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The Journal of Neuroscience, August 15, 2007, 27(33):8779-8789; doi:10.1523/JNEUROSCI.1599-07.2007
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Neurobiology of Disease
Progressive Motor Neuronopathy: A Critical Role of the Tubulin Chaperone TBCE in Axonal Tubulin Routing from the Golgi Apparatus
Michael K. E. Schaefer,1,2 Henning Schmalbruch,3 Emmanuelle Buhler,1,2 Catherine Lopez,1,2 Natalia Martin,4 Jean-Louis Guénet,4 andGeorg Haase1,2 1Inserm, Unité 29, Equipe Avenir, 13273 Marseille, France, 2Aix Marseille Université, Institut de Neurobiologie de la Méditerranée, 13284 Marseille, France, 3Panum Institute, University of Copenhagen, DK-2200 Copenhagen, Denmark, and 4Institut Pasteur, 75015 Paris, France
Abstract
Top
Abstract
Introduction
Axonal degeneration represents one of the earliest pathological features in motor neuron diseases. We here studied the underlying molecular mechanisms in progressive motor neuronopathy (pmn) mice mutated in the tubulin-specific chaperone TBCE. We demonstrate that TBCE is a peripheral membrane-associated protein that accumulates at the Golgi apparatus. In pmn mice, TBCE is destabilized and disappears from the Golgi apparatus of motor neurons, and microtubules are lost in distal axons. The axonal microtubule loss proceeds retrogradely in parallel with the axonal dying back process. These degenerative changes are inhibited in a dose-dependent manner by transgenic TBCE complementation that restores TBCE expression at the Golgi apparatus. In cultured motor neurons, the pmn mutation, interference RNA-mediated TBCE depletion, and brefeldin A-mediated Golgi disruption all compromise axonal tubulin routing. We conclude that motor axons critically depend on axonal tubulin routing from the Golgi apparatus, a process that involves TBCE and possibly other tubulin chaperones.
Key words: motor neuron disease; ALS; axon degeneration; tubulin chaperone; microtubules; Golgi apparatus
Introduction
Human motor neuron diseases such as amyotrophic lateral sclerosis (ALS) and spinal muscular atrophy (SMA) are incurable and fatal disorders characterized by loss of motor neuron cell bodies, axonal degeneration, and skeletal muscle denervation (for review, see Boillee et al., 2006; Pasinelli and Brown, 2006
We here studied this question in mice with progressive motor neuronopathy (pmn). Homozygous pmn mice suffer from a severe motor neuron disease characterized by axonal dying back (Schmalbruch et al., 1991
We identify TBCE as a tubulin chaperone that accumulates at the cis-Golgi apparatus and demonstrate its requirement for axonal tubulin routing. In spinal motor neurons of early symptomatic pmn mice, the TBCE protein is destabilized, leading to a drastic reduction in tubulin levels and microtubule densities in distal axons. Axonal microtubule loss progresses from distal to proximal, correlates with axonal degeneration, and is inhibited by transgenic TBCE protein expression. These data help to explain the axonal dying back process in pmn mice and provide a mechanistic link between motor axon maintenance and TBCE function at the Golgi apparatus.
Materials and Methods
Antibodies and reagents. Antiserum against TBCE (SA53) was generated by immunizing a rabbit with a mixture of two peptides corresponding to amino acids 87–102 and 389–402 of mouse TBCE (Eurogentec, Liege, Belgium). A second anti-TBCE antiserum (GP52) was generated against the same peptides. In control experiments, antisera were preabsorbed with antigenic peptides or recombinant green fluorescent protein (GFP)–TBCE protein (G. Haase and A. Elmarjou, unpublished observation). Antibodies and their dilutions in immunocytochemistry were as follows: TBCE (1:300),-tubulin (1:1000; Sigma, St. Louis, MO), ßIII-tubulin (TuJ1; 1:2000; Babco, Richmond, CA), GFP (monoclonal antibody, 1:1000; Roche, Indianapolis, IN), myelin basic protein (1:500; Chemicon, Temecula, CA), neurofilament medium chain (NN18, 1:2000; Sigma), S-100 (SH-B1, 1:1000; Sigma), and GM130, p115, Vti1a, and Vti1b (1:250; Becton Dickinson, Walton, KY). Fluorochrome- or horse radish peroxidase-conjugated secondary antibodies were from Invitrogen (Carlsbad, CA) or Jackson ImmunoResearch (West Grove, PA).
