Project Description
Project Overview
To maximize control over a biological system, it would beneficial to have quick, reversible control over each step in gene expression, from transcription to translation to post-translational processing. Much work has been done to create switchable promoters, toggled by pulses of light, to control rates of transcription for genes of interest. The MIT iGEM team aims to take this concept and apply it to post-translational control, more specifically protein targeting in yeast. Our goal is to make a system in which a pulse of light causes a protein of interest to localize to one part of the cell. When pulsed with another wavelength of light, the protein will diffuse. In this way, a user can easily control both localization and delocalization of a protein of interest.
Our system takes advantage of the machinery used by plants and algae to respond to changing light conditions. Small pigmented proteins called phytochromes allow plants and algae to sense the amount and quality of the light available to them and to adjust rates of transcription accordingly. They are composed of a small pigment called a chromophore covalently bonded to a polypeptide. PhyB, our phytochrome of interest, binds to a chromophore called phycocyanobilin, or PCB. In red light, PhyB changes conformation into it’s active form and can bind to a transcription factor called PIF3. A pulse of far-red light returns the phytochrome to its inactive state. This mechanism provides the foundation of a a fast, reversible switch.
We have two main goals for our project. Our first goal is to be able to engineer yeast to produce the chromophore PCB endogenously. Right now, PCB has to be extracted from plants or cyanobacteria or from strains of E. coli that have been designed to produce PCB. We would like the switch to be self-contained in the strain we engineer, so we would like to engineer a strain of yeast to produce PCB. Our second goal is to engineer a system that adopts the PhyB-PIF3 switch to control protein localization within the cell. We plan to have either PhyB or PIF3 constitutively anchored to the target desired (e.g. mitochondrial membrane, nuclear membrane, vacuole etc). The other will then be bound to our protein of interest and will diffuse within the cell. When pulsed with red light, the PIF3 and PhyB will bind, causing the protein of interest to localize to the target.
Such a system would be useful in creating a reversible switch for synchronizing a culture of cells in one part of the cell cycle without having to deal with temperature sensitive mutants or adding chemicals externally to arrest the cell cycle. It would also be beneficial to study the kinetics of localization and delocalization, as well as provide an easy on-off switch for expression of essential genes. Light switchable transcriptional regulation has shown to be an effective way of increasing or decreasing gene expression quickly. By applying the concept of light switching to post-translational control as well, we aim to have greater control not only over gene expression, but also how the protein functions within the cell.
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Information
Members
Undergraduates
- Brian Ross, MIT '11
- Department of Biological Engineering
- Alexandra Doolittle, MIT '11
- Department of Biological Engineering
- Cory Li, MIT '12
- Department of Electrical Engineering
- Dominic McDonald, MIT '10
- Department of Chemical Engineering
Graduate
- Brian Belmont
- Department of Biological Engineering
- Jeffrey Wagner
- Department of Biological Engineering
- Nathan Klapoetke
- Department of Biological Engineering
- David Nielsen
- Department of Chemical Engineering
- Scott Carlson
- Department of Biological Engineering
- Stephen Goldfless
- Department of Biological Engineering
- Shawn Finney-Manchester
- Department of Chemical Engineering
- T.L. To
- Department of Chemical Engineering
Professors
- Prof. Narendra Maheshri
- Department of Chemical Engineering
- Prof. Natalie Kuldell
- Department of Biological Engineering
- Prof. Kristala Prather
- Department of Chemical Engineering
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