Team:Utah State/Experiments
From 2009.igem.org
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<a href="https://2009.igem.org/Team:Utah_State/Introduction">Introduction</a><br /> | <a href="https://2009.igem.org/Team:Utah_State/Introduction">Introduction</a><br /> | ||
<a href="https://2009.igem.org/Team:Utah_State/Broad-HostVectors">Broad-Host Vectors</a><br /> | <a href="https://2009.igem.org/Team:Utah_State/Broad-HostVectors">Broad-Host Vectors</a><br /> | ||
- | <a href="https://2009.igem.org/Team:Utah_State/Secretion">Secretion</a> | + | <a href="https://2009.igem.org/Team:Utah_State/Secretion">Secretion</a><br /> |
- | <a href="https://2009.igem.org/Team:Utah_State/Experiments">Experiments</a> | + | <a href="https://2009.igem.org/Team:Utah_State/Experiments">Experiments</a><br /> |
- | <a href="https://2009.igem.org/Team:Utah_State/FutureWork">Future Work</a> | + | <a href="https://2009.igem.org/Team:Utah_State/FutureWork">Future Work</a><br /> |
- | <a href="https://2009.igem.org/Team:Utah_State/References">References</a> | + | <a href="https://2009.igem.org/Team:Utah_State/References">References</a><br /> |
</tr> | </tr> | ||
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<div align="center"><img src="https://static.igem.org/mediawiki/2009/8/82/PRL1383A_Plasmid_Map.jpg"" align = "middle" height="300" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /> </div> | <div align="center"><img src="https://static.igem.org/mediawiki/2009/8/82/PRL1383A_Plasmid_Map.jpg"" align = "middle" height="300" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /> </div> | ||
<div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | <div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | ||
- | <b>Figure | + | <b>Figure 1.</b> Plasmid map of pRL1383a |
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<div align="center"><img src="https://static.igem.org/mediawiki/2009/a/af/PCPP33_Plasmid_Map.jpg"" align = "middle" height="300" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /> </div> | <div align="center"><img src="https://static.igem.org/mediawiki/2009/a/af/PCPP33_Plasmid_Map.jpg"" align = "middle" height="300" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /> </div> | ||
<div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | <div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | ||
- | <b>Figure | + | <b>Figure 2.</b> Plasmid map of pCPP33 |
</div> | </div> | ||
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<p class="class">Apart from being shown effective in the Synechosystis PCC 6803 (Marraccini 1993), pRL1383a is an ideal candidate for use as a BioBrick-compatible broad-host range vector because the BioBrick restriction sites are absent within the vector sequence. To convert pRL1383a into a BioBrick format, the existing multiple cloning site, which is flanked by a BamHI site and a HindIII site, was utilized. First, modified primers were synthesized from BioBrick primers VR and VF2. These primers were modified by adding extra nucleotides to insert the desired restriction enzyme sites into the PCR product. A BamHI site was added to 5’ end of the forward primer (VF2) and a HindIII site was added to the 5’ end of the reverse primer (VR). These primers were used to amplify an existing, tested BioBrick part by PCR. For this purpose, we selected BBa_I20260 because it does not contain BamHI or HindIII sites, and successful ligation is readily testable as it is a GFP -producing construct. The addition of IPTG is typically necessary to induce GFP production in this particular device. However, when using Top10 <i>E. coli</i> cells it is produced continuously because these cells lack a lac repressor (insert invitrogen link). After cutting the vector at the multiple cloning site using BamHI and HindIII, the BioBrick insert obtained by PCR with modified ends was ligated into the backbone. The vector was then transformed using Top10 One Shot® chemically competent <i>E. coli</i> and tested for successful insertion using PCR and restriction digests.</p> | <p class="class">Apart from being shown effective in the Synechosystis PCC 6803 (Marraccini 1993), pRL1383a is an ideal candidate for use as a BioBrick-compatible broad-host range vector because the BioBrick restriction sites are absent within the vector sequence. To convert pRL1383a into a BioBrick format, the existing multiple cloning site, which is flanked by a BamHI site and a HindIII site, was utilized. First, modified primers were synthesized from BioBrick primers VR and VF2. These primers were modified by adding extra nucleotides to insert the desired restriction enzyme sites into the PCR product. A BamHI site was added to 5’ end of the forward primer (VF2) and a HindIII site was added to the 5’ end of the reverse primer (VR). These primers were used to amplify an existing, tested BioBrick part by PCR. For this purpose, we selected BBa_I20260 because it does not contain BamHI or HindIII sites, and successful ligation is readily testable as it is a GFP -producing construct. The addition of IPTG is typically necessary to induce GFP production in this particular device. However, when using Top10 <i>E. coli</i> cells it is produced continuously because these cells lack a lac repressor (insert invitrogen link). After cutting the vector at the multiple cloning site using BamHI and HindIII, the BioBrick insert obtained by PCR with modified ends was ligated into the backbone. The vector was then transformed using Top10 One Shot® chemically competent <i>E. coli</i> and tested for successful insertion using PCR and restriction digests.</p> | ||
