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Team:Paris Bettencourt/MultiHost
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| + | Electroporation protocol adapted from Cao et al. article (2011) that has given us some stable results over time. Because of the resistance of ''Bacillus subtilis'' to electro-poration higher voltages are needed to the point of destroying the population, all the different sugars used are meant to stabilize the membrane of the cells. | ||
| + | |||
| + | '''Day 1: preparation''' | ||
| + | *Growth medium: | ||
| + | **LB + 0.5 mol.L<sup>-1</sup> sorbitol → expected final volume: 52 mL for 1 cell culture (including 1 mL for taring the absorbance machine) | ||
| + | ***msorbitol ≈ 4,736 g | ||
| + | *Electro-poration medium: | ||
| + | **de-ionized water + 0.5 mol.L<sup>-1</sup> sorbitol + 0.5 mol.L<sup>-1</sup> mannitol + 0.5 mol.L<sup>-1</sup> trehalose + 10% glycerol (v/v) → expected final volume ≈ 40 mL for 1 round of poration | ||
| + | ***m<sub>sorbitol</sub> = m<sub>mannitol</sub> ≈ 3,643 g | ||
| + | ***m<sub>trehalose</sub> ≈ 7,566 g | ||
| + | ***V<sub>99,5 % glycerol</sub> ≈ 4 mL | ||
| + | *Recovery medium: | ||
| + | **LB + 0.5 mol.L<sup>-1</sup> sorbitol + 0.38 mol.L<sup>-1</sup> mannitol → expected final volume: ≈ 1.1 ml per poly... tube (Approximately 10 tubes ≈ 11 mL total) | ||
| + | ***m<sub>sorbitol</sub> ≈ 1,002 g (for 10 tubes) | ||
| + | ***m<sub>mannitol</sub> ≈ 0,761 g (for 10 tubes) | ||
| + | *Sterilise the solution: Filtration or autoclave. | ||
| + | *Inoculate a falcon containing 10 ml of LB with your ''subtilis'' strain and let it grow overnight (37°C with shaking). | ||
| + | |||
| + | '''Day 2: electro-poration''' | ||
| + | # Monitor the OD600 of your overnight culture. | ||
| + | # In a 500 ml erlenmeyer: dilute your culture into 50mL of Growth Medium so that the OD 600 is 0.01. | ||
| + | # Let the culture grow (37°C with shaking) until OD600 is between 0.85 and 1. | ||
| + | # Cool the cells on ice for 5 minutes. | ||
| + | # NOTE: KEEP ALL YOUR MATERIAL ON ICE AND ALWAYS MANIPULATE ON ICE FROM NOW ON, KEEP AS STERILE AS POSSIBLE. | ||
| + | # Distribute evenly the culture into two falcons and centrifuge at 3000g for 10 minutes. | ||
| + | # Get rid of supernatant, tap the falcon upside down on a piece of paper to get rid of as much solution possible. Detach the pellet. | ||
| + | # Add 20 mL of ice-cold electro-poration medium to one falcon, suspend the cells and transfer the content to the other falcon. Re-suspend. | ||
| + | # Centrifuge 3000g for 10 minutes. | ||
| + | # Remove supernatant, detach pellet, add 10 mL of ice-cold electro-poration medium. Centrifuge. | ||
| + | #Repeat step 10 with 5 mL, 2.5 mL and finally add 0.625 mL (1/80 of initial volume). | ||
| + | # During the centrifugation time, prepare the poly... tubes (label them) with recovery medium in them and put the cuvettes on ice: 1 of each at least has to be a control of cells without DNA, then 1 for each transformant you wish to make. | ||
| + | # Transfer in a cuvette: 60 μL of cells + 1 μL of DNA (50ng/μL; none if control). | ||
| + | # Pulse the cuvette. | ||
| + | # Transfer immediately the content into the poly... tube (STERILE CONDITIONS). | ||
| + | # Repeat 13, 14 and 15 for the number of prepared cuvettes. | ||
| + | # Incubate the poly... tubes at 37°C for 3 to 6 hours. | ||
| + | # Prepare plates with antibiotics (none for the control). | ||
| + | # Note: ≈ 25 ml of LBA per petri dish, make sure the antibiotic is well diluted, labeling should be obvious. | ||
| + | # Plate max 150 μL of transformed cells per petri dish and let grow overnight. | ||
Revision as of 08:39, 29 August 2011
Electroporation protocol adapted from Cao et al. article (2011) that has given us some stable results over time. Because of the resistance of Bacillus subtilis to electro-poration higher voltages are needed to the point of destroying the population, all the different sugars used are meant to stabilize the membrane of the cells.
