A System for Studying Mechanisms of Neuromuscular Junction Development and Maintenance Valérie Vilmont1,‡, Bruno Cadot1, Gilles Ouanounou2 and Edgar R

A System for Studying Mechanisms of Neuromuscular Junction Development and Maintenance Valérie Vilmont1,‡, Bruno Cadot1, Gilles Ouanounou2 and Edgar R

© 2016. Published by The Company of Biologists Ltd | Development (2016) 143, 2464-2477 doi:10.1242/dev.130278 TECHNIQUES AND RESOURCES RESEARCH ARTICLE A system for studying mechanisms of neuromuscular junction development and maintenance Valérie Vilmont1,‡, Bruno Cadot1, Gilles Ouanounou2 and Edgar R. Gomes1,3,*,‡ ABSTRACT different animal models and cell lines (Chen et al., 2014; Corti et al., The neuromuscular junction (NMJ), a cellular synapse between a 2012; Lenzi et al., 2015) with the hope of recapitulating some motor neuron and a skeletal muscle fiber, enables the translation of features of neuromuscular diseases and understanding the triggers chemical cues into physical activity. The development of this special of one of their common hallmarks: the disruption of the structure has been subject to numerous investigations, but its neuromuscular junction (NMJ). The NMJ is one of the most complexity renders in vivo studies particularly difficult to perform. studied synapses. It is formed of three key elements: the lower motor In vitro modeling of the neuromuscular junction represents a powerful neuron (the pre-synaptic compartment), the skeletal muscle (the tool to delineate fully the fine tuning of events that lead to subcellular post-synaptic compartment) and the Schwann cell (Sanes and specialization at the pre-synaptic and post-synaptic sites. Here, we Lichtman, 1999). The NMJ is formed in a step-wise manner describe a novel heterologous co-culture in vitro method using rat following a series of cues involving these three cellular components spinal cord explants with dorsal root ganglia and murine primary and its role is basically to ensure the skeletal muscle functionality. myoblasts to study neuromuscular junctions. This system allows the Following an action potential down the motor neuron axon, synaptic formation and long-term survival of highly differentiated myofibers, vesicles will fuse with the membrane at the half-terminal of the axon motor neurons, supporting glial cells and functional neuromuscular releasing neurotransmitters into the synaptic cleft. The post-synaptic junctions with post-synaptic specialization. Therefore, fundamental membrane of the muscle fiber is specialized to respond efficiently to aspects of NMJ formation and maintenance can be studied using the the neurotransmitter release and will convert the chemical signal to a described system, which can be adapted to model multiple mechanical signal in the form of muscular contraction (Das et al., NMJ-associated disorders. 2010). In some cases, the dialog between these cellular components is compromised and leads to instability of the NMJ and in worst KEY WORDS: Co-culture, Differentiation, Myofiber, NMJ cases, like in ALS and SMA, eventually axon retraction and muscle atrophy. INTRODUCTION In order to study NMJ physiology and pathology, different The ongoing development of new experimental approaches has in vivo systems are used, such as mouse diaphragm or Drosophila proved to be useful for modeling a number of adverse health abdominal segments (Packard et al., 2002; Perez-Garcia and conditions, including neuromuscular diseases (Chew et al., 2015; Burden, 2012). However, these systems do not allow observation Lenzi et al., 2015; Sandoe and Eggan, 2013; Tu et al., 1996). and manipulation over long periods of time in live NMJ. Therefore, Neuromuscular pathologies encompass a wide range of subgroups, understanding the development of the NMJ often needs transgenic including (1) myopathies such as Duchenne’s and Becker’s organisms, generation of which is time consuming and sometimes muscular dystrophies (Flanigan, 2014); (2) motor neuron diseases impossible. To overcome these problems, different in vitro co- (MNDs) such as amyotrophic lateral sclerosis (ALS), progressive culture systems have been set up in which motor neuron and bulbar palsy, pseudobulbar palsy and spinal muscular atrophy skeletal muscle are grown together in order to recapitulate the (SMA) (de Boer et al., 2014; Edens et al., 2015; Karam et al., 2010; formation and eventual disruption of the NMJ. To date, co-culture Tu et al., 1996); and (3) auto-immune neuromuscular diseases such methods established from various species have been described, as myasthenia gravis and Lambert–Eaton myastenic syndrome including mouse (Morimoto et al., 2013; Zahavi et al., 2015), rat (Ha and Richman, 2015; Lang et al., 2003). Researchers have set up (Das et al., 2010; Southam et al., 2013), Xenopus (Lu et al., 1996; Peng et al., 2003) and chick (Frank and Fischbach, 1979), and also heterologous co-cultures built from motor neuron and muscle 1 Myology Research Center, UM76-INSERM U974-CNRS FRE 3617 Sorbonne cells obtained from different species, such as rat-human (Askanas Universités, UPMC UniversitéParis 06, Paris, France. 