- | <p class="class">Another broad host range vector, pCPP33, previously shown effective in Pseudomonas Putida,was standardized using similar methods. While the complete sequence of this plasmid is not available, it was shown that there are no BioBrick restriction sites outside the multiple cloning site (Figure | + | <p class="class">Another broad host range vector, pCPP33, previously shown effective in Pseudomonas Putida,was standardized using similar methods. While the complete sequence of this plasmid is not available, it was shown that there are no BioBrick restriction sites outside the multiple cloning site (Figure 2). The multiple cloning site of this vector is flanked by EcoRI and HindIII. This allowed the PCR product of BBa_I20260 to again be used by cutting with HindIII and EcoRI restriction enzymes. Restriction digests and gel analysis were used to test for the insert.</p> |
<b><i><font size="2.5" face="Helvetica, Arial, San Serif" color =#000033> | <b><i><font size="2.5" face="Helvetica, Arial, San Serif" color =#000033> | ||
- | Broad Host | + | Broad Host Conjugation |
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<p class="class">Because of the use of three different cells in our transformation procedure, the selection criteria for each component needed to be unique. In addition, we selected helper plasmids which had been known to work with the intended recipient cell.</p> | <p class="class">Because of the use of three different cells in our transformation procedure, the selection criteria for each component needed to be unique. In addition, we selected helper plasmids which had been known to work with the intended recipient cell.</p> | ||
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- | <div align="center"><img src="https://static.igem.org/mediawiki/igem.org/4/4a/PCPP33_tri-p_table.png" align = "middle" height=" | + | <div align="center"><img src="https://static.igem.org/mediawiki/igem.org/4/4a/PCPP33_tri-p_table.png" align = "middle" height="150" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /> </div> |
<div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | <div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | ||
<b>Table 1</b> Components and selection criteria used in conjugation with the broad-host vector PCPP33 | <b>Table 1</b> Components and selection criteria used in conjugation with the broad-host vector PCPP33 | ||
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- | <div align="center"><img src="https://static.igem.org/mediawiki/igem.org/f/f2/PRL1383A_tri-p_table.png" align = "middle" height=" | + | <div align="center"><img src="https://static.igem.org/mediawiki/igem.org/f/f2/PRL1383A_tri-p_table.png" align = "middle" height="150" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /> </div> |
<div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | <div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | ||
<b>Table 2</b> Components and selection criteria used in conjugation with the broad-host vector PRL1383A | <b>Table 2</b> Components and selection criteria used in conjugation with the broad-host vector PRL1383A | ||
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- | <div align="center"><img src="https://static.igem.org/mediawiki/2009/7/77/R_spaeroides_PCPP33.JPG" align = "left" height=" | + | <div align="center"><img src="https://static.igem.org/mediawiki/2009/7/77/R_spaeroides_PCPP33.JPG" align = "left" height="150" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /><img src="https://static.igem.org/mediawiki/2009/1/1e/P_putida_PCPP33.JPG" align = "left" height="150" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /><img src="https://static.igem.org/mediawiki/2009/d/da/Synechocystis_PCPP33.JPG" align = "left" height="150" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /> </div> |
<div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | <div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | ||
- | <b>Figure | + | <b>Figure 3.</b> Results of the tri-parental mating between pCPP33 and R. <i>sphaeroides</I>, P. <i>putida</i>, and Synechocystis sp., respectively. Each plate is shown alongside a negative control |
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<b><font size="2.5" face="Arial, Helvetica, San Serif" color =#231f20>Phasin:</font></b><br> | <b><font size="2.5" face="Arial, Helvetica, San Serif" color =#231f20>Phasin:</font></b><br> | ||
<p class="class"> | <p class="class"> | ||
