Difference between revisions of "Team:Glasgow/Project/Overview/RBS"
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<div class="col-md-6"> | <div class="col-md-6"> | ||
<h5 style="font-size:25px">Aim</h5> | <h5 style="font-size:25px">Aim</h5> | ||
− | <p> | + | <p>To optimise bioluminescence in <i>Escherichia coli</i> by creating a range of Ribosome Binding Sites (RBS) for each of the six genes in the <i>luxCDABEG</i> operon from <i>Aliivibrio fisheri</i>, originally submitted to the registry as a single BioBrick in 2010 by the Cambridge team.</p> |
<h5 style="font-size:25px">Results</h5> | <h5 style="font-size:25px">Results</h5> | ||
<p> | <p> | ||
− | - Designed RBS library with 32 variants for each lux gene | + | - Designed RBS library with 32 variants for each <i>lux</i> gene |
</br> | </br> | ||
</br> | </br> | ||
− | - Made luxABG and luxCDE constructs from the RBS library | + | - Made <i>luxABG</i> and <i>luxCDE</i> constructs from the RBS library – over 1000 RBS variantions for each construct |
</br> | </br> | ||
</br> | </br> | ||
− | - Showed that cells are able to uptake decanal from the environment and produce light when luxAB or luxABG is expressed | + | - Showed that cells are able to uptake decanal from the environment and produce light when <i>luxAB</i> or <i>luxABG</i> is expressed |
</br> | </br> | ||
</br> | </br> | ||
− | - Visualised RBS library for luxAB, luxABG and luxCDE | + | - Visualised RBS library for <i>luxAB</i>, <i>luxABG</i> and <i>luxCDE</i> constructs and determined optimal RBS arrangements for E. coli |
</p> | </p> | ||
</div> | </div> | ||
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Documented and submitted: | Documented and submitted: | ||
<ul> | <ul> | ||
− | <li>BBa_K1725340 – | + | <li>BBa_K1725340 – I0500-RBS-<i>luxA</i>-RBS-<i>luxB</i>-RBS-<i>luxG</i> </li> |
− | <li>BBa_K1725341 – | + | <li>BBa_K1725341 – I0500-RBS-<i>luxA</i>-RBS-<i>luxB</i>-RBS-<i>luxG</i>-K1725080-RBS-<i>luxC</i>-RBS-<i>luxD</i>-RBS-<i>luxE</i></li> |
</ul> | </ul> | ||
Documented only: | Documented only: | ||
<ul> | <ul> | ||
<li> BBa_K1725301-BBa_K1725332 – RBS library</li> | <li> BBa_K1725301-BBa_K1725332 – RBS library</li> | ||
− | <li> BBa_K1725342 – | + | <li> BBa_K1725342 – K1725080-RBS-<i>luxC</i>-RBS-<i>luxD</i>-RBS-<i>luxE</i> (High decanal production)</li> |
− | <li> BBa_K1725343 – | + | <li> BBa_K1725343 – K1725080-RBS-<i>luxC</i>-RBS-<i>luxD</i>-RBS-<i>luxE</i> (Low decanal production)</li> |
</ul> | </ul> | ||
</br> | </br> |
Revision as of 14:25, 16 September 2015
RBS library
Summary
Aim
To optimise bioluminescence in Escherichia coli by creating a range of Ribosome Binding Sites (RBS) for each of the six genes in the luxCDABEG operon from Aliivibrio fisheri, originally submitted to the registry as a single BioBrick in 2010 by the Cambridge team.
Results
- Designed RBS library with 32 variants for each lux gene - Made luxABG and luxCDE constructs from the RBS library – over 1000 RBS variantions for each construct - Showed that cells are able to uptake decanal from the environment and produce light when luxAB or luxABG is expressed - Visualised RBS library for luxAB, luxABG and luxCDE constructs and determined optimal RBS arrangements for E. coli
Biobricks
Documented and submitted:
- BBa_K1725340 – I0500-RBS-luxA-RBS-luxB-RBS-luxG
- BBa_K1725341 – I0500-RBS-luxA-RBS-luxB-RBS-luxG-K1725080-RBS-luxC-RBS-luxD-RBS-luxE
- BBa_K1725301-BBa_K1725332 – RBS library
- BBa_K1725342 – K1725080-RBS-luxC-RBS-luxD-RBS-luxE (High decanal production)
- BBa_K1725343 – K1725080-RBS-luxC-RBS-luxD-RBS-luxE (Low decanal production)
Motivation
For the Bioluminescence part of our project we used lux operon from Vibrio fischeri introduced to the iGEM for the first time by Cambridge team in 2010. The have used five lux genes for the assembly of the lux operon: luxA, B, C, D and E with luxA and luxB encoding bacterial luciferase and luxC, luxD and luxE encoding enzyme complex that synthesises tetradecanal, a substrate for the luciferase. This year were are adding sixth lux gene to the assembly – luxG which is known to encode a flavin reductase that provides reduced flavin mononucleotide for the bioluminescence reaction resulting in an enhanced light ouptput. Initially we decided to optimise bioluminescence in E. coli by rearranging whole Lux operon and placing a defined relatively-weak (REF) ribosome binding site – B0032 – upstream of each of the six lux genes (Link to Cara’s Bioluminescence page). Taking this approach further, we thought of adjusting bioluminescence to E. coli by creating a B0032-derived ribosome binding site library for each lux gene. The idea behind this was to create a range of RBS combinations in a lux operon and therefore, generate E. coli strains of different bioluminescence intensity (FIGURE). We assumed that the most favourable RBS arrangements in lux operon should be observed in the E. coli colonies emitting the most light.
Design
For the construction of the RBS library, we used a master sequence based on the RBS B0032 (FIGURE). 4 nucleotides close to the actual ribosome binding site were randomised giving 32 different B0032-derived RBS variants. The predicted efficiency of each RBS library member was estimated using RBS Library Calculator (REF http://msb.embopress.org/content/10/6/731) for every lux gene (FIGURE with graphs). Technically, with 32 different RBS variants for each of the six lux genes, final RBS library for lux operon would have over a billion different RBS arrangements (Figure, show calculations??).Strategy and approaches
Randomised PCR and Cloning, Cloning, Cloning
Testing pBAD.luxAB
Inviting Mr. Bright to the party: luxG
Story about luxCDE
Results
- Cell-cell comunication - Decanal experiments - Spectrum experiments and comparison to Cambridge operonReferences