Lidstrom:Competent Cell Preparation
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(New page: Back to Protocols ==Chemically Competent E. Coli== Notes: *You need fresh cells. **Often people inoculate a few mL of the culture for overnight growth, then use 20...) |
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**Often people inoculate a few mL of the culture for overnight growth, then use 200 uL to inoculate the ~50 mL of culture they will make competent. | **Often people inoculate a few mL of the culture for overnight growth, then use 200 uL to inoculate the ~50 mL of culture they will make competent. | ||
**Some people in our lab believe you want to start with a fresh plate and don't even use one that is a few days old. Other people (Mila) are mostly concerned about the OD being right at the time of harvest. | **Some people in our lab believe you want to start with a fresh plate and don't even use one that is a few days old. Other people (Mila) are mostly concerned about the OD being right at the time of harvest. | ||
| + | *You need to flash freeze the cells at the end of the procedure. You can do this by pouring liquid nitrogen over them, or you can freeze your tubes at -80oC the night before, put your aliquots in, and stick them back at -80oC. | ||
| - | == | + | ===Amanda/Janet Protocol for Chemically Competent Cells === |
| - | * | + | ==== Supplies needed: ==== |
| + | * Plate of E. Coli colonies | ||
| + | * SOB-Mg growth medium | ||
| + | * Sterilized 500 mL Erlenmeyer flasks | ||
| + | * 50 mL screw-cap polypropylene tubes | ||
| + | * Freezer tubes (1.5 mL) | ||
| + | * SOC medium for recovery after heat shock (LB/TB is fine instead) | ||
| + | ==== Method ==== | ||
| + | # Pick several colonies off a freshly streaked plate into ~1 mL SOB-Mg growth medium | ||
| + | ## Grow cells overnight or several hours in media with appropriate antibiotics if available. | ||
| + | ## Use more inoculum in the next step if cultures weren't grown overnight. | ||
| + | # Inoculate 50 mL SOB-Mg growth medium with this culture. Use between 1 uL to 1 mL stationary phase culture per mL of medium. | ||
| + | # Incubate at 275 rpm, 37<sup>o</sup>C until OD<sub>600</sub> is about 0.3, which corresponds to ~ 5*10<sup>7</sup>cells/mL | ||
| + | # Collect in sterile 50 mL polypropylene centrifuge tube(s) and chill on ice for 10 minutes | ||
| + | # Pellet the cells at 750 - 1,000g (2500 rpm) for 14 min at 4<sup>o</sup>C. Decant the supernatant and invert tubes to remove excess culture medium. | ||
| + | # Disperse cells in ~1/3 volume of CCMB by gentle vortexing or rapping of the centrifuge tube. | ||
| + | # Incubate on ice for 20 minutes | ||
| + | # Centrifuge at 2500 rpm for 10 min at 4<sup>o</sup>C | ||
| + | # Resuspend cells in CCMB at 1/12 the original culture volume | ||
| + | # Make aliquots in eppendorf tubes, ideally on ice | ||
| + | # Flash freeze with liquid nitrogen | ||
| + | # Store at -80oC to preserve them for many months | ||
| + | ====Recipes:==== | ||
| + | *SOB-Mg growth medium | ||
| + | *CCMB | ||
| + | |||
| + | ===Nicole/Andrew protocol for Chemically Competent cells=== | ||
| + | '''Materials and reagents''' | ||
| + | * E. coli line (Top 10, S17-1, BL21-AL, BL21-D3, JM109, Qiagen) | ||
| + | * TFB I (transformation buffer) | ||
| + | * TFB II | ||
| + | |||
| + | ; TFB I (100 ml) | ||
| + | :30 mM acetate K (0.294 g) | ||
| + | :100 mM RbCl (1.21 g) | ||
| + | :10 mM CaCl2 (0.14 g) | ||
| + | :50 mM MnCl2 (1.0 g) | ||
| + | :15% glycerol (15 ml) | ||
| + | :dH2O | ||
| + | :pH = 5.8 (use acetic acid to adjust) | ||
| + | |||
| + | ; TFB II 100 ml | ||
| + | :10 mM MOPS (0.21 g) | ||
| + | :75 mM CaCl2 (1.1 g) | ||
| + | :10 mM RbCl (0.12 g) | ||
| + | :15% glycerol (15 ml) | ||
| + | :dH2O | ||
| + | :pH = 6.5 (use KOH to adjust) | ||
| + | |||
| + | '''Protocol''' | ||
| + | * 2 days '''before''' making cells, streak out the line of E. coli to make on LB plates (+strep for Top 10 and S17-1) | ||
| + | * 1 day before: | ||
| + | ::inoculate 4 white capped test tubes or disposable 14 ml clear-top falcon tubes with 1 ml of LB (+strep) | ||
| + | ::freeze appropriate color, autoclaved epi tubes in -80°C (80+ tubes) | ||
