Team:KU Leuven/Project/Glucosemodel/MeS

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  <h3 class="bg-green">The Honeydew System</h3>
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     <a href="https://2013.igem.org/Team:KU_Leuven/Project/Glucosemodel/Design">
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     <h3>Honeydew model</h3> </a>
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     <h3>Designing the Honeydew System</h3> </a>
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     <p>Design of the honeydew model</p>
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     <p>Want to know more about our constructs?</p>
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     <h3>E-β-Farnesene construction</h3>
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     <p>BanAphids produce EBF!</p>
     <p>BanAphids produce EBF!</p>
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     <h3>Methyl Salicylate</h3> </a>
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     <h3>Methyl Salicylate construction</h3> </a>
     <p>You are here!</p>
     <p>You are here!</p>
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     <a href="https://2013.igem.org/Team:KU_Leuven/Project/Glucosemodel/qPCR">
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     <h3>Methyl Salicylate - qPCR</h3> </a>
     <p>Wetlab data for the MeS model</p>
     <p>Wetlab data for the MeS model</p>
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   <p align="justify">Methyl salicylate is an organic ester also known as <b>wintergreen oil</b>. It is produced by different species of plants. It is converted from <b>chorismate with salicylate as an intermediate</b>. In <i>E. coli</i>, chorismate is used as a precursor for the amino acids phenylalanine, tryptophane and tyrosine. It is produced from erythrose-4-phosphate (Ery4P) and phosphoenolpyruvate (PEP) through the shikimate pathway (Sprenger <i>et al.</i>, 2007). Chorismate is also the precursor of isochorismate, which is used for the biosythesis of quinones, siderophores and folic acid (Dosselaere and Vanderleyden, 2001). <b>In this page we will discuss the <a href="#pathway">pathway</a> that leads up to methyl salicylate and the <a href="#bricks">biobricks</a> that we made.</b> We will end with characterisation of these biobricks using a <a href="#Smell Test">smell</a> test and an <a href="#SDS PAGE">SDS-PAGE</a>.</p>
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   <p align="justify">Methyl salicylate (MeS) or wintergreen oil is a plant hormone. It is converted from <b>chorismate</b> with <b>salicylate</b> as an intermediate. <b>In this page we will discuss the <a href="#pathway">pathway</a> that leads up to methyl salicylate and the <a href="#Our bricks">biobricks</a> that we made.</b> We will end with characterisation of these biobricks using a <a href="#Smell Test">smell</a> test, an <a href="#SDS PAGE">SDS-PAGE</a> and <a href="#Headspace GC"> GC analyses</a>.</p>
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    <h3>MeS brick background</h3> </a>
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    <p>Genes, pathway and improvements</p>
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    <p>Bricks and wetlab overview</p>
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   <p align="justify">The conversion of Ery4P and PEP to DAHP (3-deoxy-D-arabinoheptulosonate 7-phosphate) is catalysed by DAHP synthase, an enzyme which exists in three isoforms, coded by the genes <i>aroF, aroG</i> and <i>aroH</i>. These isoforms are selectively inhibited by tyrosine, phenylalanine and tryptophan, respectively. In <i>E. coli</i>, about 80%, 20% and 1% of the enzyme activities are contributed by the DAHPS phenotypes of the <i>aroG, aroF</i> and <i>aroH</i> products, respectively (Ikeda <i>et al.</i>, 2006).<br/>
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   <p align="justify">The conversion of Ery4P and PEP to DAHP (3-deoxy-D-arabinoheptulosonate 7-phosphate) is catalysed by DAHP synthase, which exists in three isoforms, coded by the genes <i>aroF, aroG</i> and <i>aroH</i>. These isoforms are selectively inhibited by Tyr, Phe and Trp, respectively. In <i>E. coli</i>, about 80% of the enzyme activity by contributed by the DAHPS of <i>aroG</i>(Ikeda <i>et al.</i>, 2006).<br/>
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This means that when there is <b>enough phenylalanine</b> produced by the cell, or enough present in the medium, the <b>production of DAHP, and hence chorismate, will stop by inhibition of the <i>aro</i> genes</b>. The <b>production of phenylalanine will stop as well by inhibition of <i>pheA</i>,</b> coding for chorismate mutase/prephenate dehydratase. <br/>
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When there is <b>enough phenylalanine</b>, the <b>production of DAHP, and hence chorismate, will stop by inhibition of the <i>aro</i> genes</b>. <br/>
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The conversion from chorismate to methyl salicylate starts with a conversion to isochorismate, catalysed by the enzyme isochorismate synthase, encoded by the <i>pchA</i> gene. This isochorismate is directly converted to salicylate by isochorismate pyruvate/lyase, encoded by the <i>pchB</i> gene. This conversion happens immediately, since the <i>pchA</i> and <i>pchB</i> gene form the <i>pchBA</i> operon which is always transcribed to one mRNA. Conversion of salicylate to methyl salicylate is catalysed by S-adenosylmethionine-dependent methyltransferase, encoded by <i>bsmt1</i> (Gaille <i>et al.</i>, 2003).  