Reagents were from the following suppliers: PBS, HBSS, HAM F-10, trypsin, culture media, and supplements (Invitrogen); Hibernate E (BrainBits, Springfield, IL); DNase I, polyornithin, laminin, glial cell line-derived neurotrophic factor (GDNF), taxol, and nocodazole (Sigma), CNTF and BDNF (R & D Systems, Minneapolis, MN), Vectashield–4',6'-diamidino-2-phenylindole (Vector Laboratories, Burlingame, CA); complete protease inhibitors and Dormicum (Roche); Hypnorm (Janssen, Beerse, Belgium); bisbenzimide and brefeldin A (BFA) (Fluka, Saint Quentin Fallavier, France); and Fluoromount (Southern Biotechnology, Birmingham, AL).
Mouse lines and genotyping. The pmn mice were maintained as +/pmn mice and Xt +/+ pmn ("Xt/pmn") mice (Brunialti et al., 1995
Mouse genotyping was done as follows. The pmn and wild-type alleles were detected using primers 5'-GTCTTACTGCTCCCTACTTG (C45F) and 5'-GTGAAAACAGAAAGGGCAGAG (C45R) and 35 cycles of amplification (95°C, 40 s; 58°C, 40 s; 72°C, 40 s), followed by DNA purification (QiaQuick; Qiagen, Hilden, Germany), 2 h incubation with the restriction enzyme MnlI (New England Biolabs, Ipswich, MA), and gel electrophoresis (3% Metaphor agarose; Tebu, Le Perray en Yvelines, France). The NSE:TBCE transgene was detected by PCR using primers 5'-CCAAGGAGATCGACTCTAGAG (NSE-7F), 5'-AAGCGACTGT-TCATATTC (TB-7R), 5'-GATCATGACCGCCGTAGG (X1), and 5'-CATGAACTTGTCCCAGGCTT (X2), 35 cycles (92°C, 40 s; 58°C, 40 s; 72°C, 1 min) and 2% agarose gel electrophoresis.
Western blots and immunohistochemistry. Tissues were dissected from deeply anesthetized mice. Proximal and distal sciatic nerve segments of 4 mm length were dissected out, respectively, at the hip level and the knee level. Mouse spinal cords and sciatic nerves were homogenized in lysis buffer (150 mM NaCl, 50 mM Tris-HCl, 2 mM EDTA, 1% Triton X-100, 0.1% SDS, pH 7.4, and protease inhibitors). NSC34 cells were directly lysed in Laemli's buffer, subjected to SDS-PAGE, Western blotting, incubated with antibodies, and revealed with the ECL plus system (GE Healthcare, Little Chalfont, UK). Western blots were scanned and analyzed by densitometry (NIH ImageJ). For immunohistochemistry, deeply anesthetized mice were perfused with 4% paraformaldehyde, and spinal cords, sciatic nerves, and phrenic nerves were dissected, postfixed overnight, and cryoprotected in 30% sucrose for 48 h. After tissue embedding, 14 µm transverse or 20 µm frontal sections of the spinal cord and 10 µm cross sections of nerves were cut on a cryostat and collected on glass slides. Sections were blocked, incubated overnight with primary antibodies, washed, incubated with fluorochrome-conjugated secondary antibodies, reacted with 0.1 µg/ml bisbenzimide, and mounted in Fluoromount.
Subcellular fractionation. Spinal cords or NSC34 cells were homogenized in buffer (50 mM Tris-HCl, pH 7.5, 2 mM EGTA, 2 mM EDTA, 5% sucrose, 0.1 mM DTT, and protease inhibitors) and centrifuged at 900 x g for 10 min at 4°C to remove nuclei and cell debris. The postnuclear supernatant was centrifuged for 1.5 h at 4°C and 60,000 rpm in a TLA-100 rotor (Beckman Coulter, Fullerton, CA) to obtain cytosol and crude membrane fractions. The membrane pellet was dissolved in homogenization buffer containing 0.5% Triton X-100 and incubated for 1 h on ice. Equal volumes of subcellular fractions were subjected to SDS-PAGE and processed as outlined above.
