Your search keyword '"Michael W. Quick"' showing total 45 results

1. Short- and Long-Lasting Consequences ofIn VivoNicotine Treatment on Hippocampal Excitability

Author

Michael W. Quick, Robin A. J. Lester, and Rachel E. Penton

Subjects

Male, Nicotine, Patch-Clamp Techniques, Time Factors, Action Potentials, Hippocampus, Tetrodotoxin, In Vitro Techniques, Hippocampal formation, Drug Administration Schedule, Article, Rats, Sprague-Dawley, chemistry.chemical_compound, In vivo, Animals, Medicine, Nicotinic Agonists, Acetylcholine receptor, 6-Cyano-7-nitroquinoxaline-2,3-dione, Dose-Response Relationship, Drug, business.industry, General Neuroscience, Excitatory Postsynaptic Potentials, Dihydro-beta-Erythroidine, Electric Stimulation, Rats, Nicotinic agonist, 2-Amino-5-phosphonovalerate, chemistry, CNQX, Excitatory postsynaptic potential, business, Excitatory Amino Acid Antagonists, Neuroscience, Sodium Channel Blockers, medicine.drug

Abstract

The potential for relapse following cessation of drug use can last for years, implying the induction of stable changes in neural circuitry. In hippocampal slices from rats treated with nicotine for 1 week, withdrawal from nicotinein vivoproduces an increase in CA1 pyramidal cell excitability that persists up to 9 months. Immediately upon drug cessation, the enhanced excitability depends on input from regions upstream of CA1, while the long-term excitability change (> 4 weeks) is expressed as an increase in the intrinsic excitability of CA1 neurons. Re-exposure to nicotinein vitrorestores hippocampal function to control levels via activation of high-affinity nicotinic acetylcholine receptors after 1 d of withdrawal, but not at times >4 weeks. Thus, nicotinein vivofirst induces homeostatic adaptations followed by other more robust neural changes. These mechanisms may contribute to hippocampal localized cue-motivated reinstatement of drug-seeking and/or cognitive deficits observed during withdrawal.

Published

2011

2. GABA transporter function, oligomerization state, and anchoring: correlates with subcellularly resolved FRET

Author

P. I. Imoukhuede, Kimberly Scott, Jia Hu, Henry A. Lester, Michael W. Quick, Fraser J. Moss, and Joanna L. Jankowsky

Subjects

GABA Plasma Membrane Transport Proteins, Physiology, PDZ domain, Cell Line, Cell membrane, Mice, 03 medical and health sciences, 0302 clinical medicine, Fluorescence Resonance Energy Transfer, medicine, Animals, Humans, GABA transporter, Cytoskeleton, gamma-Aminobutyric Acid, 030304 developmental biology, Tutorial Research Article, 0303 health sciences, biology, Cell Membrane, Biological Transport, Actin cytoskeleton, medicine.anatomical_structure, Förster resonance energy transfer, Biochemistry, biology.protein, Biophysics, Postsynaptic density, 030217 neurology & neurosurgery

Abstract

The mouse gamma-aminobutyric acid (GABA) transporter mGAT1 was expressed in neuroblastoma 2a cells. 19 mGAT1 designs incorporating fluorescent proteins were functionally characterized by [(3)H]GABA uptake in assays that responded to several experimental variables, including the mutations and pharmacological manipulation of the cytoskeleton. Oligomerization and subsequent trafficking of mGAT1 were studied in several subcellular regions of live cells using localized fluorescence, acceptor photobleach Förster resonance energy transfer (FRET), and pixel-by-pixel analysis of normalized FRET (NFRET) images. Nine constructs were functionally indistinguishable from wild-type mGAT1 and provided information about normal mGAT1 assembly and trafficking. The remainder had compromised [(3)H]GABA uptake due to observable oligomerization and/or trafficking deficits; the data help to determine regions of mGAT1 sequence involved in these processes. Acceptor photobleach FRET detected mGAT1 oligomerization, but richer information was obtained from analyzing the distribution of all-pixel NFRET amplitudes. We also analyzed such distributions restricted to cellular subregions. Distributions were fit to either two or three Gaussian components. Two of the components, present for all mGAT1 constructs that oligomerized, may represent dimers and high-order oligomers (probably tetramers), respectively. Only wild-type functioning constructs displayed three components; the additional component apparently had the highest mean NFRET amplitude. Near the cell periphery, wild-type functioning constructs displayed the highest NFRET. In this subregion, the highest NFRET component represented approximately 30% of all pixels, similar to the percentage of mGAT1 from the acutely recycling pool resident in the plasma membrane in the basal state. Blocking the mGAT1 C terminus postsynaptic density 95/discs large/zona occludens 1 (PDZ)-interacting domain abolished the highest amplitude component from the NFRET distributions. Disrupting the actin cytoskeleton in cells expressing wild-type functioning transporters moved the highest amplitude component from the cell periphery to perinuclear regions. Thus, pixel-by-pixel NFRET analysis resolved three distinct forms of GAT1: dimers, high-order oligomers, and transporters associated via PDZ-mediated interactions with the actin cytoskeleton and/or with the exocyst.

Published

2009

3. Substrate-mediated regulation of γ-aminobutyric acid transporter 1 in rat brain

Author

Michael W. Quick and Jia Hu

Subjects

GABA Plasma Membrane Transport Proteins, Neurotransmitter transporter, Nipecotic Acids, Biotin, Down-Regulation, Bicuculline, Article, Exocytosis, gamma-Aminobutyric acid, GABA transporter 1, GABA Antagonists, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Pregnancy, Serine, medicine, Animals, Immunoprecipitation, Protein phosphorylation, Phosphorylation, Cells, Cultured, gamma-Aminobutyric Acid, Brain Chemistry, Neurons, Pharmacology, biology, Tyrosine phosphorylation, Transporter, Receptors, GABA-A, Endocytosis, Rats, Cell biology, chemistry, biology.protein, Female, GLUT4, medicine.drug

Abstract

The uptake of neurotransmitter by plasma membrane transporters is a principal method for regulating extracellular transmitter levels. Neurotransmitter-mediated signals in turn are able to regulate transporter expression and function. Thus, there is a continual interplay between transporters and the transmitters they transport. Previously we showed that extracellular gamma-aminobutyric acid (GABA) increases the expression of the GABA transporter 1 (GAT1) on a time scale of minutes by acting via the transporter to slow transporter internalization. This mechanism requires in part direct tyrosine phosphorylation of the transporter. In the present study we show that the presence of GABA on a longer time scale causes a net decrease in GAT surface expression. The decrease in expression represents the contributions of transporter-mediated up-regulation and a more substantial GABA-receptor-mediated down-regulation. This receptor-mediated down-regulation is the result of both changes in the rates of transporter trafficking and in the number of transporters available for trafficking. As with transporter-mediated regulation of GAT1, the receptor-mediated regulation is associated with changes in the direct phosphorylation of GAT1. These data suggest that multiple pathways, perhaps converging upon mechanisms involving protein phosphorylation, act to regulate GAT1 expression in neurons.

Published

2008

4. Regulating the Conducting States of a Mammalian Serotonin Transporter

Author

Michael W. Quick

Subjects

Embryo, Nonmammalian, Patch-Clamp Techniques, Time Factors, Vesicular Transport Proteins, Syntaxin 1, Kidney, Choline, Membrane Potentials, Xenopus laevis, Serotonin Agents, 0302 clinical medicine, Cocaine, Thalamus, Drug Interactions, Botulinum Toxins, Type A, Cells, Cultured, Serotonin transporter, Neurons, Serotonin Plasma Membrane Transport Proteins, Membrane potential, 0303 health sciences, Membrane Glycoproteins, General Neuroscience, Depolarization, Biochemistry, Isotope Labeling, Antigens, Surface, Selective Serotonin Reuptake Inhibitors, Serotonin, Microinjections, N-Methyl-3,4-methylenedioxyamphetamine, Recombinant Fusion Proteins, Neuroscience(all), Immunoblotting, Nerve Tissue Proteins, Biology, Tritium, Protein–protein interaction, 03 medical and health sciences, Munc18 Proteins, Fluoxetine, Animals, Humans, Molecular Biology, 5-HT receptor, 030304 developmental biology, Binding Sites, Dose-Response Relationship, Drug, Sodium, Electric Conductivity, Membrane Transport Proteins, Proteins, Transporter, Embryo, Mammalian, Peptide Fragments, Rats, Mutation, Oocytes, Biophysics, biology.protein, Radiopharmaceuticals, Carrier Proteins, Flux (metabolism), 030217 neurology & neurosurgery

Abstract

Serotonin transporters (SERTs), sites of psychostimulant action, display multiple conducting states in expression systems. These include a substrate-independent transient conductance, two separate substrate-independent leak conductances associated with Na + and H + , and a substrate-dependent conductance of variable stoichiometry, which exceeds that predicted from electroneutral substrate transport. The present data show that the SNARE protein syntaxin 1A binds the N-terminal tail of SERT, and this interaction regulates two SERT-conducting states. First, substrate-induced currents are absent because Na + flux becomes strictly coupled to 5HT transport. Second, Na + -mediated leak currents are eliminated. These two SERT-conducting states are present endogenously in thalamocortical neurons, act to depolarize the membrane potential, and are modulated by molecules that disrupt SERT and syntaxin 1A interactions. These data show that protein interactions govern SERT activity and suggest that both cell excitability and psychostimulant-mediated effects will be dependent upon the state of association among SERT and its interacting partners.

Published

2003

5. Syntaxin 1A Inhibits GABA Flux, Efflux, and Exchange Mediated by the Rat Brain GABA Transporter GAT1

Author

Michael W. Quick, Dan Wang, Scott L. Deken, and Terri L. Whitworth

Subjects

GABA Plasma Membrane Transport Proteins, Vesicle docking, Organic Anion Transporters, Syntaxin 1, Nerve Tissue Proteins, Hippocampus, Xenopus laevis, Animals, Syntaxin, GABA transporter, Binding site, gamma-Aminobutyric Acid, Ion channel, Pharmacology, Binding Sites, biology, Membrane Proteins, Membrane Transport Proteins, Biological Transport, Transporter, Rats, Cell biology, nervous system, Antigens, Surface, Oocytes, biology.protein, Molecular Medicine, Carrier Proteins, Cotransporter, Flux (metabolism)

Abstract

GABA transporters control extracellular GABA levels by coupling transmitter uptake to the sodium and chloride cotransport. The rat brain GABA transporter GAT1 and other members of this family are regulated by direct interactions with syntaxin 1A, a protein involved in vesicle docking and in the regulation of several ion channels and transporters. We have shown previously that syntaxin 1A exerts its effects on GAT1 by decreasing the net uptake of GABA and its associated ions through interactions with aspartic acid residues in the N-terminal tail of GAT1. This reduction in net uptake could be caused by many steps in the transport cycle, including substrate binding, substrate flux, substrate efflux, or reorientation of the unliganded transporter. To address this question, we performed GABA flux assays, measured flux- and efflux-associated ion currents, and assessed GABA exchange in multiple experimental systems expressing syntaxin 1A and wild-type GAT1 or GAT1 mutants. Syntaxin 1A caused similar reductions in forward and reverse transport that did not involve changes in apparent transport affinities for sodium, chloride, or GABA. The syntaxin 1A-mediated reduction in GABA flux and efflux was mimicked by mutations in GAT1 at the syntaxin 1A binding site. The binding site GAT1 mutant also caused a reduction in exchange. These data suggest that syntaxin 1A exerts its effects, directly or indirectly, on GAT1 function through interactions with GAT1's N-terminal tail and that the inhibition occurs at a step in the translocation process after substrate binding but which involves both unidirectional transport and transmitter exchange.