Day 1: preparation
- Growth medium:
- LB + 0.5 mol.L-1 sorbitol → expected final volume: 52 mL for 1 cell culture (including 1 mL for taring the absorbance machine)
- msorbitol ≈ 4,736 g
- LB + 0.5 mol.L-1 sorbitol → expected final volume: 52 mL for 1 cell culture (including 1 mL for taring the absorbance machine)
- Electro-poration medium:
- de-ionized water + 0.5 mol.L-1 sorbitol + 0.5 mol.L-1 mannitol + 0.5 mol.L-1 trehalose + 10% glycerol (v/v) → expected final volume ≈ 40 mL for 1 round of poration
- msorbitol = mmannitol ≈ 3,643 g
- mtrehalose ≈ 7,566 g
- V99,5 % glycerol ≈ 4 mL
- de-ionized water + 0.5 mol.L-1 sorbitol + 0.5 mol.L-1 mannitol + 0.5 mol.L-1 trehalose + 10% glycerol (v/v) → expected final volume ≈ 40 mL for 1 round of poration
- Recovery medium:
- LB + 0.5 mol.L-1 sorbitol + 0.38 mol.L-1 mannitol → expected final volume: ≈ 1.1 ml per poly... tube (Approximately 10 tubes ≈ 11 mL total)
- msorbitol ≈ 1,002 g (for 10 tubes)
- mmannitol ≈ 0,761 g (for 10 tubes)
- LB + 0.5 mol.L-1 sorbitol + 0.38 mol.L-1 mannitol → expected final volume: ≈ 1.1 ml per poly... tube (Approximately 10 tubes ≈ 11 mL total)
- Sterilise the solution: Filtration or autoclave.
- Inoculate a falcon containing 10 ml of LB with your subtilis strain and let it grow overnight (37°C with shaking).
Day 2: electro-poration
- Monitor the OD600 of your overnight culture.
- In a 500 ml erlenmeyer: dilute your culture into 50mL of Growth Medium so that the OD 600 is 0.01.
- Let the culture grow (37°C with shaking) until OD600 is between 0.85 and 1.
- Cool the cells on ice for 5 minutes.
- NOTE: KEEP ALL YOUR MATERIAL ON ICE AND ALWAYS MANIPULATE ON ICE FROM NOW ON, KEEP AS STERILE AS POSSIBLE.
- Distribute evenly the culture into two falcons and centrifuge at 3000g for 10 minutes.
- Get rid of supernatant, tap the falcon upside down on a piece of paper to get rid of as much solution possible. Detach the pellet.
- Add 20 mL of ice-cold electro-poration medium to one falcon, suspend the cells and transfer the content to the other falcon. Re-suspend.
- Centrifuge 3000g for 10 minutes.
- Remove supernatant, detach pellet, add 10 mL of ice-cold electro-poration medium. Centrifuge.
- Repeat step 10 with 5 mL, 2.5 mL and finally add 0.625 mL (1/80 of initial volume).
- During the centrifugation time, prepare the poly... tubes (label them) with recovery medium in them and put the cuvettes on ice: 1 of each at least has to be a control of cells without DNA, then 1 for each transformant you wish to make.
- Transfer in a cuvette: 60 μL of cells + 1 μL of DNA (50ng/μL; none if control).
- Pulse the cuvette.
- Transfer immediately the content into the poly... tube (STERILE CONDITIONS).
- Repeat 13, 14 and 15 for the number of prepared cuvettes.
- Incubate the poly... tubes at 37°C for 3 to 6 hours.
- Prepare plates with antibiotics (none for the control).
- Note: ≈ 25 ml of LBA per petri dish, make sure the antibiotic is well diluted, labeling should be obvious.
- Plate max 150 μL of transformed cells per petri dish and let grow overnight.
