DOI: 10.1073/pnas.0710611105. Protein exchange dynamics at chemoreceptor clusters in <i>Escherichia coli</i>

Protein exchange dynamics at chemoreceptor clusters in Escherichia coli

10.1073/pnas.0710611105

Crossref journal-article

Proceedings of the National Academy of Sciences

Proceedings of the National Academy of Sciences (341)

Abstract

Signal processing in bacterial chemotaxis relies on large sensory complexes consisting of thousands of protein molecules. These clusters create a scaffold that increases the efficiency of pathway reactions and amplifies and integrates chemotactic signals. The cluster core in Escherichia coli comprises a ternary complex composed of receptors, kinase CheA, and adaptor protein CheW. All other chemotaxis proteins localize to clusters by binding either directly to receptors or to CheA. Here, we used fluorescence recovery after photobleaching (FRAP) to investigate the turnover of chemotaxis proteins at the cluster and their mobility in the cytoplasm. We found that cluster exchange kinetics were protein-specific and took place on several characteristic time scales that correspond to excitation, adaptation, and cell division, respectively. We further applied analytical and numerical data fitting to analyze intracellular protein diffusion and to estimate the rate constants of cluster equilibration in vivo . Our results indicate that the rates of protein turnover at the cluster have evolved to ensure optimal performance of the chemotaxis pathway.

Bibliography

Schulmeister, S., Ruttorf, M., Thiem, S., Kentner, D., Lebiedz, D., & Sourjik, V. (2008). Protein exchange dynamics at chemoreceptor clusters in Escherichia coli. Proceedings of the National Academy of Sciences, 105(17), 6403â6408.

Authors 6

Sonja Schulmeister (first)
Michaela Ruttorf (additional)
Sebastian Thiem (additional)
David Kentner (additional)
Dirk Lebiedz (additional)
Victor Sourjik (additional)

References 48 Referenced 75

Dates

Type	When
Created	17 years, 4 months ago (April 22, 2008, 1:23 a.m.)
Deposited	3 years, 4 months ago (April 12, 2022, 4:07 p.m.)
Indexed	2 months, 4 weeks ago (June 4, 2025, 6:30 a.m.)
Issued	17 years, 4 months ago (April 29, 2008)
Published	17 years, 4 months ago (April 29, 2008)
Published Online	17 years, 4 months ago (April 29, 2008)
Published Print	17 years, 4 months ago (April 29, 2008)

Funders 0

None

BibTeX

@article{Schulmeister_2008, title={Protein exchange dynamics at chemoreceptor clusters in Escherichia coli}, volume={105}, ISSN={1091-6490}, url={http://dx.doi.org/10.1073/pnas.0710611105}, DOI={10.1073/pnas.0710611105}, number={17}, journal={Proceedings of the National Academy of Sciences}, publisher={Proceedings of the National Academy of Sciences}, author={Schulmeister, Sonja and Ruttorf, Michaela and Thiem, Sebastian and Kentner, David and Lebiedz, Dirk and Sourjik, Victor}, year={2008}, month=apr, pages={6403–6408} }

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  "abstract": "<jats:p>\n            Signal processing in bacterial chemotaxis relies on large sensory complexes consisting of thousands of protein molecules. These clusters create a scaffold that increases the efficiency of pathway reactions and amplifies and integrates chemotactic signals. The cluster core in\n            <jats:italic>Escherichia coli</jats:italic>\n            comprises a ternary complex composed of receptors, kinase CheA, and adaptor protein CheW. All other chemotaxis proteins localize to clusters by binding either directly to receptors or to CheA. Here, we used fluorescence recovery after photobleaching (FRAP) to investigate the turnover of chemotaxis proteins at the cluster and their mobility in the cytoplasm. We found that cluster exchange kinetics were protein-specific and took place on several characteristic time scales that correspond to excitation, adaptation, and cell division, respectively. We further applied analytical and numerical data fitting to analyze intracellular protein diffusion and to estimate the rate constants of cluster equilibration\n            <jats:italic>in vivo</jats:italic>\n            . Our results indicate that the rates of protein turnover at the cluster have evolved to ensure optimal performance of the chemotaxis pathway.\n          </jats:p>",
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