- | The phasin (PhaP) sequence was isolated from the genomic DNA of Cupriavidus necator (also known as Ralstonia eutropha). There are four different phasin genes in the genomic DNA of this organism. This particular phasin was selected based on references in literature, although no information was acquired that indicated that one phasin gene would yield better production over another. The primers were designed so that the Silver-fusion prefix and suffix were overhanging, thereby resulting in a final product that is Silver-fusion compatible. The 579 bp phasin sequence was found to contain a PstI site. The PstI site was mutated using site-directed mutagenesis | + | The phasin (PhaP) sequence was isolated from the genomic DNA of Cupriavidus necator (also known as Ralstonia eutropha). There are four different phasin genes in the genomic DNA of this organism. This particular phasin was selected based on references in literature, although no information was acquired that indicated that one phasin gene would yield better production over another. The primers were designed so that the Silver-fusion prefix and suffix were overhanging, thereby resulting in a final product that is Silver-fusion compatible. The 579 bp phasin sequence was found to contain a PstI site. The PstI site was mutated using site-directed mutagenesis. Sequencing confirmed that this site was successfully removed. </p> |
<b><font size="2.5" face="Arial, Helvetica, San Serif" color =#231f20>GFP:</font></b><br> | <b><font size="2.5" face="Arial, Helvetica, San Serif" color =#231f20>GFP:</font></b><br> | ||
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- | A new Silver-Fusion compatible GFP BioBrick part was constructed for this project via a similar mechanism as the phasin construct. This particular GFP was previously mutated for improved fluorescence photostability (Crameri, 1996). The excitation and emission wavelengths for this GFP are 395 nm and 501 nm, respectively. That being said, GFP-positive cells emit a bright green fluorescence when exposed to shorter-wavelength UV light, such as on a transilluminator. Primers were synthesized for isolation of the sequence and, like the phasin-specific primers, designed so that the Silver-fusion prefix and suffix were inserted on the ends of the sequence (see primers). Figure | + | A new Silver-Fusion compatible GFP BioBrick part was constructed for this project via a similar mechanism as the phasin construct. This particular GFP was previously mutated for improved fluorescence photostability (Crameri, 1996). The excitation and emission wavelengths for this GFP are 395 nm and 501 nm, respectively. That being said, GFP-positive cells emit a bright green fluorescence when exposed to shorter-wavelength UV light, such as on a transilluminator. Primers were synthesized for isolation of the sequence and, like the phasin-specific primers, designed so that the Silver-fusion prefix and suffix were inserted on the ends of the sequence (see primers). Figure 4 shows GFP- Top10 <i>E. coli</i> colonies (left) and unfused GFP+ Top10 <i>E. coli</i> colonies (right). This figure shows that the GFP construct is functional and easily detectable.</p><br> |
<div align="center"><img src="https://static.igem.org/mediawiki/2009/9/93/GFPglowingUSU.jpg"" align = "middle" height="200" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /> </div> | <div align="center"><img src="https://static.igem.org/mediawiki/2009/9/93/GFPglowingUSU.jpg"" align = "middle" height="200" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /> </div> | ||
<div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | <div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | ||
- | <b>Figure | + | <b>Figure 4.</b> Plate with GFP- cells (left) next to plate with GFP+ cells(right) |
</div> | </div> | ||
<br><b><font size="2.5" face="Arial, Helvetica, San Serif" color =#231f20>Bioplastic Production:</font></b><br> | <br><b><font size="2.5" face="Arial, Helvetica, San Serif" color =#231f20>Bioplastic Production:</font></b><br> | ||
- | <p class="class">A plasmid harboring the genes for PHB production (pBHR68) was used in these experiments. This plasmid contains the sequence for ampicillin resistance and contains a ColE1 origin of replication. <i>E. coli</i> harboring pBHR68 were cultured according to methods outlined by Kang et al (2008) and production of PHB was verified using 1H NMR analysis. The spectrum obtained from this experiment is given as Figure | + | <p class="class">A plasmid harboring the genes for PHB production (pBHR68) was used in these experiments. This plasmid contains the sequence for ampicillin resistance and contains a ColE1 origin of replication. <i>E. coli</i> harboring pBHR68 were cultured according to methods outlined by Kang et al (2008) and production of PHB was verified using 1H NMR analysis. The spectrum obtained from this experiment is given as Figure 5. The observed peaks at 1.24 ppm, 2.54 ppm, and 5.2 ppm correspond with those observed in standard polyhydroxyalkanaote samples.</p> |
<Br> | <Br> | ||
<div align="center"><img src="https://static.igem.org/mediawiki/2009/4/43/NMRusu.jpg"" align = "middle" height="200" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /> </div> | <div align="center"><img src="https://static.igem.org/mediawiki/2009/4/43/NMRusu.jpg"" align = "middle" height="200" style="padding:.5px; border-style:solid; border-color:#999" alt="Team USU" /> </div> | ||
<div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | <div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | ||
- | <b>Figure | + | <b>Figure 5.</b> Proton NMR spectra for PHB production in recombinant <i>E. coli</i> |
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<b><font size="2.5" face="Arial, Helvetica, San Serif" color =#231f20>SDS-PAGE Analysis</font></b><br> | <b><font size="2.5" face="Arial, Helvetica, San Serif" color =#231f20>SDS-PAGE Analysis</font></b><br> | ||