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The conversion from chorismate to MeS starts with a conversion to isochorismate, catalysed by isochorismate synthase, encoded by <b><i>pchA</i></b>. Isochorismate is directly converted to salicylate by isochorismate pyruvate/lyase, encoded by <b><i>pchB</i></b>. This conversion happens immediately, since <i>pchA</i> and <i>pchB</i> form the <b><i>pchBA</i></b> operon which is always transcribed to one mRNA. Conversion of salicylate to MeS is catalysed by S-adenosylmethionine-dependent methyltransferase, encoded by <b><i>bsmt1</i></b> (Gaille <i>et al.</i>, 2003).  
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   <p align="justify">The <b>iGEM team of MIT 2006 already constructed a Biobrick </b>(<a href="http://parts.igem.org/Part:BBa_J45700" target="_blank">BBa_J45700</a>) encoding the <i>pchBA</i> and <i>bsmt1</i> genes, so introducing this brick should induce the production of methyl salicylate, since chorismate is a common metabolite in <i>E. coli</i>. The MIT team discovered however that there was almost no methyl salicylate production observed, only when salicylic acid was added to the medium. <b>Our experiments with this Biobrick confirmed this lack of methyl salicylate production </b>(see the smell test in the MeS journal). There had to be something wrong with the conversion of chorismate to salicylate. One possibility is that there is something wrong with the enzymes produced by the <i>pchBA</i> genes. Another one is that there is a lack of chorismate present in the cell. We have attempted to increase the productivity of the MIT 2006 brick by using stronger ribosome binding sites. Also, <b>we replaced the <i>lac</i> promoter by a TetR-repressible promoter, so the lacI produced in our system doesn't interfere with the transcription of <i>pchBA</i>.</b>.
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   <p align="justify">The <b>iGEM team of MIT 2006 already constructed a Biobrick </b>(<a href="http://parts.igem.org/Part:BBa_J45700" target="_blank">BBa_J45700</a>) encoding <i>pchBA</i> and <i>bsmt1</i>, for the production of MeS. However, the MIT team only observed MeS production when salicylic acid was added to the medium. <b>Our experiments with this Biobrick confirmed this lack of MeS production </b>(see the smell test below). There had to be something wrong with the conversion of chorismate to salicylate. One possibility is that there is something wrong with the enzymes produced by the <i>pchBA</i> genes. Another one is that there is a lack of chorismate present in the cell. We have attempted to increase the productivity of the MIT 2006 brick by using stronger ribosome binding sites. Also, <b>we replaced the <i>lac</i> promoter by a TetR-repressible promoter, so the lacI produced in our system doesn't interfere with the transcription of <i>pchBA</i>.</b>.
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   <h3>The Chorismate Problem</h3>
   <h3>The Chorismate Problem</h3>
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   <p align="justify">Since chorismate is the precursor for three amino acids in <i>E. coli</i>, we believe that there is not much of the chorismate left to be converted to methyl salicylate, since the cell needs to keep producing a steady amount of essential amino acids.<br/>
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   <p align="justify">Since chorismate is the precursor for three amino acids in <i>E. coli</i>, we believe that there is not much of the chorismate left to be converted to MeS.<br/>
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To overcome this problem, we looked at a study by Sun <i>et al.</i> (2011), in which a synthetic pathway was introduced for the production of mandelic acid from chorismate. They achieved this by deleting different genes encoding enzymes that catalyse competing pathways, as well as by introducing a feedback-insensitive DAHP synthase mutant to increase the carbon flow down the shikimate pathway. This last method gave us inspiration to overcome our own problem.<br/>
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To overcome this problem, we looked at a study by Sun <i>et al.</i> (2011), in which a synthetic pathway was introduced for the production of mandelic acid from chorismate. They achieved this by deleting different genes encoding enzymes that catalyse competing pathways, as well as by <b>introducing a feedback-insensitive DAHP synthase mutant to increase the carbon flow down the shikimate pathway</b>. This last method gave us inspiration to overcome our own problem.<br/>
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If we look at the pathway in Figure 2, we can conclude that if the amino acids are present in the medium, the conversion of chorismate to these amino acids will be inhibited allosterically, as wel as the production of DAHP. <b>Our plan is to mutate the <i>aroG</i> gene in a manner that the enzymatic function still remains, but that it is insensitive to allosteric inhibition by phenylalanine. We only mutate the <i>aroG</i> gene since this isoform is responsible for 80% of DAHP synthase activity </b> (Hu <i>et al.</i>, 2003).</p>
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If Tyr, Phe or Trp are present in the medium, the conversion of chorismate to these amino acids will be inhibited allosterically, as wel as the production of DAHP (Figure 2). <b>Our plan is to mutate the <i>aroG</i> gene in a manner that the enzymatic function still remains, but that it is insensitive to allosteric inhibition by phenylalanine. We only mutate the <i>aroG</i> gene since this isoform is responsible for 80% of DAHP synthase activity </b> (Hu <i>et al.</i>, 2003).</p>
