Difference between revisions of "Team:SDU-Denmark/Tour54"

 
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<p> <i> "In a dark place we find ourselves, and a little more knowledge lights our way." - <b>George Lucas</b></i></p>
  
 
<h1 align="center"> Interlab study </h1>
 
<h1 align="center"> Interlab study </h1>
  
 
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<a class="popupImg alignLeft" style="width:230px" target="_blank" href="https://static.igem.org/mediawiki/2015/0/07/SDU2015_InterlabStudy_big.png" title="">
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<span class="intro">Our team has been participating</span> in the iGEM <a href="https://2015.igem.org/Tracks/Measurement/Interlab_study" target="_blank">Interlab Study</a>, to help further characterize three different promoters. This was done by using GFP-fluorescence as a way of measuring how strong each of the promoters are compared to each other.
   <img src="https://static.igem.org/mediawiki/2015/7/74/SDU2015_InterlabStudy_thumbnail.png" style="width:230px"/>
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    <b> Figure 1:</b> 
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<span class="intro">We have participated in the iGEM interlabstudy.</span>
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<div class="thumbinner" style="width:255px;height:335px;">
The focus of this study were to characterize three different promoters, using a gene encoding GFP.
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<a class="popupImg alignRight" style="width:250px" target="_blank" href="https://static.igem.org/mediawiki/2015/e/ef/SDU2015_InterlabStudy_GFP.png" title="">
GFP is the reporter protein of choice, as it has a low folding time, and can be quantified through fluorescence, instead of RNA.
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   <img src="https://static.igem.org/mediawiki/2015/3/3d/SDU2015_InterlabStudy_GFP_thumbnail.png" style="width:250px"/> </a>
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<div class="thumbcaption">Figure 1:The three constructs made for this experiment.
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Our biobricks were assembled through standard biobrick assembly.
 
  
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</span class="intro">The three constructs</span> were made through standard biobrick assembly, inserting GFP into plasmids containing different promoters.
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<span class="intro">The three constructs were made</span> through iGEM standard biobrick assembly, inserting <i>gfp</i> into pSB1C3 plasmids containing the different promoters. The <i>gfp</i>-gene were originally cut out of pSB1A2, before ligation with each of the three promotes. Transformation of the constructs was done into <i>E. coli</i> K12 Top10, because it has been optimized for transformation and high levels of plasmid synthetisati<span class="sourceReference">on</span>.
The final construct were transformed into <i>E. coli</i> K12 TOP10.
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<span class="tooltip">
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  <span class="tooltipHeader">Reference:</span>One Shot® Top10 Chemically Competent <i>E. coli</i>. Catalog number: C4040-10. Visited: 17.09.15.<a target="_blank" href="https://www.thermofisher.com/order/catalog/product/C404010 "> [ThermoFisher] </a>
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According to iGEM headquarter protocol, biological triplets and technical triplicates was made for each promoter. Each construct has been sequenced and verified with colony PCR. For the complete protocol click <a href="https://static.igem.org/mediawiki/2015/5/5a/SDU_2015_Protocol_003_-_Interlab_Study.pdf" target="_blank">here</a>. <br>
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Each construct were sequenced; two of the constructs were correctly assembled, the third had the correct promoter, but the remaining did not match <i>gfp</i>.
 
