Team:ETHZ Basel/Biology
From 2010.igem.org
Biology & Wet Lab: Overview
The core idea of E. lemming is based on the spatial localization of one of the species of the chemotaxis network, so called Che proteins. Through localizing, the effective concentration of the Che protein is decreased at its site of action, affecting its activity on its downstream partners. Anchoring is achieved with the help of light-sensitive proteins (LSPs) that dimerize upon a light signal. The Che protein is fused to one of the LSPs, while the other LSP is fused to a so called anchor protein. Dimerization of the LSPs results in spatial re-localization of the Che protein, which, as a final measurable output, induces an altered ratio between tumbling and directed flagellar movement. Read more about the Molecular Mechanism.
The fusion proteins were constructed according to the Cloning Strategy BBF RFC28, a method for the combinatorial multi-part assembly based on the type II restriction enzmye AarI.
In the section Implementation, you find details on the experimental design such as the ideal conditions for the observation of chemotaxis behavior (strain, media, growth temperature, growth phase etc.) and the functionality and expression level testing of the fusion proteins.
The Archeal Light Receptor is another approach to implement the light-inducible synthetic network via the fusion of archeal and eubactarial parts.
For sure, we thought about Human Practices and Safety during our project. This section summarizes our findings on potential risk and safety issues.