Retrograde labeling of motor neurons. Mice were anesthetized with Hypnorm/Dormicum (fentanyl at 0.5 mg/ml, fluanisone at 2.5 mg/ml, and midazolam at 1.25 mg/ml; 6 ml/kg body weight, s.c.). Under a stereomicroscope, a ventral incision was made on the right side of the neck, the cervical plexus was isolated, and the phrenic nerve was identified. The phrenic nerve was cut without opening the pleural cavity, and a piece of hemostatic sponge (Spongostan; Ferrosan, Soeborg, Denmark) 1 x 1 x 1 mm in size was soaked in 10% Fluoro-ruby (Chemicon) in Ringer's solution with 2% DMSO, and applied to the proximal stump. Labeling by dextran tracers is restricted to cut axons (Richmond et al., 1994
Fluorescent, light, and electron microscopy. Confocal microscopy was performed with upright or inverted LSM 510 microscopes (Zeiss, Oberkochen, Germany) using 63x, 40x, or 10x objectives. For light and electron microscopy, glutaraldehyde-fixed nerves and roots were postfixed with osmic tetroxide and embedded in epoxy resin. For light microscopy, cross sections 3 µm thick were stained with p-phenylenediamine, photographed with a 40x oil immersion objective, and printed to 1200 times. Thin cross sections for electron microscopy were stained with uranyl acetate and lead citrate. To facilitate identifying microtubules, the sections were tilted in the electron microscope (CM100; Philips, Eindhoven, The Netherlands) by means of a goniometer to obtain exact cross sections. The magnification of the microscope was calibrated against a replica of a diffraction grating (2160 lines/mm). With the aid of a digitizer tablet, all apparently intact myelinated axons were counted on light micrographs of the phrenic nerves, axonal areas were measured, and microtubules were counted on electron micrographs printed to
60,000 times. The investigator (H.S.) was blinded with respect to the genotype of the animals.
Expression plasmids and small interference RNAs. Expression vectors for GFP–TBCE, hemagglutinin–TBCE, and FLAG–TBCE were generated by subcloning mouse wild-type TBCE cDNA using pCAGGS–GFP (Jacquier et al., 2006
Cell cultures and in vitro assays. Motor neurons were prepared from embryonic day 12 spinal cords, electroporated with DNA plasmids and/or siRNAs, and cultured in the presence of the neurotrophic factors BDNF, CNTF, and GDNF (Raoul et al., 2002
For quantification of GFP–
Microtubule growth assays were performed as described by Ahmad and Baas (1995)
-tubulin to visualize microtubules and centrosomes, respectively. Images were obtained by confocal microscopy in sections of 2.5 µm optical thickness covering the centrosome using identical acquisition parameters. Mean ßIII-tubulin fluorescence and the length of microtubules emanating from the centrosome were measured using MetaMorph and NIH ImageJ software, respectively.
Statistical analyses. Experiments were performed in duplicate or triplicate and repeated at least once. Data were analyzed with Excel (Microsoft, Seattle, WA); statistical testing and linear regression analysis were performed with SigmaStat 3.1 (Systat, Evanston, IL). When data showed a Gaussian distribution, they were analyzed with Student's t test (two-tailed, unpaired); otherwise the Mann–Whitney U test was used.