2FRE CNRS 3693 (U.N.I.C), Unitéde Neuroscience, Information et ComplexitéCNRS, Bât. 33, 1 Ave de la et al., 1987), mouse-human (Son et al., 2011) and mouse-chick Terasse, Gif sur Yvette 91198, France. 3Instituto de Medicina Molecular, Faculdade (Soundararajan et al., 2007). However, these co-culture methods de Medicina da Universidade de Lisboa, Lisboa, Portugal. * resulted in the formation of immature myofibers (thin muscle fiber, Present address: Instituto de Medicina Molecular, Faculdade de Medicina da Universidade de Lisboa, Avenida Professor Egas Moniz, 1649-028 Lisboa, with centrally localized nuclei and no transversal triads) with Portugal. immature sarcomeric structures (Das et al., 2007, 2009; Southam ‡ Authors for correspondence ([email protected]; et al., 2013). Moreover, previous models did not take advantage of [email protected]) their co-culture system to analyze other post-synaptic structures such as the formation of muscle-specific tyrosine kinase (MuSK) B.C., 0000-0002-1888-3898; E.R.G., 0000-0002-6941-4872 and Rapsyn (also known as Rapsn) clusters which are formed as This is an Open Access article distributed under the terms of the Creative Commons Attribution agrin-induced signaling sparks off and which are essential to the License (http://creativecommons.org/licenses/by/3.0), which permits unrestricted use, distribution and reproduction in any medium provided that the original work is properly attributed. formation of acetylcholine receptor (AChR) clusters. Here, we describe a new functional co-culture system in which muscle fibers Received 28 August 2015; Accepted 12 May 2016 from primary murine myoblasts are brought to advanced DEVELOPMENT 2464 TECHNIQUES AND RESOURCES Development (2016) 143, 2464-2477 doi:10.1242/dev.130278 differentiation and form highly matured NMJs with motor neurons NMJ active zones (Nishimune, 2012; Sanes and Hall, 1979). In derived from rat spinal cord. The muscle fibers show hallmarks of addition, Matrigel provided a three-dimensional matrix for our cells mature skeletal muscle fiber: peripheral nuclei, transversal triads, to grow and differentiate. Myofibers were then switched to myofibrils and organization into three-dimensional bundles differentiation (Fig. 1, Day −3). Twenty-four hours later (Fig. 1, performing synchronized contraction. Furthermore, the NMJ Day −2), another layer of Matrigel was added to the cells to showed pretzel-like morphology reminiscent of in vivo synapses. cover the differentiating muscle fibers (Fig. 1). Forty-eight We used this co-culture model to investigate the formation of the hours later (Fig.1, Day 0), whole transverse sections of the post-synaptic apparatus beyond the clustering of AChRs and we spinal cord with attached dorsal root ganglia (DRGs) without investigated the role of motor neuron firing on muscle removal of the ventral part, i.e. the ventral horn, where efferent development and differentiation. We found that AChRs form nerves are believed to emanate (Blits et al., 2004), were plated on clusters at motor neuron-muscle contacts, that the post- and pre- myotubes (Fig. 1). Medium was also supplemented with growth synapses show hallmarks of maturation and that these NMJs are factors [brain-derived neurotrophic factor (BDNF), ciliary functionally active. neurotrophic factor (CNTF) and glial cell-derived neurotrophic factor (GDNF)] involved in the maturation of NMJs (Peng et al., RESULTS 2003; Sakuma and Yamaguchi, 2011; Tuttle and Matthew, 1995; Development of a heterologous co-culture system Zahavi et al., 2015). After 12 days, myofibers showed We have previously described a method for obtaining highly high contractile activity; in order to reduce the possibility of differentiated myofibers in vitro, which is potentially useful for detachment of the neuron-muscle structures from the dish, we used studying myoblast fusion, nuclear movement, myofiber tetrodotoxin 1 µM (TTX). This treatment not only reduced myofiber differentiation and formation of agrin-induced AChR clusters contractions, but also enhanced formation of neuromuscular (Falcone et al., 2014). However, this method is not suitable for junctions. Time-course analysis showed that at 14 days after studying formation of NMJs and the post-synaptic apparatus as well starting the co-culture, fully mature myofibers and functional as mechanisms of denervation-dependent muscle atrophy, due to the NMJs were present. In addition, we found that the co-culture could lack of two of the basic cell types forming the NMJ: neurons and be kept over longer time periods (at least 30 days) without affecting Schwann cells. We therefore developed an easy co-culture system the viability of the neurons or myofibers, suggesting that we

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