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Self-Organization of the Bacterial Cell

Project description

Protein dynamics underlying bacterial cell division

In light of the increasing prevalence of antibiotic resistance, insight into the mechanism by which bacterial cells grow and divide is central to the development of new and effective antibiotics. However, studying protein dynamics in living bacterial cells has proved challenging. Funded by the European Research Council, the SELFORGANICELL project aims to study bacterial cell division by employing a synthetic biology approach. Using protein biochemistry and high-resolution microscopy techniques to decipher the biochemical network underlying cell division, the research will focus on the spatial and temporal organisation of cell division proteins. Overall, the project will enhance our understanding of complex biochemical systems that give rise to living cells.

Objective

One of the most remarkable features of biological systems is their ability to self-organize in space and time. Even a relatively simple cell like the bacterium Escherichia coli has a precisely regulated cellular anatomy, which emerges from dynamic interactions between proteins and the cell membrane. Self-organization allows the cell to perform extremely challenging tasks. For example, for cell division, more than ten different proteins assemble into a complex, yet highly dynamic machine, which controls the invagination of the cell while constantly remodeling itself. Although the individual components involved have been largely identified, how they act together to accomplish this challenge is not understood. It has become clear that sophisticated biochemical networks give rise to intracellular organization, but we have yet to uncover the underlying mechanistic principles.
In this research proposal, I aim to develop a detailed mechanistic understanding of the self-organizing, emergent properties of the cell. To this end, my research group will develop novel in vitro reconstitution experiments combined with high-resolution fluorescence microscopy and theoretical modeling. Following this “bottom-up” approach, we will quantitatively analyze collective protein dynamics and emergent mechanochemical properties of the bacterial cell division machinery. I aim to answer the following fundamental questions:
1) What is the biochemical network giving rise to the dynamic assembly of the divisome?
2) How do the components of the divisome interact to generate force?
3) How do peptidoglycan synthases build the cell wall?
By comparing protein dynamics in vitro with those measured in vivo, we will provide a link between molecular properties and the processes found in the living cell. This project will not only improve our understanding of the bacterial cell, but also open new research avenues for eukaryotic cell biology, synthetic biology and biophysics.

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Topic(s)

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Funding Scheme

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ERC-STG - Starting Grant

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Call for proposal

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(opens in new window) ERC-2015-STG

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Host institution

INSTITUTE OF SCIENCE AND TECHNOLOGY AUSTRIA
Net EU contribution

Net EU financial contribution. The sum of money that the participant receives, deducted by the EU contribution to its linked third party. It considers the distribution of the EU financial contribution between direct beneficiaries of the project and other types of participants, like third-party participants.

€ 1 496 686,99
Address
Am Campus 1
3400 KLOSTERNEUBURG
Austria

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Region
Ostösterreich Niederösterreich Wiener Umland/Nordteil
Activity type
Higher or Secondary Education Establishments
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Total cost

The total costs incurred by this organisation to participate in the project, including direct and indirect costs. This amount is a subset of the overall project budget.

€ 1 496 686,99

Beneficiaries (1)

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