Probing the effect of clustering on EphA2 receptor signaling efficiency by subcellular control of ligand-receptor mobility

Clustering of ligand:receptor complexes on the cell membrane is widely presumed to have functional consequences for subsequent signal transduction. However, it is experimentally challenging to selectively manipulate receptor clustering without altering other biochemical aspects of the cellular system. Here, we develop a microfabrication strategy to produce substrates displaying mobile and immobile ligands that are separated by roughly 1 µm, and thus experience an identical cytoplasmic signaling state, enabling precision comparison of downstream signaling reactions. Applying this approach to characterize the ephrinA1:EphA2 signaling system reveals that EphA2 clustering enhances both receptor phosphorylation and downstream signaling activity. Single-molecule imaging clearly resolves increased molecular binding dwell times at EphA2 clusters for both Grb2:SOS and NCK:N-WASP signaling modules. This type of intracellular comparison enables a substantially higher degree of quantitative analysis than is possible when comparisons must be made between different cells and essentially eliminates the effects of cellular response to ligand manipulation.

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Probe the effect of clustering on EphA2 receptor signaling efficiency by subcellular control of ligand-receptor mobility

10.1101/2021.02.16.431455 ◽

2021 ◽

Author(s):

Zhongwen Chen ◽

Dongmyung Oh ◽

Kabir H. Biswas ◽

Ronen Zaidel-Bar ◽

Jay T. Groves

Keyword(s):

Signal Transduction ◽

Single Molecule ◽

Cellular Response ◽

Dwell Time ◽

Signaling System ◽

Molecular Binding ◽

Downstream Signaling ◽

Functional Consequences ◽

Signaling Modules ◽

Signaling Efficiency

AbstractClustering of ligand:receptor complexes on the cell membrane is widely presumed to have functional consequences for subsequent signal transduction. However, it is experimentally challenging to selectively manipulate receptor clustering without altering other biochemical aspects of the cellular system. Here, we develop a microfabrication strategy to produce substrates displaying mobile and immobile ligands that are separated by roughly one micron and thus experience an identical cytoplasmic signaling state, enabling precision comparison of downstream signaling reactions. Applying this approach to characterize the ephrinA1:EphA2 signaling system reveals that EphA2 clustering enhances receptor phosphorylation. Single molecule imaging clearly resolves increased molecular binding dwell time at EphA2 clusters for both Grb2:SOS and NCK:NWASP signaling modules. This type of intracellular comparison enables a substantially higher degree of quantitative analysis than is possible when comparisons must be made between different cells and essentially eliminates the effects of cellular response to ligand manipulation.

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Resolving the Brassinosteroids Signal Transduction Mechanisms by Single-Molecule Assays

Biophysical Journal ◽

10.1016/j.bpj.2013.11.3974 ◽

2014 ◽

Vol 106 (2) ◽

pp. 719a

Author(s):

Song Song ◽

Haijiao Wang ◽

Xue-Lu Wang ◽

Yan-Wen Tan

Keyword(s):

Signal Transduction ◽

Single Molecule ◽

Transduction Mechanisms

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Clus-DoC: a combined cluster detection and colocalization analysis for single-molecule localization microscopy data

Molecular Biology of the Cell ◽

10.1091/mbc.e16-07-0478 ◽

2016 ◽

Vol 27 (22) ◽

pp. 3627-3636 ◽

Cited By ~ 35

Author(s):

Sophie V. Pageon ◽

Philip R. Nicovich ◽

Mahdie Mollazade ◽

Thibault Tabarin ◽

Katharina Gaus

Keyword(s):

T Cell ◽

T Cell Activation ◽

Single Molecule ◽

Cell Activation ◽

Spatial Organization ◽

Focal Adhesions ◽

Cell Receptor ◽

Intact Cells ◽

Analysis Strategy ◽

Signaling Activity

Advances in fluorescence microscopy are providing increasing evidence that the spatial organization of proteins in cell membranes may facilitate signal initiation and integration for appropriate cellular responses. Our understanding of how changes in spatial organization are linked to function has been hampered by the inability to directly measure signaling activity or protein association at the level of individual proteins in intact cells. Here we solve this measurement challenge by developing Clus-DoC, an analysis strategy that quantifies both the spatial distribution of a protein and its colocalization status. We apply this approach to the triggering of the T-cell receptor during T-cell activation, as well as to the functionality of focal adhesions in fibroblasts, thereby demonstrating an experimental and analytical workflow that can be used to quantify signaling activity and protein colocalization at the level of individual proteins.

