amp
- grow at 30°C

2013-06-20

too little cells: use aliquot from 2013-06-06
use all available DNA (14 µl) and 100 µl cells (complete aliquot)
grow in SOC + IPTG(1mM) at 300 rpm for 3h
spin cells down, decant supernatant, resuspend in remainder of medium
plate 10 µl, rest on Cm + IPTG

@@ Line 1: / Line 1: @@
 == 2013-06-17 ==
-[[File:Heidelberg_BAP1-colony-PCR2013-06-17.png|100px|thumb|left|Colony-PCR of BAP1-pKD46 electroporated with PCR amplificate of pLF03 grown on Cm+IPTG. Lanes 1-6: annealing at 66°C; lanes 8-11: touch-down 66->60°C; lane 6: NEB 2-log; lane 1,7: negative control (BAP1-pLF03); lane 2,8: colony-PCR of colony electroporated with gel-extracted PCR product; rest: colony-PCRs of colonies electroporated with PCR-purified PCR product.]]
+[[File:Heidelberg_BAP1-colony-PCR2013-06-17.png|100px|thumb|Colony-PCR of BAP1-pKD46 electroporated with PCR amplificate of pLF03 grown on Cm+IPTG. Lanes 1-6: annealing at 66°C; lanes 8-11: touch-down 66->60°C; lane 6: NEB 2-log; lane 1,7: negative control (BAP1-pLF03); lane 2,8: colony-PCR of colony electroporated with gel-extracted PCR product; rest: colony-PCRs of colonies electroporated with PCR-purified PCR product.]]
 * repeat colony PCR, use 1 µl of liquid culture from gel-extracted plate, pick colonies from PCR-purified plate (Taq, 25 µl total volume)
 * 2 conditions:
@@ Line 74: / Line 74: @@
 | 1  || 4 || inf
 |}
-[[File:Heidelberg_PLF03_PCR2013-06-19_purified.png|100px|thumb|left|Gel electrophoresis of the purified PCR amplificate. Lane 1: NEB 2-log ladder; lane 2: purified PCR with Phusion Flash (1 µl of product were put on gel)]]
+[[File:Heidelberg_PLF03_PCR2013-06-19_purified.png|100px|thumb|Gel electrophoresis of the purified PCR amplificate. Lane 1: NEB 2-log ladder; lane 2: purified PCR with Phusion Flash (1 µl of product were put on gel)]]
 * pool products, [[Isopropanol PCR purification|purify]] (digestion only 3 h)
 * nanoDrop: 2088 ng/µl -> remeasure: 532 ng/µl