Difference between revisions of "Team:Chalmers-Gothenburg/Project/constructs"

Latest revision as of 15:59, 30 October 2017

Chalmers Gothenburg iGEM 2017

Introduction

In this section all constructs used in the project are summarized. Assembly of fragments was accomplished with Gibson assembly, PCR overlaps with primers containing overhangs and homologous recombination in yeast, which often worked best. The DNA fragments were designed in Snapgene and Benchling. Primer design included use of software from NEBuilders, such as the Tm-Calculator. The DNA fragments where ordered from IDT, ATUM and Genscript. In addition primers were ordered from Eurofins.

Incorporation of GPCRs in the genome

The Cas9 vector

The vector contains the gene for Cas9 and markers for ampicillin and kanamycin, as shown in Figure 1.

**Figure 1.** Cas9-vector which contains the gene for Cas9 and the markers ampicillin and kanamycin.

gRNA constructs

The constructs contain gRNA able to cut STE2 and STE3 respectively. In both constructs, a P_SNR52 promoter, a gRNA scaffold and a T_SUP4 terminator are included. The construct used for cutting STE2 is shown in Figure 2, and the construct used for cutting STE3 in Figure 3.

**Figure 2.** gRNA construct for deletion of *STE2*.

**Figure 3.** gRNA construct for deletion of *STE3*.

GPCR constructs

Ri7

The Ri7 construct consists of the gene for Ri7, a P_TEF1 promoter, a T_CYC1 terminator and two sequences overlapping with the upstream and downstream regions of STE2 which makes it possible to use homologous recombination for integration. See Figure 4.

**Figure 4.** Ri7 construct with the P_TEF1 promotor and the Ri7 gene, a terminator and overlaps with the sequences surrounding *STE2*.

Olfr1258

The Olfr1258 construct is similar to the Ri7 construct and consists of the gene for Olfr1258, a P_TEF1 promoter, a T_CYC1 terminator and two sequences overlapping with the upstream and downstream regions of STE3 which makes it possible to use homologous recombination for integration. See Figure 5.

Switch constructs

The switch consists of a promoter flanked by two mutated loxP regions. After activation of the pheromone pathway by VOCs, the P_FUS1 promoter transcribes the Cre-recombinase which switches the orientation of the promoter. The promoter switch causes the transcription of either the gRNA or the Cas9 depending on the gene of interest.

Cre-Cas9 construct

The construct contains the genes for Cre-recombinase, GFP and Cas9. The Cre-recombinase is activated by the pheromone pathway, transcribed under the P_FUS1 promoter and terminated by the T_CYC1 terminator, see Figure 6.

To ensure expression of Cas9 only when the VOC is present, Cre-recombinase and loxP-sites are used. The P_FUS1 promoter is only activated when the pheromone pathway is activated by VOC binding to the GPCR. This means that Cre-recombinase is only active and can invert the P_TEF1 promoter when VOC’s are present. The loxP-sites are mutated to ensure that once the switch is flipped, it can not go back to its original orientation and Cas9 is constantly expressed. If the P_TEF1 promoter is not inverted due to the lack of Cre-recombinase GFP will be transcribed instead. In that way one can determine whether the flip of promoter worked or not. The GFP and Cas9 are followed by the terminators T_ADH1 and T_FBA1 respectively.

The gblocks where ordered from IDT technologies and therefore the constructs where order in sizes in 1000 bp with overlaps. At the ends of the construct there is overlaps with the pRS416 that was used for transformation into yeast. pRS416 contains a URA3 marker, see Figure 7.

**Figure 7.** pRS416 containing a *URA3* marker.

Cre-gRNA construct

The construct contains the genes for Cre recombinase, mCherry and gRNA for disruption of ADE2. The Cre recombinase is transcribed under the P_FUS1 promoter, activated by the pheromone pathway and terminated by the T_CYC1 terminator, see Figure 8.

