Team:HKU HongKong/Project/Background.html

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<link rel="alternate" type="application/atom+xml" title="2011.igem.org Atom feed" href="/wiki/index.php?title=Special:RecentChanges&amp;feed=atom" /> <title>Team:HKU Hong Kong - 2012</title>
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Background</a></li></font>
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Future Implications</a></li></font>
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Protocols</a></li></font>
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Bio Bricks</a></li></font>
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Results</a></li></font>
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&nbsp;&nbsp;Attributions&nbsp;&nbsp;</a></li>
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    <li><font size="10"><a href="https://2012.igem.org/Team:HKU_HongKong/Data/Mol_Protocols.html">&nbsp;Molecular Cloning&nbsp;</a></li></font>
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<li><font size="10"><a href="https://2012.igem.org/Team:HKU_HongKong/Data/pvdQ_Protocols.html">&nbsp;pvdQ Expression Analysis&nbsp;</a></li></font>
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<font face="Trebuchet MS" size="6" color="#232323">Abstract</font></span><p style="text-align: left">
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<font face="Trebuchet MS" size="6">Abstract</font></span></h2>
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&nbsp;<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">
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<p style="text-align: left; font-style: normal; font-variant: normal; font-weight: normal; font-size: 13px; vertical-align: baseline; color: rgb(85, 85, 85); font-family: Lato, Tahoma, Arial, sans-serif; letter-spacing: normal; line-height: 19.5px; orphans: 2; text-indent: 0px; text-transform: none; white-space: normal; widows: 2; word-spacing: 0px; -webkit-text-size-adjust: auto; -webkit-text-stroke-width: 0px; border: 0px none; margin-left: 0px; margin-right: 0px; margin-top: 0px; margin-bottom: 20px; padding: 0px">
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<font face="Trebuchet MS" size="2" color="#232323">HKU’s iGEM team aims to  
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&nbsp;</p>
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introduce an acyl homoerine lactone (AHL)-degrading genetic system into the  
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<p style="text-align: left; font-style: normal; font-variant: normal; font-weight: normal; font-size: 13px; vertical-align: baseline; color: #232323; font-family: Lato, Tahoma, Arial, sans-serif; letter-spacing: normal; line-height: 19.5px; orphans: 2; text-indent: 0px; text-transform: none; white-space: normal; widows: 2; word-spacing: 0px; -webkit-text-size-adjust: auto; -webkit-text-stroke-width: 0px; border: 0px none; margin-left: 0px; margin-right: 0px; margin-top: 0px; margin-bottom: 20px; padding: 0px">
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non-biolfilm-forming and non-virulent BL21 <i>Escherichia coli</i> strain.  
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HKU’s iGEM team aims to introduce  
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PvdQ, an enzyme naturally produced by <i>Pseudomonas aeruginosa</i>, is an  
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an acyl homoerine lactone (AHL)-degrading genetic system into the non-biolfilm-forming  
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acylase that functions to degrade long chain AHLs that bacteria like <i>
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and non-virulent BL21 Escherichia coli strain. PvdQ, an enzyme naturally  
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Pseudomonas putida or aeruginosa </i>itself<i> </i>utilize for biofilm  
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produced by Pseudomonas aeruginosa, is an acylase that functions to  
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formation. Biofilms are population density-dependent structures formed by  
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degrade long chain AHLs that bacteria like Pseudomonas putida or  
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quorum sensing bacteria that produce and secrete auto-inducers, which signal  
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aeruginosa itself utilize for biofilm formation. Biofilms are population  
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selective gene transcription. These signaling molecules, namely the AHLs,  
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density-dependent structures formed by quorum sensing bacteria that  
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are responsible for most bacterial pathogenicity including the opportunistic  
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produce and secrete auto-inducers, which signal selective gene  
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respiratory infections caused by <i>P.aeuroginosa</i> in immunocompromised  
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transcription. These signaling molecules, namely the AHLs, are  
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patients. </font></p>
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responsible for most bacterial pathogenicity including the opportunistic  
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">&nbsp;</p>
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respiratory infections caused by P.aeuroginosa in immunocompromised  
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">
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patients. </p>
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<font face="Trebuchet MS" size="2" color="#232323">As a step towards combating  
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<p style="text-align: left; font-style: normal; font-variant: normal; font-weight: normal; font-size: 13px; vertical-align: baseline; color: #232323; font-family: Lato, Tahoma, Arial, sans-serif; letter-spacing: normal; line-height: 19.5px; orphans: 2; text-indent: 0px; text-transform: none; white-space: normal; widows: 2; word-spacing: 0px; -webkit-text-size-adjust: auto; -webkit-text-stroke-width: 0px; border: 0px none; margin-left: 0px; margin-right: 0px; margin-top: 0px; margin-bottom: 20px; padding: 0px">
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these infections, <i>E.coli </i>can be effectively used as a protein factory  
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As a step towards combating these infections, E.coli can be effectively  
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to maximize pvdQ yield in vitro or ex vivo. Our most preliminary biobrick is  
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used as a protein factory to maximize pvdQ yield in vitro or ex vivo.  
