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-<div id="tokyotech" style=" font:bold ;left ; font-size: 30px; color: #1E90FF; padding: 10px;">
-Assays for Positive feedback system  </div>
-</div class="whitebox">
-{{tokyotechmenubar}}
-<div class="whitebox">
-<div id="tokyotech" style=" font:Arial ;left ; font-size: 15px; color: #000000; padding: 30px;">
-__NOTOC__
-=Materials & Methods=
-==1.Construction==
-[[https://2012.igem.org/Team:Tokyo_Tech/Project#Assays_for_Positive_feedback_system Back to "feedback system"]]
-<div id="tokyotech" style=" font:bold ;left ; font-size: 20px; color: #1E90FF; padding: 10px;">
-A) Sender cells </div>
-pSB6A1-Ptet-LuxR / pSB3K3-Plux-LasI (JM2.300)…Plux-LasI cell
-[[File:positivefeedbackassay13tokyotech.png|300px|center]]
-pSB6A1-Ptrc-LasR / pSB3K3-Plas-LuxI (JM2.300)…Plas-LuxI cell
-[[File:positivefeedbackassay14tokyotech.png|300px|center|]]
-pSB6A1-Ptet-LuxR / pSB3K3-ΔP-LasI (JM2.300)…ΔP-LasI cell
-[[File:positivefeedbackassay5tokyotech.png|300px|center|]]
-pSB6A1-Ptrc-LasR / pSB3K3-ΔP-LuxI (JM2.300)…ΔP-LuxI cell
-[[File:positivefeedbackassay6tokyotech.png|300px|center]]
-<br><br><br><br><br><br>
-<div id="tokyotech" style=" font:bold ;left ; font-size: 20px; color: #1E90FF; padding: 10px;">
-B) Reporter cells </div>
-pSB6A1-Ptrc-LasR / pSB3K3-Plas-GFP (JM2.300)…Las reporter cell
-[[File:positivefeedbackassay7tokyotech.png|300px|center]]
-pSB6A1-Ptet-LuxR / pSB3K3-Plux-GFP (JM2.300)…Lux reporter cell
-[[File:positivefeedbackassay8tokyotech.png|300px|center]]
-pSB6A1-Ptrc-LasR / pSB3K3-ΔP-GFP (JM2.300)…negative control
-[[File:positivefeedbackassay9tokyotech.png|300px|center]]
-pSB6A1-Ptrc-LasR / pSB3K3-pλ-GFP (JM2.300)…positive control
-[[File:positivefeedbackassay10tokyotech.png|300px|center]]
-pSB6A1-Ptet-LuxR / pSB3K3-ΔP-GFP (JM2.300)…negative control
-[[File:positivefeedbackassay11tokyotech.png|300px|center]]
-pSB6A1-Ptet-LuxR / pSB3K3-pλ-GFP (JM2.300)…positive control
-[[File:positivefeedbackassay12tokyotech.png|300px|center]]
-==3.Protocol==
-===3OC6HSL-dependent 3OC12HSL production module===
-[[https://2012.igem.org/Team:Tokyo_Tech/Project#Construction_of_the_3OC6HSL-dependent_3OC12HSL_production_module Back to "Construction of the 3OC6HSL-dependent 3OC12HSL production module"]]
-. collect liquid culture
-<div id="tokyotechprotocol" style=" font:bold ;left ; font-size: 13px; color: #000000; padding: 10px;">
-.1 Prepare overnight culture of inducer cell at 37°C for 12hours.
-.2 Take 30μl of the overnight culture of inducer cell into LB(3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml).(→fresh culture)
-.3 Incubate the flesh culture of inducer cell until the observed OD600 reaches around 0.50. Centrifuge the cell at 5000g, 25°C, 1 min, suspend it with 1ml LB + antibiotics (Amp 50μg/ml).
-.4 Take 30μl cell suspensions into LB(3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml) + 5μM 3OC6HSL(3μl) and LB(3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml) + DMSO(3μl).
-.5 Incubate the 3OC12HSL producer cells for another 4 hours at 37°C.
-.6 Centrifuge the 3OC12HSL producer cells at 9000g, 4°C, 1 min, and filter the cultured cells.
-.7 Dilute the filtrate by LB + antibiotics (Amp + Kan) in 1:30.
-</div>
-Reporter assay
-<div id="tokyotechprotocol" style=" font:bold ;left ; font-size: 13px; color: #000000; padding: 10px;">
-.1 Prepare overnight culture of reporter cell at 37°C for 12hours.
-.2 Take 30μl of the overnight culture of reporter cell into LB(3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml). (→fresh culture)
-.3 Incubate the flesh culture of reporter cell until the observed OD600 reaches around 0.50, and gather the supernatant of culture of inducer cell.
-.4 Centrifuge the reporter cell at 5000g, 25°C, 1 min, and take it into LB + antibiotics (Amp 50μg/ml + Kan 30μg/ml).
-.5 Add 30μl samples of process 2.4 to filtrate + LB(3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml) from process 1.7
-{| class="wikitable" cellpadding="2"
-| align="center" style="background:#f0f0f0;"|'''3OC6HSL'''
-| align="center" style="background:#f0f0f0;"|'''Plux'''
-|-
-| +||+
-|-
-| -||+
-|-
-| +|| -
-|-
-| -|| -
-|}
-.6	Incubate the reporter cells for 4 hours at 37°C.
-.7	Flow cytometer measurements for GFP expression of reporter cells.
-</div>
-[[https://2012.igem.org/Team:Tokyo_Tech/Project#Construction_of_the_3OC6HSL-dependent_3OC12HSL_production_module Back to "Construction of the 3OC6HSL-dependent 3OC12HSL production module"]]
-===3OC12HSL-dependent 3OC6HSL production module===
-[[https://2012.igem.org/Team:Tokyo_Tech/Project#Construction_of_the_3OC12HSL-dependent_3OC6HSL_production_module Back to "Construction of the 3OC12HSL-dependent 3OC6HSL production module"]]