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  <p align="justify">It is proven that a Pro150Leu point mutation is Phe-insensitive. This mutation is used as a positive control in a study by Hu <i>et al.</i> (2003) in which they compare the effects of different mutation in the <i>aroG</i> gene on the specific enzymatic activity. The results showed that a Leu175Asp mutation also lead to a Phe-insensitive enzyme. Leu175 is located at the bottom of the possible inhibitor binding pocket, and it is believed to be a critical residue.<br/>
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    <p align="justify">It is proven that a Pro150Leu point mutation is Phe-insensitive. This mutation is used as a positive control in a study by Hu <i>et al.</i> (2003) in which they compare the effects of different mutations in the <i>aroG</i> gene on the specific enzymatic activity. The results showed that a Leu175Asp mutation also lead to a Phe-insensitive enzyme. Leu175 is located at the bottom of the possible inhibitor binding pocket, and it is believed to be a critical residue.<br/>
For reasons still unknown, L175D mutation showed an increased specific enzymatic activity compared to the wild type. In more recent studies, L175D is mostly used to obtain a Phe-insensitive DAHPS (Lin <i>et al.</i>, 2012). That is why we will try to <b>introduce a plasmid containing a L175D mutated <i>aroG</i> gene</b>.<br/>
For reasons still unknown, L175D mutation showed an increased specific enzymatic activity compared to the wild type. In more recent studies, L175D is mostly used to obtain a Phe-insensitive DAHPS (Lin <i>et al.</i>, 2012). That is why we will try to <b>introduce a plasmid containing a L175D mutated <i>aroG</i> gene</b>.<br/>
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It is also proven that transcription of the normal DAHP synthase gene will be inhibited when phenylalanine is present in the medium, so only the mutated form will be produced (Adhja & Gottesman, 1984).
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It is also proven that transcription of the normal DAHP synthase gene will be inhibited when phenylalanine is present in the medium, so only the mutated form will be produced (Adhja & Gottesman, 1984). The unmutated version (P150 and L175) of DAHP synthase is shown in the upper two figures, with the inhibitor phenylalanine in the binding pocket on the right. Below it is shown that the <b>two mutations, P150L and L175D, clearly occupy the binding pocket and thereby sterically hinder the binding of phenylalanine</b>.
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    <p align="center"><img src="https://static.igem.org/mediawiki/2013/7/7f/Original.png" alt="The unmutated DAHP synthase shows a clear Phe binding pocket between residues 150 and 175." width="200" align="center"></p>
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<p align="center">The unmutated DAHP synthase shows a clear Phe binding pocket between residues 150 and 175.</p>
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    <p align="center"><img src="https://static.igem.org/mediawiki/2013/1/1f/OriginalPhe.png" alt="Phe binds in the binding pocket between proline and leucine." width="200"></p>
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<p align="center">Phe binds in the binding pocket between proline and leucine.</p>
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    <p align="center"><img src="https://static.igem.org/mediawiki/2013/1/1a/Mutated.png" alt="Leucine and asparagine sidechains fill up the Phe binding pocket." width="200"></p>
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<p align="center">Leucine and asparagine sidechains fill up the Phe binding pocket.</p>
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    <p align="center"><img src="https://static.igem.org/mediawiki/2013/a/a5/MutatedPhe.png" alt="The binding of Phe is sterically hindered by Leu150 and Asn175." width="200"></p>
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<p align="center">The binding of Phe is sterically hindered by Leu150 and Asn175.</p>
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<b>We created the following BioBricks for the methyl salicylate part:</b>
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    <p align="justify">We characterised the MeS BioBrick by means of <a href="#Smell Test">a smell test</a> as well as characterising this brick with <a href="#Headspace GC">Headspace GC</a>,<a href="#GC-MS analysis of MeS in ethyl acetate extracts"> GC-MS analysis of MeS in ethyl acetate extracts</a> and <a href="#SDS PAGE">SDS PAGE analysis</a>. </p>
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<a href="http://parts.igem.org/Part:BBa_K1060000" target="_blank">BBa_K1060000</a> coding biobrick of DAHP synthase, encoded by the <i>aroG</i> gene from <i>E. coli</i> in the pSB1C3 backbone. The insert is 1053 bp long.
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<p align="justify" class="greytext"> Figure 9 | <i>aroG</i> coding sequence (1053 bp) in pSB1C3 backbone (2070 bp). Digestion confirmation, cut with <i>EcoRI</i> and <i>PstI</i> restriction sites. Sequence confirmed. </p>
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<a href="http://parts.igem.org/Part:BBa_K1060003" target="_blank">BBa_K1060003</a> generator biobrick. It is a twin of the <a href="http://parts.igem.org/Part:BBa_J47500" target="_blank">BBa_J47500</a> biobrick made by the 2006 MIT team, put into a pSB1C3 backbone. The coding sequence is 3255 bp long.
 