Results
Retrograde progression of axonal microtubule loss in pmn mice
Homozygous pmn mice develop first signs of muscle atrophy and paresis at 2 weeks of age and die by respiratory failure 4 to 5 weeks later (Schmalbruch et al., 1991
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Figure 1. Axonal microtubules and tubulin levels in pmn mice. A, B, Electron micrographs showing entire cross sections through distal phrenic nerves from 15-d-old early symptomatic pmn mice and wild-type (wt) littermate mice. C, D, High-power electron micrographs from distal phrenic nerve axons at day 15. Microtubules (arrows) in pmn phrenic nerve axons are rarefied, whereas intermediate filaments are preserved. E, F, High-power electron micrographs from C4 ventral roots at day 15. G, H, High-power electron micrographs from C4 ventral roots at day 28. Scale bars: A, B, 1 µm; C–H, 0.5 µm. I, Diagram showing that axonal microtubule densities in pmn phrenic nerves mice are reduced by 61 and 56%, respectively, at the distal and intermediate level compared with those in wild-type nerves (***p < 0.0001, Student's t test). No significant microtubule loss is observed in cervical and lumbar ventral root motor axons of 15-d-old pmn mice. A total of 378 individual axon cross sections were analyzed. J, Diagram showing reduction of microtubule densities in C4 ventral roots of 28-d-old pmn mice (***p < 0.0001, Student's t test). K, Western blot analysis showing protein levels of ßIII-tubulin and ß-actin in lysates from lumbar spinal cord and proximal and distal sciatic nerves at day 15. Note the reduction of ßIII-tubulin in distal sciatic nerves of pmn mice.
In normal phrenic nerves, we counted a mean of 15.2 ± 2.3 microtubules/µm2 cross-sectional area of the distal axon (means of mean ± SD). In distal phrenic nerves of pmn mice, axonal microtubule densities were reduced to 6.0 ± 1.6 microtubules/µm2, corresponding to 39 ± 10% of normal (p < 0.0001) (Fig. 1C,D,I). A similar reduction in axonal microtubule density (44 ± 9% of normal; p < 0.0001) was found at the intermediate level (Fig. 1I). Interestingly however, C4 ventral roots from pmn mice displayed no significant reduction in axonal microtubule density (89 ± 5% of wild type) (Fig. 1E,F,I). Lumbar ventral roots that supply the most severely affected territories in pmn mice also showed normal axonal microtubule densities (97 ± 22% of wild type) (Fig. 1I). These findings were further supported by Western blot analysis of neuronal ßIII-tubulin levels in distal and proximal sciatic nerves and lumbar spinal cord of 15-d-old mice. In pmn mice, the ßIII-tubulin levels were significantly reduced in distal sciatic nerves but normal in proximal nerves and spinal cord (Fig. 1K).To analyze the temporal progression of microtubule loss in pmn mice, we studied C4 cervical ventral roots of 28-d-old pmn mice (Fig. 1G,H). At this advanced disease stage, microtubule densities were reduced to 40 ± 13% of normal (Fig. 1J). Axonal microtubule loss in pmn motor nerves thus first manifests distally and then progresses from distal to proximal, in parallel with the axonal dying back neuronopathy.
Consequences of microtubule loss on axon degeneration
We then investigated the requirement of microtubules for motor axon maintenance. To this purpose, we analyzed not only pmn and wild-type mice but also two lines of transgenic pmn mice complemented with wild-type TBCE (Martin et al., 2002
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Figure 2. Requirements of microtubules for axon maintenance. A, Electron micrographs of distal phrenic nerves show irregularly shaped myelin sheaths and myelin debris as signs of axonal atrophy and degeneration in 15-d-old pmn mice compared with wild-type littermate mice. Signs of axonal degeneration are attenuated in transgenic TBCEPA pmn mice and virtually absent in TBCEPC pmn mice. B, Diagram showing axonal microtubule densities in distal phrenic nerves of wild-type, pmn, TBCEPA pmn, and TBCEPC pmn mice. C, Diagram showing number of myelinated axons in the distal phrenic nerves of mice with the indicated genotypes. D, Histogram showing a close correlation between the number of myelinated fibers (y-axis) and axonal microtubule density (x-axis) in individual phrenic nerves (p < 0.001; , pmn;
, wild type;
, TBCEPA pmn;
, TBCEPA wild type;
, TBCEPC pmn;
, TBCEPC wild type. Scale bar, 10 µm.
