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Details of Grant 

EPSRC Reference: EP/T002875/1
Title: Molecular Mechanics of Enzymes
Principal Investigator: Vollmer, Professor F
Other Investigators:
Littlechild, Professor JA Winlove, Professor CP Gow, Professor N
Researcher Co-Investigators:
Project Partners:
Department: Physics and Astronomy
Organisation: University of Exeter
Scheme: Standard Research
Starts: 01 April 2019 Ends: 31 March 2022 Value (£): 2,086,999
EPSRC Research Topic Classifications:
Analytical Science Biophysics
Chemical Biology
EPSRC Industrial Sector Classifications:
No relevance to Underpinning Sectors
Related Grants:
Panel History:
Panel DatePanel NameOutcome
19 Mar 2019 Building Collaboration at the Physics of Life Interface Announced
Summary on Grant Application Form
Laser light can be used to perform multiple roles, including sensing, manipulating and moving objects within a laser trap (so-called optical tweezers). It is remarkable that the application of light allows one to exert minute optical forces on individual protein molecules. By pulling on individual molecules it has been possible to study DNA and protein structures in great detail. The pulling and unfolding of proteins has revealed the intramolecular forces that give them their three-dimensional structure. Optical tweezer experiments have also allowed the direct measurement of pico-Newton forces that are exerted by individual motor proteins. However, optical tweezers and other single-molecule techniques are currently not sensitive enough to resolve femto-Newton (fN) forces, and hence not all molecular forces can yet be investigated. An important, but so far poorly understood example is the miniscule fN forces that are exerted by active enzymes when they are catalysing reactions in living systems.

This research programme will develop an entirely novel and much more sensitive alternative optical tweezer technology. The nanosensors developed in this programme will provide optical 'hands' that can probe and feel-out fN forces of enzymes. This allows precise sensing of the energetics of conformational changes of enzymes, i.e. their own deforming motion, for the first time. Such measurements will provide fundamental insights into the forces that drive the conformational changes that are required for catalysis. We will visualise the enzyme movements and this will allow us to develop more accurate models to predict how these very important molecular machines function. Our approach will unravel nature's design principles for a class of nanomachines that carry out most of the important biochemistry and molecular signalling that make our bodies work.

The technology developed in this programme will not only sense forces exerted by enzymes, but allows us to manipulate the complex motions of active enzymes. Such control offers the possibility of making some patterns of molecular organisation in an enzyme more likely than another, and can be used to control enzymatic activity. Demonstrating this capability will prepare the ground for future manipulation and exploitation of synthetic biomolecular machinery and designing enzymes for specific chemical or medical tasks.

Our pathway to impact work will demonstrate the extreme sensitivity of our technology in healthcare diagnostic tests that we will develop for human pathogens. Nanosensors will be modified by attaching enzymes. This will allow us to measure pathogen-specific signals during enzymatic breakdown of different sugars present on cell-walls of the human fungal pathogen Candida albicans - a pathogenic fungus that causes around 250,000 blood stream infections per year. This measurement will enable a more rapid identification of fungal pathogens than current microbial diagnostics of infections based on cell cultures. This approach will be tested on samples provided by the Fungal Immunology Group, AFGrica, located in Cape Town, South Africa.

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Organisation Website: http://www.ex.ac.uk