| + | :::- white tube = Top 10 | ||
| + | :::- yellow tube = S17-1 | ||
| + | :::- pink tube = BL21-AL | ||
| + | :::- purple tube = BL21-D3 | ||
| + | :::- green tube = JM109 | ||
| + | :::- blue tube = Qiagen | ||
| + | |||
| + | |||
| + | # Grow cells in 5 ml LB (+5 ul strep for Top 10 and S17-1 cells) overnight | ||
| + | # Transfer 1 ml of cells to 50 ml LB (use falcon tube) and grow at 37°C for 90 min | ||
| + | #:- want OD of '''0.4 or 0.5''' before starting next steps | ||
| + | # Place on ice (0°C) for 1 min | ||
| + | # Spin at 6000g, 0°C for 5 min | ||
| + | # Add 15 ml cold dH2O | ||
| + | # Spin at 6000g, 0°C for 5 min, pour off super | ||
| + | # Add 10 ml cold TFB I to pellet | ||
| + | # Incubate on ice for 15 min | ||
| + | # Spin at 6000g, 0°C for 5 min, pour off super | ||
| + | # Add 1 ml cold TFB II to pellet | ||
| + | # Incubate on ice for 30 min | ||
| + | # Aliquot 50 ul into -80°C epi tubes (or into tubes sitting in dry ice) | ||
| + | # Immediately store at -80°C | ||
| + | ***;Best method: | ||
| + | ***:take tubes out of freezer | ||
| + | ***:open all caps | ||
| + | ***:pipette 50 ul into each | ||
| + | ***:close caps | ||
| + | ***:back in -80°C | ||
| + | ***:VERY QUICKLY! | ||
| + | |||
| + | |||
| + | '''TEST CELLS BEFORE STOCKING FOR GENERAL USE''' | ||
| + | * For contamination | ||
| + | :#Scrape a sample from frozen stock | ||
| + | :#Streak on LB (no abx) | ||
| + | :#Grow at 37°C overnight | ||
| + | :#Check for contamination (E. coli should be translucent and yellowish) – If none is present test competency | ||
| + | *For competency | ||
| + | :Use PCM184 plasmid stock (and Amp or Kan/Tet) | ||
| + | :Follow protocol for transformation | ||
| + | |||
| + | ==Electrocompetent Cells== | ||
| + | *You can make your own electro-competent cells for electroporation. | ||
| + | #Grow a small (~ 2 mL) overnight culture with appropriate antibiotic(s) | ||
| + | #Use overnight to inoculate: generally use ~ 200 uL/50 mL | ||
| + | #Let grow for about 3-4 h (OD 0.4-0.6 or so), then centrifuge and wash 2-3 times with 10% glycerol (everything on ice). | ||
| + | #Resuspend the pellet in a small volume, ideally up to 1/500<sup>ths</sup> of the culture volume. | ||
| + | ## See graph below. [[User:Janet B. Matsen|Janet]] did this experiment. The really concentrated cells performed well despite having clumped into a serious "booger" during recovery (pre-plating) that was mostly unspreadable. | ||
| + | #Aliquot into 1.5 ml centrifuge tubes (0.1 ml in each), then flash freeze with liquid nitrogen. Store at -80C. | ||
| + | *Note: you can dilute your re-suspension, measure OD, and calculate the cell concentration if you care. See [[Electrocompetent_Cells| this page]]. Would allow you to calculate efficiency. | ||
| + | [[image:2012_11 electroporation - number of colonies versus competent cell density.jpg|thumb|center|electroporation: number of colonies versus competent cell density]] | ||
Revision as of 22:21, 17 November 2012
Back to Protocols
Contents |
Chemically Competent E. Coli
Notes:
- You need fresh cells.
- Often people inoculate a few mL of the culture for overnight growth, then use 200 uL to inoculate the ~50 mL of culture they will make competent.
- Some people in our lab believe you want to start with a fresh plate and don't even use one that is a few days old. Other people (Mila) are mostly concerned about the OD being right at the time of harvest.
- You need to flash freeze the cells at the end of the procedure. You can do this by pouring liquid nitrogen over them, or you can freeze your tubes at -80oC the night before, put your aliquots in, and stick them back at -80oC.
Amanda/Janet Protocol for Chemically Competent Cells
Supplies needed:
- Plate of E. Coli colonies
- SOB-Mg growth medium
- Sterilized 500 mL Erlenmeyer flasks
- 50 mL screw-cap polypropylene tubes
- Freezer tubes (1.5 mL)
- SOC medium for recovery after heat shock (LB/TB is fine instead)
Method
- Pick several colonies off a freshly streaked plate into ~1 mL SOB-Mg growth medium
- Grow cells overnight or several hours in media with appropriate antibiotics if available.
