Effector Contributions to Gβγ-mediated Signaling as Revealed by Muscarinic Potassium Channel Gating

Tatyana T. Ivanova-Nikolova; Gerda E. Breitwieser

doi:10.1085/jgp.109.2.245

Effector Contributions to Gβγ-mediated Signaling as Revealed by Muscarinic Potassium Channel Gating

The Journal of General Physiology ◽

10.1085/jgp.109.2.245 ◽

1997 ◽

Vol 109 (2) ◽

pp. 245-253 ◽

Cited By ~ 32

Author(s):

Tatyana T. Ivanova-Nikolova ◽

Gerda E. Breitwieser

Keyword(s):

G Proteins ◽

Channel Gating ◽

K Channel ◽

Heterotrimeric G Proteins ◽

K Channels ◽

Protein Activation ◽

G Protein Activation ◽

Extracellular Stimuli ◽

Acetylcholine Concentration ◽

Signaling Process

Receptor-mediated activation of heterotrimeric G proteins leading to dissociation of the Gα subunit from Gβγ is a highly conserved signaling strategy used by numerous extracellular stimuli. Although Gβγ subunits regulate a variety of effectors, including kinases, cyclases, phospholipases, and ion channels (Clapham, D.E., and E.J. Neer. 1993. Nature (Lond.). 365:403–406), few tools exist for probing instantaneous Gβγ-effector interactions, and little is known about the kinetic contributions of effectors to the signaling process. In this study, we used the atrial muscarinic K+ channel, which is activated by direct interactions with Gβγ subunits (Logothetis, D.E., Y. Kurachi, J. Galper, E.J. Neer, and D.E. Clap. 1987. Nature (Lond.). 325:321–326; Wickman, K., J.A. Iniguez-Liuhi, P.A. Davenport, R. Taussig, G.B. Krapivinsky, M.E. Linder, A.G. Gilman, and D.E. Clapham. 1994. Nature (Lond.). 366: 654–663; Huang, C.-L., P.A. Slesinger, P.J. Casey, Y.N. Jan, and L.Y. Jan. 1995. Neuron. 15:1133–1143), as a sensitive reporter of the dynamics of Gβγ-effector interactions. Muscarinic K+ channels exhibit bursting behavior upon G protein activation, shifting between three distinct functional modes, characterized by the frequency of channel openings during individual bursts. Acetylcholine concentration (and by inference, the concentration of activated Gβγ) controls the fraction of time spent in each mode without changing either the burst duration or channel gating within individual modes. The picture which emerges is of a Gβγ effector with allosteric regulation and an intrinsic “off” switch which serves to limit its own activation. These two features combine to establish exquisite channel sensitivity to changes in Gβγ concentration, and may be indicative of the factors regulating other Gβγ-modulated effectors.

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Coupling of the human A1 adenosine receptor to different heterotrimeric G proteins: evidence for agonist-specific G protein activation

British Journal of Pharmacology ◽

10.1038/sj.bjp.0705925 ◽

2004 ◽

Vol 143 (6) ◽

pp. 705-714 ◽

Cited By ~ 52

Author(s):

Yolande Cordeaux ◽

Adriaan P IJzerman ◽

Stephen J Hill

Keyword(s):

G Protein ◽

G Proteins ◽

Adenosine Receptor ◽

Heterotrimeric G Proteins ◽

A1 Adenosine Receptor ◽

Protein Activation ◽

G Protein Activation

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Mutations in the ‘DRY’ motif of the CB1 cannabinoid receptor result in biased receptor variants

Journal of Molecular Endocrinology ◽

10.1530/jme-14-0219 ◽

2014 ◽

Vol 54 (1) ◽

pp. 75-89 ◽

Cited By ~ 15

Author(s):

Pál Gyombolai ◽

András D Tóth ◽

Dániel Tímár ◽

Gábor Turu ◽

László Hunyady

Keyword(s):

