Visualising a bacterial stress response: gene product localisations movements and gene regulation at single molecule level in live bacterial cells
Lead Research Organisation:
Imperial College London
Department Name: National Heart and Lung Institute
Abstract
Bacteria comprise one of the most abundant life forms on the planet, and contribute hugely to, for example, the major carbon, nitrogen, sulphur and phosporus cycles and transformations that characterise a functional and healthy global living environment. Despite huge advances in understanding how the components of the bacterial cell work, little is known about how they are organised within the living cell, nor how such organisations impact upon the functionality of the cell. Using a method that enables us to visualise single molecules within living cells, we will look in a quantitative way at the dynamics of the cellular components that let the cell survive a stress that damages its membrane. In effect we will be studying the cell in action, and will be able to describe the cell in its pre-stressed state as well as in its adapted state. Gaining an appreciation and understanding of how the cells components are organised for function is important in establishing principles of signaling and the networks of interactions that allow cells to grow and adapt to new environments.
Technical Summary
To date, much of our in depth understanding of cell functionality has been at the level of the detailed biochemical/biophysical characterisations of key cellular components. Advances in the field of single molecule, single cell imaging now make it possible to obtain quantitative information on the cellular localisations, interactions, dynamics and gene expressions of key effector and control proteins in important microbial cells. We plan to examine at the single molecule and single cell level how the E.coli cell adapts to stress that causes its inner membrane to lose integrity. This stress is important in a range of significant contexts, including protein export scenarios that support virulence in bacteria. One protein we will study, PspA, has a homologue in VIPP1, needed for thylakoid biogenesis. We will study in vivo (i) the states of self association of PspA and its localisations, to understand how it switches from negative regulator to effector, (ii) the localisations and dynamics of the effector protein PspG, the localisations and self associations of the transcriptional control protein PspF, and finally (iii) the expression dynamics of the pspG promoter. The latter will for the first time allow us to determine if expression of an activated and complexly controlled promoter does or does not show the geometric distribution of expression bursts seen with simple repression control as in lac. At present it is even unknown whether expression bursts are generally seen or not. The gene expression studies are important in understanding how variations in expression levels between cells might be caused, and for deducing whether different types of gene regulation strategies give rise to rather different types of outputs. Different types of outputs may well be better suited to some purposes than others, dependepending upon the type of gene product being produced.
Publications
Engl C
(2009)
In vivo localizations of membrane stress controllers PspA and PspG in Escherichia coli.
in Molecular microbiology
Fusco G
(2017)
Structural basis of membrane disruption and cellular toxicity by a-synuclein oligomers.
in Science (New York, N.Y.)
Gilburt JAH
(2017)
Dynamic Equilibrium of the Aurora A Kinase Activation Loop Revealed by Single-Molecule Spectroscopy.
in Angewandte Chemie (International ed. in English)
Gilburt JAH
(2019)
Ligand discrimination between active and inactive activation loop conformations of Aurora-A kinase is unmodified by phosphorylation.
in Chemical science
Huvet M
(2011)
The evolution of the phage shock protein response system: interplay between protein function, genomic organization, and system function.
in Molecular biology and evolution
Huvet M
(2009)
Model-based evolutionary analysis: the natural history of phage-shock stress response.
in Biochemical Society transactions
Joly N
(2009)
A lower-order oligomer form of phage shock protein A (PspA) stably associates with the hexameric AAA(+) transcription activator protein PspF for negative regulation.
in Journal of molecular biology
Jovanovic G
(2014)
The N-terminal amphipathic helices determine regulatory and effector functions of phage shock protein A (PspA) in Escherichia coli.
in Journal of molecular biology
Lenn T
(2011)
Measuring the stoichiometry of functional PspA complexes in living bacterial cells by single molecule photobleaching.
in Chemical communications (Cambridge, England)
Mehta P
(2013)
Dynamics and stoichiometry of a regulated enhancer-binding protein in live Escherichia coli cells.
