Team:Wisconsin-Madison/Parts

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Revision as of 18:59, 18 October 2009

PARTS

Basic Parts GSMT Gene GSMT is a plasmid gene (854 bp) that codes for the enzyme that catalyze the first reaction in the salt tolerant pathway that we are interested. GSMT stands for Glycine Sarcosine N-Methyl Transferase. It catalyzes the conversion from glycine to sarcosine, using SAM as a methyl donor. In our project, we have this GSMT synthesized using MR. Gene. Naturally, this gene can be found in Galdieria sulphuraria, an extremephile that establishes high resistance to osmotic stress as well as acidic, thermal stresses and toxic metals. We PCR amplified gene GSMT with iGEM designated cutting sites and ribosome binding sites and biobricked it with pSB1A2. Found HERE in Registry SDMT Gene SDMT is a plasmid gene (900 bp) that codes for the enzyme that catalyze the first reaction in the salt tolerant pathway that we are interested. This enzyme of this pathway is SDMT, which stands for Sarcosine Dimethylglycine Methyl Transferase. It catalyzes two steps of methylation, both that of sarcosine and dimethylglycine, to our final product, betaine, again using SAM as the methyl donor. The gene we used came from Galdieria sulphuraria, an extremephile that establishes high resistance to osmotic stress as well as acidic, thermal stresses and toxic metals. In our project, we really appreciate that Center for Eukaryotic Structural Genomics at University of Wisconsin-Madison graciously gave us the plasmid containing this gene. We PCR amplified gene SDMT with iGEM designated cutting sites and ribosome binding sites and biobricked it with pSB1A2. Found HERE in Registry ProU Promoter Found HERE in Registry MetK Gene Found HERE in Registry NudF Gene NudF is a plasmid gene (560 bp) that codes for the protein responsible for the enzymatic reaction in mevalonent pathway to form Dimethylallyl pyrophosphate (DMAPP). Specifically, in our project, we used it in the last step of mevalonate pathway to produce biofuels iso-pentenol. We PCR amplified gene nudF with iGEM designated cutting sites and ribosome binding sites and biobricked it with pSB1A2. Found HERE in Registry Photo System Promoter Found HERE in Registry Composite Parts ProU : RBS + RFP + TERM Photo System Promoter : pRL1383 Pro U Promoter :

@@ Line 1: / Line 1: @@
 {{Wisconsin-Madison Template}}
-{| class="wikitable" border="0" align="center" width=790px
-|style="text-align:left" style="vertical-|
 <center>
   '''PARTS'''
 </center>
+{| class="wikitable" border="0" align="center" width=750px
+|style="text-align:left" style="vertical-|
-If you choose to include a '''Parts Submitted to the Registry''' page, please list your parts here.  This is not necessary but it may be a nice list to keep track of.
+<center>
+ '''Basic Parts'''
+</center>
+<center>
+'''GSMT Gene'''
+</center>
+GSMT is a plasmid gene (854 bp) that codes for the enzyme that catalyze the first reaction in the salt tolerant pathway that we are interested. GSMT stands for Glycine Sarcosine N-Methyl Transferase. It catalyzes the conversion from glycine to sarcosine, using SAM as a methyl donor. In our project, we have this GSMT synthesized using MR. Gene. Naturally, this gene can be found in Galdieria sulphuraria, an extremephile that establishes high resistance to osmotic stress as well as acidic, thermal stresses and toxic metals. We PCR amplified gene GSMT with iGEM designated cutting sites and ribosome binding sites and biobricked it with pSB1A2.
+<center>Found [http://partsregistry.org/Part:BBa_K220002 HERE] in Registry</center>
+<center>
+'''SDMT Gene'''
+</center>
+SDMT is a plasmid gene (900 bp) that codes for the enzyme that catalyze the first reaction in the salt tolerant pathway that we are interested. This enzyme of this pathway is SDMT, which stands for Sarcosine Dimethylglycine Methyl Transferase. It catalyzes two steps of methylation, both that of sarcosine and dimethylglycine, to our final product, betaine, again using SAM as the methyl donor. The gene we used came from Galdieria sulphuraria, an extremephile that establishes high resistance to osmotic stress as well as acidic, thermal stresses and toxic metals. In our project, we really appreciate that Center for Eukaryotic Structural Genomics at University of Wisconsin-Madison graciously gave us the plasmid containing this gene. We PCR amplified gene SDMT with iGEM designated cutting sites and ribosome binding sites and biobricked it with pSB1A2.
+<center>Found [http://partsregistry.org/Part:BBa_K220000 HERE] in Registry</center>
+<center>
+'''ProU Promoter'''
+</center>
+<center>Found [http://partsregistry.org/Part:BBa_K220004 HERE] in Registry</center>
+<center>
+'''MetK Gene'''
+</center>
+<center>Found [http://partsregistry.org/Part:BBa_K220005 HERE] in Registry</center>
+<center>
+'''NudF Gene'''
+</center>
+NudF is a plasmid gene (560 bp) that codes for the protein responsible for the enzymatic reaction in mevalonent pathway to form Dimethylallyl pyrophosphate (DMAPP). Specifically, in our project, we used it in the last step of mevalonate pathway to produce biofuels iso-pentenol. We PCR amplified gene nudF with iGEM designated cutting sites and ribosome binding sites and biobricked it with pSB1A2.
+<center>Found [http://partsregistry.org/Part:BBa_K220003 HERE] in Registry</center>
+<center>
+'''Photo System Promoter'''
+</center>
+<center>Found [http://partsregistry.org/Part:BBa_K220006 HERE] in Registry</center>
+<center>
+ '''Composite Parts'''
+</center>
+<center>
+'''ProU : RBS + RFP + TERM'''
+</center>
+<center>
+'''Photo System Promoter : pRL1383'''
+</center>
+<center>
+'''Pro U Promoter : '''
+</center>