- Use more inoculum in the next step if cultures weren't grown overnight.
- Inoculate 50 mL SOB-Mg growth medium with this culture. Use between 1 uL to 1 mL stationary phase culture per mL of medium.
- Incubate at 275 rpm, 37oC until OD600 is about 0.3, which corresponds to ~ 5*107cells/mL
- Collect in sterile 50 mL polypropylene centrifuge tube(s) and chill on ice for 10 minutes
- Pellet the cells at 750 - 1,000g (2500 rpm) for 14 min at 4oC. Decant the supernatant and invert tubes to remove excess culture medium.
- Disperse cells in ~1/3 volume of CCMB by gentle vortexing or rapping of the centrifuge tube.
- Incubate on ice for 20 minutes
- Centrifuge at 2500 rpm for 10 min at 4oC
- Resuspend cells in CCMB at 1/12 the original culture volume
- Make aliquots in eppendorf tubes, ideally on ice
- Flash freeze with liquid nitrogen
- Store at -80oC to preserve them for many months
Recipes:
- SOB-Mg growth medium
- CCMB
Nicole/Andrew protocol for Chemically Competent cells
Materials and reagents
- E. coli line (Top 10, S17-1, BL21-AL, BL21-D3, JM109, Qiagen)
- TFB I (transformation buffer)
- TFB II
- TFB I (100 ml)
- 30 mM acetate K (0.294 g)
- 100 mM RbCl (1.21 g)
- 10 mM CaCl2 (0.14 g)
- 50 mM MnCl2 (1.0 g)
- 15% glycerol (15 ml)
- dH2O
- pH = 5.8 (use acetic acid to adjust)
- TFB II 100 ml
- 10 mM MOPS (0.21 g)
- 75 mM CaCl2 (1.1 g)
- 10 mM RbCl (0.12 g)
- 15% glycerol (15 ml)
- dH2O
- pH = 6.5 (use KOH to adjust)
Protocol
- 2 days before making cells, streak out the line of E. coli to make on LB plates (+strep for Top 10 and S17-1)
- 1 day before:
- inoculate 4 white capped test tubes or disposable 14 ml clear-top falcon tubes with 1 ml of LB (+strep)
- freeze appropriate color, autoclaved epi tubes in -80°C (80+ tubes)
- - white tube = Top 10
- - yellow tube = S17-1
- - pink tube = BL21-AL
- - purple tube = BL21-D3
- - green tube = JM109
- - blue tube = Qiagen
- Grow cells in 5 ml LB (+5 ul strep for Top 10 and S17-1 cells) overnight
- Transfer 1 ml of cells to 50 ml LB (use falcon tube) and grow at 37°C for 90 min
- - want OD of 0.4 or 0.5 before starting next steps
- Place on ice (0°C) for 1 min
- Spin at 6000g, 0°C for 5 min
- Add 15 ml cold dH2O
- Spin at 6000g, 0°C for 5 min, pour off super
- Add 10 ml cold TFB I to pellet
- Incubate on ice for 15 min
- Spin at 6000g, 0°C for 5 min, pour off super
- Add 1 ml cold TFB II to pellet
- Incubate on ice for 30 min
- Aliquot 50 ul into -80°C epi tubes (or into tubes sitting in dry ice)
- Immediately store at -80°C
- Best method
- take tubes out of freezer
- open all caps
- pipette 50 ul into each
- close caps
- back in -80°C
- VERY QUICKLY!
TEST CELLS BEFORE STOCKING FOR GENERAL USE
- For contamination
- Scrape a sample from frozen stock
- Streak on LB (no abx)
- Grow at 37°C overnight
- Check for contamination (E. coli should be translucent and yellowish) – If none is present test competency
- For competency
- Use PCM184 plasmid stock (and Amp or Kan/Tet)
- Follow protocol for transformation
Electrocompetent Cells
- You can make your own electro-competent cells for electroporation.
- Grow a small (~ 2 mL) overnight culture with appropriate antibiotic(s)
- Use overnight to inoculate: generally use ~ 200 uL/50 mL
- Let grow for about 3-4 h (OD 0.4-0.6 or so), then centrifuge and wash 2-3 times with 10% glycerol (everything on ice).
- Resuspend the pellet in a small volume, ideally up to 1/500ths of the culture volume.
- See graph below. Janet did this experiment. The really concentrated cells performed well despite having clumped into a serious "booger" during recovery (pre-plating) that was mostly unspreadable.
- Aliquot into 1.5 ml centrifuge tubes (0.1 ml in each), then flash freeze with liquid nitrogen. Store at -80C.
- Note: you can dilute your re-suspension, measure OD, and calculate the cell concentration if you care. See this page. Would allow you to calculate efficiency.