G Protein ◽

G Proteins ◽

Double Mutant ◽

Cannabinoid Receptor ◽

Camp Accumulation ◽

Protein Activation ◽

Cb1 Cannabinoid Receptor ◽

G Protein Activation ◽

Dry Motif

The role of the highly conserved ‘DRY’ motif in the signaling of the CB1cannabinoid receptor (CB1R) was investigated by inducing single-, double-, and triple-alanine mutations into this site of the receptor. We found that the CB1R-R3.50A mutant displays a partial decrease in its ability to activate heterotrimeric Goproteins (∼80% of WT CB1R (CB1R-WT)). Moreover, this mutant showed an enhanced basal β-arrestin2 (β-arr2) recruitment. More strikingly, the double-mutant CB1R-D3.49A/R3.50A was biased toward β-arrs, as it gained a robustly increased β-arr1 and β-arr2 recruitment ability compared with the WT receptor, while its G-protein activation was decreased. In contrast, the double-mutant CB1R-R3.50A/Y3.51A proved to be G-protein-biased, as it was practically unable to recruit β-arrs in response to agonist stimulus, while still activating G-proteins, although at a reduced level (∼70% of CB1R-WT). Agonist-induced ERK1/2 activation of the CB1R mutants showed a good correlation with their β-arr recruitment ability but not with their G-protein activation or inhibition of cAMP accumulation. Our results suggest that G-protein activation and β-arr binding of the CB1R are mediated by distinct receptor conformations, and the conserved ‘DRY’ motif plays different roles in the stabilization of these conformations, thus mediating both G-protein- and β-arr-mediated functions of CB1R.

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Cell surface beta-1,4-galactosyltransferase-I activates G protein-dependent exocytotic signaling

Development ◽

10.1242/dev.128.5.645 ◽

2001 ◽

Vol 128 (5) ◽

pp. 645-654

Author(s):

X. Shi ◽

S. Amindari ◽

K. Paruchuru ◽

D. Skalla ◽

H. Burkin ◽

...

Keyword(s):

G Protein ◽

G Proteins ◽

Pertussis Toxin ◽

Zona Pellucida ◽

Acrosome Reaction ◽

Cytoplasmic Domain ◽

Protein Activation ◽

Acrosomal Exocytosis ◽

G Protein Activation ◽

Galactosyltransferase I

ZP3 is a protein in the mammalian egg coat (zona pellucida) that binds sperm and stimulates acrosomal exocytosis, enabling sperm to penetrate the zona pellucida. The nature of the ZP3 receptor/s on sperm is a matter of considerable debate, but most evidence suggests that ZP3 binds to beta-1,4-galactosyltransferase-I (GalTase) on the sperm surface. It has been suggested that ZP3 induces the acrosome reaction by crosslinking GalTase, activating a heterotrimeric G protein. In this regard, acrosomal exocytosis is sensitive to pertussis toxin and the GalTase cytoplasmic domain can precipitate G(i) from sperm lysates. Sperm from mice that overexpress GalTase bind more soluble ZP3 and show accelerated G protein activation, whereas sperm from mice with a targeted deletion in GalTase have markedly less ability to bind soluble ZP3, undergo the ZP3-induced acrosome reaction, and penetrate the zona pellucida. We have examined the ability of GalTase to function as a ZP3 receptor and to activate heterotrimeric G proteins using Xenopus laevis oocytes as a heterologous expression system. Oocytes that express GalTase bound ZP3 but did not bind other zona pellucida glycoproteins. After oocyte maturation, ZP3 or GalTase antibodies were able to trigger cortical granule exocytosis and activation of GalTase-expressing eggs. Pertussis toxin inhibited GalTase-induced egg activation. Consistent with G protein activation, both ZP3 and anti-GalTase antibodies increased GTP-gamma[(35)S] binding as well as GTPase activity in membranes from eggs expressing GalTase. Finally, mutagenesis of a putative G protein activation motif within the GalTase cytoplasmic domain eliminated G protein activation in response to ZP3 or anti-GalTase antibodies. These results demonstrate directly that GalTase functions as a ZP3 receptor and following aggregation, is capable of activating pertussis toxin-sensitive G proteins leading to exocytosis.