Published

2003

6. Plasma Membrane GABA Transporters Reside on Distinct Vesicles and Undergo Rapid Regulated Recycling

Author

Scott L. Deken, Michael W. Quick, and Dan Wang

Subjects

GABA Plasma Membrane Transport Proteins, Vesicle fusion, Biotin, Organic Anion Transporters, CHO Cells, Brief Communication, Hippocampus, Clathrin, Synaptic vesicle, Cricetinae, Animals, GABA transporter, Cells, Cultured, Dynamin, Brain Chemistry, Neurons, biology, General Neuroscience, Vesicle, Cell Membrane, Membrane Proteins, Membrane Transport Proteins, Avidin, Rats, Cell biology, Protein Transport, Synapses, biology.protein, GABAergic, Synaptic Vesicles, Synaptic signaling, Carrier Proteins, Synaptosomes

Abstract

Plasma membrane neurotransmitter transporters affect synaptic signaling through transmitter sequestration. Transporters redistribute to and from the plasma membrane, suggesting a role for trafficking in regulating synaptic transmitter levels. One method for controlling transmitter levels would be to regulate transporter redistribution in parallel with transmitter release. Thus, how similar are these processes? We show that the trafficking of the GABA transporter GAT1 resembles the trafficking of neurotransmitter-filled synaptic vesicles: (1) transporters located on the plasma membrane are internalized and reinserted into the plasma membrane on the order of minutes; (2) the rate of recycling is depolarization and calcium dependent; (3) GAT1 internalization is associated with clathrin and dynamin; and (4) intracellular GAT1 is associated with multiple compartments and, more importantly, is found on a distinct class of vesicles. These vesicles are clear, ∼50 nm in diameter, and contain many proteins found on neurotransmitter-containing small synaptic vesicles; however, they appear to lack several traditional small synaptic vesicle proteins, such as synaptophysin and the vesicular GABA transporter. These data provide additional support for the hypothesis that GABA transporters traffic in parallel with neurotransmitter-containing small synaptic vesicles and also raise the possibility that some fraction of vesicles found in GABAergic neurons may not be participating in transmitter release but rather in the rapid regulated redistribution of membrane proteins involved in transmitter uptake.

Published

2003

7. An evolutionarily conserved dileucine motif in Shal K+ channels mediates dendritic targeting

Author

Don B. Arnold, Jacqueline F. Rivera, Emily R. Liman, Michael W. Quick, and Shoeb Ahmad

Subjects

Cell type, Potassium Channels, CD8 Antigens, Recombinant Fusion Proteins, Amino Acid Motifs, Molecular Sequence Data, In Vitro Techniques, Biology, Conserved sequence, Leucine, Animals, Amino Acid Sequence, Peptide sequence, Peroxisomal targeting signal, Cells, Cultured, Conserved Sequence, Kv1.3 Potassium Channel, Shal Potassium Channels, Voltage-gated ion channel, Pyramidal Cells, General Neuroscience, Dendrites, Endocytosis, Potassium channel, Rats, Cell biology, Transport protein, Protein Transport, nervous system, Biochemistry, Potassium Channels, Voltage-Gated, Kv1.4 Potassium Channel, Neuroscience

Abstract

The molecular mechanisms underlying polarized sorting of proteins in neurons are poorly understood. Here we report the identification of a 16 amino-acid, dileucine-containing motif that mediates dendritic targeting in a variety of neuronal cell types in slices of rat brain. This motif is present in the carboxy (C) termini of Shal-family K+ channels and is highly conserved from C. elegans to humans. It is necessary for dendritic targeting of potassium channel Kv4.2 and is sufficient to target the axonally localized channels Kv1.3 and Kv1.4 to the dendrites. It can also mediate dendritic targeting of a non-channel protein, CD8.

Published

2003

8. The Interaction between Syntaxin 1A and Cystic Fibrosis Transmembrane Conductance Regulator Cl− Channels Is Mechanistically Distinct from Syntaxin 1A-SNARE Interactions

Author

Kevin L. Kirk, Michael W. Quick, Radhika Ganeshan, Anke Di, and Deborah J. Nelson

Subjects

Recombinant Fusion Proteins, Xenopus, Molecular Sequence Data, Vesicular Transport Proteins, Cystic Fibrosis Transmembrane Conductance Regulator, Syntaxin 1, Nerve Tissue Proteins, Transfection, Biochemistry, Protein Structure, Secondary, Cell Line, Mice, Chloride Channels, Cricetinae, Animals, Humans, Protein Isoforms, Syntaxin, Amino Acid Sequence, Qc-SNARE Proteins, Molecular Biology, SNARE complex assembly, Regulation of gene expression, biology, Chemistry, STX1A, Membrane Proteins, Lipid bilayer fusion, Cell Biology, Qb-SNARE Proteins, Syntaxin 3, Cystic fibrosis transmembrane conductance regulator, Cell biology, Electrophysiology, Kinetics, Amino Acid Substitution, nervous system, Antigens, Surface, Mutagenesis, Site-Directed, Oocytes, biology.protein, Female, biological phenomena, cell phenomena, and immunity, Carrier Proteins, SNARE Proteins, SNARE complex

Abstract

Syntaxin 1A binds to and inhibits epithelial cystic fibrosis transmembrane conductance regulator (CFTR) Cl(-) channels and synaptic Ca(2+) channels in addition to participating in SNARE complex assembly and membrane fusion. We exploited the isoform-specific nature of the interaction between syntaxin 1A and CFTR to identify residues in the H3 domain of this SNARE (SNARE motif) that influence CFTR binding and regulation. Mutating isoform-specific residues that map to the surface of syntaxin 1A in the SNARE complex led to the identification of two sets of hydrophilic residues that are important for binding to and regulating CFTR channels or for binding to the syntaxin regulatory protein Munc-18a. None of these mutations affected syntaxin 1A binding to other SNAREs or the assembly and stability of SNARE complexes in vitro. Conversely, the syntaxin 1A-CFTR interaction was unaffected by mutating hydrophobic residues in the H3 domain that influence SNARE complex stability and Ca(2+) channel regulation. Thus, CFTR channel regulation by syntaxin 1A involves hydrophilic interactions that are mechanistically distinct from the hydrophobic interactions that mediate SNARE complex formation and Ca(2+) channel regulation by this t-SNARE.

Published

2003

9. Number, Density, and Surface/Cytoplasmic Distribution of GABA Transporters at Presynaptic Structures of Knock-In Mice Carrying GABA Transporter Subtype 1–Green Fluorescent Protein Fusions

Author

Dan Wang, Norman Davidson, Irina Sokolova, Stephen R. Quake, Michael W. Quick, Ming Li, Kimmo Jensen, Purnima Deshpande, Henry A. Lester, Istvan Mody, and Chi-Sung Chiu

Subjects

GABA Plasma Membrane Transport Proteins, Cytoplasm, DNA, Complementary, Patch-Clamp Techniques, Recombinant Fusion Proteins, Green Fluorescent Proteins, Purkinje cell, Presynaptic Terminals, Organic Anion Transporters, Mice, Transgenic, Kidney, Hippocampus, Synaptic Transmission, Cell Line, GABA transporter 1, Green fluorescent protein, Mice, Basket cell, Cerebellum, medicine, Animals, Humans, GABA transporter, Biotinylation, ARTICLE, gamma-Aminobutyric Acid, Neurons, biology, Chandelier cell, Stem Cells, General Neuroscience, Cell Membrane, Membrane Proteins, Membrane Transport Proteins, Luminescent Proteins, medicine.anatomical_structure, Microscopy, Fluorescence, nervous system, Biochemistry, Organ Specificity, Biophysics, biology.protein, GABAergic, Carrier Proteins

Abstract

GABA transporter subtype 1 (GAT1) molecules were counted near GABAergic synapses, to a resolution of approximately 0.5 microm. Fusions between GAT1 and green fluorescent protein (GFP) were tested in heterologous expression systems, and a construct was selected that shows function, expression level, and trafficking similar to that of wild-type (WT) GAT1. A strain of knock-in mice was constructed that expresses this mGAT1-GFP fusion in place of the WT GAT1 gene. The pattern of fluorescence in brain slices agreed with previous immunocytochemical observations. [3H]GABA uptake, synaptic electrophysiology, and subcellular localization of the mGAT1-GFP construct were also compared with WT mice. Quantitative fluorescence microscopy was used to measure the density of mGAT1-GFP at presynaptic structures in CNS preparations from the knock-in mice. Fluorescence measurements were calibrated with transparent beads and gels that have known GFP densities. Surface biotinylation defined the fraction of transporters on the surface versus those in the nearby cytoplasm. The data show that the presynaptic boutons of GABAergic interneurons in cerebellum and hippocampus have a membrane density of 800-1300 GAT1 molecules per square micrometer, and the axons that connect boutons have a linear density of 640 GAT1 molecules per micrometer. A cerebellar basket cell bouton, a pinceau surrounding a Purkinje cell axon, and a cortical chandelier cell cartridge carry 9000, 7.8 million, and 430,000 GAT1 molecules, respectively; 61-63% of these molecules are on the surface membrane. In cultures from hippocampus, the set of fluorescent cells equals the set of GABAergic interneurons. Knock-in mice carrying GFP fusions of membrane proteins provide quantitative data required for understanding the details of synaptic transmission in living neurons.

Published

2002

10. Substrates and temperature differentiate ion flux from serotonin flux in a serotonin transporter

Author

Matthew L. Beckman and Michael W. Quick

Subjects

Neurotransmitter transporter, Serotonin, Xenopus, Astrophysics::High Energy Astrophysical Phenomena, Nerve Tissue Proteins, Gating, Biology, Membrane Potentials, Ion, Cellular and Molecular Neuroscience, Chlorides, Animals, Drosophila Proteins, Ion transporter, Ion channel, 5-HT receptor, Ions, Serotonin Plasma Membrane Transport Proteins, Pharmacology, Membrane potential, Neurotransmitter Agents, Ion Transport, Membrane Glycoproteins, Dose-Response Relationship, Drug, Sodium, Temperature, Membrane Transport Proteins, Permeation, Biochemistry, Oocytes, Biophysics, Drosophila, Female, Carrier Proteins

Abstract

Neurotransmitter transporters couple the transport of transmitter against its concentration gradient to the electrochemical potential of associated ions which are also transported. Recent studies of some neurotransmitter transporters show them to have properties of both traditional carriers and substrate-dependent ion channels, in that ion fluxes are in excess of that predicted from stoichiometric substrate fluxes. Whether these properties are comparable for all transporters, the extent to which these permeation states are independent, and whether the relationship between these two states can be regulated are not well understood. To address these questions, we expressed the Drosophila serotonin (5HT) transporter (dSERT) in Xenopus oocytes and measured both substrate-elicited ion flux and 5HT flux at various temperatures and substrate concentrations. We find that the ion flux and 5HT flux components of the transport process have a significant temperature dependence suggesting that ion flux and transmitter flux arise from a similar thermodynamically-coupled process involving large conformational changes (e.g., gating). These data are in contrast to those shown for glutamate transporters, suggesting a different permeation process for 5HT transporters. The relationship between ion flux and 5HT flux is differentially regulated by chloride and 5HT, suggesting that these permeation states are distinct. The difference in half-maximal 5HT concentration necessary to mediate ion flux and 5HT flux occurs at submicromolar 5HT concentrations suggesting that the relative participation of dSERT in ion flux and 5HT flux will be determined by the synaptic 5HT concentration.

