Acetylcholine Receptor (AChR) Clustering Is Regulated Both by Glycogen Synthase Kinase 3β (GSK3β)-dependent Phosphorylation and the Level of CLIP-associated Protein 2 (CLASP2) Mediating the Capture of Microtubule Plus-ends

The postsynaptic apparatus of the neuromuscular junction (NMJ) traps and anchors acetylcholine receptors (AChRs) at high density at the synapse. We have previously shown that microtubule (MT) capture by CLASP2, a MT plus-end-tracking protein (+TIP), increases the size and receptor density of AChR clusters at the NMJ through the delivery of AChRs and that this is regulated by a pathway involving neuronal agrin and several postsynaptic kinases, including GSK3. Phosphorylation by GSK3 has been shown to cause CLASP2 dissociation from MT ends, and nine potential phosphorylation sites for GSK3 have been mapped on CLASP2. How CLASP2 phosphorylation regulates MT capture at the NMJ and how this controls the size of AChR clusters are not yet understood. To examine this, we used myotubes cultured on agrin patches that induce AChR clustering in a two-dimensional manner. We show that expression of a CLASP2 mutant, in which the nine GSK3 target serines are mutated to alanine (CLASP2–9XS/9XA) and are resistant to GSK3β-dependent phosphorylation, promotes MT capture at clusters and increases AChR cluster size, compared with myotubes that express similar levels of wild type CLASP2 or that are noninfected. Conversely, myotubes expressing a phosphomimetic form of CLASP2 (CLASP2–8XS/D) show enrichment of immobile mutant CLASP2 in clusters, but MT capture and AChR cluster size are reduced. Taken together, our data suggest that both GSK3β-dependent phosphorylation and the level of CLASP2 play a role in the maintenance of AChR cluster size through the regulated capture and release of MT plus-ends.

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Molecular events in synaptogenesis: nerve-muscle adhesion and postsynaptic differentiation

AJP Cell Physiology ◽

10.1152/ajpcell.1988.254.3.c345 ◽

1988 ◽

Vol 254 (3) ◽

pp. C345-C364 ◽

Cited By ~ 91

Author(s):

R. J. Bloch ◽

D. W. Pumplin

Keyword(s):

Cell Surface ◽

Muscle Cell ◽

Acetylcholine Receptors ◽

Membrane Skeleton ◽

Postsynaptic Membrane ◽

Molecular Assembly ◽

Trophic Factors ◽

Achr Cluster ◽

Nerve Muscle ◽

Achr Clustering

The clustering of acetylcholine receptors (AChR) in the postsynaptic membrane of newly innervated muscle fibers is one of the earliest events in the development of the vertebrate neuromuscular junction. Here, we describe two hypotheses that can account for AChR clustering in response to innervation. The "trophic factor" hypothesis proposes that the neuron releases a soluble factor that interacts with the muscle cell in a specific manner and that this interaction results in the local accumulation of AChR. The "contact and adhesion" hypothesis proposes that the binding of the nerve to the muscle cell surface is itself sufficient to induce AChR clustering, without the participation of soluble factors. We present a model for the molecular assembly of AChR clusters based on the contact and adhesion hypothesis. The model involves the sequential assembly of three distinct membrane domains. The first domain to form serves to attach microfilaments to the cytoplasmic surface of the muscle cell membrane at sites of muscle-nerve adhesion. The second domain to form is clathrin-coated membrane; it serves as a site of insertion of additional membrane elements, including AChR. Upon insertion of AChR into the cell surface, a membrane skeleton assembles by anchoring itself to the AChR. The skeleton, composed in part of actin and spectrin, binds and immobilizes significant numbers of AChR, thereby forming the third membrane domain of the AChR cluster. We make several predictions that should distinguish this model of AChR clustering from one that invokes soluble, trophic factors.

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A Single Pulse of Agrin Triggers a Pathway That Acts To Cluster Acetylcholine Receptors

Molecular and Cellular Biology ◽

10.1128/mcb.24.18.7841-7854.2004 ◽

2004 ◽

Vol 24 (18) ◽

pp. 7841-7854 ◽

Cited By ~ 29

Author(s):

Peggy Mittaud ◽

Alain A. Camilleri ◽

Raffaella Willmann ◽

Susanne Erb-Vögtli ◽

Steven J. Burden ◽

...

