Dendritic and Postsynaptic Protein Synthetic Machinery

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The Journal of Neuroscience, January 1, 1999, 19(1):168-179

Dendritic and Postsynaptic Protein Synthetic Machinery
Alejandra Gardiol, Claudia Racca, and Antoine Triller
Laboratoire de Biologie Cellulaire de la Synapse Normale et Pathologique, Institut National de la Santé et de la Recherche Médicale U497, Ecole Normale Supérieure, 75005 Paris, France

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

There is a growing body of evidence that local protein synthesis beneath synapses may provide a novel mechanism underlyingplastic phenomena. In vivo and in vitro biochemical data showthat dendrites can perform translation and glycosylation. Usingantibodies directed against the eukaryotic protein synthetic machinery,we sought to identify the structures implicated in nonperinucleartranslation, namely dendritic and postsynaptic protein synthesis.We performed a morphological and immunocytochemical analysis ofventromedial horn rat spinal cord neurons using both light andelectronmicroscopy.
We show at the cellular level that, in vivo, protein synthesis macrocomplexes (ribosomes and eIF-2) as well as the endomembranoussystem implicated in cotranslational and posttranslational modifications(endoplasmic reticulum and Golgi cisternae) penetrated some dendrites.Membrane-limited organelles of different shape and size are presentclose to the postsynaptic differentiations of most synapses, independentlyof their localization on the neuronal surface. We demonstrate(1) that some cisternae are immunoreactive for antibodies againstribosomal proteins and eIF-2, and (2) that markers of endoplasmicreticulum (BiP), intermediate compartment, and Golgi complex (rab1,CTR433, TGN38) label subsets of these subsynapticorganelles.
Therefore, these findings indicate that synapses are equipped with the essential elements required for the synthesis and insertionof a well folded and glycosylated transmembraneprotein.

Key words: glycine receptor; dendritic mRNA; spinal cord; subsynaptic cisternea; Golgi apparatus; endoplasmic reticulum; immunocytochemistry; confocal microscopy; electron microscopy

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Local protein synthesis from mRNAs transported to discrete subcellular locations is now viewed as an alternative way to targetproteins to specific microdomains. In neurons, many mRNAs arelocalized within dendrites (Steward et al., 1996; Steward, 1997).The presence of mRNAs encoding neurotransmitter receptors (Miyashiroet al., 1994; Racca et al., 1997a) raises questions about theirperisynaptic synthesis, posttranslational modifications, and subsequentinsertion at the postsynaptic membrane. The first morphologicalindications for a local synthesis derive from the visualizationof synapse-associated polyribosomes in dendrites (Bodian, 1965;Steward and Levy, 1982; Steward and Reeves, 1988; for review,see also Steward and Banker, 1992). It is currently believed thatthe endomembranous system involved in the secretory process, namelyrough endoplasmic reticulum (RER) and Golgi apparatus, can extendinto proximal portions of the dendritic shaft (Peters et al.,1991). Immunofluorescence studies have demonstrated the presenceof components of the translational machinery (Tiedge and Brosius,1996) and of elements of the endoplasmic reticulum (ER) and Golgiapparatus within some dendrites of cultured hippocampal and neocorticalneurons (De Camilli et al., 1986; Lowenstein et al., 1994; Krijnse-Lockeret al., 1995; Torre and Steward, 1996). In addition to these morphologicalfindings, biochemical studies have shown an incorporation of precursorsof both protein synthesis and glycosylation within dendrites (Raoand Steward, 1991; Torre and Steward, 1992, 1996). These experimentsindicate that nonsomatic compartments can perform all the synthesissteps of an integral membrane protein such as a neurotransmitterreceptor. However, there is still no evidence for an endomembranoussystem permitting juxtasynaptic synthesis and posttranslationalmodifications.

