Team:Chiba/Calendar-Home/18 October 2008
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(New page: 朝senderをwashして菌液10mlとLB-agar10mlを混ぜて固まらないうちにプレートに流し込む。 receiverをニトロセルロースで写し取り、senderのプレー...) |
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- | + | >[[Team:Chiba|Home]] | [[Team:Chiba/Notebook|Notebook]] | |
+ | [[Team:Chiba/Calendar-Home/17 October 2008|17 October 2008 <]]|[[Team:Chiba/Calendar-Home/19 October 2008|> 19 October 2008]] | ||
- | + | ==Laboratory work== | |
+ | ===Team:Demo-Rs=== | ||
+ | 17 October~ | ||
+ | #Sender Wash | ||
+ | ##Centrifuged 2 tubes containing([http://partsregistry.org/Part:BBa_T9002 BBa_T9002](JW1908))at 20°C,3600rpm for 6min and discarded supernatant. | ||
+ | ##Added 10mL LB-Amp to each tube. | ||
+ | ##Repeated wash twice. | ||
+ | #Creating bacterial plates | ||
+ | ##LB-Amp pre-cultured Sender([http://partsregistry.org/Part:BBa_S03623 BBa_S03623](JW1908)) tube 1 (10mL) was mixed with LB-Amp-agar(50°C)(10ml)to produce sender containing bacterialplate-1. | ||
+ | #Lifted with nitrocellulose | ||
+ | ##Receiver([http://partsregistry.org/Part:BBa_T9002 BBa_T9002](JW1908))colony was transfered to a nitrocellulose filter and placed on each of Sender([http://partsregistry.org/Part:BBa_S03623 BBa_S03623](JW1908))containing bacterial plate (1~3) and Sender-absent negative control plate (t=0). Determined the time required for the colonies to fluoresce depending on the bacterial concentration (100 and 1000-fold dilution). | ||
+ | #Method to detect fluorescence | ||
+ | ##Plates cultured at 37°C were exposed to UV (312nm) light once every 30 minutes to observe GFP fluorescence. | ||
+ | |||
+ | ==results== | ||
+ | [[Image:Team-Chiba-P1000911.JPG|150px]] | ||
+ | [[Image:Team-Chiba-P1000915.JPG|150px]] | ||
+ | [[Image:Team-Chiba-P1000923.JPG|145px]] | ||
+ | [[Image:Team-Chiba-P1000931.JPG|143px]] | ||
+ | [[Image:Team-Chiba-P1000936.JPG|140px]] | ||
+ | 0h 0.5h 1.0h 1.5h 2.0h |
Latest revision as of 00:40, 30 October 2008
17 October 2008 <|> 19 October 2008
Laboratory work
Team:Demo-Rs
17 October~
- Sender Wash
- Centrifuged 2 tubes containing([http://partsregistry.org/Part:BBa_T9002 BBa_T9002](JW1908))at 20°C,3600rpm for 6min and discarded supernatant.
- Added 10mL LB-Amp to each tube.
- Repeated wash twice.
- Creating bacterial plates
- LB-Amp pre-cultured Sender([http://partsregistry.org/Part:BBa_S03623 BBa_S03623](JW1908)) tube 1 (10mL) was mixed with LB-Amp-agar(50°C)(10ml)to produce sender containing bacterialplate-1.
- Lifted with nitrocellulose
- Receiver([http://partsregistry.org/Part:BBa_T9002 BBa_T9002](JW1908))colony was transfered to a nitrocellulose filter and placed on each of Sender([http://partsregistry.org/Part:BBa_S03623 BBa_S03623](JW1908))containing bacterial plate (1~3) and Sender-absent negative control plate (t=0). Determined the time required for the colonies to fluoresce depending on the bacterial concentration (100 and 1000-fold dilution).
- Method to detect fluorescence
- Plates cultured at 37°C were exposed to UV (312nm) light once every 30 minutes to observe GFP fluorescence.
results
0h 0.5h 1.0h 1.5h 2.0h