Team:Amsterdam/project/protocols/

From 2012.igem.org

(Difference between revisions)
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Growthcuves should be measured in for the pSB1AT3 + Mtase construct containing bacteria. This is critical because all tests should be performed on plasmids extracted from cultures that are either in the log (exponential) phase or fully grown cultures. Bought conditions should be used for bought IPTG+ and IPTG- cultures.
Growthcuves should be measured in for the pSB1AT3 + Mtase construct containing bacteria. This is critical because all tests should be performed on plasmids extracted from cultures that are either in the log (exponential) phase or fully grown cultures. Bought conditions should be used for bought IPTG+ and IPTG- cultures.
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'''Setup'''
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'''Setup'''<br\>
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Starting media:
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'''Starting media:'''<br\>
*100ml LB
*100ml LB
*100ml LB containing 100milliM IPTG
*100ml LB containing 100milliM IPTG
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Starting bacteria:
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'''Starting bacteria:'''<br\>
*2x 10ul pSB1AT3 + MTase containing bacteria form overnight (stationary phase) culture
*2x 10ul pSB1AT3 + MTase containing bacteria form overnight (stationary phase) culture
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Other requirements:
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'''Other requirements:'''<br\>
*1ml cuvette accepting spectrophotometer
*1ml cuvette accepting spectrophotometer
*44x 1ml cuvette
*44x 1ml cuvette
*1x 1ml Demi or MilliQ containing cuvette (for calibration)
*1x 1ml Demi or MilliQ containing cuvette (for calibration)
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Experiment
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'''Experiment'''<br\>
*1.Add 10ul pSB1AT3 + MTase containing bacteria from overnight (stationary phase) culture to 100ml LB and to a 100ml LB containing 100milliM IPTG media
*1.Add 10ul pSB1AT3 + MTase containing bacteria from overnight (stationary phase) culture to 100ml LB and to a 100ml LB containing 100milliM IPTG media
*2.Incubate at 37 C in shaker
*2.Incubate at 37 C in shaker
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*5.Next day measure OD again for bought cultures, and 30 min later (to confirm that the culture is actually stationary at this time)
*5.Next day measure OD again for bought cultures, and 30 min later (to confirm that the culture is actually stationary at this time)
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'''Expectation'''
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'''Expectation'''<br\>
Literature suggests that (if there is enough medium available) the culture will be in the log fase after 1h till about 6h.
Literature suggests that (if there is enough medium available) the culture will be in the log fase after 1h till about 6h.
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These experiments will tell us if the leakiness of the promoter is enough to cause all sites to be methylated. And will (in conjunction with the results from step 3) later tell us something the influence of growth rate  on the equilibrium between methylation loss (due to plasmid replication and death) and gain (due to leakiness of the promoter).
These experiments will tell us if the leakiness of the promoter is enough to cause all sites to be methylated. And will (in conjunction with the results from step 3) later tell us something the influence of growth rate  on the equilibrium between methylation loss (due to plasmid replication and death) and gain (due to leakiness of the promoter).
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'''Setup'''
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'''Setup'''<br\>
-
Starting media:
+
'''Starting media:'''<br\>
*10ml LB
*10ml LB
*10ml LB containing 100milliM IPTG
*10ml LB containing 100milliM IPTG
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Starting bacteria:
+
'''Starting bacteria:'''<br\>
*2x 10ul pSB1AT3 + MTase containing bacteria form overnight (stationary fase) culture
*2x 10ul pSB1AT3 + MTase containing bacteria form overnight (stationary fase) culture
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Other requirements:
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'''Other requirements:'''<br\>
*Miniprep kit
*Miniprep kit
*Nanodrop machine
*Nanodrop machine
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*Standard ladder
*Standard ladder
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Experiment
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'''Experiment'''<br\>
*1.Add 10ul pSB1AT3 + MTase containing bacteria from overnight (stationary phase) culture to 10ml LB and to a 10ml LB containing 100milliM IPTG media
*1.Add 10ul pSB1AT3 + MTase containing bacteria from overnight (stationary phase) culture to 10ml LB and to a 10ml LB containing 100milliM IPTG media
*2.Put cultures in shaker and incubate at 37C
*2.Put cultures in shaker and incubate at 37C
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*8.Run DNA from both cultures for all variations on gel, with the ladder on both sides and in the middle. Exact layout: **Ladder, IPTG- DNA digested by ScaI, IPTG- DNA digested by ScaI + EcoRI, IPTG- DNA digested by EcoRI, IPTG- DNA digested by None, Ladder, IPTG+ DNA digested by ScaI, IPTG+ DNA digested by ScaI + EcoRI, IPTG+ DNA digested by EcoRI, IPTG+ DNA digested by None, Ladder.