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a constitutive promoter that drives baseline, exponential expression of pvdQ.  
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Our most preliminary biobrick is a constitutive promoter that drives  
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This genetic pathway is advantageous because the pvdQ gene is constitutively  
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baseline, exponential expression of pvdQ. This genetic pathway is  
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transcribed regardless of environmental and endogenous factors.&nbsp; </font></p>
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advantageous because the pvdQ gene is constitutively transcribed  
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">
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regardless of environmental and endogenous factors.&nbsp; </p>
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<font face="Trebuchet MS" size="2" color="#232323">&nbsp;</font></p>
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<p style="text-align: left; font-style: normal; font-variant: normal; font-weight: normal; font-size: 13px; vertical-align: baseline; color: rgb(85, 85, 85); font-family: Lato, Tahoma, Arial, sans-serif; letter-spacing: normal; line-height: 19.5px; orphans: 2; text-indent: 0px; text-transform: none; white-space: normal; widows: 2; word-spacing: 0px; -webkit-text-size-adjust: auto; -webkit-text-stroke-width: 0px; border: 0px none; margin-left: 0px; margin-right: 0px; margin-top: 0px; margin-bottom: 20px; padding: 0px">
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">
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<font color="#232323">&nbsp;This synthetic genetic pathway is an auto-inductive system where pvdQ  
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<font face="Trebuchet MS" size="2" color="#232323">This synthetic genetic pathway  
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protein production will specifically depend on the presence of N-dodecanoyl-L-Homoserine  
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is an auto-inductive system where pvdQ protein production will specifically  
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lactone and its coupling to the LuxR protein. Furthermore, several  
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depend on the presence of N-dodecanoyl-L-Homoserine lactone and its coupling  
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derivatives of the genetic system design can desirably optimize pvdQ  
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to the LuxR protein. Furthermore, several derivatives of the genetic system  
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yield. For instance, implementation of a positive feedback loop will  
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design can desirably optimize pvdQ yield. For instance, implementation of a  
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upregulate luxR production by the simple placement of the luxR gene  
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positive feedback loop will upregulate luxR production by the simple  
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downstream of PluxR Larger amounts of luxR will therefore bind a greater  
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placement of the luxR gene downstream of P<sub>luxR</sub> Larger amounts of  
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number of AHL molecules secreted by P.aeuroginosa biofilms, thereby  
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luxR will therefore bind a greater number of AHL molecules secreted by <i>
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activating the acylase gene’s expression at a low cell density. Hence,  
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P.aeuroginosa</i> biofilms, thereby activating the acylase gene’s expression  
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the final biobrick produced by iGEM HKU is an AHL-inducible acylase  
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at a low cell density. Hence, the final biobrick produced by iGEM HKU is an  
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system. </font> </p>
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AHL-inducible acylase system. </font></p>
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<p style="text-align: left; font-style: normal; font-variant: normal; font-weight: normal; font-size: 13px; vertical-align: baseline; color: #232323; font-family: Lato, Tahoma, Arial, sans-serif; letter-spacing: normal; line-height: 19.5px; orphans: 2; text-indent: 0px; text-transform: none; white-space: normal; widows: 2; word-spacing: 0px; -webkit-text-size-adjust: auto; -webkit-text-stroke-width: 0px; border: 0px none; margin-left: 0px; margin-right: 0px; margin-top: 0px; margin-bottom: 20px; padding: 0px">
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&nbsp;Although the synthetic E.coli cannot be introduced into infected humans  
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or soil and water (sources of P.aueroginosa) itself, it can be used to  
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mass-produce pvdQ which can then be packaged into small protein-delivery  
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<font face="Trebuchet MS" size="2" color="#232323">Although the synthetic <i>
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bores. These structures can be stimulated to efficiently release pvdQ at  
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E.coli</i> cannot be introduced into infected humans or soil and water  
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the desired location, mimicking conventional drug-delivery systems.  
