Difference between revisions of "Team:Newcastle/Results"

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           <h2 style="font-family: Rubik; text-align: left; margin-top: 1%"> Background Information </h2>
 
           <h2 style="font-family: Rubik; text-align: left; margin-top: 1%"> Background Information </h2>
           <p>Text goes here.</p>
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           <p>Though the concept of engineering promoters to bind and sense targeted molecules is not a new concept in Synthetic Biology as demonstrated by the work several iGEM teams over the years, there are limitations with taking such guided approach.  
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Though a system is identified for the chosen target molecule, there is no variants in which to compare such system against. They also lack the ability to test many targeted molecules in parallel as each molecule would require their own engineered promoter. 
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In order to combat these limitations, we propose the creation of a library of synthetically engineered promoter that can be screened against targeted molecules in order to isolate a promoter being regulated by such molecule.
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           <h2 style="font-family: Rubik; text-align: left; margin-top: 1%"> Design Stage </h2>
 
           <h2 style="font-family: Rubik; text-align: left; margin-top: 1%"> Design Stage </h2>
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           <p>The Escherichia coli lactose (lac) operon is one of the most stud-ied paradigm for gene expression control (Becker et al., 2012). The lac system is ubiquitously used as a manner of controlling transcription in a range of different scenarios (Becker et al., 2012).
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It is also often used as a starting point for engineering and design of synthetic promoter variations as demonstrated by the work of Liu et al. in 2004. It was therefore chosen as the starting base for the design of the promoter library in this study.
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Promoter libraries can be created by varying many different as-pects of a wildtype promoter such as the upstream element prior to the -35 region, the downstream element, after the -10 region prior to -1, and its core sequence, between the -35 and -10 regions (Schlabach et al., 2010). In this study, we propose to use the PLac promoter sequence as our wildtype for creating promoter designs varying different areas of its sequence. One of such variation will be the substitution of the -35 and -10 currently found in PLac with the -35 (TTGACA) and -10 (TATAAT) regions found to be the most commonly occurring in E. coli natural promoters (Hawley and McClure, 1983, DeBoer, 1985, Harley and Reynolds, 1987). These were chosen to be the constant region between different promoter designs.
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By analyzing the findings of Harley and Reynolds (1987) and Lisser and Margalit (1993), the decision to vary the number of base pairs in the region present between the -35 and -10 elements to 17 base pairs instead of the 18 present in the wildtype PLac. Variations of the upstream and downstream regions where the lac operon would normally bind to will also be investigated in this study by the production of three different promoter designs resulting in a diverse promoter library.
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           <h2 style="font-family: Rubik; text-align: left; margin-top: 1%"> Implementation </h2>
 
           <h2 style="font-family: Rubik; text-align: left; margin-top: 1%"> Implementation </h2>

Revision as of 18:47, 31 October 2017

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Our Experimental Results



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Framework

Framework Chassis

Biochemical Adaptor

Target

Detector Modules

Multicellular Framework Testing

C12 HSL: Connector 1

Processor Modules

Framework in Cell Free Protein Synthesis Systems

C4 HSL: Connector 2

Reporter Modules



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