Difference between revisions of "Part:BBa K2062005:Experience"

Revision as of 04:11, 24 October 2016

Applications of BBa_K2062005

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 __NOTOC__
-  <h2>Transformation of <em>P. putida</em> KT2440</h2>
-  <p>
-    In order to avoid the virulence factors of
-    <em>Pseudomonas aeruginosa</em>, bacterial strains with
-    similar or shared metabolic pathways to the one
-    above were chosen as potential candidates. The
-    final candidates were <em>Pseudomonas putida</em> and
-    <em>Staphylococcus epidermidis</em>. Although
-    <em>S. epidermidis</em> doesn’t share the same exact
-    pathway as <em>P. aeruginosa</em>, it is a
-    naturally-occurring skin microbiome and only need
-    two additional enzymes, RhlA and RhlB, to produce
-    mono-rhamnolipids. Genes rhlA and rhlB necessary
-    for mono-rhamnolipid synthesis were extracted from
-    the <em>P. aeruginosa P14</em> bacterial strain. These
-    genes were cloned into the modified plasmid pNJ3.1
-    using standard cloning methods for transformation
-    into the desired bacterial strains (Figure 2). The
-    plasmid pC194 and a shuttle vector strain,
-    <em>S. aureus</em> RN4220 (details on <em>S. epidermidis</em>
-    transformation are discussed in the experiments
-    and result section) were used for <em>S. epidermidis</em>
-    transformations with the same basic design (Figure
-). The conversion of mono-rhamnolipids to
-    di-rhamnolipids requires the additional gene rhlC,
-    which was also extracted from P14 strain and
-    cloned into the same pNJ3.1 vector (Figure 4).
-  </p>
-  <figure>
-    <img src="https://static.igem.org/mediawiki/parts/a/a4/RhlAB_circuit.png"
-	 alt="RhlAB Plasmid Circuit" width="500">
-  </figure>
 ===Applications of BBa_K2062005===