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(New page: BE 140L Spring 2011 Team MANG '''Goal''': Evaluate induction of stress by toxic genes in the promoter set for toxR. In essence, put Pbad-toxR in the cell, put a stress promoter-GFP in the ...) |
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BE 140L Spring 2011 Team MANG | BE 140L Spring 2011 Team MANG | ||
<br>'''M'''arcus Macaulay | |||
<br>'''A'''veree Chang | |||
<br>'''N'''ikit Patel | |||
<br>'''G'''ary Dixon | |||
'''Goal''': Evaluate induction of stress by toxic genes in the promoter set for toxR. In essence, put Pbad-toxR in the cell, put a stress promoter-GFP in the cell, add arabinose until it starts getting toxic, measure the GFP on a plate reader (the Tecan). | '''Goal''': Evaluate induction of stress by toxic genes in the promoter set for toxR. In essence, put Pbad-toxR in the cell, put a stress promoter-GFP in the cell, add arabinose until it starts getting toxic, measure the GFP on a plate reader (the Tecan). | ||
'''Schedule''' | '''Schedule''' | ||
<br>'''Tues (4/5)''': Marcus comes in at 9am transforms ToxR plasmid into MC1061 compitent cells. Plate on SPEC. | |||
* Placed plated toxR cells in 37 degree C incubator labeled with M.A.N.G, date and time. | |||
<br>'''Wed (4/6)''': Nikit comes in at 9pm pick a colony and culture it in 3ml LB (tell GSI). | |||
* Marcus went in at 15:10 and picked colonies. | |||
* Labeled tube with red tape (BE 140L, Team M.A.N.G, date+time), placed in Warm Room (448A Stanley) in rack on the shaker closest to entry door on left side of room. | |||
* Stored our plated colonies in class room lab's glass door refridgerator on 2nd rack from top, Labeled accordingly. | |||
* See [[Picking Colonies]] for in-depth procedures as suggested by S. Boyarskiy. | |||
<br>'''Thur (4/7)''': | |||
# Gary comes in at 9:30am. He dilutes the saturated 3ml culture into a flask full of 27ml LB. After 2 hours, performs small scale competence protocol. After resuspending in TSS (90ul x the number of starting ml of cells) freeze the cells in -80. | |||
# Nikit and Marcus prepares 6 strips | |||
<br>'''Mon (4/11)''': Gary and Averee come in and perform large scale transformation: | |||
All stress promoters:GFP + one Con:GFP + 1 (-) control (36 transformations) | |||
The negative control was plated onto its own round S/K plate. | |||
<br> | |||
<br>'''Tuesday 4/12''' | |||
<br> | |||
Nikit picks colonies and we all plan our next move during class time. | |||
---- | |||
;for Tuesday (4/5) | |||
* 200µL of MC1061 competent cells | |||
* 1 toxR miniprep | |||
* spec plate | |||
---- | |||
'''Procedure''': | |||
'''Transformation #1''' (Marcus) - we need 1750 uL TSS mixture | |||
# Thaw a 200 uL aliquot of MC1061 competent cells on ice | |||
# Add 50uL of water | |||
# Add 30 uL of KCM to the cells | |||
# Put your toxR miniprep mixture on ice, let cool a minute or two (for Miniprep product, dilute by 10, then use 1uL of dilution) | |||
# Add 70 uL of the cell cocktail to the miniprep,, stir to mix | |||
# Let sit on ice for 10 min | |||
# Heat shock for 90 seconds at 42 (longer incubation may work better) | |||
# Put back on ice for 1 min | |||
# Add 100uL of 2YT, let shake in the 37 degree incubator for 1 hour | |||
# Plate 70+ uL on SPEC plate, let incubate at 37 degrees overnight | |||
'''Preparing Competent Cells''': | |||
# Pick colony from Spec plate and grow in 3mL liquid media overnight (14-16 hrs.) | |||
# Dilute 10% in fresh media. (Add 3mL culture in 27mL media flask) = 30mL solution | |||
# Take OD measurements every half hour to make sure cells are in mid-log phase. ~ 2 hours. | |||
# Do competent cell prep by adding 90uL of TSS for every mL of media left in the tube. | |||
# Freeze flask? | |||
'''Transformation #2''' | |||
# Thaw a 1800 uL (200 uL ea) aliquot of MC1061/toxR competent cells on ice | |||
# Add 450 uL (50 uL ea) of water to the cells (if greater volume is desired) | |||
# Add 270 uL (30 uL ea) of KCM to the cells | |||
# Put your miniprep mixture on ice, let cool a minute or two (for Miniprep product, dilute by 10, then use 1uL of dilution) | |||
# Add 30 uL of the cell cocktail to the miniprep, stir to mix | |||
# Let sit on ice for 10 min | |||
# Heat shock for 90 seconds at 42 (longer incubation may work better) | |||
# Put back on ice for 1 min | |||
# Add 100uL of 2YT, let shake in the 37 degree incubator for 1 hour | |||
# Plate 70+ uL on selective antibiotics on petri strips, let incubate at 37 degrees overnight | |||
Latest revision as of 13:09, 11 April 2011
BE 140L Spring 2011 Team MANG
Marcus Macaulay
Averee Chang
Nikit Patel
Gary Dixon
Goal: Evaluate induction of stress by toxic genes in the promoter set for toxR. In essence, put Pbad-toxR in the cell, put a stress promoter-GFP in the cell, add arabinose until it starts getting toxic, measure the GFP on a plate reader (the Tecan).
