Team:Tokyo Metropolitan/Notebook/Fiber/2010/08/17
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==2010/8/17 Tuesday (watachin)== | ==2010/8/17 Tuesday (watachin)== | ||
- | ===Experiment: | + | ===Experiment:Electrophoresis=== |
- | '''Member''' | + | :'''Member''' |
- | NEX and watachin | + | :NEX and watachin |
- | ''' | + | :'''Material''' |
- | *pSB1A3(25ng/μl) 22μl | + | :*pSB1A3(25ng/μl) 22μl |
- | * | + | :*10×Loading buffer 2.2μl |
- | *DNA Marker 5μl | + | :*DNA Marker 5μl |
- | * | + | :*1×TAE buffer |
- | *1% agarose gel | + | :*1% agarose gel |
- | '''Procedure''' | + | :'''Procedure''' |
- | #Set agarose gel and add TAE buffer in electrophoresis tank. | + | :#Set agarose gel and add TAE buffer in electrophoresis tank. |
- | #Mix Loading Buffer and pSB1C3 ,then put them in well (marker sets another well). | + | :#Mix Loading Buffer and pSB1C3 ,then put them in well (marker sets another well). |
- | #Load DNA at 100V for two thirds of total volume (about 15 minutes). | + | :#Load DNA at 100V for two thirds of total volume (about 15 minutes). |
- | #Image the consequence of electrophoresis. | + | :#Image the consequence of electrophoresis. |
- | '''Result''' | + | :'''Result''' |
[[Image:2010-08-17-ef.jpg]] | [[Image:2010-08-17-ef.jpg]] | ||
- | failure | + | :failure |
- | Plasmid concentration was too low. | + | :Plasmid concentration was too low. |
===Experiment:Transformation of pSB1A3=== | ===Experiment:Transformation of pSB1A3=== | ||
- | '''Member''' | + | :'''Member''' |
- | NEX and watachin | + | :NEX and watachin |
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
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+ | :'''Material''' | ||
+ | :*pSB1A3 1μl | ||
+ | :*competent cell (DH5α) 50μl | ||
+ | :*LB + amp plate | ||
+ | :'''Procedure''' | ||
+ | :#mix pSB1A3 and DH5α | ||
+ | :#on ice (30min) | ||
+ | :#heat shock 42℃ (45sec) | ||
+ | :#on ice (2min) | ||
+ | :#inoculate onto plate | ||
+ | :#incubate cells at 37℃ | ||
<br/> | <br/> |
Latest revision as of 21:38, 26 October 2010
E.coli Fiber Project Notebook
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2010/8/17 Tuesday (watachin)
Experiment:Electrophoresis
- Member
- NEX and watachin
- Material
- pSB1A3(25ng/μl) 22μl
- 10×Loading buffer 2.2μl
- DNA Marker 5μl
- 1×TAE buffer
- 1% agarose gel
- Procedure
- Set agarose gel and add TAE buffer in electrophoresis tank.
- Mix Loading Buffer and pSB1C3 ,then put them in well (marker sets another well).
- Load DNA at 100V for two thirds of total volume (about 15 minutes).
- Image the consequence of electrophoresis.
- Result
- failure
- Plasmid concentration was too low.
Experiment:Transformation of pSB1A3
- Member
- NEX and watachin
- Material
- pSB1A3 1μl
- competent cell (DH5α) 50μl
- LB + amp plate
- Procedure
- mix pSB1A3 and DH5α
- on ice (30min)
- heat shock 42℃ (45sec)
- on ice (2min)
- inoculate onto plate
- incubate cells at 37℃