Regulators of G Protein Signaling and Transient Activation of Signaling

Hao, Nan; Yıldırım, Necmettin; Wang, Yuqi; Elston, Timothy C.; Dohlman, Henrik G.

doi:10.1074/jbc.m308432200

Cited by 65 publications

(45 citation statements)

References 43 publications

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“…The model is distinct from previous models (27)(28)(29)(30)(31)(32)(33) in that (i) it includes GAP, which many previous models have excluded; (ii) it is based on a general mechanism that allows several modes of coupling of G proteins with active receptors and GAPs, including a ternary complex of receptor, G protein, and GAP; and (iii) it is based on data pertaining to a single mammalian GTPase cycle module; i.e., the m1 muscarinic acetylcholine receptor (m1 MAchR), Gq, and RGS4 (34)(35)(36)(37). The predictions of the model elucidate how changes in concentrations of molecules can result in a variety of G protein signaling properties, both in terms of dynamics as well as steady-state behavior, and how these properties are governed by the kinetics of the GTPase-cycle module.…”

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confidence: 80%

Computational modeling reveals how interplay between components of a GTPase-cycle module regulates signal transduction

Bornheimer

Maurya

Farquhar

et al. 2004

Proc. Natl. Acad. Sci. U.S.A.

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Heterotrimeric G protein signaling is regulated by signaling modules composed of heterotrimeric G proteins, active G proteincoupled receptors (Rs), which activate G proteins, and GTPaseactivating proteins (GAPs), which deactivate G proteins. We term these modules GTPase-cycle modules. The local concentrations of these proteins are spatially regulated between plasma membrane microdomains and between the plasma membrane and cytosol, but no data or models are available that quantitatively explain the effect of such regulation on signaling. We present a computational model of the GTPase-cycle module that predicts that the interplay of local G protein, R, and GAP concentrations gives rise to 16 distinct signaling regimes and numerous intermediate signaling phenomena. The regimes suggest alternative modes of the GTPasecycle module that occur based on defined local concentrations of the component proteins. In one mode, signaling occurs while G protein and receptor are unclustered and GAP eliminates signaling; in another, G protein and receptor are clustered and GAP can rapidly modulate signaling but does not eliminate it. Experimental data from multiple GTPase-cycle modules is interpreted in light of these predictions. The latter mode explains previously paradoxical data in which GAP does not alter maximal current amplitude of G protein-activated ion channels, but hastens signaling. The predictions indicate how variations in local concentrations of the component proteins create GTPase-cycle modules with distinctive phenotypes. They provide a quantitative framework for investigating how regulation of local concentrations of components of the GTPase-cycle module affects signaling.T he timing and amplitude of signaling in cellular signaling networks depends on the local concentrations and kinetics of component proteins. The complexity of these networks has precluded comprehensive quantitative analysis of signaling. However, the networks can be divided into discrete signaling modules that can be quantitatively modeled and analyzed independently (1-5). Later, such models of modules can be experimentally verified and then reconnected to build larger signaling networks.G protein-mediated signaling networks (6) are ideal for such quantitative analysis. A key signaling module in these networks is the GTPase-cycle module, which controls signaling by regulating G protein activity. This module consists of a heterotrimeric G protein, a guanine nucleotide exchange factor (GEF) such as agonist-bound and active G protein-coupled receptor, a GTPase-activating protein (GAP) such as regulator of G protein signaling (RGS) protein or phospholipase C-␤, GTP, GDP, and P i . The extent of G protein activation reflects the balance between the rates of GDP͞GTP exchange, which activates the G protein, and GTP hydrolysis, which deactivates it (7-9). GEFs facilitate GDP͞GTP exchange (9), and GAPs accelerate GTP hydrolysis (10, 11). Additional roles of GEFs (12) and GAPs (10,11,13,14) are not included in this module. At present, we lack quantitativ...

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mentioning

confidence: 80%

Computational modeling reveals how interplay between components of a GTPase-cycle module regulates signal transduction

Bornheimer

Maurya

Farquhar

et al. 2004

Proc. Natl. Acad. Sci. U.S.A.

