Team:Osaka/Meeting
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From [[Team:Osaka/Notebook|Notebook]] | From [[Team:Osaka/Notebook|Notebook]] | ||
- | = | + | =Material and Methods= |
- | + | ==Preparing CaCl<sub>2</sub>competent cell== | |
- | ;#Pick a single colony (Nova Blue) and inoculate 5 ml LB | + | ;#Pick a single colony (strain -> Nova Blue) and inoculate 5 ml LB |
;#Incubate overnight at 37°C | ;#Incubate overnight at 37°C | ||
;#Inoculate 30 ml LB with 1ml of o/n preculture in sterile 100 ml erlenmeyer | ;#Inoculate 30 ml LB with 1ml of o/n preculture in sterile 100 ml erlenmeyer | ||
Line 29: | Line 29: | ||
;#stock at -80℃ | ;#stock at -80℃ | ||
- | == | + | ==Transformation of chemical competent cell== |
- | + | ;#Thaw competent cells on ice | |
- | + | ;#Mix 2~5 ul pDNA and 100 ul competent cells in 1.5 ml pre-chiled sterile tube | |
- | + | ;#On ice for 30min | |
- | + | ;#Heat shock 42℃ for 2~1min | |
- | + | ;#On ice for 5min | |
- | ;; | + | ;#Add 900 ul LB |
- | ;; | + | ;#Incubate at 37℃ for 1hour (During this, warm plates at 42℃) |
- | ;;;;;# | + | ;#Harvest cells by centrifuge (14krpm, 1min, r.t.) |
- | ;;;;;# | + | ;#Discard 900~800 ul of supernatant |
- | ;;;;;# | + | ;#Resuspend pellet by pipetting |
- | ;;;;;# | + | ;#Plating all cells on the plate with appropriate antibiotics by glass beads |
- | ;; | + | ;#Incubate overnight at 37°C |
+ | ;#Watch the plate and find colony | ||
+ | |||
+ | ==Plasmid mini prep (QIAprep Spin Miniprep kit)== | ||
+ | ;#Pick a single colony from transformed cells and inoculate 5 ml LB with the appropriate selective antibiotics (Amp->5 ul, Kan->25 ul) | ||
+ | ;#Incubate overnight at 37°C | ||
+ | ;#Harvest the cells by centrifugation 13krpm, 1min, r.t. | ||
+ | ;#Resuspend pelleted cells in '''250 ul Buffer P1'''. No cell clumps should be visible after resuspension of the pellet. So, pipetting an vortex well!.P1 buffer must be stocked at 4°C | ||
+ | ;#Add '''250 ul Buffer P2''' and inventing the tubes 4-6times | ||
+ | ;#Add '''350 ul Buffer N3''' and inventing the tubes 4-6times soon after step 5 | ||
+ | ;#Centrifuge:15krpm, 10min, 4°C | ||
+ | ;#Transfer the supernatants to the Ecospin column (economical..) or QlAprep spin column by pipetting | ||
+ | ;#Centrifuge: 13krpm, 1min, r.t. | ||
+ | ;#Reapply the flow-through to column for improving yield | ||
+ | ;#Centrifuge: 13krpm, 1min, r.t. and discard the flow-through | ||
+ | ;#Add '''500 ul Buffer PB''' in column | ||
+ | ;#Centrifuge: 13krpm, 1min, r.t. and discard the flow-through | ||
+ | ;#Add '''750 ul Buffer PE''' in column | ||
+ | ;#Centrifuge: 13krpm, 1min, r.t. and discard the flow-through | ||
+ | ;#Centrifuge: 14krpm, 3min, r.t. to remove residual wash buffer. And then, discard the flow-through | ||
+ | ;#Place the column in a clean 1.5 ml tube. Add 100~50 ul Buffer EB or sterile water to the center of each column | ||
+ | ;#Keep at r.t. for 3~5min | ||
+ | ;#Centrifuge:15krpm, 1min | ||
+ | ;#stock -30°C | ||
+ | |||
+ | ==Restriction Digestion== | ||
+ | For cloning experiments, the final volume should be 20 or 50 | ||