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Role of G proteins in stimulation of Na-H exchange by cell shrinkage

AJP Cell Physiology ◽

10.1152/ajpcell.1992.262.2.c533 ◽

1992 ◽

Vol 262 (2) ◽

pp. C533-C536 ◽

Cited By ~ 41

Author(s):

B. A. Davis ◽

E. M. Hogan ◽

W. F. Boron

Keyword(s):

G Protein ◽

G Proteins ◽

Transport Processes ◽

Cell Shrinkage ◽

Protein Activation ◽

Kinase C ◽

G Protein Activation ◽

Barnacle Muscle Fibers ◽

Stimulation Of

Many cells respond to shrinkage by stimulating specific ion transport processes (e.g., Na-H exchange). However, it is not known how the cell senses this volume change, nor how this signal is transduced to an ion transporter. We have studied the activation of Na-H exchange in internally dialyzed barnacle muscle fibers, measuring intracellular pH (pHi) with glass microelectrodes. When cells are dialyzed to a pHi of approximately 7.2, Na-H exchange is active only in shrunken cells. We found that the shrinkage-induced stimulation of Na-H exchange, elicited by increasing medium osmolality from 975 to 1,600 mosmol/kgH2O, is inhibited approximately 72% by including in the dialysis fluid 1 mM guanosine 5'-O-(2-thiodiphosphate). The latter is an antagonist of G protein activation. Even in unshrunken cells, Na-H exchange is activated by dialyzing the cell with 1 mM guanosine 5'-O-(3-thiotriphosphate), which causes the prolonged activation of G proteins. Activation of Na-H exchange is also elicited in unshrunken cells by injecting cholera toxin, which activates certain G proteins. Neither exposing cells to 100 nM phorbol 12-myristate 13-acetate nor dialyzing them with a solution containing 20 microM adenosine 3',5'-cyclic monophosphate (cAMP) (or 50 microM dibutyryl cAMP) plus 0.5 mM 3-isobutyl-1-methylxanthine substantially stimulates the exchanger. Thus our data suggest that a G protein plays a key role in the transduction of the shrinkage signal to the Na-H exchanger via a pathway that involves neither protein kinase C nor cAMP.

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Structural basis for GPCR-independent activation of heterotrimeric Gi proteins

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.1906658116 ◽

2019 ◽

Vol 116 (33) ◽

pp. 16394-16403 ◽

Cited By ~ 15

Author(s):

Nicholas A. Kalogriopoulos ◽

Steven D. Rees ◽

Tony Ngo ◽

Noah J. Kopcho ◽

Andrey V. Ilatovskiy ◽

...

Keyword(s):

G Protein ◽

G Proteins ◽

Structural Changes ◽

Control Cell ◽

Structural Basis ◽

Common Mechanism ◽

Hydrophobic Core ◽

Nucleotide Exchange ◽

Protein Activation ◽

G Protein Activation

Heterotrimeric G proteins are key molecular switches that control cell behavior. The canonical activation of G proteins by agonist-occupied G protein-coupled receptors (GPCRs) has recently been elucidated from the structural perspective. In contrast, the structural basis for GPCR-independent G protein activation by a novel family of guanine-nucleotide exchange modulators (GEMs) remains unknown. Here, we present a 2.0-Å crystal structure of Gαi in complex with the GEM motif of GIV/Girdin. Nucleotide exchange assays, molecular dynamics simulations, and hydrogen–deuterium exchange experiments demonstrate that GEM binding to the conformational switch II causes structural changes that allosterically propagate to the hydrophobic core of the Gαi GTPase domain. Rearrangement of the hydrophobic core appears to be a common mechanism by which GPCRs and GEMs activate G proteins, although with different efficiency. Atomic-level insights presented here will aid structure-based efforts to selectively target the noncanonical G protein activation.

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Calcium sensitization produced by G protein activation in airway smooth muscle

AJP Lung Cellular and Molecular Physiology ◽

10.1152/ajplung.2001.281.3.l631 ◽

2001 ◽

Vol 281 (3) ◽

pp. L631-L638 ◽

Cited By ~ 15

Author(s):

Hayashi Yoshimura ◽

Keith A. Jones ◽

William J. Perkins ◽

Tetsuya Kai ◽

David O. Warner

Keyword(s):

