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<h5>Methods</h5> | <h5>Methods</h5> | ||
<ol> | <ol> | ||
− | <li>Locate the devices listed above in the distribution kit and resuspend them in 10uL of dH20</ | + | <li>Locate the devices listed above in the distribution kit and resuspend them in 10uL of dH20</li> |
− | < | + | <li>Transform each device into 50uL of competent cells</li> |
− | < | + | <li>Plate the transformations onto LB plates with chloramphenicol and incubate overnight at 37C</li> |
</ol> | </ol> | ||
Revision as of 18:55, 12 October 2017
InterLab Study
Overview
Directly comparing measurements is a challenge for many synthetic biology researchers. Fluorescent measurement is difficult for researchers to compare because it can be analyzed and reported in a variety of ways. Through the InterLab 2017 study, the iGEM Measurement Committee seeks to provide researchers with a standard for measuring expression of GFP in a plate reader.
iGEM Teams worldwide contributed to the InterLab study by transforming DH5a E. coli with six test devices (BBa_J364000, BBa_J364001, BBa_J364002, BBa_J364003, BBa_J364004, and BBa_J364005), as well as a positive (BBa_I20270), and negative control (BBa_R0040). Teams then measured the fluorescence of the bacteria in a plate reader over a 6-hour period.
Materials and Methods
OD 600
Materials:
- 1ml LUDOX
- H20
- Cuvette
Methods
- Add 1 mL LUDOX into a cuvette
- Add 1 mL H2O into a separate cuvette
- Measure the absorbance at 600 nm of all samples using a spectrophotometer *Approved by the InterLab Committee*
- Record the data
- fluorescein
- 10ml 1xPBS
- 96 well plate, black with flat, transparent/clear bottom
- Prepare 2x fluorescein stock solution (100 uM) by resuspending fluorescein in 1 mL of 1xPBS
- Prepare 1mL of 50 uM (1x) fluorescein solution by diluting 500 uL of the 2x fluorescein stock solution with 500 uL of 1xPBS
- Conduct serial dilutions of fluorescein in the well plate
- 100 uL of PBS added into wells A2, B2, C2, D2... A12, B12
- 200 uL of fluorescein 1x stock solution added to A1, B1, C1, D1
- 100 uL fluorescein stock solution transferred from A1 into A2
- A2 mixed by pipetting up and down, then 100 uL transferred to A3
- A3 mixed by pipetting up and down, then 100 uL transferred to A4
- Continue through A11, DO NOT continue dilution into A12
- Step 3 repeated for rows B-D
- Fluorescence for all samples measured using the plate reader
Fluorescein Fluorescence Standard Curve
Materials
Methods
Materials
- Competent cells (Escherichia coli strain DH5α)
- LB media
- Chloramphenicol
- Incubator at 37°C
- Devices
- BBa_J364000
- BBa_J364001
- BBa_J364002
- BBa_J364003
- BBa_J364004
- BBa_J364005
- BBa_I20270
- BBa_R0040
Methods
- Locate the devices listed above in the distribution kit and resuspend them in 10uL of dH20
- Transform each device into 50uL of competent cells
- Plate the transformations onto LB plates with chloramphenicol and incubate overnight at 37C