Team:ITESM-CEM/Project/Experiments
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<sub2><a href="#One" style="color: #FFF;">PCR's</a></sub2> | <sub2><a href="#One" style="color: #FFF;">PCR's</a></sub2> | ||
<sub2><a href="#Two" style="color: #FFF;">Mammalian Cell Transfection</a></sub2> | <sub2><a href="#Two" style="color: #FFF;">Mammalian Cell Transfection</a></sub2> | ||
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<sub2><a href="#Four" style="color: #FFF;">Protein Expression</a></sub2> | <sub2><a href="#Four" style="color: #FFF;">Protein Expression</a></sub2> | ||
<sub2><a href="#Five" style="color: #FFF;">NeoR Characterization</a></sub2> | <sub2><a href="#Five" style="color: #FFF;">NeoR Characterization</a></sub2> | ||
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- | <a name="One"><h2>PCR for | + | <a name="One"><h2>PCR for sequence isolation.</h2></a> |
- | <h4> | + | <h4>PCR 25 ul Mix for Mammalian expression Biobricks</h4> |
<p style="text-align: justify; text-justify: inter-word;"> | <p style="text-align: justify; text-justify: inter-word;"> | ||
-6.75 µl – Molecular grade water<br> | -6.75 µl – Molecular grade water<br> | ||
- | -1 µl – DNA template<br> | + | -1 µl – DNA template (1 ng)<br> |
- | -1.25 µl – Primer F<br> | + | -1.25 µl – Primer F (100 uM)<br> |
- | -1.25 µl – Primer R<br> | + | -1.25 µl – Primer R (100 uM)<br> |
- | -2.25 µl – DMSO<br> | + | -2.25 µl – DMSO 99%<br> |
- | -12.5 µl – NEB | + | -12.5 µl – NEB Q5 High Fidelity 2X Master Mix</p><br> |
<h4>PCR programs</h4> | <h4>PCR programs</h4> | ||
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BGHPA</p><br> | BGHPA</p><br> | ||
- | <p> | + | <p class="centeredImage"><img src="https://static.igem.org/mediawiki/2014/a/af/PCR_cycle_5.jpg" width="600" height="235" hspace="20" BORDER=10></p><br> |
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<p style="text-align: justify; text-justify: inter-word;">pcDNA 3.1 Myc-His A is an expression plasmid that contains BGHPA, a constitutive promoter and an origin of replication that work in mammalian cells. To see if the plasmid was working correctly, a cassette was expressed with GFP to see if the plasmid worked in a specific eukaryotic cell line (Marc145), so the enzyme could be inserted and the analysis of functionality of the enzyme by substrate degradation could be started. </p><br> | <p style="text-align: justify; text-justify: inter-word;">pcDNA 3.1 Myc-His A is an expression plasmid that contains BGHPA, a constitutive promoter and an origin of replication that work in mammalian cells. To see if the plasmid was working correctly, a cassette was expressed with GFP to see if the plasmid worked in a specific eukaryotic cell line (Marc145), so the enzyme could be inserted and the analysis of functionality of the enzyme by substrate degradation could be started. </p><br> | ||
- | <p> | + | <p class="centeredImage"><img src="https://static.igem.org/mediawiki/2014/2/2a/Dehyd_pcDNA.jpg" width="600" height="213" hspace="20" BORDER=10></p><br> |
<p><pie><b>Image 1.</b>Cells before (left) and after (right) transfection with plasmid pcDNA 3.1 Myc-His A with 7-dehydratase gene using lipofectamine as a transfecting agent. </p></pie> | <p><pie><b>Image 1.</b>Cells before (left) and after (right) transfection with plasmid pcDNA 3.1 Myc-His A with 7-dehydratase gene using lipofectamine as a transfecting agent. </p></pie> | ||
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<p style="text-align: justify; text-justify: inter-word;">As fluorescence of this enzyme cannot be detected, its characterization is going to be determined by an antibiotic resistance at a certain concentration (Neomycin), where cells are able to keep dividing, except for the ones without the resistance gene.</p> | <p style="text-align: justify; text-justify: inter-word;">As fluorescence of this enzyme cannot be detected, its characterization is going to be determined by an antibiotic resistance at a certain concentration (Neomycin), where cells are able to keep dividing, except for the ones without the resistance gene.</p> | ||
