Team:EPF-Lausanne

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===Another approach: Melanopsin===
===Another approach: Melanopsin===

Revision as of 18:00, 25 September 2012


Contents

The "SWITCH" Project

In a nutshell

Our project is all about implementing a light activated genetic switch in mammalian cells. The production of complex proteins that require proper folding is becoming an increasingly commonplace task, particularly in the pharmaceutical industry amongst others. Mammalian cells are an ideal environment to make these proteins but producing them at the right time and optimal rate requires an expression system controlled by a specific signal. Until now these systems have mostly been limited to chemical signals which have many drawbacks. By using a light activated expression system, we hope to modify mammalian cells to respond to a light signal, rather than a chemical signal, by initiating gene expression for a protein of interest.

A new expression system: LovTAP fusion protein

Our main goal this summer was to implement a previously untested expression system in mammalian cells. The LovTAP-VP16 fusion protein we used is based on a previously tested fusion protein, LovTAP, which binds to a specific sequence of DNA once it is activated with blue light. By attaching an activating domain to the protein that is known to work in mammalian cells, we hoped to enable LovTAP to bind DNA after exposure to light and regulate expression of a gene next to its binding site in a mammalian cell line.

Team-EPF-Lausanne transfection graphic.jpg


Team-EPF-Lausanne activation.png


Team-EPF-Lausanne transfection graphic.jpg

Another approach: Melanopsin

We also worked with another light activated expression system that has already been proven to work. Martin Fusseneger et al. have designed a pathway that makes extensive use of gene expression pathways already present in the cell. By adding a light activated receptor on the cell membrane they promote the release of calcium into the cytoplasm upon exposure to light. This activates the native cellular response to an increased calcium concentration and promoter proteins sensitive to calcium will signal for the expression of genes with specific promoter sites. By introducing a new gene with a calcium sensitive promoter next to it, we can use light to induce its expression.

CHO cells & Co

The light activated expression systems we worked on would be extremely convenient for production of proteins in an industrial context and CHO (chinese hamster ovary) cells are the workhorses of industrial protein production. For our project, we transfected these cells with each expression system and conducted a variety of tests. Along with the CHO cell line we also chose to test these light activated systems using HEK (human embryonic kidney) cells since the melanopsin system had already been demonstrated to work in this cell type. The melanopsin system would provide data to compare against our LovTAP-VP16 system.


In each different cell line we tested a transfection containing a light-sensitive protein and a target gene or readout. We chose to express easily detectable fluorescent proteins so that we could compare the efficiency of both systems in turning on a particular gene. The fluorescent protein gene could eventually be replaced by a gene coding for a medically-relevant protein of interest to the pharmaceutical industry.

Not Only Pharma

The use of our switch is not limited to the pharmaceutical industry. LovTAP-VP16 switch can also be used in the experimental biology to observe temporal gene expression suppression. Our project have multitude of other valuable applications, yet achieving them requires comprehension and consent of general public. That's why, in addition to our experimental work, we've presented our project and the scope of synthetic biology at different occasions, and attempted to engage in a two-sided dialog by polling different populations to get their opinion about synthetic biology.

Check the rest of our wiki to see our project more in detail!