Keyword(s):

Tyrosine Kinase ◽

Acetylcholine Receptors ◽

Cluster Formation ◽

Single Pulse ◽

Achr Cluster ◽

Abl Kinases ◽

Temporal Aspects ◽

Kinase Cascade ◽

Spatial Specificity ◽

Achr Clustering

ABSTRACT Agrin triggers signaling mechanisms of high temporal and spatial specificity to achieve phosphorylation, clustering, and stabilization of postsynaptic acetylcholine receptors (AChRs). Agrin transiently activates the kinase MuSK; MuSK activation has largely vanished when AChR clusters appear. Thus, a tyrosine kinase cascade acts downstream from MuSK, as illustrated by the agrin-evoked long-lasting activation of Src family kinases (SFKs) and their requirement for AChR cluster stabilization. We have investigated this cascade and report that pharmacological inhibition of SFKs reduces early but not later agrin-induced phosphorylation of MuSK and AChRs, while inhibition of Abl kinases reduces late phosphorylation. Interestingly, SFK inhibition applied selectively during agrin-induced AChR cluster formation caused rapid cluster dispersal later upon agrin withdrawal. We also report that a single 5-min agrin pulse, followed by extensive washing, triggered long-lasting MuSK and AChR phosphorylation and efficient AChR clustering. Following the pulse, MuSK phosphorylation increased and, beyond a certain level, caused maximal clustering. These data reveal novel temporal aspects of tyrosine kinase action in agrin signaling. First, during AChR cluster formation, SFKs initiate early phosphorylation and an AChR stabilization program that acts much later. Second, a kinase mechanism rapidly activated by agrin acts thereafter autonomously in agrin's absence to further increase MuSK phosphorylation and cluster AChRs.

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Degradation of Mcl-1 by β-TrCP Mediates Glycogen Synthase Kinase 3-Induced Tumor Suppression and Chemosensitization

Molecular and Cellular Biology ◽

10.1128/mcb.00620-06 ◽

2006 ◽

Vol 27 (11) ◽

pp. 4006-4017 ◽

Cited By ~ 263

Author(s):

Qingqing Ding ◽

Xianghuo He ◽

Jung-Mao Hsu ◽

Weiya Xia ◽

Chun-Te Chen ◽

...

Keyword(s):

Embryonic Development ◽

Tumor Suppression ◽

Glycogen Synthase ◽

Tissue Homeostasis ◽

Glycogen Synthase Kinase ◽

Glycogen Synthase Kinase 3 ◽

Phosphorylation Sites ◽

Wild Type ◽

Gsk 3Β ◽

Induced Apoptosis

ABSTRACT Apoptosis is critical for embryonic development, tissue homeostasis, and tumorigenesis and is determined largely by the Bcl-2 family of antiapoptotic and prosurvival regulators. Here, we report that glycogen synthase kinase 3 (GSK-3) was required for Mcl-1 degradation, and we identified a novel mechanism for proteasome-mediated Mcl-1 turnover in which GSK-3β associates with and phosphorylates Mcl-1 at one consensus motif (155 STDG159 SLPS163 T; phosphorylation sites are in italics), which will lead to the association of Mcl-1 with the E3 ligase β-TrCP, and β-TrCP then facilitates the ubiquitination and degradation of phosphorylated Mcl-1. A variant of Mcl-1 (Mcl-1-3A), which abolishes the phosphorylations by GSK-3β and then cannot be ubiquitinated by β-TrCP, is much more stable than wild-type Mcl-1 and able to block the proapoptotic function of GSK-3β and enhance chemoresistance. Our results indicate that the turnover of Mcl-1 by β-TrCP is an essential mechanism for GSK-3β-induced apoptosis and contributes to GSK-3β-mediated tumor suppression and chemosensitization.

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Rabbit skeletal muscle glycogen synthase expressed in COS cells. Identification of regulatory phosphorylation sites.

Journal of Biological Chemistry ◽

10.1016/s0021-9258(18)47282-1 ◽

1994 ◽

Vol 269 (41) ◽

pp. 25534-25542

Author(s):

A V Skurat ◽

Y Wang ◽

P J Roach

Keyword(s):

Skeletal Muscle ◽

Muscle Glycogen ◽

Glycogen Synthase ◽

Rabbit Skeletal Muscle ◽

Phosphorylation Sites ◽

Cos Cells ◽

Skeletal Muscle Glycogen ◽

Regulatory Phosphorylation

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Multiple phosphorylation of rabbit skeletal muscle glycogen synthase. Evidence for interactions among phosphorylation sites and the resolution of electrophoretically distinct forms of the subunit.