- | + | <p class="centeredImage"><img src="https://static.igem.org/mediawiki/2014/8/8f/Dehyd_pcDNA2.jpg" width="350" height="476" hspace="20" BORDER=10></p><br> | |
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<a name="Five"><h2>NeoR characterization</h2></a> | <a name="Five"><h2>NeoR characterization</h2></a> | ||
- | <p style="text-align: justify; text-justify: inter-word;"> The scope of our | + | <p style="text-align: justify; text-justify: inter-word;"> The scope of our project is to express a new synthetic pathway in mammalian cells in order to make them able to metabolize 7-ketocholesterol. Just like bacteria, mammalian cells also have a selective gene to identify successfully transformed organisms. NeoR is a gene that encodes an aminoglycoside 3'-phosphotransferase enzyme, which provides a resistance to Neomycin and its derivatives. The antibiotic that will be used to select the successfully transformed mammalian cells is G418®, a Neomycin derivative which only affects mammalian cells. <br><br> |
- | However | + | However, this exceeded the possibilities given the time constrains. Therefore a characterization in a mammalian cell culture was not done due to time limitations. The NeoR gene was characterized using an <u>E.coli</u> culture and Neomycin as selective antibiotic. The NeoR gene was obtained by PCR from pcDNA3.1(-)/ Myc-His A, and following iGEM instructions, the gene was introduced in the plasmid pSB1C3 as it is shown in the following picture.<br></p> |
<p class="centeredImage"><img src="https://static.igem.org/mediawiki/2014/e/ef/Plasmido_BBa_K1313004.jpg" width="443" height="351" hspace="20"></p> | <p class="centeredImage"><img src="https://static.igem.org/mediawiki/2014/e/ef/Plasmido_BBa_K1313004.jpg" width="443" height="351" hspace="20"></p> | ||
<h4>Procedure</h4> | <h4>Procedure</h4> | ||
- | <p style="text-align: justify; text-justify: inter-word;">The characterization was made using two groups: the | + | <p style="text-align: justify; text-justify: inter-word;">The characterization was made using two groups: the samples and a control group. The samples were made using an <u>E.coli</u> DH5-α inoculum, transformed with the NeoR gene inserted in psB1C3 using the constitutive promoter BBa_K823012. The control group used an untransformed <u>E.coli</u> DH5-α inoculum. <br><br> |
- | Both groups consisted on thirteen essay tubes with 5 ml of LB media each one with a different concentration on Neomycin as shown in table 1 and 2. The tubes were cultured on a shaker for 18 hours at 250 rpm. Afterwards each tube had its optical density measured at 600 nm using as | + | Both groups consisted on thirteen essay tubes with 5 ml of LB media each one with a different concentration on Neomycin as shown in table 1 and 2. The tubes were cultured on a shaker for 18 hours at 250 rpm/37ºC. Afterwards, each tube had its optical density measured at 600 nm using as LB media as a blank with the same antibiotic concentration. Five neomycin concentrations were chosen to perform petri dish cultures but only with the trouble group to perform a C.F.U. count. |
</p> | </p> | ||
+ | <p><pie><b>Table 1.</b> Control group without neomycin</p></pie><br> | ||
+ | <p class="centeredImage"><img src="https://static.igem.org/mediawiki/2014/a/a7/ControlTable.jpg" height="366" width="700" align="middle" hspace="10" BORDER=10><br></p><br> | ||
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+ | <p><pie><b>Table 2.</b> Positive Group with neomycin</p></pie><br> | ||
+ | <p class="centeredImage"><img src="https://static.igem.org/mediawiki/2014/1/1d/NeoR_positivo.jpg" height="411" width="700" align="middle" hspace="10" BORDER=10><br></p><br> | ||
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Latest revision as of 03:54, 18 October 2014
ITESM-CEM | Enzy7-K me |
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