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<p align="justify" class="greytext">Figure 10 | Methyl salicylate producing construct (3255 bp) in pSB1C3 backbone (2070 bp). Digestion confirmation, cut with <i>EcoRI</i> and <i>PstI</i> restriction sites. Sequence confirmed. </p>
 
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<a href="http://parts.igem.org/Part:BBa_K1060004" target="_blank">BBa_K1060004</a> intermediate biobrick consisting of <i>bsmt1</i> followed by a double terminator. It is in the pSB1C3 backbone and the insert is 1177 bp long. Sequence confirmed.
 
-
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<a href="http://parts.igem.org/Part:BBa_K1060005" target="_blank">BBa_K1060005</a> intermediate biobrick consisting of <i>pchBA</i> followed by a double terminator. It is in the pSB1C3 backbone and the insert is 1839 bp long. Sequence confirmed.</p>
 
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   <p align="justify">To functionally test our Methyl salicylate production brick (<a href="http://parts.igem.org/Part:BBa_K1060003" target="_blank">BBa_K1060003</a>), we prepared 68 microcentrifuge tubes with <i>E.coli</I> expressing the MeS construct to conduct a blind smell test. This experiment consisted of 4 sets, different in incubation time and temperature. The first set was grown at room temperature for 24 hours, the second was incubated at 37ºC for 24 hours, the third was grown at 37ºC for 8 hours and the last set was grown at room temperature for 8 hours. In each set, we inoculated our brick <a href="http://parts.igem.org/Part:BBa_K1060003" target="_blank">BBa_K1060003</a> with IPTG, IPTG + salicylate (concentration range from 0.01mM to 1mM), and IPTG + chorismate (concentration range from 0.01mM to 1mM), the same for MIT 2006 brick <a href="http://parts.igem.org/Part:BBa_K1060003" target="_blank">BBa_J45700</a>. In addition, the same combinations of additives were introduced in parallel for our negative controls (non-MeS producing <i>E. Coli</i>). <br/>
   <p align="justify">To functionally test our Methyl salicylate production brick (<a href="http://parts.igem.org/Part:BBa_K1060003" target="_blank">BBa_K1060003</a>), we prepared 68 microcentrifuge tubes with <i>E.coli</I> expressing the MeS construct to conduct a blind smell test. This experiment consisted of 4 sets, different in incubation time and temperature. The first set was grown at room temperature for 24 hours, the second was incubated at 37ºC for 24 hours, the third was grown at 37ºC for 8 hours and the last set was grown at room temperature for 8 hours. In each set, we inoculated our brick <a href="http://parts.igem.org/Part:BBa_K1060003" target="_blank">BBa_K1060003</a> with IPTG, IPTG + salicylate (concentration range from 0.01mM to 1mM), and IPTG + chorismate (concentration range from 0.01mM to 1mM), the same for MIT 2006 brick <a href="http://parts.igem.org/Part:BBa_K1060003" target="_blank">BBa_J45700</a>. In addition, the same combinations of additives were introduced in parallel for our negative controls (non-MeS producing <i>E. Coli</i>). <br/>
We asked 11 people to participate in this blind test and calculated the percentage of people who smelled MeS. We can conclude that <b>the MeS/wintergreen smell was stronger after 24 hours incubation time compared to 8 hours. Growing the bacteria at 37 degrees also produced a more pronounced smell than those at room temperature. What’s more, in the microcentrifuge tubes where 0.1mM or 1mM salicylate was added, the smell became more obvious both after 8 and 24hrs of growth. The positive effect of adding chorismate became noticable after 24 hours</b>. The reason why chorismate requires more time to show an effect may be that chorismate is the very first precursor of the methyl salicylate production pathway, whereas the salicylate is an intermediate closer to the end product. As such, the impact of salicylate on the end product will become noticeable sooner. Most importantly, our brick worked in terms of producing methyl salicylate. <br/>
We asked 11 people to participate in this blind test and calculated the percentage of people who smelled MeS. We can conclude that <b>the MeS/wintergreen smell was stronger after 24 hours incubation time compared to 8 hours. Growing the bacteria at 37 degrees also produced a more pronounced smell than those at room temperature. What’s more, in the microcentrifuge tubes where 0.1mM or 1mM salicylate was added, the smell became more obvious both after 8 and 24hrs of growth. The positive effect of adding chorismate became noticable after 24 hours</b>. The reason why chorismate requires more time to show an effect may be that chorismate is the very first precursor of the methyl salicylate production pathway, whereas the salicylate is an intermediate closer to the end product. As such, the impact of salicylate on the end product will become noticeable sooner. Most importantly, our brick worked in terms of producing methyl salicylate. <br/>
The results are shown below:</p>
The results are shown below:</p>
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     <p align="justify">Figure 8 | Incubate at room temperature for 8 hours</p>
     <p align="justify">Figure 8 | Incubate at room temperature for 8 hours</p>
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    <p align="center"><img src="https://static.igem.org/mediawiki/2013/5/55/Smell_test.jpg"></a></p>
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    <p align="justify">Figure 9 | Brief summary of smell test data</p>
