Team:Paris/Protocols Culture
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+ | <span/ id="bottom">[https://2009.igem.org/ iGEM ] > [[Team:Paris#top | Paris]] > [[Team:Paris/Protocols#top | Protocols]] > [[Team:Paris/Protocols_Culture#bottom | Culture Protocols]] | ||
{{Template:Paris2009}} | {{Template:Paris2009}} | ||
{{Template:Paris2009_menu}} | {{Template:Paris2009_menu}} | ||
- | == Protocols == | + | |
- | <center> | + | |
+ | |||
+ | == Culture Protocols == | ||
+ | <html> | ||
+ | <style type="text/css"> | ||
+ | #left-side { | ||
+ | position: absolute; | ||
+ | height: 23px; | ||
+ | width: 30px; | ||
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+ | margin-top:10px; | ||
+ | padding-top: 7px; | ||
+ | background: url(https://static.igem.org/mediawiki/2009/1/1b/Left_menu_pari.png); | ||
+ | z-index:4; | ||
+ | } | ||
+ | |||
+ | #middle-side { | ||
+ | height: 25px; | ||
+ | width: 560px; | ||
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+ | </style> | ||
+ | <div id="left-side"></div> | ||
+ | <div id="middle-side"><center> | ||
+ | <a class="menu_sub"href="https://2009.igem.org/Team:Paris/Protocols#bottom"> Main </a>| | ||
+ | <a class="menu_sub" href="https://2009.igem.org/Team:Paris/ProtocolsA#bottom"> Microscope Protocols</a>| | ||
+ | <a class="menu_sub"href="https://2009.igem.org/Team:Paris/ProtocolsB#bottom"> Adapted Protocols</a>| | ||
+ | <a class="menu_sub_active"href="https://2009.igem.org/Team:Paris/Protocols_Culture#bottom"> Culture Protocols</a>| | ||
+ | <a class="menu_sub"href="https://2009.igem.org/Team:Paris/ProtocolsMB#bottom"> Molecular biology</a> | ||
+ | </center> | ||
+ | </div> | ||
+ | |||
+ | <div id="right-side"></div> | ||
+ | |||
+ | </html> | ||
# Over Night | # Over Night | ||
- | # | + | #[[team:Paris/Protocols_Culture#Bacterial transformation|Bacterial transformation]] |
#[[team:Paris/Protocols_Culture#Competent bacteria|Competent bacteria]] | #[[team:Paris/Protocols_Culture#Competent bacteria|Competent bacteria]] | ||
#[[team:Paris/Protocols_Culture#Glycerol stock|Glycerol stock]] | #[[team:Paris/Protocols_Culture#Glycerol stock|Glycerol stock]] | ||
+ | #[[team:Paris/Protocols_Culture#Ferric citrate growth medium|Ferric citrate growth medium]] | ||
<html> | <html> | ||
</div> | </div> | ||
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- | == | + | ==Bacterial transformation== |
* 250µl of DH5α competent bacteria (by RbCl) | * 250µl of DH5α competent bacteria (by RbCl) | ||
* Add 2µl of DNA (ex Biobrick) | * Add 2µl of DNA (ex Biobrick) | ||
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# Vortex gently | # Vortex gently | ||
# Stock at -80°C | # Stock at -80°C | ||
+ | |||
+ | <html> | ||
+ | </div> | ||
+ | <div id="paris_content_boxtop"> | ||
+ | </div> | ||
+ | <div id="paris_content"> | ||
+ | </html> | ||
+ | |||
+ | ==Ferric citrate growth medium== | ||
+ | |||
+ | Growth on ferric citrate as the sole iron source was tested on Fec agar plates containing NB medium, 1.5% nutrient agar, 0.2 mM 2,2'-dipyridyl, and 1 mM citrate. (ref Surface Signaling in Ferric Citrate Transport Gene Induction: Interaction of the FecA, FecR, and FecI Regulatory Proteins. Enz et al, 1999) |
Latest revision as of 15:11, 19 October 2009
iGEM > Paris > Protocols > Culture Protocols
Contents |
Culture Protocols
Bacterial transformation
- 250µl of DH5α competent bacteria (by RbCl)
- Add 2µl of DNA (ex Biobrick)
- Incubation during 20min on ice
- Heat choc 45second at 42°C
- Leave on ice 2min
- Add 1ml of LB preheated at 42°C
- Incubation 1 hour at 37°C under agitation
- Put 100µl of culture under plate
- Centrifuge 2min at 6rpm MAX for 2 min
- Put 100µl of concentrated culture
- Incubate overnight at 37°C
CaCl2 (iGEM Paris2007)
Prepare CaCl2 0.1M
- Add 7,351g of CaCl2.2 H2O (FM 147,02) in 500 mL H2O
- dissolve the CaCl2 by mixing the suspension with the help of a magnetic stirrer
- Filter the solution with a cell-culture unit of filtration
- Aliquotes the filtered solution: 25mL in a 50 mL Falcon. Storage at +4°C
Steps
- Use non competent bacteria (ex: MG1655) stocked in 1.5 mL LB (20% Glycerol): put a sterile tip in the 1.5 mL stock tube and then place it in a 50 mL Falcon with 5 ml LB medium.