We have recently shown that glycine receptor $alpha$ subunit (GlyR $alpha$ ) mRNAs are located near synapses in close association withsubsynaptic cisternae (Racca et al., 1997a). The nature and functionof these membrane-limited structures are still speculative: theirassociation with mRNA under the synapse suggests that they participatein proteinsynthesis.

The aim of the present work was to characterize the dendritic and perisynaptic constituents potentially involved in the synthesisand glycosylation of synaptic proteins in vivo. We have now characterizedby immunocytochemistry, using both light microscopy (LM) and electronmicroscopy (EM), the distribution of the translational machineryand organelles of the secretory pathway, in neurons of the ventromedialhorn of rat spinal cord. We show with LM that initiation factors,ribosomes, ER, and Golgi complex penetrate dendrites. At the ultrastructurallevel we find that subsynaptic cisternae are: (1) decorated byanti-eIF-2 (initiation factor of the translation) immunoreactivity(IR) and present immunocytochemical characteristics of RER (anti-ribosomalP proteins, ribosomes; and BiP, ER chaperone); (2) surroundedby rab1 (ER to Golgi traffic) immunoreactivity; and (3) labeledwith CTR433 (medial Golgi) and anti-TGN38 (trans-Golgi) antibodies.These data indicate that membrane-limited elements located nearsynapses may have different functional characteristics. We postulatethat they form a complex subsynaptic apparatus involved in thelocal synthesis, glycosylation, and insertion of proteins in thesynaptic plasmamembrane.

Some of the results have been presented in abstract form (Gardiol et al., 1997).

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Several antibodies (Table 1) directed against the protein synthetic machinery including the organelles were used for LM andEM.


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Table 1. Antibodies used to characterize molecular complexes and organelles involved in protein synthesis

Tissue preparation. Adult Sprague Dawley female rats (150-170 gm; Janvier, France) were deeply anesthetized with sodium pentobarbital(60 mg/kg body weight, i.p.) and perfused intracardially witheither 4% paraformaldehyde (PFA) in 0.1 M PBS, pH 7.2, for LMexperiments and in situ hybridization (ISH) or 4% PFA and 0.1%glutaraldehyde in PBS followed by 4% PFA in PBS for EM immunocytochemistry.Spinal cords were removed and post-fixed overnight at 4°C in 4%PFA in PBS. Vibratome sections were collected in cold PBS andprocessed as described for each specificprotocol.

Fluorescent immunocytochemistry. Vibratome sections (50 µm) were incubated for 20 min in 50 mM NH₄Cl in PBS to quench thefree aldehyde groups. After PBS rinses (3 × 10 min), sectionswere preincubated for 10 min in 0.1% Triton X-100 and 0.1% bovinegelatin in PBS. Primary antibodies (Table 1) were incubated inthe same buffer overnight at 4°C. Sections were then rinsed inPBS (4 × 10 min) and incubated for 2 hr at room temperature withfluorescent secondary antibodies (1:500 in 0.1% bovine gelatinin PBS): carboxymethyl indocyanine (Cy3)-goat anti-mouse or anti-rabbitIgG (Jackson ImmunoResearch, West Grove, PA) or fluorescein isothiocyanate(FITC)-goat anti-human IgG (Jackson ImmunoResearch), dependingon the primary antibody host. Incubations were followed by PBSwashes (4 × 10 min). Finally, sections were mounted on slideswith Vectashield (Vector Laboratories, Burlingame, CA) and observedwith (1) a Leica epiluorescent microscope and images acquiredusing a Hamamatsu CCD camera or (2) a Molecular Dynamics confocallaser scanning microscope. In these and following experiments,the background noise was reduced by applying a Gaussian filterto the confocal optical sections. Omission of any primary antibodyor any single step in the development of fluorescent immunocytochemistryresulted in no labeling of anycells.