Published

2001

11. Nicotinic acetylcholine receptor subunit mRNA expression and channel function in medial habenula neurons

Author

Michael W. Quick, Elise B. Sheffield, and Robin A. J. Lester

Subjects

Nicotine, medicine.medical_specialty, Patch-Clamp Techniques, Xenopus, Protein subunit, Cell Separation, Receptors, Nicotinic, Biology, Kidney, Cell Line, Cellular and Molecular Neuroscience, Internal medicine, Gene expression, medicine, Animals, Nicotinic Agonists, RNA, Messenger, Actin, Ion channel, Acetylcholine receptor, Neurons, Pharmacology, Habenula, Reverse Transcriptase Polymerase Chain Reaction, Rats, Cell biology, Electrophysiology, Nicotinic acetylcholine receptor, medicine.anatomical_structure, Endocrinology, Animals, Newborn, Oocytes, Neuron

Abstract

Relationships between nicotinic acetylcholine receptor (nAChR) channel function and nAChR subunit mRNA expression were explored in acutely isolated rat medial habenula (MHb) neurons using a combination of whole-cell recording and single cell RT-PCR techniques. Following amplification using subunit-specific primers, subunits could be categorized in one of three ways: (i) present in 95-100% cells: alpha3, alpha4, alpha5, beta2 and beta4; (ii) never present: alpha2; and (iii) sometimes present ( approximately 40% cells): alpha6, alpha7 and beta3. These data imply that alpha2 subunits do not participate in nAChRs on MHb cells, that alpha6, alpha7 and beta3 subunits are not necessary for functional channels but may contribute in some cells, and that nAChRs may require combinations of all or subsets of alpha3, alpha4, alpha5, beta2 and beta4 subunits. Little difference in the patterns of subunit expression between nicotine-sensitive and insensitive cells were revealed based on this qualitative analysis, implying that gene transcription per se may be an insufficient determinant of nAChR channel function. Normalization of nAChR subunit levels to the amount of actin mRNA, however, revealed that cells with functional channels were associated with high levels (0.78 relative to actin; 11/12 cells) of all of the category (i) subunits: alpha3, alpha4, alpha5, beta2 and beta4. Conversely, one or more of these subunits was always low (0.40 relative to actin) in all cells with no detectable response to nicotine. Thus the formation of functional nAChR channels on MHb cells may require critical levels of several subunit mRNAs.

Published

2000

12. Potassium-Coupled Chloride Cotransport Controls Intracellular Chloride in Rat Neocortical Pyramidal Neurons

Author

R. Anthony DeFazio, Michael W. Quick, John J. Hablitz, and Sotirios Keros

Subjects

Intracellular Fluid, Aging, medicine.medical_specialty, Patch-Clamp Techniques, Neocortex, In Vitro Techniques, Biology, Chlorides, Furosemide, Internal medicine, medicine, Extracellular, Animals, RNA, Messenger, Patch clamp, ARTICLE, Diuretics, Reversal potential, Evoked Potentials, gamma-Aminobutyric Acid, Ion Transport, Dose-Response Relationship, Drug, Symporters, Reverse Transcriptase Polymerase Chain Reaction, GABAA receptor, Pyramidal Cells, General Neuroscience, Gene Expression Regulation, Developmental, Depolarization, Rats, Endocrinology, Symporter, Potassium, Biophysics, Thermodynamics, Carrier Proteins, Cotransporter, Intracellular

Abstract

Chloride (Cl−) homeostasis is critical for many cell functions including cell signaling and volume regulation. The action of GABA at GABAAreceptors is primarily determined by the concentration of intracellular Cl−. Developmental regulation of intracellular Cl−results in a depolarizing response to GABA in immature neocortical neurons and a hyperpolarizing or shunting response in mature neocortical neurons. One protein that participates in Cl−homeostasis is the neuron-specific K+–Cl−cotransporter (KCC2). Thermodynamic considerations predict that in the physiological ranges of intracellular Cl−and extracellular K+concentrations, KCC2 can act to either extrude or accumulate Cl−. To test this hypothesis, we examined KCC2 function in pyramidal cells from rat neocortical slices in mature (18–28 d postnatal) and immature (3–6 d postnatal) rats. Intracellular Cl−concentration was estimated from the reversal potential of whole-cell currents evoked by local application of exogenous GABA. Both increasing and decreasing the extracellular K+concentration resulted in a concomitant change in intracellular Cl−concentration in neurons from mature rats. KCC2 inhibition by furosemide caused a change in the intracellular Cl−concentration that depended on the concentration of pipette Cl−; in recordings with low pipette Cl−, furosemide lowered intracellular Cl−, whereas in recordings with elevated pipette Cl−, furosemide raised intracellular Cl−. In neurons from neonatal rats, manipulation of extracellular K+had no effect on intracellular Cl−concentration, consistent with the minimal KCC2 mRNA levels observed in neocortical neurons from immature animals. These data demonstrate a physiologically relevant and developmentally regulated role for KCC2 in Cl−homeostasis via both Cl−extrusion and accumulation.

Published

2000

13. Functional Regulation of γ-Aminobutyric Acid Transporters by Direct Tyrosine Phosphorylation

Author

Amy Stafford, Robert M. Law, and Michael W. Quick

Subjects

GABA Plasma Membrane Transport Proteins, Organic Anion Transporters, Nerve Tissue Proteins, Protein tyrosine phosphatase, SH2 domain, Hippocampus, Biochemistry, Receptor tyrosine kinase, chemistry.chemical_compound, Animals, Phosphorylation, Molecular Biology, gamma-Aminobutyric Acid, Neurons, biology, Brain-Derived Neurotrophic Factor, Membrane Proteins, Membrane Transport Proteins, Biological Transport, Tyrosine phosphorylation, Cell Biology, Protein-Tyrosine Kinases, Cell Compartmentation, Rats, Up-Regulation, Cell biology, Animals, Newborn, chemistry, Mutation, ROR1, biology.protein, Tyrosine, Protein Tyrosine Phosphatases, Carrier Proteins, Platelet-derived growth factor receptor, Signal Transduction, Proto-oncogene tyrosine-protein kinase Src

Abstract

Tyrosine phosphorylation regulates multiple cell signaling pathways and functionally modulates a number of ion channels and receptors. Neurotransmitter transporters, which act to clear transmitter from the synaptic cleft, are regulated by multiple second messenger pathways that exert their effects, at least in part, by causing a redistribution of the transporter protein to or from the cell surface. To test the hypothesis that tyrosine phosphorylation affects transporter function and to determine its mechanism of action, we examined the regulation of the rat brain gamma-aminobutyric acid (GABA) transporter GAT1 expressed endogenously in hippocampal neurons and expressed heterologously in Chinese hamster ovary cells. Inhibitors of tyrosine kinases decreased GABA uptake; inhibitors of tyrosine phosphatases increased GABA uptake. The decrease in uptake seen with tyrosine kinase inhibitors was correlated with a decrease in tyrosine phosphorylation of GAT1 and resulted in a redistribution of the transporter from the cell surface to intracellular locations. A mutant GAT1 construct that was refractory to tyrosine phosphorylation could not be regulated by tyrosine kinase inhibitors. Activators of protein kinase C, which are known to cause a redistribution of GAT1 from the cell surface, were additive to the effects of tyrosine kinase inhibitors suggesting that multiple signaling pathways control transporter redistribution. Application of brain-derived neurotrophic factor, which activates receptor tyrosine kinases, up-regulated GAT1 function suggesting one potential trigger for the cellular regulation of GAT1 signaling by tyrosine phosphorylation. These data support the hypothesis that transporter expression and function is controlled by the interplay of multiple cell signaling cascades.

Published

2000

14. Upregulation of Surface α4β2 Nicotinic Receptors Is Initiated by Receptor Desensitization after Chronic Exposure to Nicotine

Author

Elise B. Sheffield, Robin A. J. Lester, Terri L. Whitworth, Catherine P. Fenster, and Michael W. Quick

Subjects

Nicotine, Xenopus, medicine.medical_treatment, Cell, Receptors, Nicotinic, Pharmacology, Tritium, Binding, Competitive, Article, Membrane Potentials, RNA, Complementary, Radioligand Assay, Downregulation and upregulation, In vivo, medicine, Animals, Nicotinic Agonists, Receptor, Desensitization (medicine), Acetylcholine receptor, Chemistry, General Neuroscience, Cell Membrane, Tobacco Use Disorder, Up-Regulation, Electrophysiology, medicine.anatomical_structure, Nicotinic agonist, Gene Expression Regulation, Mutagenesis, Chronic Disease, Oocytes, medicine.drug

Abstract

It is hypothesized that desensitization of neuronal nicotinic acetylcholine receptors (nAChRs) induced by chronic exposure to nicotine initiates upregulation of nAChR number. To test this hypothesis directly, oocytes expressing α4β2 receptors were chronically incubated (24–48 hr) in nicotine, and the resulting changes in specific [3H]nicotine binding to surface receptors on intact oocytes were compared with functional receptor desensitization. Four lines of evidence strongly support the hypothesis. (1) The half-maximal nicotine concentration necessary to produce desensitization (9.7 nm) was the same as that needed to induce upregulation (9.9 nm). (2) The concentration of [3H]nicotine for half-maximal binding to surface nAChRs on intact oocytes was also similar (11.1 nm), as predicted from cyclical desensitization models. (3) Functional desensitization of α3β4 receptors required 10-fold higher nicotine concentrations, and this was mirrored by a 10-fold shift in concentrations necessary for upregulation. (4) Mutant α4β2 receptors that do not recover fully from desensitization, but not wild-type channels, were upregulated after acute (1 hr) applications of nicotine. Interestingly, the nicotine concentration required for half-maximal binding of α4β2 receptors in total cell membrane homogenates was 20-fold lower than that measured for surface nAChRs in intact oocytes. These data suggest that cell homogenate binding assays may not accurately reflect thein vivodesensitization affinity of surface nAChRs and may account for some of the previously reported differences in the efficacy of nicotine for inducing nAChR desensitization and upregulation.

Published

1999

15. Regulation of γ-Aminobutyric Acid (GABA) Transporters by Extracellular GABA

Author

Michael W. Quick and Eve M. Bernstein

Subjects

GABA Plasma Membrane Transport Proteins, Synaptic cleft, Organic Anion Transporters, CHO Cells, GABAB receptor, Hippocampus, Biochemistry, chemistry.chemical_compound, Cricetinae, Extracellular, Nipecotic acid, Animals, GABA transporter, Molecular Biology, Cells, Cultured, gamma-Aminobutyric Acid, biology, GABAA receptor, Membrane Proteins, Membrane Transport Proteins, Transporter, Cell Biology, Endocytosis, Rats, Cell biology, nervous system, chemistry, biology.protein, Carrier Proteins

Abstract

gamma-Aminobutyric acid (GABA) transporters on neurons and glia at or near the synapse function to remove GABA from the synaptic cleft. Recent evidence suggests that GABA transporter function can be regulated, although the initial triggers for such regulation are not known. One hypothesis is that transporter function is modulated by extracellular GABA concentration, thus providing a feedback mechanism for the control of neurotransmitter levels at the synapse. To test this hypothesis, GABA uptake assays were performed on primary dissociated rat hippocampal cultures that endogenously express GABA transporters and on mammalian cells stably expressing the cloned rat brain GABA transporter GAT1. In both experimental systems, extracellular GABA induces chronic changes in GABA transport that occur in a dose-dependent and time-dependent manner. In addition to GABA, ACHC and nipecotic acid, both substrates of GAT1, up-regulate transport; GAT1 transport inhibitors that are not transporter substrates down-regulate transport. These changes occur in the presence of blockers of both GABAA and GABAB receptors, occur in the presence of protein synthesis inhibitors, and are not influenced by intracellular GABA. Surface biotinylation experiments reveal that the increase in transport is correlated with an increase in surface transporter expression. This increase in surface expression is due, at least in part, to a slowing of GAT1 internalization in the presence of extracellular GABA. These data suggest that the GABA transporter fine-tunes its function in response to extracellular GABA and would act to maintain a constant level of neurotransmitter at the synaptic cleft.

