IGEM:IMPERIAL/2007/Projects/Hrp System/Systems/Hrp Device 1/TestingValidation/Protocolplux

Promoter pLux Protocol
For the followling protcol is for preparation of a culture and one set of 8 inducer concentration ranges. We wish to carry out 4 repeats of concentration and so carry out this protocol x4 in parrelel.

Protocol
Preparing the Over night Cultures Day 1 volume culture = (0.1/ O.D.600 )*10ml
 * Inoculate 5ml of M9 minimal media containing 50 μg/mL Ampicillin with 10μl of stored culture containing pLac test construct.
 * Incubate at 37°C for overnight in a shaker.
 * Allows selected growth of E.coli with vector
 * Incubate M9 Amp Media 37o
 * Remove the overnight culture from incubator and measure Optical Density at 600nm (O.D.600) of a 4ml sample.  Click here for technique on spectrometer.
 * Calculate the volume of culture needed to give a O.D.600 in a 10ml volume, use simple calculate:
 * With the calculated volume of culture add pre-warmed M9 media to make total volume of 10ml
 * Return the 10ml culture to the incubator and incubate at 37oC for 2 hours.
 * The purpose of inoculating a new media is because over night E.coli will go into the stationary phase, but by inoculating a new medium we are returned cells to the exponential phase
 * Whilst the cultures are incubating prepare the standard dilutions of IPTG.(PROCESS)

2 hours Incubation volume culture = (0.1/ O.D.600 )*15ml
 * Remove culture and measure O.D.600.
 * Calculate the volume of culture needed to give a O.D.600 in a 15ml volume, use simple calculate:
 * With the calculated volume of culture add pre-warmed M9 media to make total volume of 15ml
 * Spin the 15ml culture in a centrifuge for 10 mins at 300 to 2000g minutes(check). Cells will form a pellet in the bottom of the tube.
 * Carefully remove the liquid in the tube (supernatant) to leave just the pellet.
 * Re-suspend the cells in 15ml of prewarmed M9 Amp and gentle vortex.
 * This is to supply fresh media, ensures the cultures remain in the exponential phase

Fluorometer Plate Reader
 * Retrieve the Plate
 * Remove 200μL of the culture from the 15ml into 10 wells.
 * Pipette samples into a 96 well plate
 * Add 2μL of pre-prepared AHL solutions to relevant well (Follow schematic)
 * In addition want the following control wells:
 * 1) 200μl of growth medium.
 * 2) Cultures without vector.
 * 3) A 200μL culture with 2μL of 0.2M AHL (Just need a high concentration to saturate promoter)
 * Place into the fluorometer and set time intervals to relevant settings to give 50 time points.

Results

 * Each concentration of inducer has four repeats each of which is composed of 50 time interval measurements.