In order to guarantee expression of gRNA only when the VOC is present, Cre recombinase and loxP-sites are used in this construct as well. Cre-recombinase is only active and can invert the P_SNR52 promoter when VOC’s are present. P_SNR52 enables transcription of, but not translation of RNA and is therefore used for creating gRNAs. The loxP-sites in this construct are mutated, loxPLE and loxPRE, in order to ensure that once the switch is flipped, it can not go back to its original direction and the gRNA is constantly expressed. A ribozyme is incorporated upstream of the gRNA in order to remove the loxP from the finished gRNA.

Like the Cre-Cas9 construct, the team wanted to insert a fluorescence marker in this construct. Due to the fact that P_SNR52 can not transcribe mRNA and therefore in order to ensure the expression of mCherry, a second promoter, P_TEF1 is added between the loxP-site together with P_SNR52, as can be seen in Figure 8. Only when the loxP-site is inverted, both gRNA and the mCherry will be transcribed. When the promoters are in the initial direction no fluorescence can be seen. However, the inversion of the promoter enables the expression of mCherry and a red fluorescence marker can be seen.

At the ends of the construct there are overlaps with pRS413. The plasmid pRS413 contains a HIS3 marker, the plasmid is illustrated in Figure 9. This construct was ordered from IDT in gblocks of 1000 bp with overlap of the parts.

**Figure 9.** The plasmid pRS413 containing a *HIS3* marker.

Testing-constructs

Several constructs were created in order to use for verification of functionality of the GPCRs. Fusion-GPCRs were designed in order to investigate the localization of the GPCR’s. Fusion GPCR’s were designed for both Ri7 and Olfr1258. In addition, a plasmid containing GFP under the P_FUS1 promoter was designed. This was done in order to investigate the ability of the GPCRs to bind the VOCs, initiate the MAPK pathway and activate the P_FUS1 promoter.

Fusion-GPCRs

In order to determine where the GPCRs were localized, fusion proteins were created. The genes for the GPCRs were connected with the gene for GFP using a small bridge of four amino acids, three glycine and one serine on the N-terminal, see Figure 10 and 11. The fusion GPCRs, Olfr1258 and Ri7, were put together with primers and the templates used were the existing construct of GPCRs and Cas9.

**Figure 10.** Fusion protein of Ri7 coupled to GFP.

**Figure 11.** Fusion protein of Olfr1258 coupled to GFP.

pGFP

This construct was created to see if the binding of VOCs to the GPCRs correctly enables the P_FUS1 promoter to express a gene. The construct encodes for a GFP gene under the control of the P_FUS1 promoter, see Figure 12. If a VOC binds to the corresponding GPCR the pheromone pathway should be initiated which should induce the P_FUS1 promoter. The construct can be transformed into a strain with either GPCR.