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  <p align="justify"> Headspace gas chromatography (HS-GC) was used for the measurement of MeS production by our <b><a href="http://parts.igem.org/Part:BBa_K1060003" target="_blank">BBa_K1060003</b></a> brick in a BL21 strain. Samples of 5 ml supernatant (centrifuged and filtersterilized) were collected in 15-ml precooled glass tubes, which were immediately closed and cooled on ice. Samples were then analyzed with a calibrated Autosystem XL gas chromatograph with a headspace sampler (HS40; Perkin-Elmer, Wellesley, Mass.) and equipped with a CP-Wax 52 CB column (length, 50 m; internal diameter, 0.32 mm; layer thickness, 1.2 μm; Chrompack; Varian, Palo Alto, Calif.). Samples were heated for 16 min at 72°C in the headspace autosampler. The injection block and flame ionization detector (FID) temperatures were kept constant at 180 and 250°C, respectively; helium was used as the carrier gas. The oven temperature was 75°C held for 6 min and then increased to 110°C at 25°C min−1 and held at 100°C for 3.5 min. Results were analyzed with Perkin-Elmer Turbochrom Navigator software.
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MeS (Sigma-Aldrich, M 6752) was used as a standard and was detected at 12.832 minutes post injection (A). Cultures of <i>E. coli</i> BL21 and BL21 harbouring BBa_K1060003 with or without 0.1 mM salicylic acid (SA) supplemented to the medium were also analyzed. <b>No MeS could be detected with the FID in the samples when no SA was added (B), while MeS could be detected when SA was supplemented (C)</b>. <br/>
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The results are shown below:</p>
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    <p> Samples were analyzed with a calibrated Autosystem XL gas chromatograph with a headspace sampler (HS40; Perkin-Elmer, Wellesley, Mass.) and equipped with a CP-Wax 52 CB column. Headspace GC was performed on pure MeS (Sigma-Aldrich) (A), on culture supernatant from a <i>E. coli</i> BL21 strain harbouring BBa_K1060003 without (B) or with 0.1 mM salicylic acid (C). MeS could be detected at 12.832 minutes in (A) and (C) but not when no salicylic acid was added.</p>
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  <a id="GC-MS analysis of MeS in ethyl acetate extracts"></a>
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  <p align="justify"> To back-up our headspace GC data, we also analyzed our our brick <b><a href="http://parts.igem.org/Part:BBa_K1060003" target="_blank">BBa_K1060003</b></a> with GC-MS with the help of Dr. Jan Baeten (Centre for Surface Chemistry and Catalysis; Prof. Dirk De Vos). Supernatant of bacterial cultures were extacted 3 times with ethyl acetate. GC-MS analyses were carried out using a 7890A Agilent gas chromatograph coupled to a 5977A mass spectrometric detector. The GC was equiped with a HP-5MS capillary column (30m x 0.25 mm x 0.25 µm). 1 µl of each sample was injected using splitless injection at a temperature of 250 °C. The initial oven temperature of 40 °C was held for 1 min., ramped at 6 °C / min. to 124 °C, then ramped at 20 °C / min. to 320 °C and finally kept at this temperature for 5 min. The transfer line and ion source were held at 320 °C and 230 °C, respectively. Mass spectra were taken between masses m/z 30-300 with an ionization potential of 70 eV. Retention indices of standards were determined by co-injection of a C7-C30 n-alkane mixture (Supelco) and were compared with published retention indices.
 +
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MeS (Sigma-Aldrich, M 6752) was used as a standard. MeS was detected as a pure peak with a retention index of RI = 1198 (lit. 1191). Ethyl acetate extractions of LB cultures (either controle BL21, BBa_K1060003 or BBa_K1060003 with 0.1 mM salicylic acid (SA) supplemented in the medium) were measured in SCAN-modus with a splitless injectie of 1 µl. No MeS was detected in the controle sample (BL21) but in both other samples MeS was present. For the sample without addition of SA, just a small amount of MeS could be observed (see figure 1).</p>
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    <p> Total ion count (TIC) and extracted ion (EIC m/z 120+152) chromatograms of hexane extract of an <i>E. coli</i> BL21 culture harbouring brick BBa_K1060003 without (A) and with 0.1 mM salicylic acid (B). The mass spectrometer was turned off between 14.5-16 min. to avoid the measurement of extremely abundant peak (which was identified as indole). MeS could be detected at 13.6 min. Inset: measured spectrum at 13.6 min, confirmed as MeS (C8H8O3).</p>
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<!--Bricks-->
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<a href="http://parts.igem.org/Part:BBa_K1060000" target="_blank">BBa_K1060000</a> coding biobrick of DAHP synthase, encoded by the <i>aroG</i> gene from <i>E. coli</i> in the pSB1C3 backbone. The insert is 1053 bp long.
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<p align="justify" class="greytext"> Figure 9 | <i>aroG</i> coding sequence (1053 bp) in pSB1C3 backbone (2070 bp). Digestion confirmation, cut with <i>EcoRI</i> and <i>PstI</i> restriction sites. Sequence confirmed. </p>
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<a href="http://parts.igem.org/Part:BBa_K1060003" target="_blank">BBa_K1060003</a> generator biobrick. It is a twin of the <a href="http://parts.igem.org/Part:BBa_J47500" target="_blank">BBa_J47500</a> biobrick made by the 2006 MIT team, put into a pSB1C3 backbone. The coding sequence is 3255 bp long.
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<p align="justify" class="greytext">Figure 10 | Methyl salicylate producing construct (3255 bp) in pSB1C3 backbone (2070 bp). Digestion confirmation, cut with <i>EcoRI</i> and <i>PstI</i> restriction sites. Sequence confirmed. </p>
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<a href="http://parts.igem.org/Part:BBa_K1060004" target="_blank">BBa_K1060004</a> intermediate biobrick consisting of <i>bsmt1</i> followed by a double terminator. It is in the pSB1C3 backbone and the insert is 1177 bp long. Sequence confirmed.
 +
<br/>
 +
<a href="http://parts.igem.org/Part:BBa_K1060005" target="_blank">BBa_K1060005</a> intermediate biobrick consisting of <i>pchBA</i> followed by a double terminator. It is in the pSB1C3 backbone and the insert is 1839 bp long. Sequence confirmed.</p>
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<!--References-->
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Latest revision as of 03:06, 29 October 2013