Smooth Muscle ◽

G Proteins ◽

Myosin Light Chain ◽

Calcium Sensitization ◽

Protein Activation ◽

Maximal Force ◽

Acute Response ◽

Regulatory Myosin Light Chain ◽

G Protein Activation ◽

Intracellular Ca

We determined whether activation of G proteins can affect the force developed for a given intracellular Ca2+ concentration ([Ca2+]; i.e., the Ca2+ sensitivity) by mechanisms in addition to changes in regulatory myosin light chain (rMLC) phosphorylation. Responses in α-toxin-permeabilized canine tracheal smooth muscle were determined with Ca2+ alone or in the presence of ACh, endothelin-1 (ET-1), or aluminum fluoride (AlF[Formula: see text]; acute or 1-h exposure). Acute exposure to each compound increased Ca2+sensitivity without changing the response to high [Ca2+] (maximal force). However, chronic exposure to AlF[Formula: see text], but not to chronic ACh or ET-1, increased maximal force by increasing the force produced for a given rMLC phosphorylation. Studies employing thiophosphorylation of rMLC showed that the increase in force produced by chronic AlF[Formula: see text] exposure required Ca2+during activation to be manifest. Unlike the acute response to receptor agonists, which is mediated solely by increases in rMLC phosphorylation, chronic direct activation of G proteins further increases Ca2+ sensitivity in airways by additional mechanisms that are independent of rMLC phosphorylation.

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Intrinsic gating properties of a cloned G protein-activated inward rectifier K+ channel.

The Journal of General Physiology ◽

10.1085/jgp.106.1.1 ◽

1995 ◽

Vol 106 (1) ◽

pp. 1-23 ◽

Cited By ~ 24

Author(s):

C A Doupnik ◽

N F Lim ◽

P Kofuji ◽

N Davidson ◽

H A Lester

Keyword(s):

G Protein ◽

K Channel ◽

Extrinsic Factors ◽

Time Resolved ◽

Time Constants ◽

Protein Activation ◽

G Protein Activation ◽

Voltage Dependent ◽

Current Activation ◽

Inwardly Rectifying

The voltage-, time-, and K(+)-dependent properties of a G protein-activated inwardly rectifying K+ channel (GIRK1/KGA/Kir3.1) cloned from rat atrium were studied in Xenopus oocytes under two-electrode voltage clamp. During maintained G protein activation and in the presence of high external K+ (VK = 0 mV), voltage jumps from VK to negative membrane potentials activated inward GIRK1 K+ currents with three distinct time-resolved current components. GIRK1 current activation consisted of an instantaneous component that was followed by two components with time constants tau f approximately 50 ms and tau s approximately 400 ms. These activation time constants were weakly voltage dependent, increasing approximately twofold with maximal hyperpolarization from VK. Voltage-dependent GIRK1 availability, revealed by tail currents at -80 mV after long prepulses, was greatest at potentials negative to VK and declined to a plateau of approximately half the maximal level at positive voltages. Voltage-dependent GIRK1 availability shifted with VK and was half maximal at VK -20 mV; the equivalent gating charge was approximately 1.6 e-. The voltage-dependent gating parameters of GIRK1 did not significantly differ for G protein activation by three heterologously expressed signaling pathways: m2 muscarinic receptors, serotonin 1A receptors, or G protein beta 1 gamma 2 subunits. Voltage dependence was also unaffected by agonist concentration. These results indicate that the voltage-dependent gating properties of GIRK1 are not due to extrinsic factors such as agonist-receptor interactions and G protein-channel coupling, but instead are analogous to the intrinsic gating behaviors of other inwardly rectifying K+ channels.

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Structure, G Protein Activation, and Functional Relevance of the Cardiac G Protein-Gated K+ Channel, IKACh

Annals of the New York Academy of Sciences ◽

10.1111/j.1749-6632.1999.tb11300.x ◽

1999 ◽

Vol 868 (1 MOLECULAR AND) ◽

pp. 386-398 ◽

Cited By ~ 21

Author(s):

KEVIN WICKMAN ◽

GRIGORY KRAPIVINSKY ◽

SHAWN COREY ◽

MATT KENNEDY ◽

JAN NEMEC ◽

...

