Difference between revisions of "Team:Dundee Schools/Results"

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  <title>Dundee Schools: Results</title>
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<li class="menu_item"> <a href="https://2016.igem.org/Team:Dundee_Schools/Safety"> SAFETY </a> </li>
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<li class="menu_item"> <div class="icon plus"></div> HUMAN PRACTICES
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<li> <a href="https://2016.igem.org/Team:Dundee_Schools/HP/Gold">Gold </a></li>
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<li> <a href="https://2016.igem.org/Team:Dundee_Schools/Integrated_Practices"> Integrated Practices </a></li>
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<li> <a href="https://2016.igem.org/Team:Dundee_Schools/Engagement"> Engagement </a></li>
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                    </ul>
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<li class="menu_item"> <div class="icon plus"></div> AWARDS
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<li> <a href="https://2016.igem.org/Team:Dundee_Schools/Model">Modelling </a></li>
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<li> <a href="https://2016.igem.org/Team:Dundee_Schools/Measurement">Medals</a></li>
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<h1 id="team_name"> Dundee Schools </h1>
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<h4 id="page_name"> Results </h4>
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<p>The hfq is an RNA binding protein specific to <i>Vibrio cholerae</i> and <i>Shigella</i> which means it targets these bacteria. OsmY is a protein often secreted by <i>E. coli</i>. This means that we can attach our spiRNA which will be formed by a plasmid in the <i>E. coli</i>. However, the spiRNA cannot bind to the OsmY therefore we made an osmY – hfq fusion so it can bind to the sRNA. Our spiRNA is made from the expression systems, <i>Ec-sRNA</i> from <i>E. coli</i> and <i>Sma-sRNA</i> from <i>Serratia marcesens</i>. Once the spiRNA is outside of the <i>E. coli</i> we want the <i>Vibrio cholerae</i> and <i>Shigella</i> to take up the sRNA so that it can block a vital DNA sequence which stops translation of a protein which makes up the tail of the <i>Vibrio cholera</i>. This protein is called fliC. So in order to see if RNA interference would work in the treatment of bacterial infections, we ran some experiments on our BioBricks. First of all we ran numerous western blots to characterise our fusion proteins (S.O.R.D.) and see if they can be secreted along with our spiRNA. We then performed motility assays to see if our spiRNA works as we expect it to.</p>
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<h5>Western Blots</h5>
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<p><img src="https://static.igem.org/mediawiki/2016/f/ff/T--Dundee_Schools--results1.png"/>We ran a western blot on our rhamnose induced OsmY-HA expressing overnight cultures. We used OsmY-HA as a positive control to make sure OsmY is being secreted. First we added 500ul overnight cultures into 50ml of LB, we incubated the cultures at 37C until we reached an OD600 of 0.4. We followed this by adding different concentrations of rhamnose; 0.1%, 0.2%, 0.4% and 0.5% (v/v). We took a 1ml sample from the induced culture and measured the OD600 and then the samples from the cultures were spun down to separate the cells and supernatant. Through running both samples on a western blot we were able to determine whether; the protein was being expressed inside of the cell, and if the protein was being secreted outside of the cell. On the whole cell western blot, we can see that our OsmY-HA is being expressed in the presence of rhamnose (Fig. 1A). On the supernatant western blot, we can see traces of our OsmY-HA outside of the cell which shows that it is being secreted (Fig. 1B).<p>
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<p><img src="https://static.igem.org/mediawiki/2016/1/10/T--Dundee_Schools--results2.png"/>Once we knew our OsmY-HA was working and being secreted out of the cell we then proceeded to the next stage, we had to make sure that our fusion protein which was made up of the osmY-Ha and Hfq from <i>E. coli</i> was also being secreted to test this we ran an identical experiment with cells expressing our osmY-Hfq-HA constructs (Fig. 1A). The same had to be performed on the fusion containing the Hfq protein from <i>Serratia marcesens</i> and it can be seen that once again the fusion is being expressed when in the presence of the Rhamnose (Fig. 1B). Once we knew that the cells were being expressed we had to perform a western blot on the supernatant of the cells; this was done on the supernatant of each of the fusion proteins as well as the osmY-Ha and on the empty vector to make sure it’s not interfering with any of the results. From the results we can see that both of the fusions are secreting our protein however the <i>Serratia</i> version seems to be more limited in comparison to the <i>E. coli</i>. We can also see that the osmY-Ha is also being secreted out of the cell very well which is to be expected.</p>
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<p><img src="https://static.igem.org/mediawiki/2016/5/51/T--Dundee_Schools--results4.png"/>However, we had to make sure that our cells were not lysing in the process and releasing their contents into their surroundings; thus we once again performed a western blot, this time using a different anti-body used to check the presence of RNA polymerase which is only found inside of the cell. From the results we can see that each different cell was very rich in RNA polymerase, however we could not detect it in the supernatant (Fig. 3).</p>
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<h5>Motility Assays</h5>
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<p><img src="https://static.igem.org/mediawiki/2016/d/d4/T--Dundee_Schools--results3.png"/>We ran motility assays to see if our spiRNA was binding to the fliC in the flagellum of a bacteria and stopping it from swimming. We used the spiRNA secreted from <i>E. coli</i> for these motility assays. We grew some empty vector on a plate as a positive control and compared it to spiRNA with a 24 bp sequence of CDS which is part of fliC. We also ran motility assays on spiRNA-RBS-CDS to see if our spiRNA was stopping the CDS being translated by ribosomes. For our empty vector plate we saw a larger colony size than the two other plates which showed a very small amount of growth. This shows that our spiRNA from <i>E. coli</i> is successfully binding to the CDS and stopping the bacteria from swimming (Fig. 4A). We then worked out the average colony area. We got a larger average colony size for our empty vector than our two plates with our spiRNA. This again shows that our spiRNA is indeed working in the way that we expected. The spiRNA seems to work better for the CDS than the RBS-CDS as we got a smaller average colony size and a smaller standard deviation, however, we would need to run some further experiments to see if this is the case.</p>
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<p>Looking at these results, it can be seen that we have managed to prove that our S.O.R.D. can be secreted and that our spiRNA from <i>E. coli</i> is able to affect the motility of bacteria. Some further experiments we could have ran would be to test our spiRNA from <i>Serratia marcesens</i> to see if it also works at reducing bacteria motility. We know Hfq is an RNA binding protein but we don’t know how this function could be affect once it is fused together with OsmY. In future, we could run an experiment called an electrophoretic mobility shift assay to see if it can still bind to the spiRNA.</p>
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  <p style="position:fixed;float:right;width:auto;color:white;margin:1.5vh 2vw 0vh 40vw;font-weight:bold;font-size:3vh;">DUNDEE SCHOOLS: FIGHTING BACTERIAL INFECTIONS</p>
 