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                <a href="https://2017.igem.org/Team:Chalmers-Gothenburg/InterLab">Interlab study</a>
                <hr>
-               <a href="https://2017.igem.org/Team:Chalmers-Gothenburg/Achievements/medal">Medals</a>
+               <a href="https://2017.igem.org/Team:Chalmers-Gothenburg/Achievements/medal">Accomplishments</a>
              </div>
            </li>
@@ Line 1,627: / Line 1,363: @@
-         <div class="header_Project_theory">
+         <div class="header_test">
-    <div class="header-text">PROJECT</div>
+	   <!-- Banner -->
-    <div class="header-subtitle">Constructs</div>
+	    <div id="banner">
-    </div>
+             <h3>Constructs</h3>
+            </div>
+        </div>
@@ Line 1,641: / Line 1,376: @@
            <nav>
              <a href="#intro" class="active">Introduction</a>
-             <a href="#background">Title 1</a>
+             <a href="#incorporation">Incorporation of GPCRs </a>
-             <a href="#biosensor">Title2</a>
+             <a href="#GPCR">GPCR constructs</a>
-             <a class="sub-level" href="#signal">Subtitle 1</a>
+             <a href="#switch">Switch constructs</a>
+            <a href="#test">Testing-constructs</a>
            </nav>
          </div>
@@ Line 1,655: / Line 1,391: @@
          <div class="dashed_line_left_first">
             <h4 class="subtitle">Introduction</h4>
           <p class="text">
-Pellentesque habitant morbi tristique senectus
+In this section all constructs used in the project are summarized. Assembly of fragments was accomplished with Gibson assembly, PCR overlaps with primers containing overhangs and homologous recombination in yeast, which often worked best. The DNA fragments were designed in Snapgene and Benchling. Primer design included use of software from NEBuilders, such as the Tm-Calculator. The DNA fragments where ordered from IDT, ATUM and Genscript. In addition primers were ordered from Eurofins.
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           </p>
             </div>
           </div>
+          <div class="target" id="incorporation">
-          <div class="target" id="background">
           <div class="dashed_line_right">
-          <h4 class="sidetitle">Title 1</h4>
+          <h4 class="subtitle">Incorporation of GPCRs in the genome</h4>
+          <h2 class="h2style">The Cas9 vector</h2>
           <p class="text">
-         Pellentesque habitant morbi tristique senectus
+The vector contains the gene for Cas9 and markers for ampicillin and kanamycin, as shown in Figure 1.
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+            </p>
-        mattis interdum. Aliquam et velit fermentum velit imperdiet
-        rhoncus. Donec accumsan molestie ornare. Duis eu odio in tortor
+         <figure>
-        ullamcorper aliquam. Vivamus molestie fermentum urna, vitae
+<img src="https://static.igem.org/mediawiki/2017/f/f1/T--Chalmers-Gothenburg--cas9-vector_map.png" style="height:563px; width:507px;">
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+<figcaption><b>Figure 1.</b> Cas9-vector which contains the gene for Cas9 and the markers ampicillin and kanamycin.
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+</figcaption>
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+</figure>
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-        tristique sapien. Suspendisse eget facilisis dolor. Integer congue
-        nisi eu magna consectetur, a bibendum nibh accumsan. Vivamus
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-        metus quam, dapibus ac volutpat ut, dapibus sit amet felis.           </p>
             </div>
        <div class="dashed_line_left">
-           <p class="text">
+           <h2 class="h2style">gRNA constructs</h2>
-Pellentesque habitant morbi tristique senectus
+         <p class="text">