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Signal Transduction and Cellular Response in RBL-2H3 Mast Cells

Chemical Immunology and Allergy - Membrane Activation in Immunologically Relevant Cells ◽

10.1159/000415508 ◽

2015 ◽

pp. 185-245

Author(s):

Janet M. Oliver ◽

JeanClare Seagrave ◽

Robert F. Stump ◽

Janet R. Pfeiffer ◽

Grace G. Deanin

Keyword(s):

Signal Transduction ◽

Mast Cells ◽

Cellular Response

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Investigations of Intercellular Mitochondrial Transfer in Neural Cells by Applied Single Molecule Genotyping

10.26686/wgtn.17145686 ◽

2021 ◽

Author(s):

◽

Matthew Rowe

Keyword(s):

Cell Line ◽

Single Molecule ◽

Cellular Response ◽

Rolling Circle Amplification ◽

Metabolic Phenotype ◽

Neural Cells ◽

Mitochondrial Transfer ◽

Mitochondrial Ribosome

<p>Over the past decade and a half, evidence for transfer of whole mitochondria between mammalian cells has emerged in the literature. The notion that mitochondria are restricted to the cell of origin has been overturned by this curious phenomenon, yet the physiological relevance of these transfer events remains unclear. This thesis investigates intercellular mitochondrial transfer in co-cultures of neural cells in vitro, to understand whether neural cells placed under stress demonstrate an enhanced rate of intercellular mitochondrial transfer. This would implicate the phenomenon as a cellular response to stress. Reliable techniques for quantitative study of intercellular mitochondrial transfer are limited so far in this field. To address this, a novel quantitative approach was developed to detect intercellular mitochondrial transfer, based on single molecule genotyping by target-primed rolling circle amplification. This enabled imaging of individual mitochondrial DNA molecules in situ, to detect those molecules which had moved between cells. Through this strategy, intercellular mitochondrial transfer was detected in new in vitro co-culture models. Primary murine pericytes derived from brain microvessels, were found to readily transfer mitochondria to a murine astrocyte cell line in vitro. Cisplatin, a DNA damaging agent; and chloramphenicol, a mitochondrial ribosome inhibitor, used to induce acute cellular injuries in the murine astrocyte cell line. These injuries were characterised and found to induce apoptosis, cause changes in growth characteristics, mitochondrial gene expression, and alter the metabolic phenotype of the cells. A derivative of the astrocyte cell line which completely lacks mitochondrial respiration, was found to model a chronic metabolic injury. As pericytes are prevalent throughout the brain, the pericyte/astrocyte co-culture model was selected to evaluate how the rate of intercellular mitochondrial transfer was altered, when the astrocytes were injured prior to co-culture. Through in situ single molecule genotyping and high throughput confocal microscopy, quantitative data was produced on how the rate of intercellular mitochondrial transfer was altered by injury in these models. The rate of intercellular mitochondrial transfer remained unaltered by chloramphenicol, however both cisplatin and the chronic metabolic injury model demonstrated reduced numbers of pericyte mitochondrial DNAs transferred into the injured astrocytes. These studies demonstrate successful application of a novel approach to study intercellular mitochondrial transfer and enable quantitative studies of this phenomenon.</p>

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Single molecule analysis of signal transduction through epidermal growth factor receptor

Seibutsu Butsuri ◽

10.2142/biophys.41.s29_2 ◽

2001 ◽

Vol 41 (supplement) ◽

pp. S29

Author(s):

M. Morimatsu ◽

K. Ota ◽

K. Hibino ◽

T. Miyauchi ◽

T. Uyemura ◽

...

Keyword(s):

Signal Transduction ◽

Epidermal Growth Factor Receptor ◽

Growth Factor ◽

Epidermal Growth Factor ◽

Single Molecule ◽

Growth Factor Receptor ◽

Epidermal Growth ◽

Single Molecule Analysis

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Sugar/osmoticum levels modulate differential abscisic acid-independent expression of two stress-responsive sucrose synthase genes in Arabidopsis

Biochemical Journal ◽

10.1042/bj3440503 ◽

1999 ◽

Vol 344 (2) ◽

pp. 503-509 ◽

Cited By ~ 47

Author(s):

Annabelle DÉJARDIN ◽

Lubomir N. SOKOLOV ◽

Leszek A. KLECZKOWSKI

Keyword(s):

