IGEM:IMPERIAL/2007/Experimental Design/Phase1/Protocol 1.2: Difference between revisions

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===Day 1===
===Day 1===
====Equipment====
====Equipment====
*Sterile conical flasks x4
*7ml tubes x4
*Incubator 30<sup>o</sup>C
*Incubator 37<sup>o</sup>C
*Fluorometer
*Gilson Pipettes
====Reagents====
*''E.coli'' DH5&alpha; culture containing parts
*LB medium
*Ampicillin stock (50 mg/ml)
*GFP Standard Solution
*AHL stock
<br>
 
'''Innoculation of Media'''
*Inoculate 10ul of stored parts in individual 2ml LB medium containing 2ul of ampicillin
*Incubate at 37°C for overnight in a shaker. '''(This is to get a good stock of cells for use in the experiment. After the overnight culture the cells will be in stationary phase)'''
 
 
===Day 2===
====Equipment====
*Spectrophotometer
*Stripettes
*Well-plate x1
*Well-plate x1
*Plate Centrifuge
*Plate Centrifuge
*4x1.5ml eppendorf tubes
 
*Gilson Pipettes
*Stripettes
*Stop watch
*Stop watch
*
====Reagents====
====Reagents====
*''E.coli'' DH5&alpha; culture containing parts
*LB medium
*LB medium
*Ampicillin stock (50 mg/ml)
*Ampicillin stock (50 mg/ml)
*GFP Standard Solution
*AHL stock
*AHL stock
<br>


'''Innoculation of Media (cont'd)'''
*In the morning, prewarm 20 mL LB Amp medium in the 37°C water bath.
*Measure and record OD600
*Inoculate a 10ml fresh culture from the o/n to bring back the OD600 to 0.1, use the prewarmed LB + Ampicilin in waterbath. '''(Using prewarmed LB prevents a temperature shock to the culture, which would increase lag time)'''


<center><amsmath>
\frac{0.1}{\mbox{OD of culture}} \times \mbox{10 mL}
</amsmath></center>
:OD of XXX culture (1st Measurement):  _________
:Amount to dilute of XXX culture = ________ mL (amount of original culture to use)
:Amount of prewarmed LB with Ampicillin to use = ________ mL (16 mL - above result)
<br>
*Return LB to 37°C waterbath. '''(This returns cells to exponential phase from stationary phase)'''
*Incubate new culture at 37°C
<br>
<br>


'''Preparation of Media'''
 
*Make 3 x 50ml LB medium with 100µl ampicillin and 1 x 100ml LB medium with 100µl ampicillin into sterile concical flasks.
*Warm to 30<sup>o</sup>C.


<br>
<br>
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<br>
<br>


*Vortex new T9002/J37016/J37020 culture.
*To start AHL incubation:
**Label each tube with AHL concentration
**Put 20ul of the AHL into 11 seperate 5ml white capped tubes
**Add appropriate amount of T9002 samples as per the table below
**Record time of inoculation in report sheet.
**Vortex each tube
<showhide>
:*Incubate all 5mL tubes in a 37°C shaker for 4 hours so GFP expression can reach steady state __HIDER__
<hide>
::<font color=green>Do not pipette the samples into the 96 well plate yet - because if the 96 well plate is put in the shaker, cross-contamination between the well is very likely to happen. </font color>
</hide></showhide>
<br>




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#Place lid back on and place back in the incubator at 30<sup>o</sup>C
#Place lid back on and place back in the incubator at 30<sup>o</sup>C
<br>
<br>




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|
|
{| border="1" cellpadding="2"
{| border="1" cellpadding="2"
!<u>Well </u> || <u>Test Construct</u> !! <u>In vitro chassis</u>
!<u>Well </u> || <u>Test Construct</u> || <u>Stock Concentration</u> !! <u>AHL (ul)</u> !! <u>Final AHL Concentration</u>
|-
|-
|<font color=blue> A1  
|<font color=blue> A1  

Revision as of 08:34, 14 August 2007


Protocol

Day 1

Equipment

  • 7ml tubes x4
  • Incubator 37oC
  • Gilson Pipettes

Reagents

  • E.coli DH5α culture containing parts
  • LB medium
  • Ampicillin stock (50 mg/ml)
  • GFP Standard Solution
  • AHL stock


Innoculation of Media

  • Inoculate 10ul of stored parts in individual 2ml LB medium containing 2ul of ampicillin
  • Incubate at 37°C for overnight in a shaker. (This is to get a good stock of cells for use in the experiment. After the overnight culture the cells will be in stationary phase)