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+The constructs contain gRNA able to cut <i>STE2</i> and <i>STE3</i> respectively. In both constructs, a P<sub><i>SNR52</i></sub> promoter, a gRNA scaffold and a T<sub><i>SUP4</i></sub> terminator are included. The construct used for cutting <i>STE2</i> is shown in Figure 2, and the construct used for cutting <i>STE3</i> in Figure 3.
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+            </p>
-        rhoncus. Donec accumsan molestie ornare. Duis eu odio in tortor
-        ullamcorper aliquam. Vivamus molestie fermentum urna, vitae
+         <figure>
-        commodo mauris consequat in. Curabitur porttitor pulvinar purus,
+<img src="https://static.igem.org/mediawiki/2017/a/aa/T--Chalmers-Gothenburg--gRNA-STE2_Map.png" style="height:217px; width:781px;">
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+<figcaption><b>Figure 2.</b> gRNA construct for deletion of <i>STE2</i>.
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+</figcaption>
-        vel semper. Nullam in turpis eleifend, venenatis ex tincidunt,
+</figure>
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-        nisi eu magna consectetur, a bibendum nibh accumsan. Vivamus
-        fermentum metus id lectus porttitor congue. Pellentesque habitant morbi
+         <figure>
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+<img src="https://static.igem.org/mediawiki/2017/9/95/T--Chalmers-Gothenburg--gRNA-STE3_Map.png" style="height:217px; width:781px;">
-        metus quam, dapibus ac volutpat ut, dapibus sit amet felis.
+<figcaption><b>Figure 3.</b> gRNA construct for deletion of <i>STE3</i>.
-         </p>
+</figcaption>
-         <p class="text">
+</figure>
-Pellentesque habitant morbi tristique senectus
+          </div>
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+         </div>
-        mattis interdum. Aliquam et velit fermentum velit imperdiet
-        rhoncus. Donec accumsan molestie ornare. Duis eu odio in tortor
+         <div class="target" id="GPCR">
-        ullamcorper aliquam. Vivamus molestie fermentum urna, vitae
-        commodo mauris consequat in. Curabitur porttitor pulvinar purus,
-        ut varius nibh tempus id. Nulla dictum lectus ut erat condimentum,
-        sit amet euismod nibh eleifend. Maecenas molestie efficitur urna
-        vel semper. Nullam in turpis eleifend, venenatis ex tincidunt,
-        tristique sapien. Suspendisse eget facilisis dolor. Integer congue
-        nisi eu magna consectetur, a bibendum nibh accumsan. Vivamus
-        fermentum metus id lectus porttitor congue. Pellentesque habitant morbi
-        tristique senectus et netus et malesuada fames ac turpis egestas. Nulla
-        metus quam, dapibus ac volutpat ut, dapibus sit amet felis.
-        </div>
         <div class="dashed_line_right">
+         <h4 class="subtitle">GPCR constructs</h4>
+          <h2 class="h2style">Ri7</h2>
+         <p class="text">
+The Ri7 construct consists of the gene for Ri7, a P<sub><i>TEF1</i></sub> promoter, a T<sub><i>CYC1</i></sub> terminator and two sequences overlapping with the upstream and downstream regions of <i>STE2</i> which makes it possible to use homologous recombination for integration. See Figure 4.
           </p>
+         <figure>
+<img src="https://static.igem.org/mediawiki/2017/c/cf/T--Chalmers-Gothenburg--Ri7_Map.png" style="height:217px; width:781px;">
+<figcaption><b>Figure 4.</b> Ri7 construct with the P<sub><i>TEF1</i></sub> promotor and the Ri7 gene, a terminator and overlaps with the sequences surrounding <i>STE2</i>.
+</figcaption>
+</figure>
+          <h2 class="h2style">Olfr1258</h2>
           <p class="text">
-Pellentesque habitant morbi tristique senectus
+The Olfr1258 construct is similar to the Ri7 construct and consists of the gene for Olfr1258, a P<sub><i>TEF1</sub></i> promoter, a T<sub><i>CYC1</i></sub> terminator and two sequences overlapping with the upstream and downstream regions of <i>STE3</i> which makes it possible to use homologous recombination for integration. See Figure 5.
-        et netus et malesuada fames ac turpis egestas. Sed consequat
-        mattis interdum. Aliquam et velit fermentum velit imperdiet
-        rhoncus. Donec accumsan molestie ornare. Duis eu odio in tortor