iGem

Secret garden

Congratulations! You've found our secret garden! Follow the instructions below and win a great prize at the World jamboree!


  • A video shows that two of our team members are having great fun at our favourite company. Do you know the name of the second member that appears in the video?
  • For one of our models we had to do very extensive computations. To prevent our own computers from overheating and to keep the temperature in our iGEM room at a normal level, we used a supercomputer. Which centre maintains this supercomputer? (Dutch abbreviation)
  • We organised a symposium with a debate, some seminars and 2 iGEM project presentations. An iGEM team came all the way from the Netherlands to present their project. What is the name of their city?

Now put all of these in this URL:https://2013.igem.org/Team:KU_Leuven/(firstname)(abbreviation)(city), (loose the brackets and put everything in lowercase) and follow the very last instruction to get your special jamboree prize!

tree ladybugcartoon

Designing the Honeydew System

Want to know more about our constructs?

E-β-Farnesene construction

BanAphids produce EBF!

Methyl salicylate (MeS) or wintergreen oil is a plant hormone. It is converted from chorismate with salicylate as an intermediate. In this page we will discuss the pathway that leads up to methyl salicylate and the biobricks that we made. We will end with characterisation of these biobricks using a smell test, an SDS-PAGE and GC analyses.

MeS

Figure 1 | Methyl Salicylate

MeS brick background

Genes, pathway and improvements

Brick characterisation

Aphid experiments, GC-MS and more

Our bricks

Bricks and wetlab overview

shikimate pathway

Figure 2 | The Shikimate Pathway

The conversion of Ery4P and PEP to DAHP (3-deoxy-D-arabinoheptulosonate 7-phosphate) is catalysed by DAHP synthase, which exists in three isoforms, coded by the genes aroF, aroG and aroH. These isoforms are selectively inhibited by Tyr, Phe and Trp, respectively. In E. coli, about 80% of the enzyme activity by contributed by the DAHPS of aroG(Ikeda et al., 2006).
When there is enough phenylalanine, the production of DAHP, and hence chorismate, will stop by inhibition of the aro genes.
The conversion from chorismate to MeS starts with a conversion to isochorismate, catalysed by isochorismate synthase, encoded by pchA. Isochorismate is directly converted to salicylate by isochorismate pyruvate/lyase, encoded by pchB. This conversion happens immediately, since pchA and pchB form the pchBA operon which is always transcribed to one mRNA. Conversion of salicylate to MeS is catalysed by S-adenosylmethionine-dependent methyltransferase, encoded by bsmt1 (Gaille et al., 2003).

A Biobrick to start from

The iGEM team of MIT 2006 already constructed a Biobrick (BBa_J45700) encoding pchBA and bsmt1, for the production of MeS. However, the MIT team only observed MeS production when salicylic acid was added to the medium. Our experiments with this Biobrick confirmed this lack of MeS production (see the smell test below). There had to be something wrong with the conversion of chorismate to salicylate. One possibility is that there is something wrong with the enzymes produced by the pchBA genes. Another one is that there is a lack of chorismate present in the cell. We have attempted to increase the productivity of the MIT 2006 brick by using stronger ribosome binding sites. Also, we replaced the lac promoter by a TetR-repressible promoter, so the lacI produced in our system doesn't interfere with the transcription of pchBA..

mesa biobrick

Figure 3 | The original methyl salicylate biobrick BBa_J45700

The Chorismate Problem

Since chorismate is the precursor for three amino acids in E. coli, we believe that there is not much of the chorismate left to be converted to MeS.
To overcome this problem, we looked at a study by Sun et al. (2011), in which a synthetic pathway was introduced for the production of mandelic acid from chorismate. They achieved this by deleting different genes encoding enzymes that catalyse competing pathways, as well as by introducing a feedback-insensitive DAHP synthase mutant to increase the carbon flow down the shikimate pathway. This last method gave us inspiration to overcome our own problem.
If Tyr, Phe or Trp are present in the medium, the conversion of chorismate to these amino acids will be inhibited allosterically, as wel as the production of DAHP (Figure 2). Our plan is to mutate the aroG gene in a manner that the enzymatic function still remains, but that it is insensitive to allosteric inhibition by phenylalanine. We only mutate the aroG gene since this isoform is responsible for 80% of DAHP synthase activity (Hu et al., 2003).