Day 2

Equipment

  • Spectrophotometer
  • Stripettes
  • Well-plate x1
  • Plate Centrifuge
  • Stop watch

Reagents

  • LB medium
  • Ampicillin stock (50 mg/ml)
  • GFP Standard Solution
  • AHL stock


Innoculation of Media (cont'd)

  • In the morning, prewarm 20 mL LB Amp medium in the 37°C water bath.
  • Measure and record OD600
  • Inoculate a 10ml fresh culture from the o/n to bring back the OD600 to 0.1, use the prewarmed LB + Ampicilin in waterbath. (Using prewarmed LB prevents a temperature shock to the culture, which would increase lag time)


<amsmath>

\frac{0.1}{\mbox{OD of culture}} \times \mbox{10 mL}

</amsmath>
OD of XXX culture (1st Measurement): _________
Amount to dilute of XXX culture = ________ mL (amount of original culture to use)
Amount of prewarmed LB with Ampicillin to use = ________ mL (16 mL - above result)


  • Return LB to 37°C waterbath. (This returns cells to exponential phase from stationary phase)
  • Incubate new culture at 37°C




Preparation of diluted series of AHL

  • Dilution series of AHL [1000 μM, 100 μM, 10 μM, 5 μM]



  • Vortex new T9002/J37016/J37020 culture.
  • To start AHL incubation:
    • Label each tube with AHL concentration
    • Put 20ul of the AHL into 11 seperate 5ml white capped tubes
    • Add appropriate amount of T9002 samples as per the table below
    • Record time of inoculation in report sheet.
    • Vortex each tube

<showhide>

  • Incubate all 5mL tubes in a 37°C shaker for 4 hours so GFP expression can reach steady state __HIDER__

<hide>

Do not pipette the samples into the 96 well plate yet - because if the 96 well plate is put in the shaker, cross-contamination between the well is very likely to happen.

</hide></showhide>


Loading Plate

  1. Follow the schematic for the plate adding everything but the DNA sample.
  2. Place the top on the plate and place in the incubator. Leave for a few minutes to heat to 30oC
  3. Remove from incubator and centrifuge for 1 minute
  4. Remove lid and Measure in the flourometer.
  5. Then to begin the reaction add .... purified DNA sample.
  6. Place lid back on and place back in the incubator at 30oC






Schematic

Well Test Construct Stock Concentration AHL (ul) Final AHL Concentration
A1 pTet Commercial E.coli extract
A2 pTet Commercial E.coli extract
A3 pTet Commercial E.coli extract
A4 pTet Our S30 Cell extract
A5 pTet Our S30 Cell extract
A6 pTet Our S30 Cell extract
A7 None Commercial E.coli extract
A8 None Our S30 Cell extract
B1 pT7 Commercial T7 extract
B2 pT7 Commercial T7 extract
B3 pT7 Commercial T7 extract
B4 pT7 Our S30 Cell extract
B5 pT7 Our S30 Cell extract
B6 pT7 Our S30 Cell extract
B7 None Commercial T7 extract
B8 None Our S30 Cell extract

T9002 96 well plate






Equipment

  • Incubator 30oC
  • Fluorometer
  • Spectrometer
  • Plate x1
  • Plate Centrifuge
  • 6x1.5ml tubes
  • Gilson Pipettes
  • Stop watch

Day 3:

Make 5 of 550 ml LB medium with 550 µl ampicillin in sterile conical flask Innoculate in 5 cultures into the the conical flasks Leave overnight at 37°C with shaking

Day 4:

Prepare a water bath at 30°C [should we use a shaking incubator?] Aliquot the 550 ml cultures into sterile tubes, 25 ml per tube Add 53.3075 ng AHL each time to increase [AHL] in steps of 10nM Begin the timer when AHL is added At 5 minute intervals for the first 40 minutes, and 10 minute intervals thereafter: Sample a 1 ml of the reaction mixture Immediately chill in ice (to slow the rate of reaction) Centrifuge at maximum speed for 30 seconds to pellet the cells Remove the supernatant and resuspend the pellet in 1ml distilled water Put in a spectrometer and excite it at 501nm and detect at 511nm [Note: Use solution at 0 minutes as a blank, assume no fluorescence is present prior to activation] These measurements should be repeated with the other 4 cultures of bacteria

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