-        ullamcorper aliquam. Vivamus molestie fermentum urna, vitae
-        commodo mauris consequat in. Curabitur porttitor pulvinar purus,
-        ut varius nibh tempus id. Nulla dictum lectus ut erat condimentum,
-        sit amet euismod nibh eleifend. Maecenas molestie efficitur urna
-        vel semper. Nullam in turpis eleifend, venenatis ex tincidunt,
-        tristique sapien. Suspendisse eget facilisis dolor. Integer congue
-        nisi eu magna consectetur, a bibendum nibh accumsan. Vivamus
-        fermentum metus id lectus porttitor congue. Pellentesque habitant morbi
-        tristique senectus et netus et malesuada fames ac turpis egestas. Nulla
-        metus quam, dapibus ac volutpat ut, dapibus sit amet felis.
           </p>
+         <figure>
+<img src="https://static.igem.org/mediawiki/2017/b/b9/T--Chalmers-Gothenburg--olfr1258_Map.png" style="height:217px; width:781px;">
+<figcaption><b>Figure 5.</b> Olfr1258 construct with the P<sub><i>TEF1</i></sub> promotor and the Olfr1258 gene, a terminator and overlaps with the sequences surrounding <i>STE3</i>.
+</figcaption>
+</figure>
          </div>
-         </div>
+      </div>
-          <div class="target" id="biosensor">
+          <div class="target" id="switch">
           <div class="dashed_line_left">
-            <h4 class="sidetitle">Title 2</h4>
+            <h4 class="sidetitle">Switch constructs</h4>
           <p class="text">
-Pellentesque habitant morbi tristique senectus
+The switch consists of a promoter flanked by two mutated loxP regions. After activation of the pheromone pathway by VOCs, the P<sub><i>FUS1</i></sub> promoter transcribes the Cre-recombinase which switches the orientation of the promoter. The promoter switch causes the transcription of either the gRNA or the Cas9 depending on the gene of interest.
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-        rhoncus. Donec accumsan molestie ornare. Duis eu odio in tortor
-        ullamcorper aliquam. Vivamus molestie fermentum urna, vitae
-        commodo mauris consequat in. Curabitur porttitor pulvinar purus,
-        ut varius nibh tempus id. Nulla dictum lectus ut erat condimentum,
-        sit amet euismod nibh eleifend. Maecenas molestie efficitur urna
-        vel semper. Nullam in turpis eleifend, venenatis ex tincidunt,
-        tristique sapien. Suspendisse eget facilisis dolor. Integer congue
-        nisi eu magna consectetur, a bibendum nibh accumsan. Vivamus
-        fermentum metus id lectus porttitor congue. Pellentesque habitant morbi
-        tristique senectus et netus et malesuada fames ac turpis egestas. Nulla
-        metus quam, dapibus ac volutpat ut, dapibus sit amet felis.
           </p>
+          <h2 class="h2style">Cre-Cas9 construct</h2>
+         <p class="text">
+The construct contains the genes for Cre-recombinase, GFP and Cas9. The Cre-recombinase is activated by the pheromone pathway, transcribed under the P<sub><i>FUS1</i></sub> promoter and terminated by the T<sub><i>CYC1</i></sub> terminator,  see Figure 6.
+         </p>
+         <figure>
+<img src="https://static.igem.org/mediawiki/2017/4/45/T--Chalmers-Gothenburg--CreCas9_Map.png" style="height:217px; width:781px;">
+<figcaption><b>Figure 6.</b> Map of the whole Cre-Cas9 construct.
+</figcaption>
+</figure>
+         <p class="text">
+To ensure expression of Cas9 only when the VOC is present, Cre-recombinase and loxP-sites are used. The P<sub><i>FUS1</i></sub> promoter is only activated when the pheromone pathway is activated by VOC binding to the GPCR. This means that Cre-recombinase is only active and can invert the P<sub><i>TEF1</i></sub> promoter when VOC’s are present. The loxP-sites are mutated to ensure that once the switch is flipped, it can not go back to its original orientation and Cas9 is constantly expressed. If the P<sub><i>TEF1</sub></i> promoter is not inverted due to the lack of Cre-recombinase GFP will be transcribed instead. In that way one can determine whether the flip of promoter worked or not. The GFP and Cas9 are followed by the terminators T<sub><i>ADH1</i></sub> and T<sub><i>FBA1</i></sub> respectively.