Figure 4 | The different pointmutations of aroG and their effect

Necessary Mutations

It is proven that a Pro150Leu point mutation is Phe-insensitive. This mutation is used as a positive control in a study by Hu et al. (2003) in which they compare the effects of different mutations in the aroG gene on the specific enzymatic activity. The results showed that a Leu175Asp mutation also lead to a Phe-insensitive enzyme. Leu175 is located at the bottom of the possible inhibitor binding pocket, and it is believed to be a critical residue.
For reasons still unknown, L175D mutation showed an increased specific enzymatic activity compared to the wild type. In more recent studies, L175D is mostly used to obtain a Phe-insensitive DAHPS (Lin et al., 2012). That is why we will try to introduce a plasmid containing a L175D mutated aroG gene.
It is also proven that transcription of the normal DAHP synthase gene will be inhibited when phenylalanine is present in the medium, so only the mutated form will be produced (Adhja & Gottesman, 1984). The unmutated version (P150 and L175) of DAHP synthase is shown in the upper two figures, with the inhibitor phenylalanine in the binding pocket on the right. Below it is shown that the two mutations, P150L and L175D, clearly occupy the binding pocket and thereby sterically hinder the binding of phenylalanine.

The unmutated DAHP synthase shows a clear Phe binding pocket between residues 150 and 175.

The unmutated DAHP synthase shows a clear Phe binding pocket between residues 150 and 175.

Phe binds in the binding pocket between proline and leucine.

Phe binds in the binding pocket between proline and leucine.

Leucine and asparagine sidechains fill up the Phe binding pocket.

Leucine and asparagine sidechains fill up the Phe binding pocket.

The binding of Phe is sterically hindered by Leu150 and Asn175.

The binding of Phe is sterically hindered by Leu150 and Asn175.

We characterised the MeS BioBrick by means of a smell test as well as characterising this brick with Headspace GC, GC-MS analysis of MeS in ethyl acetate extracts and SDS PAGE analysis.

To functionally test our Methyl salicylate production brick (BBa_K1060003), we prepared 68 microcentrifuge tubes with E.coli expressing the MeS construct to conduct a blind smell test. This experiment consisted of 4 sets, different in incubation time and temperature. The first set was grown at room temperature for 24 hours, the second was incubated at 37ºC for 24 hours, the third was grown at 37ºC for 8 hours and the last set was grown at room temperature for 8 hours. In each set, we inoculated our brick BBa_K1060003 with IPTG, IPTG + salicylate (concentration range from 0.01mM to 1mM), and IPTG + chorismate (concentration range from 0.01mM to 1mM), the same for MIT 2006 brick BBa_J45700. In addition, the same combinations of additives were introduced in parallel for our negative controls (non-MeS producing E. Coli).
We asked 11 people to participate in this blind test and calculated the percentage of people who smelled MeS. We can conclude that the MeS/wintergreen smell was stronger after 24 hours incubation time compared to 8 hours. Growing the bacteria at 37 degrees also produced a more pronounced smell than those at room temperature. What’s more, in the microcentrifuge tubes where 0.1mM or 1mM salicylate was added, the smell became more obvious both after 8 and 24hrs of growth. The positive effect of adding chorismate became noticable after 24 hours. The reason why chorismate requires more time to show an effect may be that chorismate is the very first precursor of the methyl salicylate production pathway, whereas the salicylate is an intermediate closer to the end product. As such, the impact of salicylate on the end product will become noticeable sooner. Most importantly, our brick worked in terms of producing methyl salicylate.
The results are shown below:

Figure 5 | Incubate at room temperature for 24 hours

Figure 7 | Incubate at 37 degrees for 8 hours

Figure 6 | Incubate at 37 degrees for 24 hours

Figure 8 | Incubate at room temperature for 8 hours

Figure 9 | Brief summary of smell test data

Headspace gas chromatography (HS-GC) was used for the measurement of MeS production by our BBa_K1060003 brick in a BL21 strain. Samples of 5 ml supernatant (centrifuged and filtersterilized) were collected in 15-ml precooled glass tubes, which were immediately closed and cooled on ice. Samples were then analyzed with a calibrated Autosystem XL gas chromatograph with a headspace sampler (HS40; Perkin-Elmer, Wellesley, Mass.) and equipped with a CP-Wax 52 CB column (length, 50 m; internal diameter, 0.32 mm; layer thickness, 1.2 μm; Chrompack; Varian, Palo Alto, Calif.). Samples were heated for 16 min at 72°C in the headspace autosampler. The injection block and flame ionization detector (FID) temperatures were kept constant at 180 and 250°C, respectively; helium was used as the carrier gas. The oven temperature was 75°C held for 6 min and then increased to 110°C at 25°C min−1 and held at 100°C for 3.5 min. Results were analyzed with Perkin-Elmer Turbochrom Navigator software. MeS (Sigma-Aldrich, M 6752) was used as a standard and was detected at 12.832 minutes post injection (A). Cultures of E. coli BL21 and BL21 harbouring BBa_K1060003 with or without 0.1 mM salicylic acid (SA) supplemented to the medium were also analyzed. No MeS could be detected with the FID in the samples when no SA was added (B), while MeS could be detected when SA was supplemented (C).
The results are shown below:

Samples were analyzed with a calibrated Autosystem XL gas chromatograph with a headspace sampler (HS40; Perkin-Elmer, Wellesley, Mass.) and equipped with a CP-Wax 52 CB column. Headspace GC was performed on pure MeS (Sigma-Aldrich) (A), on culture supernatant from a E. coli BL21 strain harbouring BBa_K1060003 without (B) or with 0.1 mM salicylic acid (C). MeS could be detected at 12.832 minutes in (A) and (C) but not when no salicylic acid was added.

