Team:Duke/project/
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- | <tr><h5> | + | <tr><h5>Rational Bioengineering of LadA Monooxygenase in a Polyethylene Biodegradation Pathway</h5> |
- | + | <p> Polyethylene, a stable and common commercial plastic, presents a costly and persistent environmental problem. We are currently engineering a polyethylene biodegradation pathway by modifying an alkane degradation pathway in which a monooxygenase enzyme, LadA, performs the initial terminal oxidation step converting the alkane into an alcohol. The alcohol can later be processed into a fatty acid to be consumed for energy in a natural fatty acid metabolic pathway. Using Molegro Virtual Docker, we computationally analyzed the substrate specificity of LadA and identified a sub-region of Insertion Region 4 (IS4), comprising of residues 300-349, as the primary residues responsible for hindering polyethylene binding. We have isolated the wild-type gene from Geobacillus thermodenitrificans and are currently engineering a LadA mutant capable of binding to polyethylene through a combination of rational design and directed evolution. A large library of mutant LadA genes, that vary in the IS4 subregion, will be synthesized, spliced into bacteriophage vector and amplified in E. coli BLT5403 host to screen for a polyethylene-binding mutant through a phage display assay. In further research, the selected mutant will be combined with enzymes in the natural alkane biodegradation pathway to form an in vitro process that degrades polyethylene.</p> | |
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Revision as of 01:20, 30 October 2008
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