Team:Tokyo Tech/Projects/Lux-Tet hybrid promoter/index.htm

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(Materials & Method)
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Lux-Tet hybrid promoter assay </div>
 
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__NOTOC__
 
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=Materials & Method=
 
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[[https://2012.igem.org/Team:Tokyo_Tech/Project#Band_detect_system Back to "Lux-Tet hybrid promoter assay"]]
 
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i. Materials & Methods
 
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1. Construction
 
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To characterize Plux/tet hybrid promoter (BBa_K934024), we constructed Plux/tet-GFP (BBa_K934025) by ligating the Plux/tet hybrid promoter (BBa_K934024) to the upstream of promoterless GFP generator (BBa_I13504).
 
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pSB3K3-PlacIq-LuxR-Ptrc-TetR / pSB6A1-Pluxtet-GFP (JM2.300)…Sample 
 
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pSB3K3-PlacIq-LuxR-Ptrc-TetR / pSB6A1-⊿P-GFP (JM2.300)…negative control
 
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pSB3K3-PlacIq-LuxR-Ptrc-TetR / pSB6A1-Plac-GFP (JM2.300)…positive control
 
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2. Strain
 
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JM2.300
 
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3. Protocol
 
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1.1 Prepare overnight culture of reporter cell at 37 ℃ for 12hours.
 
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1.2 Take 30 μl of the overnight culture of reporter cells into LB (3 ml) + antibiotics (Amp 50 μg/ml + Kan 30 μg/ml). (→fresh culture)
 
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1.3 Dilute the flesh culture in 1:50 by the following conditions:
 
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A) LB
 
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B) LB + aTc (500 ng/ ml)
 
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C) LB + 3OC6HSL (1 μM )
 
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D) LB + aTc (500 ng/ml) + 3OC6HSL (1 μM )
 
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1.4 Incubate the fresh culture of diluted inducer cell for 2 hours.
 
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1.5 Flow cytometer measurements for GFP expression of reporter cell.
 

Latest revision as of 00:04, 27 October 2012

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