-. collect liquid culture
-<div id="tokyotechprotocol" style=" font:bold ;left ; font-size: 13px; color: #000000; padding: 10px;">
-.1 Prepare overnight culture of inducer cell at 37°C for 12hours.
-.2 Take 30μl of the overnight culture of inducer cell into LB(3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml).(→fresh culture)
-.3 Incubate the flesh culture of inducer cell until the observed OD600 reaches around 0.50. Centrifuge the cell at 5000g, 25°C, 1 min, suspend it with 1ml LB + antibiotics (Amp 50μg/ml).
-.4 Take 30μl cell suspensions into LB(3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml) + 5μM 3OC6HSL(3μl) and LB(3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml) + DMSO(3μl).
-.5 Incubate the 3OC12HSL producer cells for another 4 hours at 37°C.
-.6 Centrifuge the 3OC12HSL producer cells at 9000g, 4°C, 1 min, and filter the cultured cells.
-.7 Dilute the filtrate by LB + antibiotics (Amp + Kan) in 1:30.
-</div>
-Reporter assay
-<div id="tokyotechprotocol" style=" font:bold ;left ; font-size: 13px; color: #000000; padding: 10px;">
-.1 Prepare overnight culture of reporter cell at 37°C for 12hours.
-.2 Take 30μl of the overnight culture of reporter cell into LB(3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml). (→fresh culture)
-.3 Incubate the flesh culture of reporter cell until the observed OD600 reaches around 0.50, and gather the supernatant of culture of inducer cell.
-.4 Centrifuge the reporter cell at 5000g, 25°C, 1 min, and take it into LB + antibiotics (Amp 50μg/ml + Kan 30μg/ml).
-.5 Add 30μl samples of process 2.4 to filtrate + LB(3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml) from process 1.7
-{| class="wikitable" cellpadding="2"
-| align="center" style="background:#f0f0f0;"|'''3OC12HSL'''
-| align="center" style="background:#f0f0f0;"|'''Plas'''
-|-
-| +||+
-|-
-| -||+
-|-
-| +|| -
-|-
-| -|| -
-|}
-.6 Induction of reporter cell for 4 hours at 37°C.
-.7 Flow cytometer measurements for GFP expression of reporter cell.
-</div>
-[[https://2012.igem.org/Team:Tokyo_Tech/Project#Construction_of_the_3OC12HSL-dependent_3OC6HSL_production_module Back to "Construction of the 3OC12HSL-dependent 3OC6HSL production module"]]
-===positive feedback assay===
-[[https://2012.igem.org/Team:Tokyo_Tech/Project#Construction_of_the_positive_feedback_system Back to "Construction of the positive feedback system"]]
-. collect liquid culture
-<div id="tokyotechprotocol" style=" font:bold ;left ; font-size: 13px; color: #000000; padding: 10px;">
-.1	Prepare overnight culture of inducer cells at 37°C for 12hours.
-.2	Take 30μl of the overnight culture of inducer cells into LB (3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml). (→fresh culture)
-.3	Incubate the flesh culture of inducer cells until the observed OD600 reaches around 0.50. Centrifuge the cells at 5000g, 25°C, 1 min, suspend it with 1ml LB + antibiotics (Amp 50μg/ml + Kan 30μg/ml).
-.4	According to the Fig.3-1-3-1-1, take 30μl cell suspensions into LB(3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml) + 3OC6HSL (5nM) or OC6HSL(2.5nM)
-[[File:positivefeedbackassay27tokyotech.png|500px|thumb|center|Fig.3-1-3-1-1]]
-.5 Incubate the inducer cell for another 4 hours at 37°C.
-.6 Centrifuge the inducer cell at 9000g, 4°C, 1 min, and filter the cultured cell.
-.7 Dilute the filtrate by LB + antibiotics (Amp 50μg/ml + Kan 30μg/ml) in 1:30.
-</div>
-Reporter assay
-<div id="tokyotechprotocol" style=" font:bold ;left ; font-size: 13px; color: #000000; padding: 10px;">
-.1	Prepare overnight culture of reporter cells at 37°C for 12hours.
-.2	Take 30μl of the overnight culture of reporter cells into LB (3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml). (→fresh culture)
-.3	Incubate the flesh culture of reporter cells until the observed OD600 reaches around 0.50, and gather the supernatant of culture of inducer cells.
-.4	Centrifuge the reporter cells at 5000g, 25°C, 1 min, and take it into LB + antibiotics (Amp 50μg/ml + Kan 30μg/ml).
-.5	Add 30μl samples of process 2.4 to filtrate + LB (3ml) + antibiotics (Amp 50μg/ml + Kan 30μg/ml) from process 1.7
-.6	Incubate the reporter cells for 4 hours at 37°C.
-.7	Flow cytometer measurements for GFP expression of reporter cells.
-</div>
-[[https://2012.igem.org/Team:Tokyo_Tech/Project#Construction_of_the_positive_feedback_system Back to "Construction of the positive feedback system"]]

Team:Tokyo Tech/Projects/positive feedback assay/index.htm

From 2012.igem.org

Latest revision as of 17:29, 26 October 2012