in Nature communications
| Description | This grant has enabled us to develop an approach based on the imaging of the photobleaching steps of a fluorescent protein tagged protein complex to determine its stoichiometry in living cells. We have found that a stable repressive PspF-PspA complex is located in the nucleoid of an E. coli cell, transiently communicating with the inner membrane via PspA. We have also established that the PspF as a hexamer stably binds only one of the two psp promoters at a time, suggesting that psp promoters will fire asynchronously. |
| Exploitation Route | The code for protein complex stoichiometry analysis based on single molecule photobleaching has been used by other labs in the US and UK. |
| Sectors | Education Environment Pharmaceuticals and Medical Biotechnology |
| Description | The code developed for the measurement of the stoichiometry of protein complexes in living cells has been adopted by several other labs in the US and UK. |
| First Year Of Impact | 2011 |
| Sector | Education,Environment,Pharmaceuticals and Medical Biotechnology |
| Impact Types | Societal Economic |
| Description | Institute of Chemical Biology DTC PhD Studentship 2 (Imperial College London) |
| Amount | £85,000 (GBP) |
| Organisation | Engineering and Physical Sciences Research Council (EPSRC) |
| Sector | Public |
| Country | United Kingdom |
| Start | 08/2013 |
| End | 09/2017 |
| Description | Project grant/Leverhulme Trust (co-PI) |
| Amount | £241,000 (GBP) |
| Organisation | The Leverhulme Trust |
| Sector | Charity/Non Profit |
| Country | United Kingdom |
| Start | 02/2013 |
| End | 01/2016 |
| Title | Single molecule data for unphosphorylated Aurora-A (Gilburt et al, Chemical Science 2019) |
| Description | Raw and partially processed single molecule intensity histogram and dwell time histogram data for the following publication: James A H Gilburt, Paul Girvan, Julian Blagg, Liming Ying, Charlotte A Dodson (2019) Ligand discrimination between active and inactive activation loop conformations of Aurora-A kinase is unmodified by phosphorylation. Chemical Science. DOI: 10.1039/c8sc03669a Please cite our publication in any use of this data. |
| Type Of Material | Database/Collection of data |
| Year Produced | 2019 |
| Provided To Others? | Yes |
| Description | Application of CRISPR-Cas9 Technology in Fast Detection of Transgenic Products |
| Organisation | Chinese Academy of Sciences |
| Department | Institute for Nutritional Sciences |
| Country | China |
| Sector | Learned Society |
| PI Contribution | Investigate the molecular mechanisms and corresponding thermodynamic parameters of the detection system using single-molecule and other biophysical techniques. |
| Collaborator Contribution | 1. Prepare main components of the detection system, including Spy-dCas9 protein, specific sgRNA, double-stranded target DNA, DNA-RNA hybrid antibody, and so on. 2. Confirm the effectiveness of the detection system by in vitro approaches, and modify the reaction conditions. 3. In cooperation with the partner, further improve the specificity and sensitivity of the detection system based on its molecular mechanisms. 4. Quantitatively detect the heterologous gene fragments in samples from transgenic products by applying the system. |
| Impact | multi-disciplinary, biosensor/biophysics/spectroscopy |
| Start Year | 2016 |
| Description | Collaboration with Guangdong University of Technology, China |
| Organisation | Guangdong University of Technology |
| Department | Institute of Biomedical and Pharmaceutical Sciences |
| Country | China |
| Sector | Academic/University |
| PI Contribution | Provide research facilities to express, purify and label protein. Host a postdoctoral researcher form the partner organisation to carry out single molecule fluorescence measurement. |
| Collaborator Contribution | Salary of the postdoctoral researcher |
| Impact | Multi-disciplinary: biochemistry, biophysics, drug discovery |
| Start Year | 2017 |
| Description | Structural and functional characterisation of a G-quadruplex in the promoter of ß1-adrenergic receptor |
| Organisation | Chinese Academy of Sciences |
| Department | Shenzhen Institute of Advanced Integration Technology |
| Country | China |
| Sector | Academic/University |
| PI Contribution | Provide guidance for the project and carry out single molecule FRET measurements. |