Published

1999

16. Neurotransmitter Transporters: Regulators of Function and Functional Regulation

Author

Matthew L. Beckman and Michael W. Quick

Subjects

Neurotransmitter transporter, Neurotransmitter Agents, Physiology, Biophysics, Nerve Tissue Proteins, Cell Biology, Human physiology, Biology, Synaptic Transmission, TRPC1, Neurotransmitter receptor, Animals, Humans, Ligand-gated ion channel, Carrier Proteins, Neuroscience, Function (biology)

Published

1998

17. Permeation Properties of Neurotransmitter Transporters

Author

Janis L. Corey, Sela Mager, Michael W. Quick, and Henry A. Lester

Subjects

Pharmacology, Neurotransmitter transporter, Neurotransmitter Agents, biology, ATPase, Permeation, Inorganic ions, Toxicology, Permeability, chemistry.chemical_compound, Membrane protein, Biochemistry, chemistry, biology.protein, Animals, Humans, Carrier Proteins, Cotransporter, Neurotransmitter

Abstract

The neurotransmitter transporters belong to three known families of intrinsic membrane proteins (Figure 1). The energy for transport, which is often against the neurotransmitter concentration gradient, is derived from the cotransport (and in some cases the counter transport) of inorganic ions. Ion-transporting ATPases establish the concentration gradients for these ions.

Published

1994

18. PICKing on transporters

Author

Scott L. Deken, Matthew L. Beckman, and Michael W. Quick

Subjects

Central nervous system, Nerve Tissue Proteins, Biology, Synapse, chemistry.chemical_compound, Extracellular, medicine, Animals, Humans, Neurotransmitter, Neurons, Dopamine Plasma Membrane Transport Proteins, Membrane Glycoproteins, Primary sites, General Neuroscience, Membrane Transport Proteins, Nuclear Proteins, Transporter, Membrane transport, Protein Structure, Tertiary, medicine.anatomical_structure, nervous system, chemistry, Neuron, Carrier Proteins, Neuroscience, Signal Transduction

Abstract

Plasma membrane neurotransmitter transporters are regulators of extracellular transmitter levels in brain and are the primary sites of action for several drugs of abuse and therapy. Studies are beginning to reveal how neurons use synaptic machinery to modulate these regulators.

Published

2001

19. Calcium/calmodulin-dependent kinase II regulates the interaction between the serotonin transporter and syntaxin 1A

Author

Anthony Phillips, Miranda Timmons, Michael W. Quick, and Marcia A. Ciccone

Subjects

Serotonin, Patch-Clamp Techniques, Microinjections, Syntaxin 1, Article, Membrane Potentials, Cellular and Molecular Neuroscience, Xenopus laevis, Synaptic vesicle docking, Ca2+/calmodulin-dependent protein kinase, Animals, Drug Interactions, Enzyme Inhibitors, Serotonin Uptake Inhibitors, Serotonin transporter, 5-HT receptor, Cells, Cultured, Pharmacology, Neurons, Serotonin Plasma Membrane Transport Proteins, Analysis of Variance, biology, Dose-Response Relationship, Drug, Brain, Embryo, Mammalian, Syntaxin 3, Cell biology, Rats, Paroxetine, biology.protein, Oocytes, Calcium-Calmodulin-Dependent Protein Kinase Type 2, Selective Serotonin Reuptake Inhibitors

Abstract

Plasma membrane serotonin transporters (SERTs) regulate serotonin (5HT) levels in brain and are a site of action of antidepressants and psychostimulant drugs of abuse. Syntaxin 1A is a component of the synaptic vesicle docking and fusion apparatus and has been shown to interact with multiple plasma membrane neurotransmitter transporters including SERT. Previously, we showed that syntaxin 1A regulates the transport stoichiometry of SERT. When not bound to syntaxin 1A, SERT shows both substrate-independent Na(+) fluxes and substrate-dependent Na(+) fluxes of variable stoichiometry; these fluxes are eliminated in the presence of syntaxin 1A as Na(+) flux becomes strictly coupled to 5HT uptake. However, not known are the endogenous signaling molecules that determine the conducting states that SERT exhibits. In the present experiments, we show that inhibitors of calcium/calmodulin-dependent kinase II (CaM kinase II) modulate the stoichiometry of 5HT flux and that this effect requires syntaxin 1A. The modulation correlates with a shift in the affinity of SERT for syntaxin 1A binding. The regulation by CaM kinase II is eliminated by a mutation in the N-terminal domain of SERT. In neonatal thalomocortical neurons that endogenously express SERT and syntaxin 1A, inhibition of CaM kinase II reveals SERT-mediated currents. These data suggest that calcium-mediated signals can serve as a trigger for regulating protein-protein interactions that control SERT conducting states.

Published

2008

20. The Caenorhabditis elegans snf-11 Gene Encodes a Sodium-dependent GABA Transporter Required for Clearance of Synaptic GABA

Author

Michael W. Quick, Paurush Saxena, Eleanor A. Mathews, Gregory P. Mullen, Robert Barstead, James B. Rand, Stephen D. Fields, John McManus, and Gary Moulder

Subjects

Neurotransmitter transporter, GABA Plasma Membrane Transport Proteins, GABA Agents, Nipecotic Acids, macromolecular substances, Neurotransmission, Synaptic Transmission, gamma-Aminobutyric acid, Postsynaptic potential, medicine, GABA transporter, Animals, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Molecular Biology, Genes, Helminth, Phylogeny, gamma-Aminobutyric Acid, biology, fungi, Sodium, Cell Biology, Articles, Cell biology, enzymes and coenzymes (carbohydrates), Phenotype, Biochemistry, nervous system, Mutation, Synapses, biology.protein, GABAergic, human activities, medicine.drug

Abstract

Sodium-dependent neurotransmitter transporters participate in the clearance and/or recycling of neurotransmitters from synaptic clefts. The snf-11 gene in Caenorhabditis elegans encodes a protein of high similarity to mammalian GABA transporters (GATs). We show here that snf-11 encodes a functional GABA transporter; SNF-11–mediated GABA transport is Na+and Cl−dependent, has an EC50value of 168 μM, and is blocked by the GAT1 inhibitor SKF89976A. The SNF-11 protein is expressed in seven GABAergic neurons, several additional neurons in the head and retrovesicular ganglion, and three groups of muscle cells. Therefore, all GABAergic synapses are associated with either presynaptic or postsynaptic (or both) expression of SNF-11. Although a snf-11 null mutation has no obvious effects on GABAergic behaviors, it leads to resistance to inhibitors of acetylcholinesterase. In vivo, a snf-11 null mutation blocks GABA uptake in at least a subset of GABAergic cells; in a cell culture system, all GABA uptake is abolished by the snf-11 mutation. We conclude that GABA transport activity is not essential for normal GABAergic function in C. elegans and that the localization of SNF-11 is consistent with a GABA clearance function rather than recycling.

Published

2006

21. Rapid upregulation of alpha7 nicotinic acetylcholine receptors by tyrosine dephosphorylation

Author

Weifeng Song, Robin A. J. Lester, Annal D. Meleth, Chang-Hoon Cho, Michael W. Quick, Esther Teo, and Katherine Leitzell

Subjects

Patch-Clamp Techniques, Time Factors, alpha7 Nicotinic Acetylcholine Receptor, Xenopus, Protein tyrosine phosphatase, Receptors, Nicotinic, Hippocampus, Receptor tyrosine kinase, Tyrosine-kinase inhibitor, Choline, Membrane Potentials, chemistry.chemical_compound, Radioligand Assay, Iodine Isotopes, Excitatory Amino Acid Agonists, Insulin, Drug Interactions, Tyrosine, Enzyme Inhibitors, Phosphorylation, biology, Reverse Transcriptase Polymerase Chain Reaction, General Neuroscience, Protein-Tyrosine Kinases, Genistein, Cell biology, Up-Regulation, Nicotinic agonist, Biochemistry, SNARE Proteins, Ion Channel Gating, psychological phenomena and processes, Platelet-derived growth factor receptor, Cellular/Molecular, N-Methylaspartate, Microinjections, medicine.drug_class, Blotting, Western, complex mixtures, Interneurons, medicine, Animals, Biotinylation, RNA, Messenger, Dose-Response Relationship, Drug, Tyrosine phosphorylation, Dose-Response Relationship, Radiation, Bungarotoxins, Acetylcholine, Electric Stimulation, Phosphoric Monoester Hydrolases, Rats, nervous system, chemistry, Mutagenesis, biology.protein, Oocytes, Vanadates

Abstract

α7 nicotinic acetylcholine receptors (nAChRs) modulate network activity in the CNS. Thus, functional regulation of α7 nAChRs could influence the flow of information through various brain nuclei. It is hypothesized here that these receptors are amenable to modulation by tyrosine phosphorylation. In bothXenopusoocytes and rat hippocampal interneurons, brief exposure to a broad-spectrum protein tyrosine kinase inhibitor, genistein, specifically and reversibly potentiated α7 nAChR-mediated responses, whereas a protein tyrosine phosphatase inhibitor, pervanadate, caused depression. Potentiation was associated with an increased expression of surface α7 subunits and was not accompanied by detectable changes in receptor open probability, implying that the increased function results from an increased number of α7 nAChRs. SolubleN-ethylmaleimide-sensitive factor attachment protein receptor-mediated exocytosis was shown to be a plausible mechanism for the rapid delivery of additional α7 nAChRs to the plasma membrane. Direct phosphorylation/dephosphorylation of α7 subunits was unlikely because mutation of all three cytoplasmic tyrosine residues did not prevent the genistein-mediated facilitation. Overall, these data are consistent with the hypothesis that the number of functional cell surface α7 nAChRs is controlled indirectly via processes involving tyrosine phosphorylation.

Published

2005

22. Trafficking of the plasma membrane gamma-aminobutyric acid transporter GAT1. Size and rates of an acutely recycling pool

Author

Dan, Wang and Michael W, Quick

Subjects

Cerebral Cortex, Dynamins, Neurons, GABA Plasma Membrane Transport Proteins, Sucrose, Time Factors, Cell Membrane, Immunoblotting, Membrane Transport Proteins, Biological Transport, CHO Cells, Clathrin, Endocytosis, Exocytosis, Rats, Kinetics, Protein Transport, Cricetinae, Animals, Tetradecanoylphorbol Acetate, Biotinylation, Calcium, Cells, Cultured, Protein Kinase C, Signal Transduction

Abstract

Plasma membrane neurotransmitter transporters rapidly traffic to and from the cell surface in neurons. This trafficking may be important in regulating neuronal signaling. Such regulation will be subject to the number of trafficking transporters and their trafficking rates. In the present study, we define an acutely recycling pool of endogenous gamma-aminobutyric acid transporters (GAT1) in cortical neurons that comprises approximately one-third of total cellular GAT1. Kinetic analysis of this pool estimates exocytosis and endocytosis time constants of 1.6 and 0.9 min, respectively, and thus approximately one-third of the recycling pool is plasma membrane resident in the basal state. Recent evidence shows that GAT1 substrates, second messengers, and interacting proteins regulate GAT1 trafficking. These triggers could act by altering trafficking rates or by changing the recycling pool size. In the present study we examine three GAT1 modulators. Calcium depletion decreases GAT1 surface expression by diminishing the recycling pool size. Sucrose increases GAT1 surface expression by blocking clathrin- and dynamin-dependent endocytosis, but it does not change the recycling pool size. Protein kinase C decreases surface GAT1 expression by increasing the endocytosis rate, but it does not change the exocytosis rate or the recycling pool size. Based upon estimates of GAT1 molecules in cortical boutons, the present data suggest that approximately 1000 transporters comprise the acutely recycling pool, of which 300 are on the surface in the basal state, and five transporters insert into the plasma membrane every second. This insertion could represent the fusion of one transporter-containing vesicle.

