Team:DTU-Denmark/pBAD SPL

From 2013.igem.org

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# USER cloning to add RFP downstream of promoter.
# USER cloning to add RFP downstream of promoter.
# Colonies were plated.
# Colonies were plated.
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# Plates were induced by spraying them with an aqueous arabinose solution.
+
# After inspection under UV-light the visually non RFP containing colonies where picked.
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# Colonies that were not red prior to induction with arabinose but that did turn red after induction with arabinose were selected and re-innoculated as liquid cultures.
+
# Plates were induced by spraying them with an 5% w/v aqueous arabinose solution.
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# Biolector: Wells were inoculated from overnight cultures of each of the selected colonies. All wells were run in duplicate.
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# The plates were again inspected under UV-light and this time the most red florescent cells were picked.
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# Colonies were grown in culture tubes and screened in parallel on BioLector. Wells on BioLector plate were loaded with culture by transferring a toothpick from each overnight culture selected and into the wells of the plate. All wells were run in duplicate.
# All duplicate colonies were run twice -- once with arabinose added at t=0, and again without arabinose.   
# All duplicate colonies were run twice -- once with arabinose added at t=0, and again without arabinose.   
# The pBAD system [http://parts.igem.org/Part:BBa_K808000 BBa_K808000] was used as a reference.
# The pBAD system [http://parts.igem.org/Part:BBa_K808000 BBa_K808000] was used as a reference.

Revision as of 16:50, 3 October 2013

pBAD SPL

Contents

pBAD synthetic promoter library

A synthetic promoter library (SPL) is a library of cells each having one promoter sequence that differs between them. This promoter is always the same and is usually upstream a fluorescent protein like GFP/RFP. The term was first coined in 1998 and used in Lactococcus lactis (Jensen, Peter Ruhdal, and Karin Hammer.). The method was adapted by 2010 DTU iGEM team to make a SPL for E.coli that enabled the modulation of constitutive gene expression with great precision. They even made a new standard for this method with the use of biobricks ([http://dspace.mit.edu/handle/1721.1/60080 RFC 63]).

We used the method to build a non-leaky arabinose inducible promoter as a tool for expressing lethal proteins in E. coli. The reason was that many of the proteins we are working with are membrane bound or integral membrane proteins and will be lethal if expressed in to high quantities.

For testing our pathways we needed to grow the transformed cell to a certain concentration and growth with the gene constitutively expressed was not working very well. We needed a inducible system but the standard arabinose inducible system was way too leaky and we got same stood with the same problem as before. Therefore we needed to either build or buy (if an possible) an inducible system with great tightness able to be induced easily. We choose to build such system.

Methods

Experimental procedure

  1. Random promoter sequences were ordered matching the sequence CTGACGNNNNNNNNNNNNNNNNNNTAWWATNNNNA.
  2. USER cloning to add RFP downstream of promoter.
  3. Colonies were plated.
  4. After inspection under UV-light the visually non RFP containing colonies where picked.
  5. Plates were induced by spraying them with an 5% w/v aqueous arabinose solution.
  6. The plates were again inspected under UV-light and this time the most red florescent cells were picked.
  7. Colonies were grown in culture tubes and screened in parallel on BioLector. Wells on BioLector plate were loaded with culture by transferring a toothpick from each overnight culture selected and into the wells of the plate. All wells were run in duplicate.
  8. All duplicate colonies were run twice -- once with arabinose added at t=0, and again without arabinose.
  9. The pBAD system [http://parts.igem.org/Part:BBa_K808000 BBa_K808000] was used as a reference.
This reverse primer sequence is incorporating randomized promoter sequences into the pBAD construct. The sequence is annotated with -10 and -35 consensus region. Note that I2-bindingsite is overlapping with the -35 region. Blue is the binding part of the primer, red is the USER made sticky ends. N=random, W=50% A and 50% T

Data analysis

  1. Data was collected from the Biolector, and analyzed using a series of R scripts written by Chris Workman (unpublished).
    • The maturation and degradation times for mCherry were both assumed to be 40 min. TODOref
    • The growth rate, mu, was estimated to be 1.28 (from an average of all wells on all plates) since we expect each strain to grow at the same rate.
    • A time window representing exponential growth was selected (between 1 and 4.5 hours).
  2. The RFP measurement for a constitutively expressed strain was used as a standard measure of growth. This is plotted on the x-axis in the detailed plots per colony below.
  3. Figures were plotted using R.

Results

Summary

Promoter activity when induced (with arabinose added) plotted vs basal activity (without arabinose; ie leakiness of the promoter). The colonies that we selected all show less activity than the the constitutive promoter, and when induced, show higher activity than the constitutive promoter. Induced vs basal.png

Details

Promoter strengths for two trials of each colony with and without arabinose.

Colony Number With arabinose 1 With arabinose 2 Without arabinose 1 Without arabinose 2
Col28.90257.86990.7270.9552
Col39.272412.11420.52480.6982
Col49.457111.45220.52310.2508
Col126.364110.53890.58970.6869
Col107.96979.79490.33920.733
Col97.856320.10940.69950.7432
Col812.231815.45480.42030.4538
Col1311.03777.33430.4820.4641
Col1515.68178.27070.81690.1343
Col1814.791615.57360.66740.6745
Col1914.212616.48980.45450.3566
Col297.185316.34670.54450.5013
Col269.77249.62690.71180.7865
Col228.41685.59580.60490.5645
Col339.19828.99870.65081.374
Col3410.69877.8830.50670.5031
Col3513.84277.54690.43630.6281
ConRef6.5067.93238.78117.9323

Dtu-Fss-plot-col2.png Dtu-Fss-plot-col3.png Dtu-Fss-plot-col4.png Dtu-Fss-plot-col12.png Dtu-Fss-plot-col10.png Dtu-Fss-plot-col9.png Dtu-Fss-plot-col8.png Dtu-Fss-plot-col13.png Dtu-Fss-plot-col15.png Dtu-Fss-plot-col18.png Dtu-Fss-plot-col19.png Dtu-Fss-plot-col29.png Dut-Fss-plot-col26.png Dtu-Fss-plot-col22.png Dtu-Fss-plot-col33.png Dtu-Fss-plot-col34.png Dtu-Fss-plot-col25.png Dtu-Fss-plot-conref.png

Example of use

The tight inducible pBAD promoter was used in our "Hello World project" to regulate the expression of GFP SF, which was tagged with a signal peptide to direct it into the periplasm. Production and folding of GFP SF is faster than the transport system of E. coli, which leads to undesired accumulation of GFP SF in the cytoplasm. Only when using a promoter with low leakiness it is possible to translocate a significant fraction of GFP SF after its production has been switched off. Thereby we get a clear signal from the periplasm with low interference from the cytoplasm.

Alt text
Overview microscopic pciture showing "Hello World" transformants.
Alt text
High resolution picture of "Hello World" transformants, showing a clear seperation of green and red fluorescence. GFP is primarily located in the periplasm while RFP is located in the cytoplasm. Fluorescence intensity measurements are taken along the cross-section indicated by the white line. Picture taken with a confocal microscope and ??? filter.
Alt text
Graph of flourescence measurement (or is this the model???) on green and red channel. It can be seen that the intensity of the red flourescence is restricted to the cytoplasm while green flourescence has it's peaks on the egdes. A weak green signal is measured for the cytoplasmic region because the periplasm envelopes the cytoplasm.


See also "Hello World project".


References

  • Jensen, Peter Ruhdal, and Karin Hammer. "The sequence of spacers between the consensus sequences modulates the strength of prokaryotic promoters." Applied and environmental microbiology 64.1 (1998): 82-87.