Signal Transduction ◽

Abscisic Acid ◽

Cold Stress ◽

Osmotic Potential ◽

Sucrose Synthase ◽

Cellular Response ◽

Expression Profiles ◽

Soluble Sugars ◽

Leaf Osmotic Potential ◽

Detached Leaves

Sucrose synthase (Sus) is a key enzyme of sucrose metabolism. Two Sus-encoding genes (Sus1 and Sus2) from Arabidopsis thaliana were found to be profoundly and differentially regulated in leaves exposed to environmental stresses (cold stress, drought or O2 deficiency). Transcript levels of Sus1 increased on exposure to cold and drought, whereas Sus2 mRNA was induced specifically by O2 deficiency. Both cold and drought exposures induced the accumulation of soluble sugars and caused a decrease in leaf osmotic potential, whereas O2 deficiency was characterized by a nearly complete depletion in sugars. Feeding abscisic acid (ABA) to detached leaves or subjecting Arabidopsis ABA-deficient mutants to cold stress conditions had no effect on the expression profiles of Sus1 or Sus2, whereas feeding metabolizable sugars (sucrose or glucose) or non-metabolizable osmotica [poly(ethylene glycol), sorbitol or mannitol] mimicked the effects of osmotic stress on Sus1 expression in detached leaves. By using various sucrose/mannitol solutions, we demonstrated that Sus1 was up-regulated by a decrease in leaf osmotic potential rather than an increase in sucrose concentration itself. We suggest that Sus1 expression is regulated via an ABA-independent signal transduction pathway that is related to the perception of a decrease in leaf osmotic potential during stresses. In contrast, the expression of Sus2 was independent of sugar/osmoticum effects, suggesting the involvement of a signal transduction mechanism distinct from that regulating Sus1 expression. The differential stress-responsive regulation of Sus genes in leaves might represent part of a general cellular response to the allocation of carbohydrates during acclimation processes.

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Real-Time 3D Imaging at the Single Molecule Level of Signal Transduction in Saccharomyces CerevisiÆ Responding to Environmental Changes

Biophysical Journal ◽

10.1016/j.bpj.2015.11.823 ◽

2016 ◽

Vol 110 (3) ◽

pp. 145a

Author(s):

Erik G. Hedlund ◽

Sviatlana Shashkova ◽

Adam J.M. Wollman ◽

Stefan Hohmann ◽

Mark C. Leake

Keyword(s):

Saccharomyces Cerevisiae ◽

Signal Transduction ◽

Real Time ◽

Single Molecule ◽

3D Imaging ◽

Environmental Changes ◽

Single Molecule Level

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Investigation of the EnvZ/OmpR Bacterial Signaling System using Single Particle Tracking and Single Molecule Force Spectroscopy

Biophysical Journal ◽

10.1016/j.bpj.2014.11.043 ◽

2015 ◽

Vol 108 (2) ◽

pp. 5a

Author(s):

Yong Hwee Foo ◽

Ricksen Surya Winardhi ◽

Jie Yan ◽

Linda Kenney

Keyword(s):

Single Molecule ◽

Particle Tracking ◽

Single Particle ◽

Force Spectroscopy ◽

Single Particle Tracking ◽

Signaling System ◽

Single Molecule Force Spectroscopy ◽

Bacterial Signaling

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Compartmentalized cAMP signalling regulates vasopressin-mediated water reabsorption by controlling aquaporin-2

Biochemical Society Transactions ◽

10.1042/bst0331316 ◽

2005 ◽

Vol 33 (6) ◽

pp. 1316-1318 ◽

Cited By ~ 13

Author(s):

V. Henn ◽

E. Stefan ◽

G.S. Baillie ◽

M.D. Houslay ◽

W. Rosenthal ◽

...

Keyword(s):

Signal Transduction ◽

Protein Interactions ◽

Cellular Response ◽

Signal Transduction Pathway ◽

Basic Research ◽

New Drugs ◽

Response Signal ◽

Water Reabsorption ◽

Signalling Molecules ◽

Anchoring Proteins

The cAMP/PKA (protein kinase A) signalling pathway is activated by a plethora of stimuli. To facilitate the specificity of a cellular response, signal transduction complexes are formed and segregated to discrete sites (compartmentalization). cAMP/PKA signalling compartments are maintained by AKAPs (A-kinase anchoring proteins) which bind PKA and other signalling proteins, and by PDEs (phosphodiesterases). The latter hydrolyse cAMP and thus limit its diffusion and terminate PKA activity. An example of a cAMP-dependent process requiring compartmentalization of cAMP/PKA signals is arginine-vasopressin-regulated water reabsorption in renal principal cells. A detailed understanding of the protein interactions within a signal transduction complex offers the possibility to design agents influencing PKA binding to a specific AKAP, the targeting of an AKAP or the interactions of AKAPs with other signalling molecules. The ability to specifically modulate selected branches of a signal transduction pathway would greatly advance basic research, and may lead to new drugs suitable for the treatment of diseases caused by dysregulation of anchored PKA signalling (e.g. renal and cardiovascular diseases).

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