To back-up our headspace GC data, we also analyzed our our brick BBa_K1060003 with GC-MS with the help of Dr. Jan Baeten (Centre for Surface Chemistry and Catalysis; Prof. Dirk De Vos). Supernatant of bacterial cultures were extacted 3 times with ethyl acetate. GC-MS analyses were carried out using a 7890A Agilent gas chromatograph coupled to a 5977A mass spectrometric detector. The GC was equiped with a HP-5MS capillary column (30m x 0.25 mm x 0.25 µm). 1 µl of each sample was injected using splitless injection at a temperature of 250 °C. The initial oven temperature of 40 °C was held for 1 min., ramped at 6 °C / min. to 124 °C, then ramped at 20 °C / min. to 320 °C and finally kept at this temperature for 5 min. The transfer line and ion source were held at 320 °C and 230 °C, respectively. Mass spectra were taken between masses m/z 30-300 with an ionization potential of 70 eV. Retention indices of standards were determined by co-injection of a C7-C30 n-alkane mixture (Supelco) and were compared with published retention indices. MeS (Sigma-Aldrich, M 6752) was used as a standard. MeS was detected as a pure peak with a retention index of RI = 1198 (lit. 1191). Ethyl acetate extractions of LB cultures (either controle BL21, BBa_K1060003 or BBa_K1060003 with 0.1 mM salicylic acid (SA) supplemented in the medium) were measured in SCAN-modus with a splitless injectie of 1 µl. No MeS was detected in the controle sample (BL21) but in both other samples MeS was present. For the sample without addition of SA, just a small amount of MeS could be observed (see figure 1).

Total ion count (TIC) and extracted ion (EIC m/z 120+152) chromatograms of hexane extract of an E. coli BL21 culture harbouring brick BBa_K1060003 without (A) and with 0.1 mM salicylic acid (B). The mass spectrometer was turned off between 14.5-16 min. to avoid the measurement of extremely abundant peak (which was identified as indole). MeS could be detected at 13.6 min. Inset: measured spectrum at 13.6 min, confirmed as MeS (C8H8O3).

Lanes a-d were induced at OD600nm 0.5, Lanes e-h were induced at OD600nm 1.0 with the indicated concentration of IPTG. Cells were grown further for 1 hrs at 25°C. An identical experiment was performed with cells grown for 6hrs after induction. Finally, the brick was also tested with cells grown at 37°C.

Similar to our set-up for the EBF synthase protein expression, we tested the MIT biobrick (BBa_J45700) and our novel MeS construct (BBa_K1060003) via protein expression. We transformed our constructs in an E.coli expression strain, grew them at various temperatures (room temperature and 37 degrees celcius) and induced expression with increasing amounts of IPTG. We also added salicylate or chorismate to the growth medium in an attempt to increase MeS production.
The figure shows results obtained with the BBa_J45700 brick. Our biobrick (BBa_K1060003) showed similar results (data not shown). Increasing the amount of IPTG did not influence the protein expression profile (compare lanes a-d or lanes e-h) but we do see some bands in the lanes a-d which we cannot see in lanes e-f (eg a band just above 55 kDa). Nonetheless, this observation can be verified with lower amounts of the protein extracts. Nonetheless, our smell test would suggest that the MeS brick does work. Hence, we need a more sensitive approach to identify the protein production of the MeS brick. Possible approaches would be via classic western blot experiment or a GC-MS set-up.

BBa_K1060000 coding biobrick of DAHP synthase, encoded by the aroG gene from E. coli in the pSB1C3 backbone. The insert is 1053 bp long.










Figure 9 | aroG coding sequence (1053 bp) in pSB1C3 backbone (2070 bp). Digestion confirmation, cut with EcoRI and PstI restriction sites. Sequence confirmed.

K1060000
K1060003.png

BBa_K1060003 generator biobrick. It is a twin of the BBa_J47500 biobrick made by the 2006 MIT team, put into a pSB1C3 backbone. The coding sequence is 3255 bp long.






Figure 10 | Methyl salicylate producing construct (3255 bp) in pSB1C3 backbone (2070 bp). Digestion confirmation, cut with EcoRI and PstI restriction sites. Sequence confirmed.

BBa_K1060004 intermediate biobrick consisting of bsmt1 followed by a double terminator. It is in the pSB1C3 backbone and the insert is 1177 bp long. Sequence confirmed.
BBa_K1060005 intermediate biobrick consisting of pchBA followed by a double terminator. It is in the pSB1C3 backbone and the insert is 1839 bp long. Sequence confirmed.

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