Difference between revisions of "Team:Imperial College/Composite Part"

Revision as of 22:13, 19 October 2016

Composite Parts

In this section we aim to present all the composite parts that we have built and used thorough our project. In addition we introduce our best composite part: the pBAD-Gp2 construct, which provides a novel non-lethal way of inhibiting the growth of bacteria.

Best Composite Part - pBAD-Gp2

This year our best composite part is the pBAD-Gp2 construct. It provides a new way to repress growth in bacteria without killing the host cell. We have demonstrated that the cell is able to recover its initial growth rate once Gp2 is no longer expressed and can recover back to a normal growth rate. We are excited to provide this new growth regulator for the synthetic biology community and for future iGEM teams.

How does the pBAD-Gp2 construct work?

In the presence of arabinose (the promoter was active from 100 μM L-arabinose), the araC transcriptional regulator activates the pBAD promoter, resulting in the production of Gp2, a protein from T7 phage. Gp2 binds reversibly to the bacterial RNA polymerase, preventing protein production, and preventing the cell from dividing.

Figure 1: Schematic of the pBAD-Gp2 construct

The part was created by cloning a synthesised sequence block that contained Gp2, an RBS and the biobrick prefix and suffix, into an pBAD construct created by the 2014 Imperial iGEM team.

The construct effectively downregulates the growth of E. coli in response to arabinose, and does so in a reversible manner. We believe it is a good alternative to existing growth control methods, especially for controlling co-culture, for several reasons. You can read more about our characterisation data on our results page.

Key advantadges →Controlling cells in this way doesn’t require the usage of supplemented or minimal media, as in the case of antibiotics and auxotrophy.
→The system can easily be induced by L-arabinose, and switched off by d-glucose, both of which are non-toxic. .
→Gp2 is particularly good for regulating population size in co-cultures, as it only affects the size of one population.

Figure 2: Growth inhibition of Top10 cells by induction of Gp2 by arabinose

Figure 3: Recovery of growth by Top10 cells after induced araBAD operon is switched off by glucose-mediated catabolite repression.

BioBrick Registry Parts Table <groupparts>iGEM2016 Imperial_College</groupparts>

@@ Line 20: / Line 20: @@
 <specialh3> Best Composite Part - pBAD-Gp2 </specialh3>
-<p><br>This year our best composite part is the pBAD-Gp2 construct. It provides a new way to repress growth in bacteria without killing the host cell. We have demonstrated that the cell is able to recover its initial growth rate once Gp2 is not expressed and can recover back to a normal growth rate. We are excited to provide this new growth regulator for the synthetic biology community and for the future iGEM teams.
+<p><br>This year our best composite part is the pBAD-Gp2 construct. It provides a new way to repress growth in bacteria without killing the host cell. We have demonstrated that the cell is able to recover its initial growth rate once Gp2 is no longer expressed and can recover back to a normal growth rate. We are excited to provide this new growth regulator for the synthetic biology community and for future iGEM teams.
 </p>
-<specialh4>Key Advantages</specialh4>
+<specialh4>How does the pBAD-Gp2 construct work?</specialh4>
-<p>→The protein is very small, and can inhibit growth within a half-hour timeframe. <br>
+<p>In the presence of arabinose (the promoter was active from 100 μM L-arabinose), the araC transcriptional regulator activates the pBAD promoter, resulting in the production of Gp2, a protein from T7 phage. Gp2 binds reversibly to the bacterial RNA polymerase, preventing protein production, and preventing the cell from dividing. <br><br>
-→The repression is robust and reversible.<br>
-→The system does not require any toxins or supplements in the media.<br>
-→Usage of the gene avoids the problem of antimicrobial resistance. <br><br>
 </p>
 <center>
@@ Line 35: / Line 32: @@
 </center>
-<p><br><br>For our best composite part, we have selected the pBAD-Gp2 part. It was created by cloning a synthesised sequence block that contained Gp2, an RBS and the biobrick prefix and suffix, into an pBAD construct created by the 2014 Imperial iGEM team. <br><br><br>
+<p><br><br>The part was created by cloning a synthesised sequence block that contained Gp2, an RBS and the biobrick prefix and suffix, into an pBAD construct created by the 2014 Imperial iGEM team. <br><br><br>
+The construct effectively downregulates the growth of E. coli in response to arabinose, and does so in a reversible manner. We believe it is a good alternative to existing growth control methods, especially for controlling co-culture, for several reasons. You can read more about our characterisation data on our results page. <br><br>
+<specialh4>Key advantadges</specialh4>
-The construct effectively and rapidly downregulates the growth of E. coli in response to arabinose, and does so in a reversible manner. We believe it is a good alternative to existing growth control methods, especially for controlling co-culture, for several reasons<br><br>
 →Controlling cells in this way doesn’t require the usage of supplemented or minimal media, as in the case of antibiotics and auxotrophy.<br>
-→The gene is already naturally in the environment within the E.coli virus T7 phage, so there aren’t major biocontainment issues or the problems associated with antimicrobial resistance.<br>
+→The system can easily be induced by L-arabinose, and switched off by d-glucose, both of which are non-toxic. .<br>
-→It is specific to E. coli, and so, while possibly toxic to other prokaryotic bacteria, will not have any effect on eukaryotes. <br>
 →Gp2 is particularly good for regulating population size in co-cultures, as it only affects the size of one population.<br><br>
 <center>