Preparing chemically competent cells (Inoue)
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Current revision (13:09, 23 February 2009) (view source) |
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==Materials== | ==Materials== | ||
* Plate of cells streaked for single colonies | * Plate of cells streaked for single colonies | ||
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==Preparation== | ==Preparation== | ||
| - | # Pick a 10 - 12 large single colonies (2-3 mm dia) from your source plate and inoculate 500 ml of sterile SOB medium (do not use LB) in a 2 liter flask. | + | # Pick a 10 - 12 large single colonies (2-3 mm dia) from your source plate and inoculate 500 ml of sterile SOB medium (do not use LB) in a 2 liter flask. Save some medium as an OD blank. |
| - | # Grow to an OD of 0.6 with vigorous shaking (200-250 rpm) at 18 degrees (important) | + | # Grow to an OD of 0.6 with vigorous shaking (200-250 rpm) at 18 degrees (important). This is slow -- approximately 35-40 hours. |
# Prechill the centrifuge to 4 degrees | # Prechill the centrifuge to 4 degrees | ||
# Remove from the incubator and place on ice for 10 minutes | # Remove from the incubator and place on ice for 10 minutes | ||
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# Place on ice for 10 minutes | # Place on ice for 10 minutes | ||
# Spin down as above. | # Spin down as above. | ||
| - | # Resuspend each pellet in 20 ml of cold TB | + | # While spinning, add 1.4 ml of DMSO to 18.6 ml of TB (7% DMSO mixture) |
| - | + | # Resuspend each pellet in 20 ml of cold TB-DMSO mixture | |
# Incubate on ice for 10 minutes | # Incubate on ice for 10 minutes | ||
# Dispense cells into pre-chilled tubes | # Dispense cells into pre-chilled tubes | ||
# Freeze cells in a dry ice / ethanol bath and store at -80 degrees indefinitely | # Freeze cells in a dry ice / ethanol bath and store at -80 degrees indefinitely | ||
| + | |||
| + | ==Thoughts on improvements== | ||
| + | * "Methods in Yeast Genetics" book (Amberg05) suggests growth the SOB + 300 mM NaCl | ||
| + | * They also control pH at 7.5, which may be a major issue | ||
| + | * Centrifuging in flat bottom centrifuge tubes may make pellet resuspension easier and less damaging | ||
| + | * Length of time on ice prior to transformation may make a big difference | ||
| + | * The Hanahan protocol specifies dry pure DMSO, while Inoue says it doesn't make a difference. Let's see. | ||
| + | * Warm plates for growing cells after transformation are claimed to be 2x to 4x more efficient. | ||
| + | * My lab uses LB for instead of SOB media...it seems to work fine for them--[[User:Melissali|mel]] 18:10, 14 June 2007 (EDT) | ||
==Related topics & references== | ==Related topics & references== | ||
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*[[Bacterial cell culture]] | *[[Bacterial cell culture]] | ||
| - | Original protocol from Inoue et al. <cite> Inoue90 </cite>. | + | Original protocol from Inoue et al. <cite> Inoue90 </cite>. Useful comments and speculation about reducing agents in <cite>Hengen96</cite>. |
<biblio> | <biblio> | ||
#Inoue90 pmid=2265755 | #Inoue90 pmid=2265755 | ||
| + | #Hengen96 pmid=8851666 | ||
</biblio> | </biblio> | ||
| - | [[Category: | + | [[Category:Protocol]] |
| + | [[Category:Escherichia coli]] | ||
Current revision
| back to protocols | ||
Contents |
Materials
Glassware & equipment
- 2 liter erlenmeyer flask (no detergent residue, rinse with 70% ethanol and DI water)
- 220 ml conical centrifuge tubes BD 35 2075
- Eppendorf 5410R refrigerated centrifuge with conical adapters
Preparation
- Pick a 10 - 12 large single colonies (2-3 mm dia) from your source plate and inoculate 500 ml of sterile SOB medium (do not use LB) in a 2 liter flask. Save some medium as an OD blank.
- Grow to an OD of 0.6 with vigorous shaking (200-250 rpm) at 18 degrees (important). This is slow -- approximately 35-40 hours.
- Prechill the centrifuge to 4 degrees
- Remove from the incubator and place on ice for 10 minutes
- Transfer to two 220 ml centrifuge tubes and spin at 3220 x g for 10 minutes at 4 degrees
- Drain the medium and resuspend each pellet first in 5 ml of ice cold TB. Add an additional 75 ml of cold TB buffer and resuspend.
- Place on ice for 10 minutes
- Spin down as above.
- While spinning, add 1.4 ml of DMSO to 18.6 ml of TB (7% DMSO mixture)
- Resuspend each pellet in 20 ml of cold TB-DMSO mixture
- Incubate on ice for 10 minutes
- Dispense cells into pre-chilled tubes
- Freeze cells in a dry ice / ethanol bath and store at -80 degrees indefinitely
Thoughts on improvements
- "Methods in Yeast Genetics" book (Amberg05) suggests growth the SOB + 300 mM NaCl
- They also control pH at 7.5, which may be a major issue
- Centrifuging in flat bottom centrifuge tubes may make pellet resuspension easier and less damaging
- Length of time on ice prior to transformation may make a big difference
- The Hanahan protocol specifies dry pure DMSO, while Inoue says it doesn't make a difference. Let's see.
- Warm plates for growing cells after transformation are claimed to be 2x to 4x more efficient.
- My lab uses LB for instead of SOB media...it seems to work fine for them--mel 18:10, 14 June 2007 (EDT)
Related topics & references
- Preparing chemically competent cells
- Preparing TSS buffer
- Transforming chemically competent cells
- Preparing electrocompetent cells
- Electroporation
- TB buffer
- Transforming chemically competent cells (Inoue)
- Bacterial cell culture
Original protocol from Inoue et al. [1]. Useful comments and speculation about reducing agents in [2].
- Inoue H, Nojima H, and Okayama H. . pmid:2265755.
- Hengen PN. . pmid:8851666.