Published

2005

23. Intracellular domains of a rat brain GABA transporter that govern transport

Author

Michael W. Quick, Shruti Arya, and Nina Hansra

Subjects

GABA Plasma Membrane Transport Proteins, Patch-Clamp Techniques, Recombinant Fusion Proteins, Xenopus, Syntaxin 1, Nerve Tissue Proteins, Biology, Structure-Activity Relationship, Protein structure, Extracellular, GABA transporter, Animals, Cells, Cultured, gamma-Aminobutyric Acid, Membrane transport protein, General Neuroscience, Brain, Membrane Proteins, Membrane Transport Proteins, Transporter, Biological Transport, Cell biology, Protein Structure, Tertiary, Rats, Protein Transport, Antigens, Surface, biology.protein, Mutagenesis, Site-Directed, Oocytes, Carrier Proteins, Brief Communications, Intracellular

Abstract

Plasma membrane neurotransmitter transporters determine in part the concentration, time course, and diffusion of extracellular transmitter. Much has been learned about how substrate translocation through the transporter occurs; however, the precise way in which transporter structure maps onto transporter function has not yet been fully elucidated. Here, biochemical and electrophysiological approaches were used to test the hypothesis that intracellular domains of the rat brain GABA transporter (GAT1) contribute to the transport process. Injection of a peptide corresponding to the presumed fourth intracellular loop of the transporter (IL4) into oocytes expressing GAT1 greatly reduced both forward and reverse transport and reduced the transport rate in a dose-dependent manner. Coinjection of the IL4 peptide with a peptide corresponding to the N-terminal cytoplasmic tail of GAT1 reversed the IL4-mediated inhibition; this reversal, and direct binding between these two domains, was prevented by mutagenesis of charged residues in either the IL4 or N-terminal domains. Furthermore, syntaxin 1A, a solubleN-ethylmaleimide-sensitive factor attachment protein receptor (SNARE) protein that inhibits GAT1 transport rates via interactions with the N-terminal tail of GAT1 was unable to regulate the GAT1 IL4 mutant. Together, these data suggest a model in which the GAT1 IL4 domain serves as a barrier for transport, and this barrier can be regulated through intra-molecular and inter-molecular interactions.

Published

2004

24. Regulation of a gamma-aminobutyric acid transporter by reciprocal tyrosine and serine phosphorylation

Author

Huai-Yu Zhang, Michael W. Quick, Dan Wang, and Jia Hu

Subjects

inorganic chemicals, GABA Plasma Membrane Transport Proteins, macromolecular substances, Protein tyrosine phosphatase, SH2 domain, environment and public health, Biochemistry, Hippocampus, Receptor tyrosine kinase, Phosphorylation cascade, chemistry.chemical_compound, Serine, Animals, Protein phosphorylation, Phosphorylation, Molecular Biology, Protein kinase C, Cells, Cultured, biology, Membrane Proteins, Membrane Transport Proteins, Tyrosine phosphorylation, Biological Transport, Cell Biology, Cell biology, Rats, enzymes and coenzymes (carbohydrates), chemistry, biology.protein, bacteria, Tyrosine, Carrier Proteins

Abstract

A feature of the rat brain gamma-aminobutyric acid transporter GAT1, and other members of the neurotransmitter transporter family, is its regulated redistribution between intracellular locations and the plasma membrane. Recent studies have focused upon defining the signaling molecules that facilitate this redistribution. Agents that promote direct tyrosine phosphorylation of GAT1 promote a relative increase in surface GAT1 levels, and this results from a slowing of the transporter internalization rate. Agents that act to increase protein kinase C (PKC) activity promote a relative decrease in surface GAT1 levels; whether this effect is caused by direct transporter phosphorylation is unknown. The opposing actions of tyrosine kinase activity and PKC activity raise the possibility that the subcellular distribution of GAT1 is associated with mutually exclusive transporter phosphorylation events. The present experiments show that GAT1 is phosphorylated on serine residues in a PKC-dependent manner, but this state is only revealed when GAT1 tyrosine phosphorylation is eliminated or greatly reduced. The relative levels of serine phosphorylation and tyrosine phosphorylation are negatively correlated. The amount of serine phosphorylation is regulated by agents that affect tyrosine phosphorylation, and vice versa. In addition, the ability of agents that affect tyrosine kinase activity to regulate GAT1 serine phosphorylation requires a change in its tyrosine phosphorylation state. These data support the ideas that GAT1 can exist in either of two mutually exclusive phosphorylation states and that the relative abundance of these states determines in part the relative subcellular distribution of the transporter.

Published

2004

25. A Regulated Interaction of Syntaxin 1A with the Antidepressant-Sensitive Norepinephrine Transporter Establishes Catecholamine Clearance Capacity

Author

Michael W. Quick, Kristopher M. Kahlig, Subramaniam Apparsundaram, Uhna Sung, Randy D. Blakely, Sally Schroeter, Valentina Savchenko, and Aurelio Galli

Subjects

Male, Botulinum Toxins, Patch-Clamp Techniques, Vesicular Transport Proteins, Syntaxin 1, Plasma protein binding, environment and public health, Reuptake, Mice, Norepinephrine, Catecholamines, Vas Deferens, Enzyme Inhibitors, Cells, Cultured, Sequence Deletion, Neurons, biology, Symporters, General Neuroscience, Antidepressive Agents, Cell biology, Transport protein, Protein Transport, Norepinephrine transporter, Antigens, Surface, biological phenomena, cell phenomena, and immunity, SNARE Proteins, Protein Binding, endocrine system, Recombinant Fusion Proteins, Enzyme Activators, Nerve Tissue Proteins, Animals, Humans, ARTICLE, Brain Chemistry, Norepinephrine Plasma Membrane Transport Proteins, urogenital system, Membrane Proteins, Transporter, Oligonucleotides, Antisense, Syntaxin 3, Protein Structure, Tertiary, Rats, Enzyme Activation, Mice, Inbred C57BL, nervous system, biology.protein, Synaptosomes

Abstract

Norepinephrine (NE) transporters (NETs) terminate noradrenergic synaptic transmission and represent a major therapeutic target for antidepressant medications. NETs and related transporters are under intrinsic regulation by receptor and kinase-linked pathways, and clarification of these pathways may suggest candidates for the development of novel therapeutic approaches. Syntaxin 1A, a presynaptic solubleN-ethylmaleimide-sensitive factor attachment protein receptor (SNARE) protein, interacts with NET and modulates NET intrinsic activity. NETs colocalize with and bind to syntaxin 1A in both native preparations and heterologous systems. Protein kinase C activation disrupts surface NET/syntaxin 1A interactions and downregulates NET activity in a syntaxin-dependent manner. Syntaxin 1A binds the NH2terminal domain of NET, and a deletion of this domain both eliminates NET/syntaxin 1A associations and prevents phorbol ester-triggered NET downregulation. Whereas syntaxin 1A supports the surface trafficking of NET proteins, its direct interaction with NET limits transporter catalytic function. These two contradictory roles of syntaxin 1A on NET appear to be linked and reveal a dynamic cycle of interactions that allow for the coordinated control between NE release and reuptake.

Published

2003

26. Desensitization of neuronal nicotinic receptors

Author

Robin A. J. Lester and Michael W. Quick

Subjects

Agonist, Nicotine, medicine.drug_class, General Neuroscience, medicine.medical_treatment, Excitotoxicity, Drug Tolerance, Biology, Receptors, Nicotinic, medicine.disease_cause, Acetylcholine, Ion Channels, Membrane Potentials, Cellular and Molecular Neuroscience, Nicotinic acetylcholine receptor, Synaptic plasticity, medicine, Animals, Humans, Receptor, Neuroscience, Ion channel, Desensitization (medicine), medicine.drug

Abstract

The loss of functional response upon continuous or repeated exposure to agonist, desensitization, is an intriguing phenomenon if not as yet a well-defined physiological mechanism. However, detailed evaluation of the properties of desensitization, especially for the superfamily of ligand-gated ion channels, reveals how the nervous system could make important use of this process that goes far beyond simply curtailing excessive receptor stimulation and the prevention of excitotoxicity. Here we will review the mechanistic basis of desensitization and discuss how the subunit-dependent properties and regulation of nicotinic acetylcholine receptor (nAChR) desensitization contribute to the functional diversity of these channels. These studies provide the essential framework for understanding how the physiological regulation of desensitization could be a major determinant of synaptic efficacy by controlling, in both the short and long term, the number of functional receptors. This type of mechanism can be extended to explain how the continuous occupation of desensitized receptors during chronic nicotine exposure contributes to drug addiction, and highlights the potential significance of prolonged nAChR desensitization that would also occur as a result of extended acetylcholine lifetime during treatment of Alzheimer's disease with cholinesterase inhibitors. Thus, a clearer picture of the importance of nAChR desensitization in both normal information processing and in various diseased states is beginning to emerge.

Published

2002

27. Role of syntaxin 1A on serotonin transporter expression in developing thalamocortical neurons

Author

Michael W. Quick

Subjects

Neurotransmitter transporter, Serotonin, Botulinum Toxins, Neurotransmitter uptake, Synaptic cleft, Presynaptic Terminals, Syntaxin 1, Nerve Tissue Proteins, Biology, Synaptic Transmission, Rats, Sprague-Dawley, chemistry.chemical_compound, Fetus, Developmental Neuroscience, Thalamus, Neural Pathways, Animals, Neurotransmitter, Serotonin transporter, Cells, Cultured, Cerebral Cortex, Serotonin Plasma Membrane Transport Proteins, Membrane Glycoproteins, Cell Membrane, Membrane Transport Proteins, Cell Differentiation, Immunohistochemistry, Syntaxin 3, Cell biology, Rats, Protein Transport, chemistry, Antigens, Surface, biology.protein, Carrier Proteins, Neuroscience, Developmental Biology

Abstract

Neurotransmitter transporters are regulated through a variety of signal transduction mechanisms which may operate in order to maintain appropriate levels of transmitter in the synaptic cleft. GABA and glycine transporters both interact with components of the neurotransmitter release, such as the SNARE protein syntaxin 1A, suggesting that protein-protein interactions are a common method for regulating members of the neurotransmitter transporter family, and thus, linking the release of transmitter to its subsequent re-uptake. In the present report, the interaction of syntaxin 1A with endogenous serotonin transporters (SERT) expressed in developing thalamocortical neurons is examined. Incubation of thalamocortical cultures with botulinum toxin C1, which specifically cleaves syntaxin 1A, decreased SERT function. Serotonin (5HT) saturation analysis showed that the effect of the toxin was to decrease maximum transport capacity with little change to the affinity of the transporter for 5HT. The 5HT uptake data were consistent with biotinylation experiments showing a decrease in the surface expression of SERT following toxin treatment. In addition, co-immunoprecipitation experiments showed that SERT and syntaxin 1A form a protein complex in these neurons. These data show that components of the transmitter release machinery interact with endogenously expressed amine transporters, and suggest a mechanism for the control of transmitter levels in disorders related to aminergic signaling.

Published

2002

28. Psychostimulants Differentially Regulate Serotonin Transporter Expression in Thalamocortical Neurons

Author

Laura C. Herndon, Terri L. Whitworth, and Michael W. Quick

Subjects

Serotonin, Time Factors, N-Methyl-3,4-methylenedioxyamphetamine, Enzyme Activators, Endogeny, Nerve Tissue Proteins, Serotonergic, Rats, Sprague-Dawley, Glutamatergic, Thalamus, medicine, Animals, Serotonin transporter, Cells, Cultured, Cerebral Cortex, Neurons, Serotonin Plasma Membrane Transport Proteins, Membrane Glycoproteins, biology, Dose-Response Relationship, Drug, General Neuroscience, Cell Membrane, Gene Expression Regulation, Developmental, Membrane Transport Proteins, Transporter, Rats, Serotonin Receptor Agonists, Protein Transport, medicine.anatomical_structure, Microscopy, Fluorescence, Cerebral cortex, biology.protein, Hallucinogens, Central Nervous System Stimulants, Serotonin Antagonists, Carrier Proteins, Neuroscience, Neural development, Rapid Communication

Abstract

5-HT transporters (SERTs) are transiently expressed in thalamocortical neurons during development, permitting these glutamatergic neurons to co-release 5-HT as a “borrowed” transmitter. The high level of SERT expression in these neurons is likely important in the serotonergic modulation of neocortical circuits and provides a system for examining endogenous SERT regulation. We tested the hypothesis that developmental expression of SERT in thalamocortical neurons is regulated by psychostimulants that are agonists and antagonists of SERT. Cultured thalamocortical neurons from embryonic day 18 rats were examined for SERT expression until P15. In untreated cultures, SERT protein levels peaked at postnatal day 3 (P3) and were absent by P10. Chronic treatment with SERT substrates (5-HT, 3,4-methylenedioxymethamphetamine) increased both peak SERT protein levels (fourfold) and the time course of SERT expression. SERT substrates also shifted the relative functional expression of SERT by redistributing intracellular SERT protein to the plasma membrane. The subcellular redistribution was prevented by PKC activators. SERT antagonists (e.g., fluoxetine, cocaine) reduced total SERT expression levels and the time course of SERT expression. These data (1) show that endogenous SERT is differentially regulated by 5-HT and psychostimulants, (2) indicate that SERT modulation occurs via changes in both total SERT protein levels and subcellular redistribution of the transporter, and (3) suggest that some of the actions of drugs of abuse in neocortical development may be attributable to alterations in SERT expression and concomitant changes in 5-HT signaling.

