Team:TzuChiU Formosa/Protocol
From 2009.igem.org
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==Protocol== | ==Protocol== | ||
- | + | https://static.igem.org/mediawiki/2009/e/ea/Project.jpg | |
- | + | A. Culture CP919 | |
- | + | ||
- | + | B. Put Aqueorin-GFP into plasmid . | |
- | + | ||
- | + | C. Transform the cp919 into the Midnight Apollo! | |
- | + | ||
- | + | D. Sense the light. | |
- | + | ||
- | + | E. In the dark, the Midnight Apollo! is activated and emit the light. | |
====Competent Cell (CP919-Cph8)==== | ====Competent Cell (CP919-Cph8)==== | ||
- | #Day1. Streak out the E.coli strain on an | + | #Day1. Streak out the E.coli strain on an LB plate (with kanamycin)and incubate at 37℃ overnight (16-20 hours). |
- | #Day2. Select a single colony and inoculate 10 ml sterile | + | #Day2. Select a single colony and inoculate 10 ml sterile LB and grow overnight (16-20 hours) in a 37℃ shaker incubator. |
- | #Day3. Add 2ml overnight culture to 250ml flask | + | #Day3. Add 2ml overnight culture to 250ml flask containing 100 ml LB. |
- | #Grow the cultures to OD600 = 0.2~0.4 (incubate | + | #Grow the cultures to OD600 = 0.2~0.4 (incubate with shaking for 75~90 min.) |
- | # | + | #Spin down the bacteria at 4℃,3000 rpm for 10 min. |
#Discard the supernatant and mix the cell pellet with 10ml FSB. | #Discard the supernatant and mix the cell pellet with 10ml FSB. | ||
#Keep the cells on ice for 3~4 hours. | #Keep the cells on ice for 3~4 hours. | ||
- | # | + | #Spin down, at 4℃,3000 rpm for 10 min. |
#Discard the supernatant and mix the cell pellet with 5ml FSB. | #Discard the supernatant and mix the cell pellet with 5ml FSB. | ||
- | #Pipet 200μl of the cell suspension into sterile 1.5ml eppendorf. Freeze these tubes | + | #Pipet 200μl of the cell suspension into sterile 1.5ml eppendorf tubes. Freeze these tubes in liquid nitrogen, then transfer them to -80℃ freezer. |
- | |||
+ | ====Tansformation Protocol ==== | ||
- | + | #Take competent cell in an eppendorf tube from -80℃ freezer put in ice. | |
+ | #Add 2ul plasmid to competent cell and place in ice for 5 minutes. | ||
+ | #Put the transformed cells into 42℃ water bath for 60 seconds. | ||
+ | #Then place the cells in ice for 2 minutes. | ||
+ | #Add 1ml LB to the cells and mixed. | ||
+ | #Put the eppendorf tube in 37℃ water bath and incubate for an hour. | ||
+ | #Spin down at 7000 rpm for 5 minutes and remove most of the supernatant. | ||
+ | #While the cells are incubated at 37℃ water bath spread 100ul Ampicilin(50mg/ml) on the plate. When the plate is dried, spread bacteria on the plate. | ||
+ | #Incubate at 37℃ incubater for 16~18 hours. | ||
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- | + | ==== PCR ==== | |
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- | + | 1. Dissolve the primers in water to have the concentration of 10nM. | |
- | |||
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- | |||
- | |||
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- | |||
- | |||
- | 5. | + | 2. PCR reaction mixer: |
+ | |||
+ | Template DNA(10ng/μl) 5 | ||
+ | 10× PCR buffer 2 | ||
+ | 10× dNTP(2mM) 2 | ||
+ | forward primer(10μM) 0.5 | ||
+ | reverse primer(10μM) 0.5 | ||
+ | Pfu DNA polymerase(2Kb) 0.1 | ||
+ | PCR water 9.9 | ||
+ | _______________________________________ | ||
+ | Total 20 μl | ||
- | :''' | + | |
+ | 3. Put the reaction mixer in a PCR tube. | ||
+ | |||
+ | 4.The PCR program is as follow : | ||
+ | :'''4.1''' | ||
:94℃ 30 seconds | :94℃ 30 seconds | ||
:60℃ 30seconds | :60℃ 30seconds | ||
Line 86: | Line 84: | ||
- | :''' | + | :'''4.2''' |
:94℃ 30 seconds | :94℃ 30 seconds | ||
:55℃ 30seconds | :55℃ 30seconds | ||
:72℃ 2 minutes | :72℃ 2 minutes | ||
:Cycle 34 times | :Cycle 34 times | ||
- | |||
+ | Extend PCR product at 72℃ for 10 minutes | ||