*8.Run DNA from both cultures for all variations on gel, with the ladder on both sides and in the middle. Exact layout: **Ladder, IPTG- DNA digested by ScaI, IPTG- DNA digested by ScaI + EcoRI, IPTG- DNA digested by EcoRI, IPTG- DNA digested by None, Ladder, IPTG+ DNA digested by ScaI, IPTG+ DNA digested by ScaI + EcoRI, IPTG+ DNA digested by EcoRI, IPTG+ DNA digested by None, Ladder.
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'''Expectation'''
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'''Expectation'''<br\>
Ideal results would be that the Positive control (IPTG+) will result in intensity shift to the uncut/1cut plasmid band in the ScaI digestion and a shift to the top band (plasmid only cut by EcoRI) in the ScaI + EcoRI digestion. Whereas for the Negative control (IPTG-) this shift would be the opposite. Pilot experiments already suggest that this shift of the Negative control is not as severe as would be desired.
Ideal results would be that the Positive control (IPTG+) will result in intensity shift to the uncut/1cut plasmid band in the ScaI digestion and a shift to the top band (plasmid only cut by EcoRI) in the ScaI + EcoRI digestion. Whereas for the Negative control (IPTG-) this shift would be the opposite. Pilot experiments already suggest that this shift of the Negative control is not as severe as would be desired.
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This experiment is done in order to determine the effect that bacterial growth has on the loss and gain of methylated sites and the equilibrium it might establish.
This experiment is done in order to determine the effect that bacterial growth has on the loss and gain of methylated sites and the equilibrium it might establish.
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'''Setup'''
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'''Setup'''<br\>
Starting media (much more than in step 3 because less DNA will be extracted per ml due to lower growth time):
Starting media (much more than in step 3 because less DNA will be extracted per ml due to lower growth time):
*100ml LB
*100ml LB
*100ml LB containing 100milliM IPTG
*100ml LB containing 100milliM IPTG
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Starting bacteria:
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'''Starting bacteria:'''<br\>
*10ul pSB1AT3 + MTase containing bacteria form step 2.4 (stationary phase) IPTG+ culture
*10ul pSB1AT3 + MTase containing bacteria form step 2.4 (stationary phase) IPTG+ culture
*10ul pSB1AT3 + MTase containing bacteria form step 2.4 (stationary phase) IPTG- culture
*10ul pSB1AT3 + MTase containing bacteria form step 2.4 (stationary phase) IPTG- culture
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Other requirements:
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'''Other requirements:'''<br\>
*Miniprep kit
*Miniprep kit
*Nanodrop machine
*Nanodrop machine
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*Standard ladder
*Standard ladder
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'''Experiment'''
+
'''Experiment'''<br\>
*1.Add 10ul pSB1AT3 + MTase containing bacteria from step 2.4 (stationary phase) IPTG+ culture to the 100ml LB containing 100milliM IPTG media
*1.Add 10ul pSB1AT3 + MTase containing bacteria from step 2.4 (stationary phase) IPTG+ culture to the 100ml LB containing 100milliM IPTG media
*2.Add 10ul pSB1AT3 + MTase containing bacteria from step 2.4 (stationary phase) IPTG- culture to the 100ml LB media
*2.Add 10ul pSB1AT3 + MTase containing bacteria from step 2.4 (stationary phase) IPTG- culture to the 100ml LB media
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*9.Run DNA from both cultures for all variations on gel, with the ladder on both sides and in the middle. Exact layout: Ladder, IPTG- DNA digested by ScaI, IPTG- DNA digested by ScaI + EcoRI, IPTG- DNA digested by EcoRI, IPTG- DNA digested by None, Ladder, IPTG+ DNA digested by ScaI, IPTG+ DNA digested by ScaI + EcoRI, IPTG+ DNA digested by EcoRI, IPTG+ DNA digested by None, Ladder.
*9.Run DNA from both cultures for all variations on gel, with the ladder on both sides and in the middle. Exact layout: Ladder, IPTG- DNA digested by ScaI, IPTG- DNA digested by ScaI + EcoRI, IPTG- DNA digested by EcoRI, IPTG- DNA digested by None, Ladder, IPTG+ DNA digested by ScaI, IPTG+ DNA digested by ScaI + EcoRI, IPTG+ DNA digested by EcoRI, IPTG+ DNA digested by None, Ladder.
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'''Expectation'''
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'''Expectation'''<br\>
In the ideal case the Positive result (IPTG+) would only show the uncut/1 cut plasmid band in the ScaI digestion and only the top band (uncut plasmid) in the ScaI + EcoRI digestion. And the opposite results in the negative control (IPTG-)
In the ideal case the Positive result (IPTG+) would only show the uncut/1 cut plasmid band in the ScaI digestion and only the top band (uncut plasmid) in the ScaI + EcoRI digestion. And the opposite results in the negative control (IPTG-)
If similar results to the expected shift in step 2 are observed than the growth rate of the culture doesn’t have any impact on the methylation gain and methylation loss equilibrium.
If similar results to the expected shift in step 2 are observed than the growth rate of the culture doesn’t have any impact on the methylation gain and methylation loss equilibrium.

Revision as of 10:26, 24 September 2012