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<p>
<a class="popupImg alignRight" style="width:200px" target="_blank" href="https://static.igem.org/mediawiki/2015/1/1f/SDU2015_InterlabStudyData.png" title="">
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<span class="intro">For the measurements conducted in this project</span> we used a FACSAriaII. The used method of the FACS were flow cytometry which functions through singling out droplets containing one cell each.
  <img src="https://static.igem.org/mediawiki/2015/a/a9/SDU2015_InterlabStudyData_thumbnail.png" style="width:200px"/>
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By exciting the proteins with light on the absorption frequency of the protein the cells will be fluorescent and emission intensity can be measured.<br>
    <b> Figure 2:</b>
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We used <i>E. coli</i> Top10 without inserted plasmids as our negative control and one of our own biobricks; pSB1C3-T18-LinkerGFP for the positive control. Top10 was used to calibrate the FACS and the arbitrary units (a.u.) was measured by gating.
</a>
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Arbitrary units are relative to the measurements, it describes how strong one reading is compared to a defined referen<span class="sourceReference">ce</span>.
<span class="intro">Once the final constructs</span> were made, each construct were veryfied through colony PCR, and sequencing.
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<span class="tooltip">
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  <span class="tooltipHeader">Reference:</span>Kate B. Bechtol, David K. Hanzel, and Bee
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Choo Liang, Amersham Biosciences, Inc. - Understanding Fluorescence.<a target="_blank" href="https://www.gelifesciences.com/gehcls_images/GELS/Related%20Content/Files/1314729545976/litdoc63002879_20110830221802.pdf "> [GelifeSciences] </a>
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<span class="intro">The three promoters are part</span> of a promoter family originally from a combinatorial library made by John Anderson in 2006. WT J23119 was made from synthetic oligonucleotides using overlap extension, and is the strongest of all the promoters in the family<span class="sourceReference">REFERENCE WORD</span>.
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<span class="tooltip">
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  <span class="tooltipHeader">Reference:</span>iGEM Parts Registry - BBa_J23119:Design. Visited: 17.09.15.<a target="_blank" href="http://parts.igem.org/Part:BBa_J23119:Design "> [Parts] </a>
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J23101 is a constitutive promoter mutated form the WT J23119, and contains one point mutation in position -33, subsstituting G with T. J23106 and J23117, like J23101, are derivatives of J23119, and are also constitutive promoters and modified in the same manner. J23106 have three mutations one in the -10 region and two in the -35 region, 8- and -9 plus -33 and -32, respectively. J23117 have two mutations in its -10 region, at position -8 and -12. All three promoters are 35 bp lo<span class="sourceReference">ng</span>.
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<span class="tooltip">
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  <span class="tooltipHeader">Reference:</span>JCAnderson. iGEM Parts Registry - Visited: 17.09.15.<a target="_blank" href="http://parts.igem.org/File:PBca1020-r0040.jpg "> [Parts] </a>
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For the measurements conducted in this project we used FACS.
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<a class="popupImg alignRight" style="width:250px" target="_blank" href="https://static.igem.org/mediawiki/2015/8/8a/SDU2015_Interlabstudy_pvalues_thumbnail.jpg" title="Results from FACS - *=p<1, **=p<0.1, ***=p<0.01, ****=p<0.0001. J23101: Construct 1. J23106: construct 2. J23117: Construct 3.<br> For full dataset, see raw data.">
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  <img src="https://static.igem.org/mediawiki/2015/8/8a/SDU2015_Interlabstudy_pvalues_thumbnail.jpg" style="width:250px"/> </a>
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<div class="thumbcaption">Figure 2: The diagram shows the flourescence measured in a.u. by FACS for the 5 constructs. The P-value derived from the data is P<0.0001, marked by ****. J23106+I13504 has the highest flourescence measured, while Top10 has the lowest.  
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FACS functions through singling out droplets containing cells, exciting the proteins by shooting light on the absorption frequency onto the cells, then by measuring the emission intensity, the fluorescence of each cell is measured.
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<a href="http://parts.igem.org/Part:BBa_I13504" target="_blank">BBa_I13504</a> is a composite part composed of and RBS-site, a FACS optimized GFPmut3b and two standard biobrick terminators. The GFPmut3b has amino acid substitutions in position 65 and 72, a Glycine and Alanine respective<span class="sourceReference">ly</span>.
When measuring we used our own construct rfirefhyiw as a positive control, and TOP10 as negative control.
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<span class="tooltip">
Each construct were in the experiment measured in both biological and technical triplicates.
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  <span class="tooltipHeader">Reference:</span>Brendan P. Cormack, Raphael H. Valdiviaa, Stanley Falkow - FACS-optimized mutants of the green fluorescent protein (GFP). DOI:10.1016/0378-1119(95)00685-0.<a target="_blank" href="http://www.sciencedirect.com/science/article/pii/0378111995006850 "> [ScienceDirect] </a>
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Although veryfied through colony PCR, one construct seemed faulty, due to irregular measurments, and inconclusive sequencing.
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<span class="intro">Top10 is the reference for the a.u. measurements</span> compared to each of the other samples.
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Our expectations of the promoters are listed from weakest to strongest in relative expression: J23117 < J23106 < J23101, based on the original measurements done in 2006.<br>
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In figure 2 a graph comparing each construct’s a.u. to the positive control, T18-Linker-GFP is depicted. The scale is logarithmic due to the relatively large difference in the measured expression levels of the promoters.  
 
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<span class="intro">Sequence data for the three constructs</span> was compared to the sequence retrieved from parts registry. It was correct for <a href="https://static.igem.org/mediawiki/2015/a/a5/Sdu_2015_J23106%2BI13504.txt" target="_blank">J23106-I13504</a> and <a href="https://static.igem.org/mediawiki/2015/3/33/Sdu_2015_J23117%2BI13504.txt" target="_blank">J23117-I13504</a>, but the data for <a href="https://static.igem.org/mediawiki/2015/1/15/Sdu_2015_J23101%2BI13504.txt" target="_blank">J23101-I13504</a> did not show the gene encoding GFP, a BLAST search showed some alignment in the beginning of the sequence, to pFM46. Promoter J23106 showed the highest fluorescence of the constructs, with J23117 having a significantly (p < 0.0001) reduced fluorescence, at 40 times lower.
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<span class="intro">The J23106 construct showed a much higher</span> fluorescence than the J23117 construct, with a mean value of 85932 a.u. compared to 814 a.u. see figure 2 for graph.
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The measurement on J23101 is inconclusive in this study, due to the wrongful sequence, possibly caused by contamination.
 