+         </p>
+         <p class="text">
+The gblocks where ordered from IDT technologies and therefore the constructs where order in sizes in 1000 bp with overlaps. At the ends of the construct there is overlaps with the pRS416 that was used for transformation into yeast. pRS416 contains a <i>URA3</i> marker, see Figure 7.
+         </p>
+         <figure>
+<img src="https://static.igem.org/mediawiki/2017/1/1a/T--Chalmers-Gothenburg--pRS416_Map.png" style="height:563px; width:507px;">
+<figcaption><b>Figure 7.</b> pRS416 containing a <i>URA3</i> marker.
+</figcaption>
+</figure>
+           </div>
+         <div class="dashed_line_right">
+          <h2 class="h2style">Cre-gRNA construct</h2>
+         <p class="text">
+The construct contains the genes for Cre recombinase, mCherry and gRNA for disruption of <i>ADE2</i>. The Cre recombinase is transcribed under the P<sub><i>FUS1</i></sub> promoter, activated by the pheromone pathway and terminated by the T<sub><i>CYC1</sub></i> terminator, see Figure 8.
+         </p>
+         <figure>
+<img src="https://static.igem.org/mediawiki/2017/2/24/T--Chalmers-Gothenburg--Cre-gRNA_construct.png" style="height:217px; width:781px;">
+<figcaption><b>Figure 8.</b> The Cre-gRNA construct.
+</figcaption>
+</figure>
+         <p class="text">
+In order to guarantee expression of gRNA only when the VOC is present, Cre recombinase and loxP-sites are used in this construct as well. Cre-recombinase is only active and can invert the P<sub><i>SNR52</i></sub> promoter when VOC’s are present. P<sub><i>SNR52</i></sub> enables transcription of,  but not translation of RNA and is therefore used for creating gRNAs. The loxP-sites in this construct are mutated, loxPLE and loxPRE, in order to ensure that once the switch is flipped, it can not go back to its original direction and the gRNA is constantly expressed. A ribozyme is incorporated upstream of the gRNA in order to remove the loxP from the finished gRNA.
+         </p>
+         <p class="text">
+Like the Cre-Cas9 construct, the team wanted to insert a fluorescence marker in this construct. Due to the fact that P<sub><i>SNR52</i></sub> can not transcribe mRNA and therefore in order to ensure the expression of mCherry, a second promoter, P<sub><i>TEF1</i></sub> is added between the loxP-site together with P<sub><i>SNR52</i></sub>, as can be seen in Figure 8. Only when the loxP-site is inverted, both gRNA and the mCherry will be transcribed. When the promoters are in the initial direction no fluorescence can be seen. However, the inversion of the promoter enables the expression of mCherry and a red fluorescence marker can be seen.
+         </p>
+         <p class="text">
+At the ends of the construct there are overlaps with pRS413. The plasmid pRS413 contains a <i>HIS3</i> marker, the plasmid is illustrated in Figure 9. This construct was ordered from IDT in gblocks of 1000 bp with overlap of the parts.
+         </p>
+         <figure>
+<img src="https://static.igem.org/mediawiki/2017/0/0f/T--Chalmers-Gothenburg--pRS413_Map.png" style="height:563px; width:507px;">
+<figcaption><b>Figure 9.</b> The plasmid pRS413 containing a <i>HIS3</i> marker.
+</figcaption>
+</figure>
             </div>
           </div>
-         <div class="target" id="signal">
+         <div class="target" id="test">
-         <div class="dashed_line_right_last">
+         <div class="dashed_line_left_last">
-          <h2 class="h2style">Subtitle 1</h2>
+           <h4 class="sidetitle">Testing-constructs</h4>
            <p class="text">
-Pellentesque habitant morbi tristique senectus
+Several constructs were created in order to use for verification of functionality of the GPCRs. Fusion-GPCRs were designed in order to investigate the localization of the GPCR’s.  Fusion GPCR’s were designed for both Ri7 and Olfr1258.  In addition, a plasmid containing GFP under the P<sub><i>FUS1</i></sub> promoter was designed. This was done in order to investigate the ability of the GPCRs to bind the VOCs, initiate the MAPK pathway and activate the P<sub><i>FUS1</i></sub> promoter.