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Revision as of 04:20, 19 October 2016

Dundee Schools

Results

The hfq is an RNA binding protein specific to Vibrio cholerae and Shigella which means it targets these bacteria. OsmY is a protein often secreted by E. coli. This means that we can attach our spiRNA which will be formed by a plasmid in the E. coli. However, the spiRNA cannot bind to the OsmY therefore we made an osmY – hfq fusion so it can bind to the sRNA. Our spiRNA is made from the expression systems, Ec-sRNA from E. coli and Sma-sRNA from Serratia marcesens. Once the spiRNA is outside of the E. coli we want the Vibrio cholerae and Shigella to take up the sRNA so that it can block a vital DNA sequence which stops translation of a protein which makes up the tail of the Vibrio cholera. This protein is called fliC. So in order to see if RNA interference would work in the treatment of bacterial infections, we ran some experiments on our BioBricks. First of all we ran numerous western blots to characterise our fusion proteins (S.O.R.D.) and see if they can be secreted along with our spiRNA. We then performed motility assays to see if our spiRNA works as we expect it to.

Western Blots

We ran a western blot on our rhamnose induced OsmY-HA expressing overnight cultures. We used OsmY-HA as a positive control to make sure OsmY is being secreted. First we added 500ul overnight cultures into 50ml of LB, we incubated the cultures at 37C until we reached an OD600 of 0.4. We followed this by adding different concentrations of rhamnose; 0.1%, 0.2%, 0.4% and 0.5% (v/v). We took a 1ml sample from the induced culture and measured the OD600 and then the samples from the cultures were spun down to separate the cells and supernatant. Through running both samples on a western blot we were able to determine whether; the protein was being expressed inside of the cell, and if the protein was being secreted outside of the cell. On the whole cell western blot, we can see that our OsmY-HA is being expressed in the presence of rhamnose (Fig. 1A). On the supernatant western blot, we can see traces of our OsmY-HA outside of the cell which shows that it is being secreted (Fig. 1B).

Once we knew our OsmY-HA was working and being secreted out of the cell we then proceeded to the next stage, we had to make sure that our fusion protein which was made up of the osmY-Ha and Hfq from E. coli was also being secreted to test this we ran an identical experiment with cells expressing our osmY-Hfq-HA constructs (Fig. 1A). The same had to be performed on the fusion containing the Hfq protein from Serratia marcesens and it can be seen that once again the fusion is being expressed when in the presence of the Rhamnose (Fig. 1B). Once we knew that the cells were being expressed we had to perform a western blot on the supernatant of the cells; this was done on the supernatant of each of the fusion proteins as well as the osmY-Ha and on the empty vector to make sure it’s not interfering with any of the results. From the results we can see that both of the fusions are secreting our protein however the Serratia version seems to be more limited in comparison to the E. coli. We can also see that the osmY-Ha is also being secreted out of the cell very well which is to be expected.

However, we had to make sure that our cells were not lysing in the process and releasing their contents into their surroundings; thus we once again performed a western blot, this time using a different anti-body used to check the presence of RNA polymerase which is only found inside of the cell. From the results we can see that each different cell was very rich in RNA polymerase, however we could not detect it in the supernatant (Fig. 3).

Motility Assays

We ran motility assays to see if our spiRNA was binding to the fliC in the flagellum of a bacteria and stopping it from swimming. We used the spiRNA secreted from E. coli for these motility assays. We grew some empty vector on a plate as a positive control and compared it to spiRNA with a 24 bp sequence of CDS which is part of fliC. We also ran motility assays on spiRNA-RBS-CDS to see if our spiRNA was stopping the CDS being translated by ribosomes. For our empty vector plate we saw a larger colony size than the two other plates which showed a very small amount of growth. This shows that our spiRNA from E. coli is successfully binding to the CDS and stopping the bacteria from swimming (Fig. 4A). We then worked out the average colony area. We got a larger average colony size for our empty vector than our two plates with our spiRNA. This again shows that our spiRNA is indeed working in the way that we expected. The spiRNA seems to work better for the CDS than the RBS-CDS as we got a smaller average colony size and a smaller standard deviation, however, we would need to run some further experiments to see if this is the case.

Looking at these results, it can be seen that we have managed to prove that our S.O.R.D. can be secreted and that our spiRNA from E. coli is able to affect the motility of bacteria. Some further experiments we could have ran would be to test our spiRNA from Serratia marcesens to see if it also works at reducing bacteria motility. We know Hfq is an RNA binding protein but we don’t know how this function could be affect once it is fused together with OsmY. In future, we could run an experiment called an electrophoretic mobility shift assay to see if it can still bind to the spiRNA.