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“…Earlier studies indicate that Ste4 represents a crucial component in the pathway, and its activity must be tightly regulated (30,40). Growing evidence suggests that ubiquitination is involved in the regulation of G protein signaling (17,18).…”

Section: Resultsmentioning

confidence: 99%

“…Thus, although Ste4 is a critical determinant of the intensity and duration of downstream MAP kinase signaling (30,40), ubiquitination does not appear to alter the abundance of Ste4 and thereby the intensity of downstream MAP kinase signaling. Rather, ubiquitination of Ste4 appears to have a very specific role in regulating the timing of polarized cell growth in response to pheromone stimulation.…”

Section: Discussionmentioning

confidence: 99%

“…Specificity of detection was established using fus3⌬ and kss1⌬ cell extracts as negative controls. The pheromone-dependent transcription assay using the green fluorescent protein reporter (FUS1-GFP) has been described previously (30,37). To monitor the loss of Ste4 over time, early log cell cultures were treated with 3 M ␣-factor for 60 min, followed by cycloheximide (10 g/ml in 0.1% ethanol, final concentrations) for up to 2 h. Growth was stopped by the addition of 10 mM NaN 3 and transfer to an ice bath.…”

Section: Methodsmentioning

confidence: 99%

“…Estimates from a large scale quantitative immunoblotting study indicated that the number of Ste4 molecules (ϳ2050/cell) is much lower than either G␣ Gpa1 (ϳ9920/cell) or G␥ Ste18 (ϳ5550/cell) (29). Moreover, as little as 2-fold overexpression of Ste4 (but not Gpa1 and Ste18) is sufficient to yield full activation of the pathway (30). Given the limiting abundance of Ste4 and its crucial roles in pheromone signaling, it is likely that a battery of mechanisms may exist to regulate its activity to ensure accurate cellular responses to pheromone treatment.…”

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confidence: 99%

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Pheromone- and RSP5-dependent Ubiquitination of the G Protein β Subunit Ste4 in Yeast

Zhu

Torres

Kelley

et al. 2011

Journal of Biological Chemistry

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Ste4 is the ␤ subunit of a heterotrimeric G protein that mediates mating responses in Saccharomyces cerevisiae. Here we show that Ste4 undergoes ubiquitination in response to pheromone stimulation. Ubiquitination of Ste4 is dependent on the E3 ligase Rsp5. Disrupting the activity of Rsp5 abolishes ubiquitination of Ste4 in vivo, and recombinant Rsp5 is capable of ubiquitinating Ste4 in vitro. We find also that Lys-340 is a major ubiquitination site on Ste4, as pheromone-induced ubiquitination of the protein is prevented when this residue is mutated to an arginine. Functionally, ubiquitination does not appear to regulate the stability of Ste4, as blocking ubiquitination has no apparent effect on either the abundance or the half-life of the protein. However, when presented with a concentration gradient of pheromone, Ste4 K340R mutant cells polarize significantly faster than wild-type cells, indicating that ubiquitination limits pheromone-directed polarized growth. Together, these findings reveal a novel stimulus-dependent posttranslational modification of a G␤ subunit, establish Ste4 as a new substrate of the E3 ligase Rsp5, and demonstrate a role for G protein ubiquitination in cell polarization.

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Microfluidic gradient platforms for controlling cellular behavior

Chung

Choo

2010

Electrophoresis

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Concentration gradients play an important role in controlling biological and pathological processes, such as metastasis, embryogenesis, axon guidance, and wound healing. Microfluidic devices fabricated by photo- and soft lithography techniques can manipulate the fluidic flow and diffusion profile to create biomolecular gradients in a temporal and spatial manner. Furthermore, microfluidic devices enable the control of cell-extracellular microenvironment interactions, including cell-cell, cell-matrix, and cell-soluble factor interaction. In this paper, we review the development of microfluidic-based gradient devices and highlight their biological applications.

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Regulators of G Protein Signaling and Transient Activation of Signaling

Cited by 65 publications

References 43 publications

Computational modeling reveals how interplay between components of a GTPase-cycle module regulates signal transduction

Computational modeling reveals how interplay between components of a GTPase-cycle module regulates signal transduction

Pheromone- and RSP5-dependent Ubiquitination of the G Protein β Subunit Ste4 in Yeast

Microfluidic gradient platforms for controlling cellular behavior

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