-        et netus et malesuada fames ac turpis egestas. Sed consequat
-        mattis interdum. Aliquam et velit fermentum velit imperdiet
-        rhoncus. Donec accumsan molestie ornare. Duis eu odio in tortor
-        ullamcorper aliquam. Vivamus molestie fermentum urna, vitae
-        commodo mauris consequat in. Curabitur porttitor pulvinar purus,
-        ut varius nibh tempus id. Nulla dictum lectus ut erat condimentum,
-        sit amet euismod nibh eleifend. Maecenas molestie efficitur urna
-        vel semper. Nullam in turpis eleifend, venenatis ex tincidunt,
-        tristique sapien. Suspendisse eget facilisis dolor. Integer congue
-        nisi eu magna consectetur, a bibendum nibh accumsan. Vivamus
-        fermentum metus id lectus porttitor congue. Pellentesque habitant morbi
-        tristique senectus et netus et malesuada fames ac turpis egestas. Nulla
-        metus quam, dapibus ac volutpat ut, dapibus sit amet felis.
             </p>
+           <h2 class="h2style">Fusion-GPCRs</h2>
+          <p class="text">
+In order to determine where the GPCRs were localized, fusion proteins were created. The genes for the GPCRs were connected with the gene for GFP using a small bridge of four amino acids, three glycine and one serine on the N-terminal, see Figure 10 and 11. The fusion GPCRs, Olfr1258 and Ri7, were put together with primers and the templates used were the existing construct of GPCRs and Cas9.
+           </p>
+         <figure>
+<img src="https://static.igem.org/mediawiki/2017/b/bc/T--Chalmers-Gothenburg--Ri7-GFP_construct_Map.png" style="height:217px; width:781px;">
+<figcaption><b>Figure 10.</b> Fusion protein of Ri7 coupled to GFP.
+</figcaption>
+</figure>
+         <figure>
+<img src="https://static.igem.org/mediawiki/2017/f/f5/T--Chalmers-Gothenburg--olfr1258-GFP_Map.png" style="height:217px; width:781px;">
+<figcaption><b>Figure 11.</b> Fusion protein of Olfr1258 coupled to GFP.
+</figcaption>
+</figure>
+           <h2 class="h2style">pGFP</h2>
+          <p class="text">
+This construct was created to see if the binding of VOCs to the GPCRs correctly enables the P<sub><i>FUS1</i></sub> promoter to express a gene. The construct encodes for a GFP gene under the control of the P<sub><i>FUS1</i></sub> promoter, see Figure 12. If a VOC binds to the corresponding GPCR the pheromone pathway should be initiated which should induce the P<sub><i>FUS1</i></sub> promoter. The construct can be transformed into a strain with either GPCR.
+           </p>
+         <figure>
+<img src="https://static.igem.org/mediawiki/2017/e/ee/T--Chalmers-Gothenburg--pGFP_Map.png" style="height:563px; width:507px;">
+<figcaption><b>Figure 12.</b> pGFP containing GFP and the markers <i>HIS3</i> and ampicillin.
+</figcaption>
+</figure>
               </div>
          </div>
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              <img src="https://static.igem.org/mediawiki/2017/a/a3/T--Chalmers-Gothenburg--IDT_gray.png" alt="IDT" class="footerimg on">
              <img src="https://static.igem.org/mediawiki/2017/f/fd/T--Chalmers-Gothenburg--IDT.png" alt="IDT" class="footerimg off">
+          </a>
+        </div>
+        <div class="footerlogo">
+          <a href="http://www.chalmers.se/en/areas-of-advance/lifescience/Pages/default.aspx" target="_blank">
+            <img src="https://static.igem.org/mediawiki/2017/6/6e/T--Chalmers-Gothenburg--Life_science_gray.png" alt="ATUM" class="footerimg on">
+            <img src="https://static.igem.org/mediawiki/2017/a/a3/T--Chalmers-Gothenburg--Life_science.png" alt="ATUM" class="footerimg off">
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          <a href="https://www.instagram.com/chalmersigem/" target="_blank">instagram</a>
        </div>
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+     </footer> <!--------------------------------- footer_170726.html STOP ---------------------------------->  </body>
-  </body>