Revision as of 00:37, 17 July 2015

wiki wiki 2

Home

Team

Project

Statistics

Enzymes

Parts

Metodology

Results

Future Projections

Parts

Throughout the project we started to learn the fundamental principles of synthetic biology to get to work on our plasmid with which we want to see gluten degradation via the enzyme Kumamax. For this we going to insert in an e. coli the parts (Biobricks) needed to make our future bacteria can degrade gluten. The parts are:

Promoter (BBa_J23119): Constitutive promoter (which works permanently) that is give in the relative fluorescence of these plasmids in the TG1 strain grown in LB medium.
RBS (BBa_K1084103): Synthetic RBS with uplifting sequence.
Vector: pSB1C3
Coding Region: KumaMax (BBa_K590087): It degrades gluten, celiac disease leading cause. Enzyme generated by rational mutation for the active site of it.
Reporter: RFP (BBa_J04450): Red fluorescence protein.
Terminator (BBa_B0015): Dual terminator consisting of the B0010 and B0012 parties. It serves to give greater efficiency in transcription.

This is a graphic model of as it has be our plasmid where we can visualize the promoter, the RBS, the enzyme KumaMax, the RFP and the terminator, joined by means of prefixes and suffixes that indicate the locations of court.

@@ Line 6: / Line 6: @@
 </head>
 <body>
+<meta content="text/html; charset=ISO-8859-1"
+ http-equiv="content-type">
+<title></title>
 <meta content="text/html; charset=ISO-8859-1"
   http-equiv="content-type">
@@ Line 329: / Line 332: @@
    <li><big><span
   style="font-family: 'Arial','sans-serif';"><strong
-  style="font-weight: bold;">Promoter (BBa_J23119</strong><span
+  style="font-weight: bold;"><a
- style="font-weight: bold;">)</span>: </span>Constitutive
+ href="http://parts.igem.org/Part:BBa_J23119">Promoter</a>
+(BBa_J23119</strong><span style="font-weight: bold;">)</span>:
+    </span>Constitutive
 promoter (which works permanently) that is give in the relative
 fluorescence of these plasmids in the TG1 strain grown in LB medium.</big></li>
-   <li><big><strong style="font-weight: bold;">RBS
+   <li><big><strong style="font-weight: bold;"><a
+ href="http://parts.igem.org/Part:BBa_K1084103">RBS</a>
 (BBa_K1084103)</strong>: Synthetic RBS with uplifting sequence.</big></li>
    <li><big><strong><span
   style="font-family: 'Arial','sans-serif';">Vector:<span
-  style="font-weight: normal;"> pET29B+</span></span></strong></big></li>
+  style="font-weight: normal;"> pSB1C3</span></span></strong></big></li>
    <li><big><strong><span
-  style="font-family: 'Arial','sans-serif';">Coding Region:
+  style="font-family: 'Arial','sans-serif';"><a
-KumaMax (BBa_K590087):</span></strong> It degrades gluten,
+ href="http://parts.igem.org/Part:BBa_K590087">Coding Region:
+KumaMax</a> (BBa_K590087):</span></strong> It
+degrades gluten,
 celiac disease leading cause. Enzyme generated by rational mutation for
 the active site of it.</big></li>
    <li><big><strong><span
-  style="font-family: 'Arial','sans-serif';">Reporter: RFP
+  style="font-family: 'Arial','sans-serif';"><a
+ href="http://parts.igem.org/Part:BBa_J04450">Reporter: RFP</a>
 (BBa_J04450):</span></strong><span
   style="font-family: Arial,sans-serif;"> Red f</span>luorescence
 protein.</big></li>
-   <li><big><span style="font-family: Arial,sans-serif;"><strong>Terminator
+   <li><big><span style="font-family: Arial,sans-serif;"><strong><a
+ href="http://parts.igem.org/Part:BBa_B0015">Terminator</a>
 (BBa_B0015):</strong> </span>Dual terminator consisting of
 the B0010 and B0012 parties. It serves to give greater efficiency in
@@ Line 377: / Line 387: @@
 </div>
 </div>
+<br>
 </body>
 </html>

Difference between revisions of "Team:San Andres/Parts"

Revision as of 00:37, 17 July 2015

Parts