+ | |||
+ | |||
+ | 5. The PCR product was examed by electrophoresis in 1% agarose. | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ====T-A cloning==== | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | |||
+ | Take an eppendorf tube and add following component one by one and mix well,incubated at 4℃ overnight. | ||
+ | |||
+ | |||
+ | 2x ligase buffer 7.5μl | ||
+ | Insert(Aeq.-GFP) 5.5μl | ||
+ | Vector(pGEM-T-easy) 1μl | ||
+ | T4 DNA exp 3/12 1μl | ||
+ | _________________________________ | ||
+ | total 15μl | ||
+ | |||
+ | |||
+ | ====Colony PCR(To verify the presence of our gene of interest)==== | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | |||
+ | #Take 10μl of bacterial culture, spin down at 14000 rpm for 10 min. | ||
+ | #Discard the supernatant | ||
+ | #Add 500μl ddH20, Vortex | ||
+ | #Boil for 20 min. | ||
+ | #Take 5μl of above bacterial lysate, and add 10x dNTP 2μl, 10x Buffer 2μl, forward primer(10μM)0.5μl reverse primer(10μM)0.5μl, Taq DNA polymerase 0.1μl, ddH20 | ||
+ | #Use the PCR to amplify our product:PCR program | ||
+ | |||
+ | 95℃ 4 min | ||
+ | 94℃ 30seconds | ||
+ | 55℃ 40seconds | ||
+ | 72℃ 2 min | ||
+ | Cycle 34 times | ||
+ | 25℃ 2 min | ||
+ | 7. The PCR product was examed by electrophoresis in 1% agarose. | ||
+ | |||
+ | ====Plasmid extraction(Homemade)==== | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | |||
+ | #Transfer 1.5ml of bacterial culture to each well(24 wells plate) | ||
+ | #pellet cells by centrifuging at 33000 rpm for 10min at 4℃ | ||
+ | #carefully remove the supernatant | ||
+ | #add 100μl of Solution 1 (*)to each well, and vortex | ||
+ | #add 200μl of Solution 2 (*)to each well, and mix gently | ||
+ | #add 150μl of Solution 3 (*)to each well | ||
+ | #spin down 3000rpm at 4℃ for 10min | ||
+ | #add 1 ml 100% EtOH to new well | ||
+ | #Transfer the supernatant to the new well, containing 100% EtOH. | ||
+ | #spin down 3300rpm at 4℃ for 30min. | ||
+ | #carefully remove the supernatant. | ||
+ | #add 75% EtOH to wash pellets, then remove the supernantant, then air dry. | ||
+ | #add 40μl ddH2O to each well, to dissolve with plasmid DNA | ||
+ | #store the plate in 4℃ | ||
+ | (*)Sol 1: 10m Miris/0.5mM HEDTA, PH 7.4 buffer. | ||
+ | Sol 2: 0.2N NaOH/1% SDS | ||
+ | Sol 3: 3M KOAC/HOAC | ||
+ | |||
+ | ====Digestion==== | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | Digestion mixture | ||
+ | |||
+ | DNA 20μl | ||
+ | 10x buffer 3μl | ||
+ | Enzyme 1μl | ||
+ | RNase H2O 6μl | ||
+ | __________________________ | ||
+ | Total 30μl | ||
+ | 3. The order for adding materials to wells is from plenty to less | ||
+ | 4. Place the plate in 37℃water bath overnight | ||
+ | |||
+ | |||
+ | |||
+ | ====Ligation==== | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | |||
+ | Take an eppendorf tube and add following component one by one and mix well,incubated at 16℃ overnight. | ||
- | |||
- | 7. | + | Insert(Aeq.-GFP) 7.5μl |
+ | Vector(pSB1A3) 5.5μl | ||
+ | 10X ligase buffer 1μl | ||
+ | T4 DNA ligase 1μl | ||
+ | _________________________________ | ||
+ | total 30μl |
Latest revision as of 01:01, 22 October 2009
Contents |
Protocol
A. Culture CP919
B. Put Aqueorin-GFP into plasmid .
C. Transform the cp919 into the Midnight Apollo!
D. Sense the light.
E. In the dark, the Midnight Apollo! is activated and emit the light.
Competent Cell (CP919-Cph8)
- Day1. Streak out the E.coli strain on an LB plate (with kanamycin)and incubate at 37℃ overnight (16-20 hours).
- Day2. Select a single colony and inoculate 10 ml sterile LB and grow overnight (16-20 hours) in a 37℃ shaker incubator.
- Day3. Add 2ml overnight culture to 250ml flask containing 100 ml LB.
- Grow the cultures to OD600 = 0.2~0.4 (incubate with shaking for 75~90 min.)