- | <p class="class">Sodium dodecyl sulfate polyacrylamide gel electrophoresis was used to analyze the protein content in transformed E. coli. As a positive control, E. coli containing the Lac/RBS/GFP/Terminator (BBa_K208045) construct were sonicated and centrifuged (see Figure | + | <p class="class">Sodium dodecyl sulfate polyacrylamide gel electrophoresis was used to analyze the protein content in transformed E. coli. As a positive control, E. coli containing the Lac/RBS/GFP/Terminator (BBa_K208045) construct were sonicated and centrifuged (see Figure 6). Additionally, E. coli cells containing an individual BioBrick part (BBa_B0015) were analyzed as a negative control. The resulting gel was stained with coomassie blue and is shown as Figure 6. The bright band at 27 kD in the GFP+ sample corresponds to the GFP protein (Bio-Rad). The absence of this band in the GFP- sample further reinforces the functionality of the GFP construct.</p> |
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<div align="center"><img src="https://static.igem.org/mediawiki/2009/d/d1/GFP_gel.png"" align = "middle" height="400" style="padding:.5px; alt="Team USU" /> </div> | <div align="center"><img src="https://static.igem.org/mediawiki/2009/d/d1/GFP_gel.png"" align = "middle" height="400" style="padding:.5px; alt="Team USU" /> </div> | ||
<div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | <div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | ||
- | <b>Figure | + | <b>Figure 6.</b> Protein gel showing a strong band corresponding to GFP |
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- | <p class="class">The geneIII secretion signal sequence fused to the phasin protein was expressed in E. coli cells. The E. coli cells were grown overnight in LB growth media and centrifuged to pellet the cells. Supernatants (5ml) were then concentrated using a Centricon Centriplus concentrator (Amicon, Beverly MA). This process concentrated proteins that were larger than 10kDa and removed molecules smaller than 10kDa. Approximately 20ug of protein were then applied to a SDS polyacrylamide gel to separate the proteins according to size. The gel was then stained with coomassie blue for protein detection, as shown in Figure | + | <p class="class">The geneIII secretion signal sequence fused to the phasin protein was expressed in E. coli cells. The E. coli cells were grown overnight in LB growth media and centrifuged to pellet the cells. Supernatants (5ml) were then concentrated using a Centricon Centriplus concentrator (Amicon, Beverly MA). This process concentrated proteins that were larger than 10kDa and removed molecules smaller than 10kDa. Approximately 20ug of protein were then applied to a SDS polyacrylamide gel to separate the proteins according to size. The gel was then stained with coomassie blue for protein detection, as shown in Figure 7. Following SDS polyacylamide gel electrophoresis (PAGE) and subsequent coomassie blue staining of the separated proteins, a protein with an approximate size of 22kDA is observed in the sample from the phasin-expressing E. coli cells that is not present in the control E. coli sample. The phasin protein has been reported by others to migrate on SDS PAGE from 14-28kDa (Pötter, 2002; York, 2002). These results indicate that the GeneIII::phasin expression construct is being produced by the E. coli cells and is being secreted outside the cell into the media.</p> |
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<div align="center"><img src="https://static.igem.org/mediawiki/2009/3/3e/PHB_gel.png"" align = "middle" height="250" style="padding:.5px; alt="Team USU" /> </div> | <div align="center"><img src="https://static.igem.org/mediawiki/2009/3/3e/PHB_gel.png"" align = "middle" height="250" style="padding:.5px; alt="Team USU" /> </div> | ||
<div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | <div align="center"><font size="2.5" face="Helvetica, Arial, San Serif" color =#231f20> | ||
- | <b>Figure | + | <b>Figure 7.</b> Protein gel showing the presence of phasin protein in supernatant samples (third well from left)<br> next to supernatant from an <i>E. coli</i> sample without a phasin-producing construct. |
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- | <p class="class">Western blotting with phasin-specific antibodies was performed to verify the observed band as phasin. | + | <p class="class">Western blotting with phasin-specific antibodies was performed to verify the observed band as phasin. Phasin antibody was kindly provided by Anthony J. Sinskey at Massachusetts Institute of Technology. The results of the western blotting were inconclusive. Non-specific binding to larger constructs was observed. Additional testing is required to further reinforce preliminary findings and confirm the secretion of phasin. The secretion of phasin would provide evidence that PHA recovery via phasin secretion is possible. Addtionally, this would reinforce that the constructed BioBricks are not only functional, but would be beneficial for use in other studies. </p> |
Latest revision as of 04:29, 12 November 2009
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