Over Night culture at 37°C / 200 rpm - 1/100 dilution in LB medium QSP 50 mL in an erlenmeyer of 250 mL
- Culture at 37°C / 200 rpm untill OD600 reach 0.6
- Fast cooling at +4°C by gently shaking the erlen in ice
- Use pre-cooled centrifuge at +4°C. Centrifuge 50 mL of the culture in 50 mL falcon: +4°C / 5 min / 4000 rpm
- Discard supernatant by inverting the tube, and resuspend the pellet with 1 mL of cold CaCl2 and mix gently the suspension by up and down
- Add cold CaCl2 QSP 20 mL and incubate 30 min / +4°C
- Centrifuge the suspension : +4°C / 5 min / 4000 rpm
- Discard supernatant by inverting the tube, and resuspend the pellet with 1 mL of cold CaCl2 and mix gently the suspension by up and down
- Transform or freeze the competent cells. Freeze the competent cells in 50 µL aliquots in the 0.1M CaCl2 medium with 15% glycerol.
- After transformation, prepare a Glycerol stock
CaCl2 (2nd Protocol)
- Inoculate 50/5 ml of LB with fresh colony or dilution of an overnight culture
- Grow up to OD600 0.5-0.8
- Leave on ice 10min
- Spin 40/2 ml of cell suspension, 5min at 4000rpm, 4°C/minispin 2min at 5000rpm, 4°C
- Resuspend the pellet in 20/1 ml CaCl2 50mM (1/2 of initial Vol)
- Leave on ice 10min
- Spin 40/2 ml of resuspension, 5min at 4000rpm, 4°C/minispin 2min at 5000rpm, 4°C
- Resuspend the pellet in 2ml/100µl CaCl2 50mM (1/20 of initial Vol)
- Leave on ice overnight before stock at -80°C
RbCl
Solutions
- Tampon I (250ml)
- Potassium acetate (C2H3KO2 30mM pH 5,8 0,733g
- RbCl 100mM 3,02g
- CaCl2 10mM 0,3741g
- MnCl250mM 2,5g
- Glycerol 15% ~37,5ml
- QS 250ml H2O ~218,5ml
- Adjust with Acetic acid (CH3COOH 100%)to pH 5,8. (Remake the solution if pH beneath 5.8
- Sterilization (filtration).
- Tampon II (125ml)
- MOPS 10mM pH 6.5 0,2382g
- RbCl 10mM 0,150g
- CaCl2 10mM 1,37gg
- Glycerol 15% ~18,75ml
- QS 1250ml H2O ~106.25ml
- Adjust pH to 6.5 with KOH 1M
- Sterilization (filtration)
Steps
- Over night culture (O.N.C)
- Competent
- 50mL of LB with 0.5mL O.N.C
- Wait for 5.6 OD600
- 10mn on ice
- centrifuge 10mn at 4000 RPM
- resuspend the bacteria pellet in 18mL Tampon I
- 10mn on ice
- centrifuge 10mn at 4000 RPM
- resuspend the bacteria pellet in 8mL Tampon II
- Alicot 250µL/tube at -80°C
- Transformation plasmid (10pg/µl)
- 250µl of RbCl competent DH5α
- 12,5µl plasmid
- Leave 20 min in ice
- 45s at 42°C
- Leave 2 min in ice
- Add 1ml of hot LB (42°C)
- 1h at 37 under agitation
- Put on plate (LB agar + Antibiotic)
- culture
- take 100µL and spread it on the plate (LB + Antibiotic)
- centrifuge 2mn the left
- take 100µL and spread it on the plate (LB + Antiobotic)
Glycerol stock
- 0,66ml of 60% glycerol into cryogenic tube
- 1,32ml of overnight bacterial culture
- Vortex gently
- Stock at -80°C
Ferric citrate growth medium
Growth on ferric citrate as the sole iron source was tested on Fec agar plates containing NB medium, 1.5% nutrient agar, 0.2 mM 2,2'-dipyridyl, and 1 mM citrate. (ref Surface Signaling in Ferric Citrate Transport Gene Induction: Interaction of the FecA, FecR, and FecI Regulatory Proteins. Enz et al, 1999)