Revision as of 15:19, 2 October 2014

TEC-CEM | Parts

ITESM-CEM | Enzy7-K me

Parts 3256

_{Our Parts}

_{List of our parts}

Our Parts

This enzyme was first detected in Chromobacterium sp. We introduced it in a plasmid backbone with chloramphenicol resistance. Its length is of 1871 nucleotides and its codons were optimized in order to use it on E.coli, it already included a stop codon, it was also modified by the addition of a glycosilation site and the peptide signal of human cathepsin.

Oxoacyl Reductase

This enzyme (7-alpha dehydratase) was detected in Rhodococcus jostii . We introduced it in a plasmid backbone with chloramphenicol resistance. Its length is of 602 nucleotides and its codons were optimized in order to use it on E.coli, it already included a stop codon, it was also modified by the addition of a glycosilation site and the peptide signal of human cathepsin.

Neomycin Resistance

Stop coding for eucaryotic cells

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    <tr>
      <td colspan="3" rowspan="3" align="left" valign="top"><ul>
-       <sub>Submenú 1</sub><sub>Submenú 2</sub><sub>Submenú 3</sub>
+       <sub><a href="https://2014.igem.org/Team:ITESM-CEM/Parts" style="color: #FFF;">Our Parts</a></sub>
-    </ul></td>
+      <sub><a href="https://2014.igem.org/Team:ITESM-CEM/List" style="color: #FFF;">List of our parts</a></sub>
+        </ul></td>
      <td><img src="images/spacer.gif" width="1" height="1" alt=""></td>
    </tr>
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 <div style="background-color: #f3f3e2; style="width:95%">
 <!--INICIO CONTENIDO-->
+<h2>Our Parts</h2>
+<p style="text-align: justify; text-justify: inter-word> The main goal of our project was to establish the construct which will help us to degrade 7-ketocholesterol consisting in the use of three specific enzymes, but for further applications we submitted them in single modules. This will serve as the basis of a future library for standardized work related with atherosclerosis.
+</p><br><br>
-<br>
+<h2>Cholesterol Oxidase</h2>
-<table class="table table-striped">
+<p style="text-align: justify; text-justify: inter-word> This enzyme was first detected in Chromobacterium sp. We introduced it in a plasmid backbone with chloramphenicol resistance. Its length is of 1871 nucleotides and its codons were optimized in order to use it on E.coli, it already included a stop codon, it was also modified by the addition of a glycosilation site and the peptide signal of human cathepsin.
-<tr>
+</p> <br><br>
-<th>Name</th>
-<th>Type</th>
-<th>Description</th>
-<th>Designer</th>
-<th>Length (bp)</th>
-</tr>
-<!-- Favorite-Name-Type-Description-Designer-Length-->
-<tr>
-<td><a href="http://parts.igem.org/Part:BBa_K1313000">BBa_K1313000</a></td>
-<td>Enzyme</td>
-<td>Colox</td>
-<td>Eddie Cano Gámez</td>
-<td>1</td>
-</tr>
-<tr>
-<td> <a href="http://parts.igem.org/Part:BBa_K1313001">BBa_K1313001</a></td>
-<td>Enzyme</td>
-<td>OxRed</td>
-<td>Eddie Cano Gámez</td>
-<td>1</td>
-</tr>
-<tr>
-<td> <a href="http://parts.igem.org/Part:BBa_K1313002"> BBa_K1313002 </a> </td>
-<td>Enzyme</td>
-<td>Dehydratase</td>
-<td>Eddie Cano Gámez</td>
-<td>1</td>
-</tr>
-<tr>
-<td> <a href="http://parts.igem.org/Part:BBa_K1313003"> BBa_K1313003 </a> </td>
-<td>Antibiotic Resistance</td>
-<td>NeoR</td>
-<td>Carlos Meza Ramírez</td>
-<td>1</td>
-</tr>
-<tr>
-<td> <a href="http://parts.igem.org/Part:BBa_K1313004"> BBa_K1313004 </a> </td>
-<td>Promoter</td>
-<td>pCMV</td>
-<td>Oliva Sánchez Montesinos</td>
-<td>1</td>
-</tr>
-<tr>
-<td> <a href="http://parts.igem.org/Part:BBa_K1313004"> BBa_K1313005 </a> </td>
-<td>Stop</td>
-<td>BGH PA</td>
-<td>Oliva Sánchez Montesinos</td>
-<td>1</td>
-</tr>
-</table>
-<h2> ColOx </h2>
+<h2>Oxoacyl Reductase</h2>
+<p style="text-align: justify; text-justify: inter-word> This enzyme was detected in Rhodococcus jostii . We introduced it in a plasmid backbone with chloramphenicol resistance. Its length is of 1007 nucleotides and its codons were optimized in order to use it on E.coli, it already included a stop codon, it was also modified by the addition of a glycosilation site and the peptide signal of human cathepsin.
+</p> <br><br>
-<P> Cholesterol oxidase is a well characterized enzyme.
+<h2>7-dehydratase</h2>
-</p>
+<p style="text-align: justify; text-justify: inter-word> This enzyme (7-alpha dehydratase) was detected in Rhodococcus jostii . We introduced it in a plasmid backbone with chloramphenicol resistance. Its length is of 602 nucleotides and its codons were optimized in order to use it on E.coli, it already included a stop codon, it was also modified by the addition of a glycosilation site and the peptide signal of human cathepsin.
+</p> <br><br>
+<h2>Neomycin Resistance</h2>
+<p style="text-align: justify; text-justify: inter-word> This selective marker was gotten from a plasmid for mammalian expression, its length is of 855 nucleotides,and it was isolated from pcDNA3.1(+)/myc-His A.
+</p><br><br>
+<h2>BGHPA</h2>
+<p style="text-align: justify; text-justify: inter-word> Stop coding for eucaryotic cells
+</p><br><br>
+<h2>PCMV</h2>
+<p style="text-align: justify; text-justify: inter-word> Promoter from Human Cytomegalovirus, this promoter works only on eucaryotic cells.
+</p><br><br><br>
+<br>
 <!--FIN CONTENIDO-->