Journal of Biological Chemistry ◽

10.1016/s0021-9258(17)44513-3 ◽

1983 ◽

Vol 258 (17) ◽

pp. 10702-10709 ◽

Cited By ~ 27

Author(s):

A A DePaoli-Roach ◽

Z Ahmad ◽

M Camici ◽

J C Lawrence ◽

P J Roach

Keyword(s):

Skeletal Muscle ◽

Muscle Glycogen ◽

Glycogen Synthase ◽

Rabbit Skeletal Muscle ◽

Phosphorylation Sites ◽

Skeletal Muscle Glycogen

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Acetylcholine Receptors

The Journal of General Physiology ◽

10.1085/jgp.60.3.248 ◽

1972 ◽

Vol 60 (3) ◽

pp. 248-262 ◽

Cited By ~ 174

Author(s):

H. Criss Hartzell ◽

Douglas M. Fambrough

Keyword(s):

Acetylcholine Receptors ◽

Time Course ◽

Plasma Membranes ◽

Scintillation Counting ◽

Receptor Density ◽

Rat Diaphragm ◽

Leg Muscles ◽

And Function ◽

Quantitative Radioautography ◽

Ach Receptors

Using 125iodine-labeled α-bungarotoxin (α-BGT-125I) and quantitative radioautography, we have studied the time-course of the change in acetylcholine (ACh) receptor distribution and density occurring in rat diaphragm after denervation. In innervated fibers, ACh receptors are localized at the neuromuscular junction and the extrajunctional receptor density is less than five receptors per square micrometer. The extrajunctional receptor density begins to increase between 2 and 3 days after denervation and increases approximately linearly to 1695 receptors/µm2 at 14 days, subsequently decreasing to 529 receptors/µm2 at 45 days. We have isolated plasma membranes from rat leg muscles at various times after denervation and find that the change in concentration of ACh receptors in the membranes measured by α-BGT-125I binding and scintillation counting follows a time-course similar to the change in ACh receptor density measured radioautographically. Furthermore, we have correlated extrajunctional ACh receptor density measured by radioautography with extrajunctional ACh sensitivity measured by iontophoretic application of ACh and intracellular recording and find that the log of ACh receptor density is related to 0.53 times the log of ACh sensitivity. These results are discussed in terms of the electrophysiological experiments on the ACh receptor and the recent, more biochemical approaches to the study of ACh receptor control and function.

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Insulin promotes glycogen synthesis in the absence of GSK3 phosphorylation in skeletal muscle

AJP Endocrinology and Metabolism ◽

10.1152/ajpendo.00481.2007 ◽

2008 ◽

Vol 294 (1) ◽

pp. E28-E35 ◽

Cited By ~ 67

Author(s):

Michale Bouskila ◽

Michael F. Hirshman ◽

Jørgen Jensen ◽

Laurie J. Goodyear ◽

Kei Sakamoto

Keyword(s):

Skeletal Muscle ◽

Glucose Uptake ◽

Muscle Glycogen ◽

Glycogen Content ◽

Glycogen Synthase ◽

Glycogen Synthesis ◽

Wild Type ◽

Muscle Glycogen Synthesis ◽

Mutant Forms

Insulin promotes dephosphorylation and activation of glycogen synthase (GS) by inactivating glycogen synthase kinase (GSK) 3 through phosphorylation. Insulin also promotes glucose uptake and glucose 6-phosphate (G-6- P) production, which allosterically activates GS. The relative importance of these two regulatory mechanisms in the activation of GS in vivo is unknown. The aim of this study was to investigate if dephosphorylation of GS mediated via GSK3 is required for normal glycogen synthesis in skeletal muscle with insulin. We employed GSK3 knockin mice in which wild-type GSK3α and -β genes are replaced with mutant forms (GSK3α/βS21A/S21A/S9A/S9A), which are nonresponsive to insulin. Although insulin failed to promote dephosphorylation and activation of GS in GSK3α/βS21A/S21A/S9A/S9Amice, glycogen content in different muscles from these mice was similar compared with wild-type mice. Basal and epinephrine-stimulated activity of muscle glycogen phosphorylase was comparable between wild-type and GSK3 knockin mice. Incubation of isolated soleus muscle in Krebs buffer containing 5.5 mM glucose in the presence or absence of insulin revealed that the levels of G-6- P, the rate of [14C]glucose incorporation into glycogen, and an increase in total glycogen content were similar between wild-type and GSK3 knockin mice. Injection of glucose containing 2-deoxy-[3H]glucose and [14C]glucose also resulted in similar rates of muscle glucose uptake and glycogen synthesis in vivo between wild-type and GSK3 knockin mice. These results suggest that insulin-mediated inhibition of GSK3 is not a rate-limiting step in muscle glycogen synthesis in mice. This suggests that allosteric regulation of GS by G-6- P may play a key role in insulin-stimulated muscle glycogen synthesis in vivo.

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Abstract 1361: Leukocyte Antigen-Related Phosphatase Regulates Insulin Sensitivity by Interaction with Snapin

Circulation ◽

10.1161/circ.118.suppl_18.s_313-b ◽

2008 ◽

Vol 118 (suppl_18) ◽

Author(s):

Aleksandr E Vendrov ◽

Igor Tchivilev ◽

Xi-Lin Niu ◽

Juxiang Li ◽

Marschall S Runge ◽

...