Published

2002

29. Substrate-induced regulation of gamma-aminobutyric acid transporter trafficking requires tyrosine phosphorylation

Author

Terri L. Whitworth and Michael W. Quick

Subjects

GABA Plasma Membrane Transport Proteins, Immunoblotting, Nipecotic Acids, Organic Anion Transporters, Protein tyrosine phosphatase, CHO Cells, Biology, SH2 domain, Ligands, Transfection, Biochemistry, Receptor tyrosine kinase, Phosphorylation cascade, chemistry.chemical_compound, Cricetinae, Animals, Protein phosphorylation, Biotinylation, Tyrosine, Phosphorylation, Molecular Biology, Binding Sites, Cell Membrane, Membrane Proteins, Membrane Transport Proteins, Tyrosine phosphorylation, Cell Biology, Protein-Tyrosine Kinases, Genistein, Precipitin Tests, Cell biology, Up-Regulation, chemistry, Mutation, biology.protein, Mutagenesis, Site-Directed, Carrier Proteins, Protein Binding, Signal Transduction

Abstract

Neurotransmitter transporters regulate synaptic transmitter levels and are themselves functionally regulated by a number of different signal transduction cascades. A common theme in transporter regulation is redistribution of transporter protein between intracellular stores and the plasma membrane. The triggers and mechanisms underlying this regulation are important in the control of extracellular transmitter concentrations and hence synaptic signaling. Previously, we demonstrated that the gamma-aminobutyric acid transporter GAT1 is regulated by direct tyrosine phosphorylation, resulting in an up-regulation of transporter expression on the plasma membrane. In the present report, we show that two tyrosine residues on GAT1 contribute to the phosphorylation and transporter redistribution. Tyrosine phosphorylation is concomitant with a decrease in the rate of transporter internalization from the plasma membrane. A decrease in GAT internalization rates also occurs in the presence of GAT1 substrates, suggesting the hypothesis that tyrosine phosphorylation is required for the substrate-induced up-regulation of GAT1 surface expression. In support of this hypothesis, incubation of GAT1-expressing cells with transporter ligands alters the amount of GAT1 tyrosine phosphorylation, and substrate-induced surface expression is unchanged in a GAT1 mutant lacking tyrosine phosphorylation sites. These data suggest a model in which substrates permit the phosphorylation of GAT1 on tyrosine residues and that the phosphorylated state of the transporter is refractory for internalization.

Published

2001

30. Transport rates of GABA transporters: regulation by the N-terminal domain and syntaxin 1A

Author

Laura Boos, Michael W. Quick, Scott L. Deken, and Matthew L. Beckman

Subjects

GABA Plasma Membrane Transport Proteins, Botulinum Toxins, Xenopus, Synaptic Membranes, Organic Anion Transporters, Syntaxin 1, Nerve Tissue Proteins, Biology, Hippocampus, Synaptic Transmission, Membrane Potentials, Cricetinae, GABA transporter, Animals, RNA, Messenger, Cells, Cultured, gamma-Aminobutyric Acid, Neurons, Voltage-dependent calcium channel, Membrane transport protein, General Neuroscience, Membrane Proteins, Membrane Transport Proteins, Transporter, Transmembrane protein, Cell biology, Protein Structure, Tertiary, Rats, Antigens, Surface, Chloride channel, biology.protein, Oocytes, Synaptic Vesicles, Carrier Proteins

Abstract

Plasma membrane GABA transporters participate in neural signaling through re-uptake of neurotransmitter. The domains of the transporter that mediate GABA translocation and regulate transport are not well understood. In the present experiments, the N-terminal cytoplasmic domain of the GABA transporter GAT1 regulated substrate transport rates. This domain directly interacted with syntaxin 1A, a SNARE protein involved in both neurotransmitter release and modulation of calcium channels and cystic fibrosis transmembrane regulator (CFTR) chloride channels. The interaction resulted in a decrease in transporter transport rates. These data demonstrate that intracellular domains of the GABA and protein-protein interactions regulate substrate translocation, and identify a direct link between the machinery involved in transmitter release and re-uptake.

Published

2000

31. CFTR chloride channel regulation by an interdomain interaction

Author

Matteo Villain, Jian Fu, Kevin L. Kirk, Anjaparavanda P. Naren, J. Edwin Blalock, Michael W. Quick, and Estelle Cormet-Boyaka

Subjects

congenital, hereditary, and neonatal diseases and abnormalities, medicine.medical_specialty, Patch-Clamp Techniques, Recombinant Fusion Proteins, Xenopus, DNA Mutational Analysis, Molecular Sequence Data, Cystic Fibrosis Transmembrane Conductance Regulator, Protein Structure, Secondary, Adenosine Triphosphate, Internal medicine, medicine, Cyclic AMP, Animals, Humans, Amino Acid Sequence, Phosphorylation, Protein kinase A, Ion channel, Multidisciplinary, Water transport, biology, Cyclic AMP-Dependent Protein Kinases, Cystic fibrosis transmembrane conductance regulator, Cell biology, Endocrinology, Amino Acid Substitution, Cytoplasm, COS Cells, Mutation, Chloride channel, biology.protein, Oocytes, Ion Channel Gating, Function (biology)

Abstract

The cystic fibrosis gene encodes a chloride channel, CFTR (cystic fibrosis transmembrane conductance regulator), that regulates salt and water transport across epithelial tissues. Phosphorylation of the cytoplasmic regulatory (R) domain by protein kinase A activates CFTR by an unknown mechanism. The amino-terminal cytoplasmic tail of CFTR was found to control protein kinase A–dependent channel gating through a physical interaction with the R domain. This regulatory activity mapped to a cluster of acidic residues in the NH 2 -terminal tail; mutating these residues proportionately inhibited R domain binding and CFTR channel function. CFTR activity appears to be governed by an interdomain interaction involving the amino-terminal tail, which is a potential target for physiologic and pharmacologic modulators of this ion channel.

Published

1999

32. Alpha3beta4 subunit-containing nicotinic receptors dominate function in rat medial habenula neurons

Author

Michael W. Quick, R.Michael Ceballos, J. Michael McIntosh, Michael R. Kasten, and Robin A. J. Lester

Subjects

Agonist, medicine.medical_specialty, Patch-Clamp Techniques, medicine.drug_class, Xenopus, Biology, In Vitro Techniques, Receptors, Nicotinic, Cellular and Molecular Neuroscience, Cytisine, chemistry.chemical_compound, Internal medicine, medicine, Animals, Patch clamp, Nicotinic Agonists, Receptor, Acetylcholine receptor, Pharmacology, Neurons, Habenula, Cell biology, Rats, Endocrinology, medicine.anatomical_structure, Nicotinic agonist, chemistry, Oocytes, Neuron

Abstract

Regional-specific differences in nicotinic acetylcholine receptors (nAChRs) were examined using the whole-cell patch clamp technique in rat medial habenula (MHb) slices. The majority of cells in the ventral two thirds of the MHb responded robustly to local pressure application of nAChR agonists. Mean agonist potency profiles in the middle and ventral thirds of the MHb were similar: cytisine was the most potent agonist and DMPP the weakest, consistent with a significant contribution of the beta4 subunit to functional nAChRs in all areas of the MHb. In acutely isolated MHb neurons, the alpha3beta4-selective toxin alpha-CTx-AuIB (1 microM) reversibly blocked approximately 75% of the nicotine-induced currents, as expected for cells solely expressing alpha3beta4 nAChRs. However, the alpha3beta2-selective toxin, alpha-CTx-MII (100 nM), blocked a variable fraction (0-90%) of the MHb nicotinic response implying that beta2 subunits may contribute to some functional receptors. We suggest that the effects of alpha-CTx-MII may arise from interaction with alpha3beta2beta4 subunit-containing nAChRs. This idea is supported by the findings (1) that alpha-CTx-MII antagonizes receptors comprised of alpha3, beta2 and beta4 subunits in Xenopus oocytes, and (2) that a mutant alpha-CTx-MII toxin[H12A], which blocks alpha3beta2beta4 receptors but not alpha3beta2 or alpha3beta4 nAChRs, also reduces nicotinic currents in some MHb neurons. Overall these data imply that most functional nAChRs on MHb cells contain at least alpha3 and beta4 subunits, and that a variable subpopulation additionally contains the beta2 subunit.

Published

1999

33. Desensitization of nicotinic receptors in the central nervous system

Author

Matthew L. Beckman, Robin A. J. Lester, P.J. O. Covernton, J. H. Hicks, Michael W. Quick, and Catherine P. Fenster

Subjects

Nicotine, Indoles, Patch-Clamp Techniques, medicine.medical_treatment, Xenopus, Central nervous system, Pharmacology, Receptors, Nicotinic, General Biochemistry, Genetics and Molecular Biology, Maleimides, Ganglion type nicotinic receptor, History and Philosophy of Science, medicine, Animals, Enzyme Inhibitors, Protein Kinase C, gamma-Aminobutyric Acid, Desensitization (medicine), Neurons, Nicotinic Receptors, Chemistry, General Neuroscience, Brain, medicine.anatomical_structure, Nicotinic agonist, Oocytes

Published

1999

34. Interaction of syntaxins with the amiloride-sensitive epithelial sodium channel

Author

Sunil Saxena, Youngsuk Oh, David G. Warnock, Michael W. Quick, and Albert Tousson

Subjects

Epithelial sodium channel, endocrine system, Xenopus, Syntaxin 1, Biochemistry, Sodium Channels, medicine, Syntaxin, Animals, Humans, Protein Isoforms, Epithelial Sodium Channels, Molecular Biology, Ion channel, Acid-sensing ion channel, urogenital system, Chemistry, Qa-SNARE Proteins, Sodium channel, Membrane Proteins, Biological Transport, Cell Biology, respiratory system, Apical membrane, Syntaxin 3, Amiloride, Cell biology, Rats, nervous system, Gene Expression Regulation, Ion Channel Gating, hormones, hormone substitutes, and hormone antagonists, medicine.drug, Protein Binding

Abstract

Amiloride-sensitive sodium channels mediate sodium entry across the apical membrane of epithelial cells in variety of tissues. The rate of Na(+) entry is controlled by the regulation of the epithelial sodium channel (ENaC) complex. Insertion/retrieval of the ENaC complex into the apical membrane as well as direct kinetic effects at the single channel level are recognized mechanisms of regulation. Recent data suggest that the syntaxin family of targeting proteins interact with and functionally regulate a number of ion channels and pumps. To evaluate the role of these proteins in regulating ENaC activity, we co-expressed rat ENaC cRNA (alpha, beta, gamma subunits) with syntaxin 1A or 3 cRNAs in Xenopus oocytes. Basal ENaC currents were inhibited by syntaxin 1A and stimulated by syntaxin 3. Both syntaxin 1A and syntaxin 3 could be co-immunoprecipitated with ENaC subunit proteins, suggesting physical interaction. Interestingly, immunofluorescence data suggest that with either syntaxin isoform the ENaC-associated epifluorescence on the oocyte surface is enhanced. These data indicate that (i) both syntaxin isoforms increase the net externalization of the ENaC channel complex, (ii) that the functional regulation is isoform specific, and (iii) suggest that ENaC may be regulated through mechanisms involving protein-protein interactions.