Double immunocytochemistry. Fifty micrometer sections were treated and permeabilized as described above for single immunocytochemistry.Double-immunolabelings were performed by incubating sections,overnight at 4°C, in presence of (1) mouse anti-BiP and rabbitanti-TGN38, (2) mouse CTR433 and rabbit anti-TGN38, (3) rabbitanti-TGN38 and mouse anti-synaptophysin, or (4) mouse CTR433 andrabbit anti-synapsin. The antibodies were diluted in the samebuffer as above (for concentrations, see Table 1). The followingday, sections were rinsed in PBS (4 × 10 min). Primary antibodieswere detected with the following combinations: Cy3-goat anti-rabbitIgG antibody (1:500) and FITC-goat anti-mouse IgG antibody (1:500)in PBS, 2 hr at room temperature; or FITC-goat anti-rabbit IgGantibody (1:500) and Cy3-goat anti-mouse IgG antibody (1:500)in PBS, 2 hr at room temperature. All of these secondary antibodieswere from JacksonImmunoResearch.

After washes in PBS (4 × 10 min), sections were mounted on slides with Vectashield (Vector Laboratories) and observed witha Leica confocal laser scanning microscope equipped with appropriatefilters for simultaneous detection of FITC and Cy3 fluorochromes.Controls included the independent omission of each single majorstep of the immunocytochemistry protocol, one at atime.

Fluorescent nonradioactive in situ hybridization and immunocytochemistry. The GlyR $alpha$ 2 oligonucleotide probe (residues 1682-1726;Kuhse et al., 1990; Malosio et al., 1991) has been described previously(Malosio et al., 1991; Racca et al., 1997a). ISH was as previouslydescribed by Racca et al. (1997a). Briefly, spinal cord, 30 µmsections were permeabilized with 0.1% Triton X-100 in PBS. Thefree-floating sections were pretreated for 3 hr at 42°C with prehybridizationbuffer (4× SSC buffer, 1× Denhardt's solution, and 10 µg/ml yeasttRNA), and then hybridized overnight at 42°C in hybridizationbuffer (50% formamide, 600 mM NaCl, 80 mM Tris-HCl, pH 7.5, 4mM EDTA, and 10 µg/ml yeast tRNA) containing 10 nM 3'end digoxigenin(DIG)-labeled oligonucleotides as previously described (Trembleauet al., 1994). The following day, sections were rinsed in 2× SSCand 1× SSC for 1 hr each, and the high stringency wash was in0.1× SSC at 42°C for 50 min. Detection of mRNAs and BiP was contemporaneouslycarried using (1) sheep anti-DIG antibody (Boehringer Mannheim,Indianapolis, IN; 1:1000 in 100 mM Tris-HCl, pH 7.5, 150 mM NaCl,2% BSA, and 0.3% Triton X-100, overnight at 4°C) and Cy3-donkeyanti-sheep IgG antibody (Jackson ImmunoResearch; 1:800 in PBS-1%BSA, 2 hr at room temperature) for ISH; and (2) anti-BiP antibody(1:200 in 100 mM Tris-HCl, pH 7.5, 150 mM NaCl, 2% BSA, and 0.3%Triton X-100, overnight at 4°C) followed by biotinylated rabbitanti-mouse IgG (Jackson ImmunoResearch; 1:500 in PBS, 2 hr atroom temperature) and FITC-streptavidin (Jackson ImmunoResearch,1:200 in PBS, 3 hr at room temperature) for BiPdetection.

Each incubation was followed by washes in PBS (3 × 10 min). Finally, sections were mounted on slides with Vectashield (VectorLaboratories) and observed with a Leica confocal laser scanningmicroscope equipped with appropriate filters for simultaneousdetection of FITC and Cy3 fluorochromes. Sense and random oligonucleotideprobes and omission of any oligonucleotides or primary antibodyor any single step in the development of fluorescent ISH and immunocytochemistryresulted in no labeling of anycells.

