Team:Amsterdam/extra/protocols
From 2012.igem.org
(Difference between revisions)
(2 intermediate revisions not shown) | |||
Line 8: | Line 8: | ||
<h1>Protocols</h1><br/> | <h1>Protocols</h1><br/> | ||
- | + | __NOTOC__ | |
<div class='clear'></div> | <div class='clear'></div> | ||
Line 237: | Line 237: | ||
'''Growth curve time points'''<br\> | '''Growth curve time points'''<br\> | ||
- | + | ||
This contained a time laps of 30min for the first period of time (lets say first 3 hours) and after that time lapses of a hour would be better. | This contained a time laps of 30min for the first period of time (lets say first 3 hours) and after that time lapses of a hour would be better. | ||
Line 252: | Line 252: | ||
*Prepare 2x 10ml pSB1AT3 + LacH cultures (in normal LB and with appropriate antibiotic added) | *Prepare 2x 10ml pSB1AT3 + LacH cultures (in normal LB and with appropriate antibiotic added) | ||
*Prepare 2x 10ml pSB1AT3 + pBAD cultures (in normal LB and with appropriate antibiotic added) | *Prepare 2x 10ml pSB1AT3 + pBAD cultures (in normal LB and with appropriate antibiotic added) | ||
- | *Incubate at approximately 37 C for 20 hours | + | *Incubate at approximately 37 C for 20 hours |
- | '''Day 2 | + | '''Day 2 '''<br\> |
Setup: | Setup: | ||
- | *Stop incubation of cultures after 20 hours of growth | + | *Stop incubation of cultures after 20 hours of growth , cultures should now be well into the stationary faze. |
*Prepare 8x a 500ml flasks containing 49.5ml of LB each | *Prepare 8x a 500ml flasks containing 49.5ml of LB each | ||
*For 4 flasks add appropriate antibiotic for culture 1 (pSB1AT3 + LacH containing bacteria from day 1 - step 1) | *For 4 flasks add appropriate antibiotic for culture 1 (pSB1AT3 + LacH containing bacteria from day 1 - step 1) | ||
Line 262: | Line 262: | ||
*To the 4 flasks from step 3 add 0.5ml of culture 1 | *To the 4 flasks from step 3 add 0.5ml of culture 1 | ||
*To the 4 flasks from step 4 add 0.5ml of culture 2 | *To the 4 flasks from step 4 add 0.5ml of culture 2 | ||
- | *Incubate new cultures (step 5 & 6) at 37 degrees for 18 hours | + | *Incubate new cultures (step 5 & 6) at 37 degrees for 18 hours |
- | '''Day 3 | + | '''Day 3 '''<br\> |
Experiment: | Experiment: | ||
*Stop incubation of cultures after 18 hours of growth (at 12:00), cultures should now be well into the stationary faze. | *Stop incubation of cultures after 18 hours of growth (at 12:00), cultures should now be well into the stationary faze. | ||
*From all 8 cultures take 1.5 ml sample and put on ice (-20 C) these are negative control reference points (IPTG- and ARA-) | *From all 8 cultures take 1.5 ml sample and put on ice (-20 C) these are negative control reference points (IPTG- and ARA-) | ||
*To 3 of 4 cultures) (day 2 – step 5) each add 100mM IPTG, these will become the IPTGex30, IPTGex60, IPTGex120 cultures | *To 3 of 4 cultures) (day 2 – step 5) each add 100mM IPTG, these will become the IPTGex30, IPTGex60, IPTGex120 cultures | ||
- | *To 3 of 4 cultures (day 2 – step 6) each add excessive amount of Arabinose | + | *To 3 of 4 cultures (day 2 – step 6) each add excessive amount of Arabinose, these will become the ARAex30, ARAex60, ARAex120 cultures |
*From all 8 cultures (IPTG-, IPTGex30, IPTGex60, IPTGex120, ARA-, ARAex30, ARAex60, ARAex120) take 1.5 ml sample and put on ice (-20 C) (IPTG t0 & ARA t0) | *From all 8 cultures (IPTG-, IPTGex30, IPTGex60, IPTGex120, ARA-, ARAex30, ARAex60, ARAex120) take 1.5 ml sample and put on ice (-20 C) (IPTG t0 & ARA t0) | ||
*At 30 min take for all 8 cultures (IPTG-, IPTGex30, IPTGex60, IPTGex120, ARA-, ARAex30, ARAex60, ARAex120) a 1.5 ml sample and put on ice (-20 C) (IPTG t30 & ARA t30) | *At 30 min take for all 8 cultures (IPTG-, IPTGex30, IPTGex60, IPTGex120, ARA-, ARAex30, ARAex60, ARAex120) a 1.5 ml sample and put on ice (-20 C) (IPTG t30 & ARA t30) |
Latest revision as of 03:55, 27 September 2012