Published

1999

35. Multiple G Protein-Coupled Receptors Initiate Protein Kinase C Redistribution of GABA Transporters in Hippocampal Neurons

Author

Eve M. Bernstein, Matthew L. Beckman, and Michael W. Quick

Subjects

GABA Plasma Membrane Transport Proteins, Neurotransmitter transporter, Intracellular Fluid, Synaptic cleft, Blotting, Western, Down-Regulation, Organic Anion Transporters, Biology, Hippocampus, chemistry.chemical_compound, GTP-Binding Proteins, GABA transporter, Animals, Biotinylation, Enzyme Inhibitors, Neurotransmitter, Cells, Cultured, Protein Kinase C, gamma-Aminobutyric Acid, G protein-coupled receptor, Neurons, General Neuroscience, Cell Membrane, Glutamate receptor, Membrane Proteins, Membrane Transport Proteins, Biological Transport, Receptors, Muscarinic, Cell biology, Rats, Receptors, Neurotransmitter, Enzyme Activation, chemistry, Receptors, Glutamate, Receptors, Serotonin, biology.protein, Synaptic signaling, Carrier Proteins, Rapid Communication

Abstract

Neurotransmitter transporters function in synaptic signaling in part through the sequestration and removal of neurotransmitter from the synaptic cleft. A recurring theme of transporters is that many can be functionally regulated by protein kinase C (PKC); some of this regulation occurs via a redistribution of the transporter protein between the plasma membrane and the cytoplasm. The endogenous triggers that lead to PKC-mediated transporter redistribution have not been elucidated. G-protein-coupled receptors that activate PKC are likely candidates to initiate transporter redistribution. We tested this hypothesis by examining the rat brain GABA transporter GAT1 endogenously expressed in hippocampal neurons. Specific agonists of G-protein-coupled acetylcholine, glutamate, and serotonin receptors downregulate GAT1 function. This functional inhibition is dose-dependent, mimicked by PKC activators, and prevented by specific receptor antagonists and PKC inhibitors. Surface biotinylation experiments show that the receptor-mediated functional inhibition correlates with a redistribution of GAT1 from the plasma membrane to intracellular locations. These data demonstrate (1) that endogenous GAT1 function can be regulated by PKC via subcellular redistribution, and (2) that signaling via several different G-protein-coupled receptors can mediate this effect. These results raise the possibility that some effects of G-protein-mediated alterations in synaptic signaling might occur through changes in the number of transporters expressed on the plasma membrane and subsequent effects on synaptic neurotransmitter levels.

Published

1999

36. Functional regulation of Galpha16 by protein kinase C

Author

Michael W. Quick and Anna M. Aragay

Subjects

G protein, Xenopus, Biochemistry, chemistry.chemical_compound, GTP-Binding Proteins, Heterotrimeric G protein, Animals, Amino Acid Sequence, Enzyme Inhibitors, Phosphorylation, Molecular Biology, Protein kinase C, Protein Kinase C, biology, Phospholipase C, Inositol trisphosphate, Cell Biology, Staurosporine, Cell biology, Enzyme Activation, Gq alpha subunit, chemistry, biology.protein, Oocytes, Tetradecanoylphorbol Acetate, Signal transduction, Signal Transduction

Abstract

Recent evidence demonstrates that the alpha subunits of some heterotrimeric GTP-binding proteins (G proteins) are subject to modification by protein kinase C (PKC). For the family of G proteins that activate the phospholipase C/inositol trisphosphate/calcium/PKC pathway, such modification could result in G protein autoregulation. To examine the potential regulation of members of the Galphaq family by PKC phosphorylation, we expressed the thyrotropin-releasing hormone (TRH) receptor in combination with Galphaq, Galpha11, Galpha14, Galpha15, or Galpha16 in Xenopus oocytes and examined the regulation of signaling by PKC activators and inhibitors. For Galpha16 and Galpha15, the two family members of hematopoietic lineage, PKC activators reduce both the magnitude and the time course of TRH-mediated responses; PKC inhibitors have the opposite effect. The PKC-mediated effects are evident in measurements of GTPase activity, suggesting that the regulation is occurring early in the signaling pathway. In vivo phosphorylation experiments demonstrate that Galpha16 is a substrate for PKC modification. By comparison, Galphaq is not phosphorylated by PKC in vivo, and oocytes expressing Galphaq are not functionally modulated by PKC. Repeated TRH stimulation of oocytes expressing Galpha16 mimics the effects of PKC activators, and this functional regulation is correlated with an increase in Galpha16 phosphorylation. A mutant Galpha16 with four consensus PKC phosphorylation sites removed is not phosphorylated in vivo, and TRH responses mediated through the mutant are not regulated by PKC. These results demonstrate that signaling involving hematopoietic G proteins is subject to PKC-mediated autoregulation, at least in part, by phosphorylation of the G protein alpha subunit.

Published

1999

37. Syntaxin 1A inhibits CFTR chloride channels by means of domain-specific protein-protein interactions

Author

Anjaparavanda P. Naren, James F. Collawn, Kevin L. Kirk, Deborah J. Nelson, and Michael W. Quick

Subjects

congenital, hereditary, and neonatal diseases and abnormalities, Vesicle fusion, Swine, Xenopus, Cystic Fibrosis Transmembrane Conductance Regulator, Syntaxin 1, Nerve Tissue Proteins, Plasma protein binding, Biology, environment and public health, Animals, Humans, Multidisciplinary, urogenital system, Lipid bilayer fusion, Biological Sciences, Syntaxin 3, Cystic fibrosis transmembrane conductance regulator, Cell biology, Membrane protein, nervous system, Antigens, Surface, COS Cells, Mutation, Chloride channel, biology.protein, LLC-PK1 Cells, biological phenomena, cell phenomena, and immunity, Protein Binding

Abstract

Previously we showed that the functional activity of the epithelial chloride channel that is encoded by the cystic fibrosis gene (CFTR) is reciprocally modulated by two components of the vesicle fusion machinery, syntaxin 1A and Munc-18. Here we report that syntaxin 1A inhibits CFTR chloride channels by means of direct and domain-specific protein–protein interactions. Syntaxin 1A stoichiometrically binds to the N-terminal cytoplasmic tail of CFTR, and this binding is blocked by Munc-18. The modulation of CFTR currents by syntaxin 1A is eliminated either by deletion of this tail or by injecting this tail as a blocking peptide into coexpressing Xenopus oocytes. The CFTR binding site on syntaxin 1A maps to the third predicted helical domain (H3) of this membrane protein. Moreover, CFTR Cl − currents are effectively inhibited by a minimal syntaxin 1A construct (i.e., the membrane-anchored H3 domain) that cannot fully substitute for wild-type syntaxin 1A in membrane fusion reactions. We also show that syntaxin 1A binds to and inhibits the activities of disease-associated mutants of CFTR, and that the chloride current activity of recombinant ΔF508 CFTR (i.e., the most common cystic fibrosis mutant) can be potentiated by disrupting its interaction with syntaxin 1A in cultured epithelial cells. Our results provide evidence for a direct physical interaction between CFTR and syntaxin 1A that limits the functional activities of normal and disease-associated forms of this chloride channel.

Published

1998

38. Protein kinase C regulates the interaction between a GABA transporter and syntaxin 1A

Author

Eve M. Bernstein, Michael W. Quick, and Matthew L. Beckman

Subjects

endocrine system, GABA Plasma Membrane Transport Proteins, Botulinum Toxins, Immunoprecipitation, Organic Anion Transporters, Syntaxin 1, Nerve Tissue Proteins, environment and public health, PC12 Cells, Sodium Channels, Article, Reuptake, SNAP23, GABA transporter, Animals, Protein kinase C, Protein Kinase C, biology, Chemistry, STX1A, urogenital system, General Neuroscience, Membrane Proteins, Membrane Transport Proteins, Transporter, Syntaxin 3, Cell biology, Rats, nervous system, Antigens, Surface, Mutation, biology.protein, biological phenomena, cell phenomena, and immunity, Carrier Proteins

Abstract

Syntaxin 1A inhibits GABA uptake of an endogenous GABA transporter in neuronal cultures from rat hippocampus and in reconstitution systems expressing the cloned rat brain GABA transporter GAT1. Evidence of interactions between syntaxin 1A and GAT1 comes from three experimental approaches: botulinum toxin cleavage of syntaxin 1A, syntaxin 1A antisense treatments, and coimmunoprecipitation of a complex containing GAT1 and syntaxin 1A. Protein kinase C (PKC), shown previously to modulate GABA transporter function, exerts its modulatory effects by regulating the availability of syntaxin 1A to interact with the transporter, and a transporter mutant that fails to interact with syntaxin 1A is not regulated by PKC. These results suggest a new target for regulation by syntaxin 1A and a novel mechanism for controlling the machinery involved in both neurotransmitter release and reuptake.

Published

1998

39. Regulation of CFTR chloride channels by syntaxin and Munc18 isoforms

Author

Dale J. Benos, Weiwen Xie, Kevin L. Kirk, Mark K. Bennett, Anjaparavanda P. Naren, Biljana Jovov, Michael W. Quick, Deborah J. Nelson, and Jonathan Pevsner

Subjects

congenital, hereditary, and neonatal diseases and abnormalities, Patch-Clamp Techniques, Protein family, Cystic Fibrosis, Colon, Xenopus, Molecular Sequence Data, Vesicular Transport Proteins, Cystic Fibrosis Transmembrane Conductance Regulator, Syntaxin 1, Nerve Tissue Proteins, Biology, Xenopus Proteins, Cell Line, Munc18 Proteins, Chlorides, Isomerism, Syntaxin, Animals, Humans, Multidisciplinary, urogenital system, Qa-SNARE Proteins, Membrane Proteins, respiratory system, biology.organism_classification, Syntaxin 3, Cystic fibrosis transmembrane conductance regulator, Recombinant Proteins, respiratory tract diseases, Cell biology, nervous system, Biochemistry, Membrane protein, Chloride channel, biology.protein, Oocytes

Abstract

The cystic fibrosis gene encodes a cyclic AMP-gated chloride channel (CFTR) that mediates electrolyte transport across the luminal surfaces of a variety of epithelial cells. The molecular mechanisms that modulate CFTR activity in epithelial tissues are poorly understood. Here we show that CFTR is regulated by an epithelially expressed syntaxin (syntaxin 1A), a membrane protein that also modulates neurosecretion and calcium-channel gating in brain. Syntaxin 1A physically interacts with CFTR chloride channels and regulates CFTR-mediated currents both in Xenopus oocytes and in epithelial cells that normally express these proteins. The physical and functional interactions between syntaxin 1A and CFTR are blocked by a syntaxin-binding protein of the Munc18 protein family (also called n-Secl). Our results indicate that CFTR function in epithelial cells is regulated by an interplay between syntaxin and Munc18 isoforms.