Pre-embedding immunogold electron microscopy. Vibratome sections (100 µm) were treated for 20 min with 50 mM NH₄Cl in PBSand preincubated in 0.1% bovine gelatin in PBS (3 hr). Then, sectionswere incubated in primary antibodies: (1) mouse anti-BiP; (2)human anti-ribosomal P proteins; (3) rabbit anti-eIF-2 $beta$ ; (4) rabbitanti-Rab1; (5) mouse CTR433; and (6) rabbit anti-TGN38 (see Table1 for dilutions and references) diluted in 0.05% Triton X-100and 0.1% bovine gelatin in PBS, at 4°C, 48hr.

Sections were rinsed in PBS (3 × 10 min), post-fixed for 5 min in 4% PFA in PBS, rinsed again, and incubated with gold-conjugatedsecondary antibodies (goat anti-rabbit, goat anti-human, goatanti-mouse, 1:50-1:100 depending on batch; Nanoprobes, Stony Brook,NY) for 24 hr in 0.1% fish gelatin (Sigma, St. Louis, MO) in PBSat 4°C. The following day sections were rinsed in 0.1% fish gelatin-PBS(3 × 10 min), PBS (1 × 10 min), then post-fixed in 1% glutaraldehydein PBS (5 min). After PBS washes (3 × 10 min), sections were rinsedseveral times in distilled water. Silver-enhancement (HQS kit;Nanoprobes) was performed in the dark for 5-7 min and stoppedby several rinses in cold distilled water. A gold-toning procedure(Trembleau et al., 1994) was used to protect silver particlesagainst osmium displacement. After PBS rinses (2 × 10 min), sectionswere osmicated, dehydrated, and flat-embedded in Araldite resin.Ultrathin sections of ventromedial spinal cord laminae (70-90nm) were countercolored with uranyl acetate and lead citrate andvisualized with a Jeol CX-II transmission electron microscopeat 80kV.

Pre-embedding immunoperoxidase electron microscopy. Sections were pretreated as described above and incubated in anti-BiPor anti-TGN38 (see Table 1 for dilutions and references) dilutedin 0.05% Triton X-100 and 0.1% bovine gelatin in PBS, at 4°C,for 48 hr. Subsequently, sections were rinsed in PBS (3 × 10 min),incubated in the biotinylated antibodies, goat anti-mouse IgG(Sigma), or goat anti-rabbit (Vector Laboratories, 2 hr at roomtemperature, 1:200 in PBS 1% BSA), and finally with avidin-biotinperoxidase complex for 1 hr at room temperature (ABC Elite kit;Vector Laboratories, 1:400 in PBS). After rinses with 50 mM Tris-HCl,pH 7.5 (3 × 5 min), the peroxidase was revealed by incubatingthe sections in 3,3'-diaminobenzidine tetrachloride (DAB) andhydrogen peroxide (Sigma-Fast; Sigma). The reacted sections wererinsed in PBS (3 × 10 min), osmicated, embedded, and processedfor EM as described above. Measurements for morphometrical analysiswere performed on micrographs at a final magnification of 18000×.

  RESULTS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

We have analyzed the distribution of components of the protein synthesis and posttranslational modification machineries inneurons of the ventromedial portion of adult rat cervical spinalcord by immunocytochemistry at both the LM and EM levels. We focusedon the distribution of markers of organelles (RER, intermediatecompartment and Golgi apparatus) and on one marker of a memberof the macromolecular complexes involved in the initiation oftranslation (eIF-2), as well as on the P proteins ofribosomes.