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Latest revision as of 03:20, 19 September 2015

"In a dark place we find ourselves, and a little more knowledge lights our way." - George Lucas

Interlab study

Our team has been participating in the iGEM Interlab Study, to help further characterize three different promoters. This was done by using GFP-fluorescence as a way of measuring how strong each of the promoters are compared to each other.

Figure 1:The three constructs made for this experiment.

The three constructs were made through iGEM standard biobrick assembly, inserting gfp into pSB1C3 plasmids containing the different promoters. The gfp-gene were originally cut out of pSB1A2, before ligation with each of the three promotes. Transformation of the constructs was done into E. coli K12 Top10, because it has been optimized for transformation and high levels of plasmid synthetisation. Reference:One Shot® Top10 Chemically Competent E. coli. Catalog number: C4040-10. Visited: 17.09.15. [ThermoFisher] According to iGEM headquarter protocol, biological triplets and technical triplicates was made for each promoter. Each construct has been sequenced and verified with colony PCR. For the complete protocol click here.
Each construct were sequenced; two of the constructs were correctly assembled, the third had the correct promoter, but the remaining did not match gfp.

For the measurements conducted in this project we used a FACSAriaII. The used method of the FACS were flow cytometry which functions through singling out droplets containing one cell each. By exciting the proteins with light on the absorption frequency of the protein the cells will be fluorescent and emission intensity can be measured.
We used E. coli Top10 without inserted plasmids as our negative control and one of our own biobricks; pSB1C3-T18-LinkerGFP for the positive control. Top10 was used to calibrate the FACS and the arbitrary units (a.u.) was measured by gating. Arbitrary units are relative to the measurements, it describes how strong one reading is compared to a defined reference. Reference:Kate B. Bechtol, David K. Hanzel, and Bee Choo Liang, Amersham Biosciences, Inc. - Understanding Fluorescence. [GelifeSciences]

The three promoters are part of a promoter family originally from a combinatorial library made by John Anderson in 2006. WT J23119 was made from synthetic oligonucleotides using overlap extension, and is the strongest of all the promoters in the familyREFERENCE WORD. Reference:iGEM Parts Registry - BBa_J23119:Design. Visited: 17.09.15. [Parts] J23101 is a constitutive promoter mutated form the WT J23119, and contains one point mutation in position -33, subsstituting G with T. J23106 and J23117, like J23101, are derivatives of J23119, and are also constitutive promoters and modified in the same manner. J23106 have three mutations one in the -10 region and two in the -35 region, 8- and -9 plus -33 and -32, respectively. J23117 have two mutations in its -10 region, at position -8 and -12. All three promoters are 35 bp long. Reference:JCAnderson. iGEM Parts Registry - Visited: 17.09.15. [Parts]

Figure 2: The diagram shows the flourescence measured in a.u. by FACS for the 5 constructs. The P-value derived from the data is P<0.0001, marked by ****. J23106+I13504 has the highest flourescence measured, while Top10 has the lowest.
BBa_I13504 is a composite part composed of and RBS-site, a FACS optimized GFPmut3b and two standard biobrick terminators. The GFPmut3b has amino acid substitutions in position 65 and 72, a Glycine and Alanine respectively. Reference:Brendan P. Cormack, Raphael H. Valdiviaa, Stanley Falkow - FACS-optimized mutants of the green fluorescent protein (GFP). DOI:10.1016/0378-1119(95)00685-0. [ScienceDirect]

Top10 is the reference for the a.u. measurements compared to each of the other samples. Our expectations of the promoters are listed from weakest to strongest in relative expression: J23117 < J23106 < J23101, based on the original measurements done in 2006.
In figure 2 a graph comparing each construct’s a.u. to the positive control, T18-Linker-GFP is depicted. The scale is logarithmic due to the relatively large difference in the measured expression levels of the promoters.

Sequence data for the three constructs was compared to the sequence retrieved from parts registry. It was correct for J23106-I13504 and J23117-I13504, but the data for J23101-I13504 did not show the gene encoding GFP, a BLAST search showed some alignment in the beginning of the sequence, to pFM46. Promoter J23106 showed the highest fluorescence of the constructs, with J23117 having a significantly (p < 0.0001) reduced fluorescence, at 40 times lower.

The J23106 construct showed a much higher fluorescence than the J23117 construct, with a mean value of 85932 a.u. compared to 814 a.u. see figure 2 for graph. The measurement on J23101 is inconclusive in this study, due to the wrongful sequence, possibly caused by contamination.