Keyword(s):

G Protein ◽

K Channel ◽

Protein Activation ◽

G Protein Activation ◽

Functional Relevance

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G-protein Activation Decreases Isoflurane Inhibition of N-type Ba2+Currents

Anesthesiology ◽

10.1097/00000542-200308000-00021 ◽

2003 ◽

Vol 99 (2) ◽

pp. 392-399 ◽

Cited By ~ 7

Author(s):

Igor M. Nikonorov ◽

Thomas J. J. Blanck ◽

Esperanza Recio-Pinto

Keyword(s):

Cholera Toxin ◽

G Protein ◽

G Proteins ◽

Pertussis Toxin ◽

Volatile Anesthetic ◽

Cell Voltage ◽

Dependent Manner ◽

Protein Activation ◽

G Protein Activation ◽

Voltage Dependent

Background G-protein activation mediates inhibition of N-type Ca2+ currents. Volatile anesthetics affect G-protein pathways at various levels, and activation of G-proteins has been shown to increase the volatile anesthetic potency for inhibiting the electrical-induced contraction in ileum. The authors investigated whether isoflurane inhibition of N-type Ba2+ currents was mediated by G-protein activation. Methods N-type Ba2+ currents were measured in the human neuronal SH-SY5Y cell line by using the whole cell voltage-clamp method. Results Isoflurane was found to have two effects on N-type Ba2+ currents. First, isoflurane reduced the magnitude of N-type Ba2+ currents to a similar extent (IC50 approximately 0.28 mm) in the absence and presence of GDPbetaS (a nonhydrolyzable GDP analog). Interestingly, GTPgammaS (a nonhydrolyzable GTP analog and G-protein activator) in a dose-dependent manner reduced the isoflurane block; 120 microm GTPgammaS completely eliminated the block of 0.3 mm isoflurane and reduced the apparent isoflurane potency by approximately 2.4 times (IC50 approximately 0.68 mm). Pretreatment with pertussis toxin or cholera toxin did not eliminate the GTPgammaS-induced protection against the isoflurane block. Furthermore, isoflurane reduced the magnitude of voltage-dependent G-protein-mediated inhibition of N-type Ba2+ currents, and this effect was eliminated by pretreatment with pertussis toxin or cholera toxin. Conclusions It was found that activation of G-proteins in a neuronal environment dramatically reduced the isoflurane potency for inhibiting N-type Ba2+ currents and, in turn, isoflurane affected the G-protein regulation of N-type Ba2+ currents.

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Modulation of N-Type Calcium Channel Activity by G-Proteins and Protein Kinase C

The Journal of General Physiology ◽

10.1085/jgp.115.3.277 ◽

2000 ◽

Vol 115 (3) ◽

pp. 277-286 ◽

Cited By ~ 55

Author(s):

Curtis F. Barrett ◽

Ann R. Rittenhouse

Keyword(s):

G Protein ◽

G Proteins ◽

Current Amplitude ◽

Whole Cell ◽

Protein Activation ◽

Kinase C ◽

Bath Application ◽

G Protein Activation ◽

Cervical Ganglion ◽

Ganglion Neurons

N-type voltage-gated calcium channel activity in rat superior cervical ganglion neurons is modulated by a variety of pathways. Activation of heterotrimeric G-proteins reduces whole-cell current amplitude, whereas phosphorylation by protein kinase C leads to an increase in current amplitude. It has been proposed that these two distinct pathways converge on the channel's pore-forming α1B subunit, such that the actions of one pathway can preclude those of the other. In this study, we have characterized further the actions of PKC on whole-cell barium currents in neonatal rat superior cervical ganglion neurons. We first examined whether the effects of G-protein–mediated inhibition and phosphorylation by PKC are mutually exclusive. G-proteins were activated by including 0.4 mM GTP or 0.1 mM GTP-γ-S in the pipette, and PKC was activated by bath application of 500 nM phorbol 12-myristate 13-acetate (PMA). We found that activated PKC was unable to reverse GTP-γ-S–induced inhibition unless prepulses were applied, indicating that reversal of inhibition by phosphorylation appears to occur only after dissociation of the G-protein from the channel. Once inhibition was relieved, activation of PKC was sufficient to prevent reinhibition of current by G-proteins, indicating that under phosphorylating conditions, channels are resistant to G-protein–mediated modulation. We then examined what effect, if any, phosphorylation by PKC has on N-type barium currents beyond antagonizing G-protein–mediated inhibition. We found that, although G-protein activation significantly affected peak current amplitude, fast inactivation, holding-potential–dependent inactivation, and voltage-dependent activation, when G-protein activation was minimized by dialysis of the cytoplasm with 0.1 mM GDP-β-S, these parameters were not affected by bath application of PMA. These results indicate that, under our recording conditions, phosphorylation by PKC has no effect on whole-cell N-type currents, other than preventing inhibition by G-proteins.

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