Team:Missouri Miners/Project


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PROJECT - Microbial Fuel Cell:

The goal of this research is the manipulation of E.Coli; granting them the ability to release electrons in an aerobic enviroment. This project utilizes geobacter's cytocromes, which makes it's extracellular electron transfer possible. The cytocromes OmcB,OmcE,OmcS, and MacA are our priority since they are the major electron smugglers out of the cell. By isolating and placing these cytocromes, some of which are naturally occur in E.Coli,into bricks we hope to make the electical application possible in other bacterial species.

Overall project

The optimization of electron shuffle within bacteria to external surfaces such as anodes is one of the primary goals of our project. Geobacter sulfurreducens is the bacteria of choice due to its ability to efficiently export electrons outside of the cell. E. coli is our desired "skeleton" bacteria for our project due to the bacteria's genome already containing many key proteins in the desired pathway. Extracellular pilin, MacA, and many other cytochromes that E. coli does not have will be isolated from Geobacter sulfurreducens and introduced into E. coli to create the most optimal pathway for generating electronmotive force in a microbial fuel cell apparatus.

A handful of problems have surfaced already in our project this year. Two of the most evident are correct plasmid engineering and Geobacter's anaerobic respiration contrasted to E. coli's aerobic respiration. Also, the role of Geobacter's pili in extracellular electron transfer is not clearly understood and could create a significant problem due to E. coli not having such pili. As a team, we will strive in the right direction harder than an emf on the internal resistivity of a toroid. Our team consists of many students working together from many diverse areas including Missouri S&T’s Electrical, Chemical, and Biological Engineering department along with the Biological Sciences.

Project Details


Laboratory techniques that have been utilized by team members working on the project:

  1. PCR amplification of the MacA and other cytochromes using PCR primers that added standard prefix and suffix sequences
  2. Cloning the cytochrome PCR products into a commercial cloning vector
  3. Digesting the cytochrome plasmids to obtain the promoter genes of interest
  4. Separating and isolating the enzyme digest fragments through gel electrophoresis
  5. Ligating the individual cytochrome promoters together
  6. Transforming bacterial cells with the recombined cytochrome plasmids
Extracellular Electron Transport Chain

Possible Applications: The applications of a interchangeable electron transfer gene part are limitless. The cytochrome cocktail could be used as a signal within bacteria. It would produce small currents which would be utilized in a similar fashion to fluorescent proteins as markers and indicators of cellular activity. Micro and nano-electronics could be adapted to use electron transfer modified bacteria as a cheap and effective power source. Medical research could benefit by using modified bacteria in areas of the body such as the stomach and intestines. The bacteria could be developed to act as a long term mobile monitor inside the human body.