Organelles and macromolecular complexes in somata and dendrites

BiP, ribosomal P proteins, eIF-2
The immunoglobulin-binding protein BiP is a chaperone protein bearing a KDEL signal thus residing in the ER (Haas and Wabl,1983; Bole et al., 1986; Villa et al., 1991; Gething and Sambrook,1992). Using a monoclonal antibody against BiP and digitalizedLM microscopy we showed an intense discontinuous immunofluorescencesignal within somata and dendrites (Fig. 1A₁, confocal;inset, CCD camera). The nucleoplasm of neurons was devoid of fluorescence,but the nuclear envelope was strongly labeled. The intense blob-shapedsomatic staining likely corresponds to the Nissl bodies aroundthe nucleus (Fig. 1A₁). Within dendrites these fluorescentblobs (Fig. 1A₂, crossed arrow) were less numerous. Furthermore,smaller sparse spots, often elongated, could be detected alongdendrites, where the total signal was lower (Fig. 1A₂,arrows). These small fluorescent spots probably correspond tocisternal elements scattered throughout the dendroplasm, includingthose under the border of the neurite most likely correspondingto the subsynaptic ER (see EM below).

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Figure 1. Somatic and dendritic distribution of BiP-, ribosomal P protein-, eIF-2 $beta$ -, CTR433-, and TGN38-IRs. A₁, A₂, Discontinuous distribution of BiP-IR in the soma and dendrites. The IR can form blobs (crossed arrows) or elongated structures (arrows). A₂, Higher magnification of the box in A₁. Note that in the nonconfocal image (A₁, inset) the IR fills the dendrite. B₁, B₂, Distribution of ribosomal P protein-IR with intense staining forming blocks (arrows) within a weaker staining (double-crossed arrows). The ribosomal P protein-IR tends to accumulate at branch points (arrowhead). C₁, C₂, eIF-2 $beta$ -IR is present throughout the somatodendritic compartment with local accumulations (arrows) within dendrites. D₁, Discontinous rab1-IR in a dendrite. D₂, Dendritic extension of CTR433-IR thread (arrows) connected with the somatic network. D₃, Dendritic extension of TGN38-IR thread (arrow) extending after the first branch point (arrowheads) and connected with the somatic network. In all cases, nuclei were devoid of labeling. A₁, A₂, B₁, B₂, C₁, C₂, and D₁ are confocal sections. D₂ and D₃ are maximum intensity projections obtained from series of confocal sections. The inset in A₁ is a CCD camera image. De, Dendrites; n, nucleus; s, soma. Scale bars, A_1-2: A₁, 20 µm; inset, 30 µm; A₂, 6 µm; B_1-2: B₁, 20 µm; B₂, 28 µm; C_1-2: C₁, C₂, 20 µm; D_1-3: D₁, 29 µm; D₂, D₃, 20 µm.

A human serum with anti-ribosomal activity obtained from a systemic lupus erythematous patient was used to localize ribosomes.It targets three ribosomal phosphoproteins (P0, P1, and P2; Elkonet al., 1985, 1986). Confocal microscopy revealed blocks of stainingwithin somatic cytosol (Fig. 1B_1,2). This heavy labelingin the perikarya and initial portions of dendrites likely correspondsto ribosomes associated with cisternae of the Nissl bodies. Thedendritic signal was more discontinuous with triangular-shapedaccumulation of ribosomes at branch points (Fig. 1B₂)and at discrete sites under the margin of dendrites (Fig. 1B₁).Occasionally, we observed a faint fluorescence signal underscoringthe dendritic border (Fig. 1B_1,2).
The association of initiation factors with the ribosomal subunits is a key event in the regulation of eukaryote protein translationrate (Rhoads, 1993). We used an antibody against eIF-2 $beta$ (Bommeret al., 1988), one of the subunits of the initiation factor-2(eIF-2). The heaviest signal was present in the soma as brightpunctiform staining (Fig. 1C₁). An intense dot-like eIF-2 $beta$ staining was also found over dendrites. These spots tended toaccumulate at discrete sites with no visible morphological features(Fig. 1C₂). As for ribosomal P proteins, the nuclei ofeIF-2-positive cells were devoid oflabeling.