- Spin down the bacteria at 4℃,3000 rpm for 10 min.
- Discard the supernatant and mix the cell pellet with 10ml FSB.
- Keep the cells on ice for 3~4 hours.
- Spin down, at 4℃,3000 rpm for 10 min.
- Discard the supernatant and mix the cell pellet with 5ml FSB.
- Pipet 200μl of the cell suspension into sterile 1.5ml eppendorf tubes. Freeze these tubes in liquid nitrogen, then transfer them to -80℃ freezer.
Tansformation Protocol
- Take competent cell in an eppendorf tube from -80℃ freezer put in ice.
- Add 2ul plasmid to competent cell and place in ice for 5 minutes.
- Put the transformed cells into 42℃ water bath for 60 seconds.
- Then place the cells in ice for 2 minutes.
- Add 1ml LB to the cells and mixed.
- Put the eppendorf tube in 37℃ water bath and incubate for an hour.
- Spin down at 7000 rpm for 5 minutes and remove most of the supernatant.
- While the cells are incubated at 37℃ water bath spread 100ul Ampicilin(50mg/ml) on the plate. When the plate is dried, spread bacteria on the plate.
- Incubate at 37℃ incubater for 16~18 hours.
PCR
1. Dissolve the primers in water to have the concentration of 10nM.
2. PCR reaction mixer:
Template DNA(10ng/μl) 5 10× PCR buffer 2 10× dNTP(2mM) 2 forward primer(10μM) 0.5 reverse primer(10μM) 0.5 Pfu DNA polymerase(2Kb) 0.1 PCR water 9.9 _______________________________________ Total 20 μl
3. Put the reaction mixer in a PCR tube.
4.The PCR program is as follow :
- 4.1
- 94℃ 30 seconds
- 60℃ 30seconds
- 72℃ 2 minutes
- Cycle 9 times
- 4.2
- 94℃ 30 seconds
- 55℃ 30seconds
- 72℃ 2 minutes
- Cycle 34 times
Extend PCR product at 72℃ for 10 minutes
5. The PCR product was examed by electrophoresis in 1% agarose.
T-A cloning
Take an eppendorf tube and add following component one by one and mix well,incubated at 4℃ overnight.
2x ligase buffer 7.5μl Insert(Aeq.-GFP) 5.5μl Vector(pGEM-T-easy) 1μl T4 DNA exp 3/12 1μl _________________________________ total 15μl
Colony PCR(To verify the presence of our gene of interest)
- Take 10μl of bacterial culture, spin down at 14000 rpm for 10 min.
- Discard the supernatant
- Add 500μl ddH20, Vortex
- Boil for 20 min.
- Take 5μl of above bacterial lysate, and add 10x dNTP 2μl, 10x Buffer 2μl, forward primer(10μM)0.5μl reverse primer(10μM)0.5μl, Taq DNA polymerase 0.1μl, ddH20
- Use the PCR to amplify our product:PCR program
95℃ 4 min 94℃ 30seconds 55℃ 40seconds 72℃ 2 min Cycle 34 times 25℃ 2 min
7. The PCR product was examed by electrophoresis in 1% agarose.
Plasmid extraction(Homemade)
- Transfer 1.5ml of bacterial culture to each well(24 wells plate)
- pellet cells by centrifuging at 33000 rpm for 10min at 4℃
- carefully remove the supernatant
- add 100μl of Solution 1 (*)to each well, and vortex
- add 200μl of Solution 2 (*)to each well, and mix gently
- add 150μl of Solution 3 (*)to each well
- spin down 3000rpm at 4℃ for 10min
- add 1 ml 100% EtOH to new well
- Transfer the supernatant to the new well, containing 100% EtOH.
- spin down 3300rpm at 4℃ for 30min.
- carefully remove the supernatant.
- add 75% EtOH to wash pellets, then remove the supernantant, then air dry.
- add 40μl ddH2O to each well, to dissolve with plasmid DNA
- store the plate in 4℃
(*)Sol 1: 10m Miris/0.5mM HEDTA, PH 7.4 buffer. Sol 2: 0.2N NaOH/1% SDS Sol 3: 3M KOAC/HOAC
Digestion
Digestion mixture
DNA 20μl 10x buffer 3μl Enzyme 1μl RNase H2O 6μl __________________________ Total 30μl
3. The order for adding materials to wells is from plenty to less 4. Place the plate in 37℃water bath overnight
Ligation
Take an eppendorf tube and add following component one by one and mix well,incubated at 16℃ overnight.
Insert(Aeq.-GFP) 7.5μl Vector(pSB1A3) 5.5μl 10X ligase buffer 1μl T4 DNA ligase 1μl _________________________________ total 30μl