Team:Imperial College/mainresults
From 2013.igem.org
Line 74: | Line 74: | ||
</html> | </html> | ||
- | <p align="justify">One of the objectives of [https://2013.igem.org/Team:Imperial_College/Waste_Degradation:_SRF Module 1] is to produce P3HB bioplastic from waste. We compared P3HB degradation by measuring the concentration of 3HB monomers, using P3HB we bought from sigma, we produced from glucose, and we produced from the waste collected from Powerday. We found that there is no significant difference among them. Thus <b>we conclude that we have made P3HB bioplastic from waste | + | <p align="justify">One of the objectives of [https://2013.igem.org/Team:Imperial_College/Waste_Degradation:_SRF Module 1] is to produce P3HB bioplastic from waste. We compared P3HB degradation by measuring the concentration of 3HB monomers, using P3HB we bought from sigma, we produced from glucose, and we produced from the waste collected from Powerday. We found that there is no significant difference among them. Thus <b>we conclude that we have made P3HB bioplastic from waste</b>.</p> |
{| class="wikitable" style="margin: 1em auto 1em auto;" | {| class="wikitable" style="margin: 1em auto 1em auto;" |
Revision as of 23:55, 4 October 2013
Main Results
Resource-full Waste
Plastic Fantastic
We made P3HB bioplastic ▼
Our model predicts increased PhaB expression boosts P3HB production ▼
In order to realistically improve our experimental design, we produced P3HB synthesis model with considerations of central metabolic pathway within the cells. Our model predicts that during the synthesis of P3HB, the concentration of PhaB enzymes is an important rate limiting factor that can actually be regulated.
We optimised P3HB bioplastic production ▼
Since our model predicts that P3HB production can be significantly improved by expressing more P3HB polymerase PhaB, we designed a [http://parts.igem.org/Part:BBa_K1149051 hybrid promoter] which, consists of the J23104 constitutive promoter and the native promoter to optimise gene expression. Our results show that we have successfully produced 11-fold more P3HB bioplastic compared with the native promoter.
We made bioplastic from mixed waste ▼
One of the objectives of Module 1 is to produce P3HB bioplastic from waste. We compared P3HB degradation by measuring the concentration of 3HB monomers, using P3HB we bought from sigma, we produced from glucose, and we produced from the waste collected from Powerday. We found that there is no significant difference among them. Thus we conclude that we have made P3HB bioplastic from waste.
We degraded P3HB ▼
We degraded P3HB we made from waste ▼
Using 3HB colourimetric assay kit, we have shown that we have degraded the P3HB made from waste into 3HB monomers. In addition, there is no significant difference in 3HB concentration between different P3HB sources. This result proves that we now have a closed loop for P3HB bioplastic recycling!