Published

1997

40. Influence of subunit composition on desensitization of neuronal acetylcholine receptors at low concentrations of nicotine

Author

B. Noerager, Michael W. Quick, Catherine P. Fenster, Robin A. J. Lester, and M. F. Rains

Subjects

medicine.medical_specialty, Nicotine, Dose-Response Relationship, Drug, Chemistry, General Neuroscience, medicine.medical_treatment, Xenopus, Articles, Endocrinology, Nicotinic agonist, Internal medicine, Homologous desensitization, medicine, Oocytes, Homomeric, Animals, Receptors, Cholinergic, Receptor, Desensitization (medicine), medicine.drug, G alpha subunit, Acetylcholine receptor

Abstract

The influence of alpha and beta subunits on the properties of nicotine-induced activation and desensitization of neuronal nicotinic acetylcholine receptors (nAChRs) expressed in Xenopus oocytes was examined. Receptors containing alpha4 subunits were more sensitive to activation by nicotine than alpha3-containing receptors. At low concentrations of nicotine, nAChRs containing beta2 subunits reached near-maximal desensitization more rapidly than beta4-containing receptors. The concentration of nicotine producing half-maximal desensitization was influenced by the particular alpha subunit expressed; similar to results for activation, alpha4-containing receptors were more sensitive to desensitizing levels of nicotine than alpha3-containing receptors. The alpha subunit also influenced the rate of recovery from desensitization; this rate was approximately inversely proportional to the apparent nicotine affinity for the desensitized state. The homomeric alpha7 receptor showed the lowest sensitivity to nicotine for both activation and desensitization; alpha7 nAChRs also demonstrated the fastest desensitization kinetics. These subunit-dependent properties remained in the presence of external calcium, although subtle, receptor subtype-specific effects on both the apparent affinities for activation and desensitization and the desensitization kinetics were noted. These data imply that the subunit composition of various nAChRs determines the degree to which receptors are desensitized and/or activated by tobacco-related levels of nicotine. The subtype-specific balance between receptor activation and desensitization should be considered important when the cellular and behavioral actions of nicotine are interpreted.

Published

1997

41. Second Messengers, Trafficking-Related Proteins, and Amino Acid Residues that Contribute to the Functional Regulation of the Rat Brain GABA Transporter GAT1

Author

Norman Davidson, Janis L. Corey, Michael W. Quick, and Henry A. Lester

Subjects

GABA Plasma Membrane Transport Proteins, Neurotransmitter uptake, Organic Anion Transporters, Biology, Second Messenger Systems, Neurotransmitter secretion, Syntaxin, GABA transporter, Animals, Amino Acids, Protein kinase C, General Neuroscience, Brain, Membrane Proteins, Membrane Transport Proteins, Proteins, Transporter, Articles, Cell biology, Rats, Biochemistry, Second messenger system, biology.protein, Oocytes, Carrier Proteins, Intracellular

Abstract

Recent evidence indicates that several members of the Na+-coupled transporter family are regulated, and this regulation in part occurs by redistribution of transporters between intracellular locations and the plasma membrane. We elucidate components of this process for both wild-type and mutant GABA transporters (GAT1) expressed inXenopusoocytes using a combination of uptake assays, immunoblots, and electrophysiological measurements of membrane capacitance, transport-associated currents, and GAT1-specific charge movements. At low GAT1 expression levels, activators of protein kinase C (PKC) induce redistribution of GAT1 from intracellular vesicles to the plasma membrane; at higher GAT1 expression levels, activators of PKC fail to induce this redistribution. However, coinjection of total rat brain mRNA with GAT1 permits PKC-mediated modulation at high transporter expression levels. This effect of brain mRNA on modulation is mimicked by coinjection of syntaxin 1a mRNA and is eliminated by injecting synaptophysin or syntaxin antisense oligonucleotides. Additionally, botulinum toxins, which inactivate proteins involved in vesicle release and recycling, reduce basal GAT1 expression and prevent PKC-induced translocation. Mutant GAT1 proteins, in which most or all of a leucine heptad repeat sequence was removed, display altered basal distribution and lack susceptibility to modulation by PKC, delineating one region of GAT1 necessary for its targeting. Thus, functional regulation of GAT1 in oocytes occurs via components common to transporters and to trafficking in both neural and non-neural cells, and suggests a relationship between factors that control neurotransmitter secretion and the components necessary for neurotransmitter uptake.

Published

1997

42. Desensitization of inositol 1,4,5-trisphosphate/Ca2+-induced Cl- currents by prolonged activation of G proteins in Xenopus oocytes

Author

Anna M. Aragay, Melvin I. Simon, Michael W. Quick, Norman Davidson, and Henry A. Lester

Subjects

endocrine system, G protein, Protein subunit, Xenopus, Inositol 1,4,5-Trisphosphate, Inhibitory postsynaptic potential, Biochemistry, chemistry.chemical_compound, Chlorides, Chloride Channels, GTP-Binding Proteins, Animals, Humans, Inositol, Receptor, Molecular Biology, G alpha subunit, biology, Receptors, Thyrotropin-Releasing Hormone, Cell Biology, biology.organism_classification, Molecular biology, Cell biology, chemistry, Oocytes, Calcium, hormones, hormone substitutes, and hormone antagonists, Caltech Library Services, Gamma subunit

Abstract

Expression of G protein alpha subunits of the Gq family with various G protein-coupled receptors induces activation of an inositol 1,4,5-trisphosphate (IP3)/Ca2+-mediated Cl- conductance in Xenopus oocytes. Our present data show that two members of this family, the human Galpha 16 subunit and the murine homologue Galpha 15, can induce both activation and inhibition of these agonist-induced currents. Although extremely low amounts (10-50 pg) of injected Galpha 16 subunit cRNA cause modest (~2-fold) enhancement of ligand-induced Cl- currents in oocytes co-injected with thyrotropin-releasing hormone (TRH) receptor cRNA 48 h postinjection, larger Galpha 16 and Galpha 15 cRNA injections cause >10-fold inhibition of TRH or 5HT2c receptor responses. The inhibition is analyzed in this study. The inhibited currents are recovered if various Gbeta gamma subunit combinations are also expressed with the Galpha subunits. The constitutively active mutant, Galpha 16Q212L, also causes a strong attenuation of the ligand-induced Cl- currents, but this inhibition is not recovered by co-expression of Gbeta gamma subunits. These results indicate that the free Galpha subunit is responsible for the inhibitory signal. Although expression of TRH receptor alone produces maximum responses approximately 48 h after injection, co-expression of TRH receptor with Galpha 16 results in enhanced responses 6-12 h postinjection, followed by complete attenuation at 36 h. Furthermore, injection of Galpha 16 cRNA alone at comparable levels gives rise to spontaneous Cl- currents within 6-12 h postinjection, suggesting that the early spontaneous activation underlies the later suppression. Expression of other G protein alpha subunits of the Gq family, at cRNA levels considerably higher than effective for Galpha 16, produces both analogous spontaneous Cl- currents and, later, inhibition of ligand-induced Cl- currents. Experiments with direct injection of IP3 and of Ca2+ suggest that this inhibition is consistent with the down-regulation of IP3 receptors. These data indicate that both enhancement and inhibition of signaling through G protein-coupled receptors can be mediated by the expression level and/or activity of an individual G protein.

Published

1996

43. A cocaine-sensitive Drosophila serotonin transporter: Cloning, expression, and electrophysiological characterization

Author

Michael W. Quick, Janis L. Corey, John Guastella, Norman Davidson, and Henry A. Lester

Subjects

Serotonin, DNA, Complementary, Xenopus, Molecular Sequence Data, Gene Expression, Genes, Insect, Nerve Tissue Proteins, Biology, Cocaine, Animals, Drosophila Proteins, Humans, Amino Acid Sequence, Cloning, Molecular, Peptide sequence, 5-HT receptor, Serotonin transporter, DNA Primers, Serotonin Plasma Membrane Transport Proteins, Membrane Glycoproteins, Multidisciplinary, Base Sequence, Sequence Homology, Amino Acid, Membrane Transport Proteins, Transporter, Rats, Electrophysiology, Transmembrane domain, Monoamine neurotransmitter, Biochemistry, Oocytes, biology.protein, Drosophila, Female, Carrier Proteins, Drosophila Protein, Research Article

Abstract

A cocaine-sensitive, high-affinity Drosophila serotonin (5-hydroxytryptamine; 5HT) transporter cDNA, denoted dSERT1, was isolated and characterized in oocytes. dSERT1 shows little transport of other monoamines and is Na+ and Cl- dependent. Sequence analysis indicates 12 putative transmembrane domains and strong homologies (approximately 50%) among dSERT1 and mammalian 5HT, norepinephrine, and dopamine transporters. Interestingly, the pharmacological properties of dSERT1, including sensitivity to antidepressants, are more similar to those of mammalian catecholamine transporters than to mammalian 5HT transporters. Two-electrode voltage-clamp analysis demonstrated 5HT-induced, voltage-dependent currents. Cloning and characterization of dSERT1 adds significantly to our knowledge of the diversity of 5HT transporters with regard to primary sequence, pharmacological profile, and permeation properties.

Published

1994

44. Steady states, charge movements, and rates for a cloned GABA transporter expressed in Xenopus oocytes

Author

Norman Davidson, Sela Mager, Cesar Labarca, Michael W. Quick, Janis Naeve, and Henry A. Lester

Subjects

GABA Plasma Membrane Transport Proteins, Organic anion transporter 1, Xenopus, Nipecotic Acids, Gene Expression, Organic Anion Transporters, Transfection, RNA, Complementary, GABA Antagonists, Chlorides, Extracellular, GABA transporter, Animals, Cloning, Molecular, gamma-Aminobutyric Acid, biology, Chemistry, General Neuroscience, Cell Membrane, Sodium, Electric Conductivity, Membrane Proteins, Membrane Transport Proteins, Transporter, GABA receptor antagonist, biology.organism_classification, Electrophysiology, Kinetics, nervous system, Biochemistry, biology.protein, Biophysics, Oocytes, RNA, Female, Carrier Proteins

Abstract

Voltage-clamp analysis was applied to study the currents associated with the uptake of extracellular gamma-aminobutyric acid (GABA) by the cloned transporter GAT1 expressed at high efficiency in Xenopus oocytes. Steady-state GABA currents were increased at higher extracellular [GABA], [Na+], and [Cl-] and at more negative potentials. The Hill coefficient for Na+ exceeded unity, suggesting the involvement of two Na+ ions. In the absence of GABA, voltage jumps produced transient currents that behaved like capacitive charge movements; these were suppressed by the uptake inhibitor SKF-89976A, were shifted to more negative potentials at lower external [Na+] and [Cl-], and had an effective valence of 1.1 elementary charge. A turnover rate per transporter of 6-13/s at maximal [GABA] (-80 mV, 96 mM NaCl, 22 degrees C) is given both by the kinetics of voltage jump relaxations and by the ratio between the maximal GABA currents and the charge movements. These quantitative data are necessary for evaluating the roles of GAT1 in synaptic function.

Published

1993

45. Regions of β4·β2 subunit chimeras that contribute to the agonist selectivity of neuronal nicotinic receptors

Author

Bruce N. Cohen, Michael W. Quick, Norman Davidson, Henry A. Lester, and Antonio Figl

Subjects

Agonist, Nicotine, medicine.drug_class, Protein subunit, Recombinant Fusion Proteins, Xenopus, DNA Mutational Analysis, Molecular Sequence Data, Biophysics, Receptors, Nicotinic, Biochemistry, chemistry.chemical_compound, Cytisine, Structure-Activity Relationship, Nicotinic receptor, Alkaloids, Structural Biology, Genetics, medicine, Extracellular, Animals, Amino Acid Sequence, Molecular Biology, Tetramethylammonium, Neurons, Pharmacology, biology, Chimera, Cell Biology, biology.organism_classification, Azocines, Acetylcholine, Cell biology, Quaternary Ammonium Compounds, chemistry, Ganglionic stimulant, Oocytes, Quinolizines, Cys-loop receptors, medicine.drug

Abstract

Fifteen chimeric nicotinic receptor beta subunits were constructed consisting of N-terminal neuronal beta 4 sequences and C-terminal beta 2 sequences. Responses to cytisine, nicotine, or tetramethylammonium were compared to acetylcholine responses for these subunits expressed in Xenopus oocytes with alpha 3 subunits. The results show that (i) two residues in the extracellular domain of chimeric beta 4.beta 2 subunits (108 beta 2F/beta 4V, 110 beta 2S/beta 4T) account for much of the relative cytisine sensitivity; and (ii) four extracellular residues of chimeric beta 4.beta 2 subunits (112 beta 2A/beta 4V, 113 beta 2V/beta 4I and 115 beta 2S/beta 4R, 116 beta 2Y/beta 4S) account for most of the relative tetramethylammonium sensitivity. The data did not permit localization of nicotine sensitivity to any particular region.