Difference between revisions of "Team:Dalhousie Halifax NS/Results"

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<h3>Bacterial Isolation</h3>
 
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<h3>Colony PCR:</h3>
 
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<h2>Chemical Analysis</h2>
 
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<h3>High-Throughput Sequencing</h3>
 
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    <p>The colony PCR that was done with the cellulose-degrading colonies can be seen on the gel to the left. A 1kb ladder can also be seen on this image. Most of the PCR reactions were successful here, so the DNA was quantified used the geldoc and was purified with ExoSapIt before being sent to GeneWiz for sequencing.</p>
 
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Revision as of 10:33, 13 October 2016

This year we managed to isolate a few cellulose degrading bacteria and identify them. We also did an extensive proof of concept for our plan to use microbiomes as a "mine" for enzymes and gathered evidence that it would, likely, enable us to identify genes that encode cellulose degrading enzymes. We showed that growth of an E. coli strain used to degrade soft-wood lumber waste would not be inhibited by the anti-microbial properties of terpenes found in trees milled for softwood lumber. We also created a couple of new biobricks containing enzymes that we identified bioinformatically from Ruminiclostridium thermocellum, a cellulose degrader identified in the porcupine microbiome. Next year we intend to move forward with the metagenomic library and isolate more enzymes that would be useful for converting soft-wood lumber waste to a source of efficient fuel (ethanol) or be useful for bioremediation.

Our Results

DNA Sequencing and Bacterial Isolation

Bacterial Isolation

Colony PCR:

The colony PCR that was done with the cellulose-degrading colonies can be seen on the gel to the left. A 1kb ladder can also be seen on this image. Most of the PCR reactions were successful here, so the DNA was quantified used the geldoc and was purified with ExoSapIt before being sent to GeneWiz for sequencing.

High-Throughput Sequencing

Chemical Analysis

For the Future

What we have planned for the future

Dalhousie iGEM 2016