</div> | </div> |
Latest revision as of 08:02, 11 August 2009
From Notebook
Contents |
Material and Methods
Preparing CaCl2competent cell
- Pick a single colony (strain -> Nova Blue) and inoculate 5 ml LB
- Incubate overnight at 37°C
- Inoculate 30 ml LB with 1ml of o/n preculture in sterile 100 ml erlenmeyer
- Incubate culture at 37°C on a shaker up to OD600=0.3~0.5 (Measure OD value first 1hr and each 30min)
- When the culture reaches an OD600 between 0.3 and 0.5, transfer the culture into 50 centrifugation tube(sterile)
- On ice for 10min
- Centrifuge:8krpm,5min,4°C
- Discard supernatant
- Resuspend each pellet in 20 ml chilled 0.1 M MgCl2 and add further 15 ml 0.1 M MgCl (total 45 ml)
- On ice for 10min
- Centrifuge:8krpm,5min,4℃
- Discard supernatant
- Resuspend each pellet in 20 ml chilled 0.1 M CaCl2 and add further 15 ml 0.1 M MgCl (total 45 ml)
- On ice 30min
- Centrifuge:8krpm,5min,4℃
- Discard supernatant carefuly
- Resuspend each pellet in 750 µl pre-chilled 0.1 M CaCl2 and 750 µl pre-chilled 50%(v/v) Glycerol
- Aliquot 500~100 ul of the mix into sterile microfuge tubes that are pre-chiled at -80℃
- stock at -80℃
Transformation of chemical competent cell
- Thaw competent cells on ice
- Mix 2~5 ul pDNA and 100 ul competent cells in 1.5 ml pre-chiled sterile tube
- On ice for 30min
- Heat shock 42℃ for 2~1min
- On ice for 5min
- Add 900 ul LB
- Incubate at 37℃ for 1hour (During this, warm plates at 42℃)
- Harvest cells by centrifuge (14krpm, 1min, r.t.)
- Discard 900~800 ul of supernatant
- Resuspend pellet by pipetting
- Plating all cells on the plate with appropriate antibiotics by glass beads
- Incubate overnight at 37°C
- Watch the plate and find colony
Plasmid mini prep (QIAprep Spin Miniprep kit)
- Pick a single colony from transformed cells and inoculate 5 ml LB with the appropriate selective antibiotics (Amp->5 ul, Kan->25 ul)
- Incubate overnight at 37°C
- Harvest the cells by centrifugation 13krpm, 1min, r.t.
- Resuspend pelleted cells in 250 ul Buffer P1. No cell clumps should be visible after resuspension of the pellet. So, pipetting an vortex well!.P1 buffer must be stocked at 4°C
- Add 250 ul Buffer P2 and inventing the tubes 4-6times
- Add 350 ul Buffer N3 and inventing the tubes 4-6times soon after step 5
- Centrifuge:15krpm, 10min, 4°C
- Transfer the supernatants to the Ecospin column (economical..) or QlAprep spin column by pipetting
- Centrifuge: 13krpm, 1min, r.t.
- Reapply the flow-through to column for improving yield
- Centrifuge: 13krpm, 1min, r.t. and discard the flow-through
- Add 500 ul Buffer PB in column
- Centrifuge: 13krpm, 1min, r.t. and discard the flow-through
- Add 750 ul Buffer PE in column
- Centrifuge: 13krpm, 1min, r.t. and discard the flow-through
- Centrifuge: 14krpm, 3min, r.t. to remove residual wash buffer. And then, discard the flow-through
- Place the column in a clean 1.5 ml tube. Add 100~50 ul Buffer EB or sterile water to the center of each column
- Keep at r.t. for 3~5min
- Centrifuge:15krpm, 1min
- stock -30°C
Restriction Digestion
For cloning experiments, the final volume should be 20 or 50