Rab1, CTR, TGN38
We used several markers to analyze the distribution of the Golgi apparatus: rab1 (Saraste et al., 1995) for the compartmentbetween the ER and the Golgi apparatus, including the cis-sideof it, CTR 433 (Jasmin et al.,1989) for the medial cisternae,and anti-TGN38 (Wilde et al., 1992) for the trans-most Golgi cisternaeand trans-Golgi network. The antibody against rab1 recognizesa small G-protein involved in the traffic between the ER and theGolgi apparatus. The CTR433 antibody recognizes an epitope ofunknown function, whereas that against TGN38 recognizes a structuralprotein involved in the budding at the trans-side of the Golgicomplex (Stanley and Howell, 1993). With the anti-rab1, smallstructures were labeled over somata and dendrites (Fig. 1D₁).For the medial and trans-Golgi markers, the labeling formed athread-shaped network enclosing the nucleus (Fig. 1D_2,3).In the initial portion of dendrites, the threads assumed a moreparallel distribution before penetrating the shaft. The labelingextended into dendrites sometimes as far as the second branchingpoint (Fig. 1D₃). The dendritic Golgi network was composedof a single tubule or of a few tubules running parallel, alongthe central core (see also Fig. 2D_1-4). As seenon projections of confocal sections (Fig. 1D_2,3), thedendritic network in continuity with the somatic one was presentonly in few dendrites issuing from a given soma. Quantificationsfor TGN38-IR indicated that in 34, 40, 22, 3, and 1% of neurons(n = 469) the Golgi-IR network penetrated one, two, three, four,and five dendrites, respectively. The number of dendrites containingGolgi elements was certainly underestimated because we could nottake into account the presence of small and discontinuous structuresthat could only be detected with high-resolution confocal microscopy(Fig. 2B_1,2, see De1) and were shown to be postsynapticwith EM (see Fig. 4)

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Figure 2. Spatial relationships of elements of the synthetic machinery. A₁, A₂, ISH signal (A₂, red, double-crossed arrows) corresponding to GlyR $alpha$ 2 mRNA is partially colocalized (A₂, yellow, arrows) with the BiP-IR (A₂, green, crossed arrow) associated with the ER. Note that a glial cell (A₁, G) presents only BiP-IR. A₁ and A₂, Low and high magnifications, respectively. B₁, B₂, TGN38- (red) and BiP- (green) IRs. One dendrite (De₂) displays a central thread (asterisk) surrounded by discontinuous TGN38-IR elements (arrows). Another dendrite (De₁) exhibits globular TGN38-IR but not thread-like IR. Note that the BiP-IR (crossed arrow) does not colocalize with TGN38-IR. C₁-C₃, CTR-IRs (red, arrows) and TGN38-IRs (green, crossed arrows) are present within the same dendrites and extend over the first branch point (arrowheads). The yellow color corresponds to superposition of fluorescent signal within the thickness of the confocal sections. D₁-D₄, Relationship between Golgi markers (red) and synaptic boutons (green). The main Golgi thread (asterisks) is located in the center of the dendrites. Some elements immunopositive for Golgi markers (arrows) are in front of synaptic boutons (arrowheads). Anti-TGN38/anti-synaptophysin and CTR433/anti-synapsin double-labelings are shown in D₁ and D₂ and D₃ and D₄, respectively. D₄ is a high magnification of the dendrite in D₃. A-D are color-coded pairs of confocal sections. For all antibodies, nuclei were devoid of labeling. De, Dendrites; n, nucleus; s, soma; G, glia. Scale bars, A_1-2: A₁, 12 µm; A₂, 5 µm; B_1-2: B₁, 14 µm; B₂, 5 µm; C_1-3: C₁, 20 µm; C₂, 12 µm; C₃, 13 µm; D_1-4: D₁, 17 µm; D₂, 6 µm; D₃, 21 µm; D₄, 7 µm.