Schedule
Tues (4/5): Marcus comes in at 9am transforms ToxR plasmid into MC1061 compitent cells. Plate on SPEC.
- Placed plated toxR cells in 37 degree C incubator labeled with M.A.N.G, date and time.
Wed (4/6): Nikit comes in at 9pm pick a colony and culture it in 3ml LB (tell GSI).
- Marcus went in at 15:10 and picked colonies.
- Labeled tube with red tape (BE 140L, Team M.A.N.G, date+time), placed in Warm Room (448A Stanley) in rack on the shaker closest to entry door on left side of room.
- Stored our plated colonies in class room lab's glass door refridgerator on 2nd rack from top, Labeled accordingly.
- See Picking Colonies for in-depth procedures as suggested by S. Boyarskiy.
Thur (4/7):
- Gary comes in at 9:30am. He dilutes the saturated 3ml culture into a flask full of 27ml LB. After 2 hours, performs small scale competence protocol. After resuspending in TSS (90ul x the number of starting ml of cells) freeze the cells in -80.
- Nikit and Marcus prepares 6 strips
Mon (4/11): Gary and Averee come in and perform large scale transformation:
All stress promoters:GFP + one Con:GFP + 1 (-) control (36 transformations)
The negative control was plated onto its own round S/K plate.
Tuesday 4/12
Nikit picks colonies and we all plan our next move during class time.
- for Tuesday (4/5)
- 200µL of MC1061 competent cells
- 1 toxR miniprep
- spec plate
Procedure:
Transformation #1 (Marcus) - we need 1750 uL TSS mixture
- Thaw a 200 uL aliquot of MC1061 competent cells on ice
- Add 50uL of water
- Add 30 uL of KCM to the cells
- Put your toxR miniprep mixture on ice, let cool a minute or two (for Miniprep product, dilute by 10, then use 1uL of dilution)
- Add 70 uL of the cell cocktail to the miniprep,, stir to mix
- Let sit on ice for 10 min
- Heat shock for 90 seconds at 42 (longer incubation may work better)
- Put back on ice for 1 min
- Add 100uL of 2YT, let shake in the 37 degree incubator for 1 hour
- Plate 70+ uL on SPEC plate, let incubate at 37 degrees overnight
Preparing Competent Cells:
- Pick colony from Spec plate and grow in 3mL liquid media overnight (14-16 hrs.)
- Dilute 10% in fresh media. (Add 3mL culture in 27mL media flask) = 30mL solution
- Take OD measurements every half hour to make sure cells are in mid-log phase. ~ 2 hours.
- Do competent cell prep by adding 90uL of TSS for every mL of media left in the tube.
- Freeze flask?
Transformation #2
- Thaw a 1800 uL (200 uL ea) aliquot of MC1061/toxR competent cells on ice
- Add 450 uL (50 uL ea) of water to the cells (if greater volume is desired)
- Add 270 uL (30 uL ea) of KCM to the cells
- Put your miniprep mixture on ice, let cool a minute or two (for Miniprep product, dilute by 10, then use 1uL of dilution)
- Add 30 uL of the cell cocktail to the miniprep, stir to mix
- Let sit on ice for 10 min
- Heat shock for 90 seconds at 42 (longer incubation may work better)
- Put back on ice for 1 min
- Add 100uL of 2YT, let shake in the 37 degree incubator for 1 hour
- Plate 70+ uL on selective antibiotics on petri strips, let incubate at 37 degrees overnight