TBCE accumulates at the Golgi apparatus of motor neurons
To investigate the role of TBCE in the maintenance of axonal microtubules, we studied its protein expression profile in the peripheral nervous system. In immunoblots of adult spinal cord extracts, our polyclonal antibody detected a single band of 59 kDa, corresponding to recombinant TBCE (Fig. 3A). On cervical spinal cord sections, TBCE was mainly expressed in ventral horn motor neurons and in neurons of superficial dorsal horn layers (Fig. 3B). To verify that TBCE is expressed in phrenic motor neurons in the cervical spinal cord, we used retrograde rhodamine–dextran labeling. We found that all of them expressed high levels of TBCE in their soma (Fig. 3C). Surprisingly, however, TBCE was barely detectable in axons, identified by neurofilament labeling (Fig. 3D) or genetic labeling (Fig. 3E) in Thy1–YFP line 16 mice (Feng et al., 2000
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Figure 3. TBCE accumulation at the Golgi apparatus of spinal motor neurons. A, Western blot analysis shows that a polyclonal antibody directed against murine TBCE detects a band of
In motor neurons, TBCE accumulated at discrete tubulovesicular structures surrounding the nucleus that were reminiscent of the Golgi apparatus (Fig. 3F–I). Double immunolabeling and confocal microscopic analysis confirmed a striking overlap (Fig. 3F,G) between TBCE and the two cis-Golgi markers GM130 (Nakamura et al., 1995Previous TBCE overexpression studies in HeLa cells had detected TBCE only in the cytoplasm (Bhamidipati et al., 2000
Golgi proteins can be membrane bound, like the Golgi matrix protein GM130 (Nakamura et al., 1995
TBCE is destabilized at the Golgi apparatus in pmn mice and is restored by transgenic TBCE complementation
To explore the molecular causes of microtubule loss in pmn mice, we analyzed whether the protein levels or subcellular localization of TBCE were modified in pmn motor neurons in vivo. Our previous in vitro studies had indicated that the pmn mutation alters the conformation and reduces the half-life of the TBCE protein (Martin et al., 2002
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Figure 4. Loss of TBCE expression at the Golgi apparatus of pmn mice and its restoration by transgenic TBCE complementation. A, B, Western blot analysis showing protein levels of TBCE and neurofilament-M (NF-M) in spinal cord lysates of wild-type (wt), pmn, TBCEPA pmn, and TBCEPC pmn mice at P15 (A) and P35 (B). C, Immunolabeling showing reduced TBCE expression in spinal cord motor neurons of pmn mice at P15. D, E, Immunolabeling showing TBCE protein expression in cervical (D) and lumbar (E) spinal cord motor neurons of wild type, pmn, TBCEPA pmn, and TBCEPC pmn mice at P15. Scale bars: C, 100 µm; D, 10 µm.
To determine the levels of TBCE protein required for motor axon maintenance, we analyzed the two lines of transgenic TBCE pmn mice. In these mice, wild-type TBCE is expressed under control of the neuron-specific NSE promoter (Forss-Petter et al., 1990Effects of TBCE depletion in motor neuron cultures
Microtubules are made of
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Figure 5. Role of TBCE in tubulin formation and axonal routing. A, TBCE depletion in NSC34 cells. Western blots showing total levels of TBCE,
In neurons, tubulins are mainly synthesized in the cell body (Eng et al., 1999Microtubule polymerization and axonal routing in pmn motor neurons
To test the consequences of the pmn mutation on microtubule polymerization, we examined pmn and wild-type motor neurons in culture. Motor neurons were purified from individual embryos, seeded, and incubated for 6 h with 10 µM nocodazole to depolymerize microtubules (Ahmad and Baas, 1995
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Figure 6. Microtubule polymerization and axonal tubulin routing in cultured pmn motor neurons. A, B, Images showing microtubule regrowth in wild-type (wt) and pmn motor neurons at 0, 1, and 30 min after nocodazole washout. Microtubules are labeled for ßIII-tubulin and centrosomes for
We next analyzed axonal tubulin routing in pmn motor neurons. Motor neurons were electroporated with GFP–The Golgi apparatus controls axonal tubulin routing in motor neurons
To test whether the Golgi apparatus is involved in axonal tubulin routing, we pharmacologically disrupted this organelle with BFA. BFA inhibits activation of ADP-ribosylation factors (Donaldson et al., 1992