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(sources of <i>P.aueroginosa</i>) itself, it can be used to mass-produce  
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While the mechanism of pvdQ delivery will not be addressed, it can be  
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pvdQ which can then be packaged into small protein-delivery bores. These  
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regarded as a potential implication of HKU’s iGEM project.
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structures can be stimulated to efficiently release pvdQ at the desired  
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location, mimicking conventional drug-delivery systems. While the mechanism  
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of pvdQ delivery will not be addressed, it can be regarded as a potential  
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">
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    <p>&nbsp;</p>
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<u><font face="Trebuchet MS" size="6" color="#232323">Materials &amp; Methods</font></u></p>
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    <p>&nbsp;</p>
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">&nbsp;</p>
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">
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<font face="Trebuchet MS" color="#232323" size="4"><i>Cloning and expressing
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pvdQ in E. coli</i></font></p>
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">&nbsp;</p>
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">
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<font face="Trebuchet MS" size="2" color="#232323"><i>pvdQ</i> was amplified
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from genomic DNA of Pseudomonas Aeruginosa. A functional biobrick is
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constructed by combining <i>pvdQ</i> and some regulatory elements (such as
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promoter and terminator). The regulatory components are obtained from the
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iGEM Distribution Kit 2012. As a result, a variety of <i>pvdQ</i> regulatory
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systems can be established. Among the various regulation systems, the luxR
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regulation system is most concerned. luxR is a gene that can encode LuxR
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which binds with AHLs and upregulates the luxRp. As a result, in our
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biobrick model, the expression of <i>pvdQ</i> will be upregulated. Increase
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in production of <i>pvdQ</i> indicates an increase in acylase activity,
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which further degrades AHLs. The product biobrick will be a AHL-inducible
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acylase system. PvdQ will only be produced when AHL is present.</font></p>
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">
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<font face="Trebuchet MS" size="2" color="#232323">&nbsp;</font></p>
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">
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<font face="Trebuchet MS" color="#232323" size="4"><i>Testing the inhibitory
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effect</i></font></p>
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">&nbsp;</p>
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">
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<font face="Trebuchet MS" size="2" color="#232323">The growth rate of
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monospecies biofilm of <i>Pseudomonas putida</i> is used to reflect the
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inhibitory effect of engineered <i>Escherichia coli</i>. This is because the
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major AHLs secreted by it involve 3-oxo-C12, which is a AHL that can be
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degraded by PvdQ and is also the major AHL produced in Pseudomonas
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areuginosa, the pathogenic microorganism. <i>pvdQ</i> expressing E. coli
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will be mixed with Pseudomonas putida and grown on agar plate. The reduction
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in biofilm formation will be assayed by crystal violet assay. The next part
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of the experiment is to add engineered E. coli to different phases of
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biofilm to validate the role of AHLs in biofilm formation.</font></p>
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<p class="MsoNormal" style="text-align:justify;text-justify:inter-ideograph">
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<font face="Trebuchet MS" size="2" color="#232323">&nbsp;</font></p>
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<p style="text-align: left">
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<br /></div>
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<span style="font-size: 14pt">Our kind Sponsors:</span></b></font></p>
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Latest revision as of 01:04, 27 September 2012

Team:HKU Hong Kong - 2012

Team:HKU HK

From 2011.igem.org