| Collaborator Contribution | Cell biology and other biophysical measurements |
| Impact | Multi-disciplinary, biophysics/biochemistry/cell biology/cardiovascular science |
| Start Year | 2016 |
| Title | LABELLED KINASES FOR DRUG DISCOVERY |
| Description | A kinase or kinase fragment comprising a first label and a second label, wherein: the kinase or kinase fragment has a first conformation and second conformation; one or both of the first and second label are fluorophores; the first label and second label comprise an interacting pair capable of interacting with each other by static quenching or Dexter quenching or PET (photoinduced electron transfer) or exciplex formation to produce a quenched pair; and wherein the first and second labels are positioned on the kinase or kinase fragment such that when the kinase or kinase fragment is in the first conformation the labels are distal to each other such that static quenching or PET or Dexter quenching or exciplex formation does not occur and when the kinase or kinase fragment is in the second conformation the labels are brought into close proximity such that static quenching or PET or Dexter quenching or exciplex formation of one or both labels occurs. |
| IP Reference | WO2018167502 |
| Protection | Patent application published |
| Year Protection Granted | 2018 |
| Licensed | No |
| Impact | The new tool is expected to be widely applicable to the kinase drug development program. |
| Description | Guest speaker of Netherhall House |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | Local |
| Primary Audience | Public/other audiences |
| Results and Impact | A public lecture titled from DNA double helix to personalised medicine no actual impacts realised to date |
| Year(s) Of Engagement Activity | 2013 |
| Description | Invited seminar/Peking University 2009 |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Participants in your research or patient groups |
| Results and Impact | Seeing is believing: single molecule fluorescence approaches to biology and medicine, Department of Chemical Biology, Peking University, Beijing, July 2009 no actual impacts realised to date |
| Year(s) Of Engagement Activity | 2009 |
| Description | Invited seminar/University of Cambridge 2009 |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Participants in your research or patient groups |
| Results and Impact | Seeing is believing: single molecule fluorescence approaches to biology and medicine, Department of Chemistry, University of Cambridge, July 2009. no actual impacts realised to date |
| Year(s) Of Engagement Activity | 2009 |
| Description | Invited seminar/University of Warwick 2010 |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | local |
| Primary Audience | Participants in your research or patient groups |
| Results and Impact | Seeing Is Believing: Single Molecule Fluorescence Approaches to Biology, Warwick Mathematics Institute, University of Warwick, May 2010. no actual impacts realised to date |
| Year(s) Of Engagement Activity | 2010 |
| Description | Visit to Guangzhou Zengcheng Economic and technological Development Zone and short presentation to the business leaders and managing team of the Development Zone |
| Form Of Engagement Activity | A formal working group, expert panel or dialogue |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Industry/Business |
| Results and Impact | Visiting R&D facilities, give short presentation about translational research activities of the group |
| Year(s) Of Engagement Activity | 2016 |
| Description | Visit to Hainan Medical School, Haikou, China |
| Form Of Engagement Activity | A formal working group, expert panel or dialogue |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Professional Practitioners |
| Results and Impact | short presentation of research and dialogue with leaders, doctors and graduate students of the medical school |
| Year(s) Of Engagement Activity | 2016 |
| Description | Visit to Sanya People's Hospital |
| Form Of Engagement Activity | A formal working group, expert panel or dialogue |
| Part Of Official Scheme? | No |
| Geographic Reach | International |
| Primary Audience | Professional Practitioners |
| Results and Impact | Visit research labs and patient wards, science exchange via short presentations. This activity marks the beginning of the Academic Platform of the Hospital. |
| Year(s) Of Engagement Activity | 2016 |