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Figure 7. Effects of BFA-mediated Golgi disassembly on axonal tubulin routing in cultured motor neurons. A, Images of TBCE/GM130-immunostained NSC34 cells after mock treatment, BFA treatment (5 h), or BFA treatment and subsequent washout (30 min). BFA induces dispersal of GM130-stained Golgi elements and complete TBCE redistribution into the cytoplasm; the BFA effects are reversible. B, Western blot analysis of NSC34 cell lysates showing that BFA treatment does not affect the overall levels of TBCE,
To test the effects of Golgi disruption on axonal tubulin routing, we electroporated motor neurons with GFP–
Discussion
Subcellular origin of axonal degeneration
Axonal degeneration, whether of traumatic, toxic, or genetic origin, often manifests as axonal dying back: distal axons are affected first, and degeneration apparently progresses from distal to proximal (Cavanagh, 1964Retrograde microtubule loss in pmn mice
We here investigated how a missense mutation in TBCE causes axonal dying back in pmn mice. We show that in normal mice, TBCE is expressed in motor neuron cell bodies in which it accumulates at the cis-Golgi apparatus. In early symptomatic pmn mice, TBCE is destabilized and lost from this organelle. Microtubules are first lost in distal motor axons and only at end stage in proximal motor axons. This retrograde microtubule loss parallels the axonal dying back: at disease onset, the extent of microtubule loss in distal phrenic nerves correlates with the severity of axonal degeneration and the axonal loss. At end stage of disease, microtubules and axonal diameters (Schmalbruch et al., 1991) are also reduced in ventral roots. We further show that neuron-specific TBCE complementation restores TBCE levels in spinal motor neurons of pmn mice and inhibits microtubule loss, axonal degeneration, and clinical disease in a dose-dependent manner. These data indicate that destabilization of TBCE in motor neurons is responsible for the axonal dying back process in pmn mice.How can a defective tubulin chaperone cause axonal dying back?
Using cultured pmn motor neurons, we show that the pmn mutation compromises the routing of newly synthesized tubulin from the cell body to the distal axon and impedes the incorporation of tubulin into growing microtubules. In vivo analyses of early symptomatic pmn mice further demonstrate that neuronal ßIII-tubulin levels are reduced in distal sciatic nerves but normal in proximal nerves and corresponding lumbar spinal cord segments. Hoffman et al. (1992)What is the role of the Golgi apparatus in axonal tubulin routing?
Studies in cultured neurons have shown that axonal tubulins are mainly synthesized in the cell soma (Eng et al., 1999Are defects in tubulin chaperones also implicated in other forms of axonal degeneration?
Human TBCE deletions have been found in children with HRD (hypoparathyroidism, growth retardation, dysmorphism) syndrome (Parvari et al., 2002Therapeutic implications
In the past, pmn mice have been instrumental in developing new axonoprotective strategies. Crossing of pmn mice with WldS mice reduced axonal degeneration and extended the lifespan of pmn mice (Ferri et al., 2003
Footnotes
Received April 10, 2007; revised May 26, 2007; accepted June 21, 2007.This work was funded by grants from Inserm (Avenir Program), Conseil Général des Bouches du Rhône, Association Française contre les Myopathies, Fédération pour la Recherche sur le Cerveau, and the Amyotrophic Lateral Sclerosis Association. M.S. received a postdoctoral fellowship from Inserm and Deutsche Forschungsgemeinschaft (Grant DFG 1261/1-1). We thank M. Szatanek (Institut Pasteur, Paris, France) and S. Corby (Inserm, Marseille, France) for genotyping, M. Bjaerg (University of Copenhagen, Copenhagen, Denmark) for expert help in histology, and A. Andrieux and D. Job (Commissariat à l'Energie Atomique, Grenoble, France), F. Lotfi, C. Faivre-Sarrailh, and C. Raoul (Inserm, Marseille, France) for helpful discussions.
Correspondence should be addressed to Dr. Georg Haase, Institut de Neurobiologie de la Méditerranée, Equipe Avenir, 13288 Marseille cedex 09, France. Email: haase{at}inmed.univ-mrs.fr
Copyright © 2007 Society for Neuroscience 0270-6474/07/278779-11$15.00/0
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