Keyword(s):

Insulin Resistance ◽

Insulin Sensitivity ◽

Glucose Uptake ◽

Glycogen Synthase ◽

Serine Phosphorylation ◽

Snare Complex ◽

Vascular Pathology ◽

Wild Type ◽

Membrane Translocation ◽

Leukocyte Antigen

Several protein tyrosine phosphatases including leukocyte antigen-related (LAR) phosphatase have been implicated in insulin resistance, which is a risk factor for atherosclerosis. We showed previously that LAR negatively regulates insulin-like growth factor-1 (IGF1) signaling in vascular smooth muscle cells (VSMC) leading to increased proliferation and migration. Absence of LAR also enhanced neointima formation in response to arterial injury in mice. However, the role of LAR-modulated signaling in the development of insulin resistance has not been elucidated. Here, we investigated the function of LAR in regulating glucose uptake and insulin sensitivity. We identified snapin, a SNARE-associated protein involved in glucose transporter Glut4 vesicle fusion with plasma membrane, as a LAR-interacting protein using a yeast two-hybrid screen. IGF1-induced serine phosphorylation of snapin, its translocation to membrane and association with SNARE complex were enhanced in VSMC lacking LAR. Similarly, PI3K-PDK1-PKCζ signaling pathway was more active in LAR-/- cells after IGF1 treatment. This resulted in enhanced Glut4 activation, its membrane translocation and association with snapin. Glut4 membrane translocation and association with snapin after IGF1 treatment were impaired in snapin+/− VSMC. IGF1 treatment also increased serine phosphorylation of GSK3 β in LAR−/− VSMC leading to increased activation of glycogen synthase. Consistent with this, enhanced glucose uptake was observed in LAR−/− VSMC compared to wild-type cells after IGF1 treatment. Basal and IGF1-induced glucose uptake were significantly lower in snapin+/− VSMC than in wild-type cells. Snapin+/− mice had higher levels of blood glucose, lower quantitative insulin sensitivity check index (QUICKI) and impaired response to insulin in insulin tolerance test (ITT) compared to wild-type mice. Decrease of QUICKI and impairment of IIT were more pronounced in snapin+/− mice fed a high-fat diet. In addition, Doppler ultrasonography indicated increased arterial stiffness in snapin+/− mice. Together, these data indicate that LAR negatively regulates snapin phosphorylation which in turn affects glucose uptake leading to the development of insulin resistance and vascular pathology.

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A mutation in the alpha 1-tubulin gene of Chlamydomonas reinhardtii confers resistance to anti-microtubule herbicides

Journal of Cell Science ◽

10.1242/jcs.106.1.209 ◽

1993 ◽

Vol 106 (1) ◽

pp. 209-218 ◽

Cited By ~ 4

Author(s):

S.W. James ◽

C.D. Silflow ◽

P. Stroom ◽

P.A. Lefebvre

Keyword(s):

Chlamydomonas Reinhardtii ◽

Resistance Mutation ◽

In Vitro Translation ◽

Predicted Amino Acid Sequence ◽

Two Dimensional ◽

Wild Type ◽

Tubulin Gene ◽

Alpha Tubulin ◽

Tubulin Genes

A mutation in the alpha 1-tubulin gene of Chlamydomonas reinhardtii was isolated by using the amiprophos-methyl-resistant mutation apm1-18 as a background to select new mutants that showed increased resistance to the drug. The upA12 mutation caused twofold resistance to amiprophos-methyl and oryzalin, and twofold hypersensitivity to the microtubule-stabilizing drug taxol, suggesting that the mutation enhanced microtubule stability. The resistance mutation was semi-dominant and mapped to the same interval on linkage group III as the alpha 1-tubulin gene. Two-dimensional gel immunoblots of proteins in the mutant cells revealed two electrophoretically altered alpha-tubulin isoforms, one of which was acetylated and incorporated into microtubules in the axoneme. The mutant isoforms co-segregated with the drug-resistance phenotypes when mutant upA12 was backcrossed to wild-type cells. Two-dimensional gel analysis of in vitro translation products showed that the non-acetylated variant alpha-tubulin was a primary gene product. DNA sequence analysis of the alpha 1-tubulin genes from mutant and wild-type cells revealed a single missense mutation, which predicted a change in codon 24 from tyrosine in wild type to histidine in mutant upA12. This alteration in the predicted amino acid sequence corroborated the approximately +1 basic charge shift observed for the variant alpha-tubulins. The mutant allele of the alpha 1-tubulin gene was designated tua1-1.

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