Spatial relationship of markers of the synthetic machinery within the somatodendritic compartment

GlyR $alpha$ 2 subunit mRNA and BiP-positive compartments
In a previous study, we showed that GlyR $alpha$ 1 and $alpha$ 2 subunit mRNAs were present in the somatodendritic compartment of neuronsof the rat spinal cord (Racca et al., 1997a, 1998). These mRNAswere found to be partially associated with cisternae, beneathsynapses (Racca et al., 1997a). Therefore, we performed double-labelingexperiments for GlyR $alpha$ 2 mRNA and BiP. We focused on GlyR $alpha$ 2 mRNAlocalization because GlyR $alpha$ 2 and $alpha$ 1 mRNAs have the same distributionpattern (Racca et al., 1997a, 1998). As shown in confocal sectionsof double-labeling experiments (Fig. 2A_1,2), the ISHsignal (red) and the immunolabeling for BiP (green) were detectedin somata and dendrites. In somata and dendrites, some spots displayedthe two IRs (yellow). In dendrites, these yellow spots were foundmainly at the border of dendrites (Fig. 2A₂). GlyR $alpha$ 2mRNA-spots (red) not associated with BiP-labeling likely correspondto transport granules of mRNA (Racca et al., 1997a). Moreover,in dendrites, high-resolution confocal microscopy revealed thatGlyR $alpha$ 2 mRNA and P ribosomal antigen are colocalized (Racca etal., 1997b).

BiP-positive compartments and TGN cisternae
The spatial relationship between the ER and the Golgi complex, particularly within dendrites, was investigated in double-immunofluorescenceexperiments (Fig. 2B_1,2) using anti-TGN38 (red) and anti-BiP(green) antibodies. As expected from single-labeling experiments,BiP and TGN38-IRs were detected in somata and dendrites (Fig.2B₁). In dendrites at higher magnification, small TGN38-IRspots (Fig. 2B₂) were detected at the border of the dendrite.They were not continuous with the centrally located apparatus.In most dendrites these small TGN38-IR spots were detected evenin the absence of central labeling (Fig. 2B_1,2, De1).High-resolution confocal microscopy observations (Fig. 2B₂)showed that BiP- and TGN38-IRs were notcolocalized.

Golgi complex
Double-labeling experiments with CTR433-TGN38, CTR433-synapsin, and TGN38-synaptophysin couples of antibodies were performedto define the distribution of the constitutive elements of theGolgi complex. Synapsin and synaptophysin are both markers ofsynaptic terminals (Bloom et al., 1979; De Camilli et al., 1983;Wiedenmann and Franke, 1985). We observed that CTR433- and TGN38-IRswere present within the same dendritic shafts (Fig. 2C_1-3;CTR433, red; TGN38, green). In confocal longitudinal sectionsof dendrites double-labeled for TGN38 and synaptophysin (Fig.2D_1,2, red and green, respectively) or CTR433 and synapsin(Fig. 2D_3,4, red and green, respectively), Golgi compartmentswere mainly localized centrally with respect to the plasma membrane,delineated by green synaptic boutons. At higher magnification(Fig. 2D₂,D₄), we observed some punctated elementsclose to synaptic boutons, beside the central thread of the Golgiapparatus. These little elements were observed with CTR433 aswell as with the anti-TGN38 antibody, independently of the presenceof the centralthread.

Ultrastructural characterization of subsynaptic cisternae

BiP inside, ribosomal P proteins outside, eIF-2 around
As expected from immunofluorescence experiments, BiP signal strongly labeled the lumenal side of the nuclear envelope (Fig.3A₁). Cisternae of the smooth endoplasmic reticulum (SER)and RER were strongly labeled (Fig. 3A₁). Bip-IR wasalso detected in vesicular-shaped elements scattered within theperikaryon. In dendrites, cisternae of different shape and sizewere observed in the most central part (Fig. 3A₂). Inaddition, BiP-IR cisternae were often seen in front of presynapticboutons that could be filled with pleiomorphic (Fig. 3A_3,4)or round vesicles (data not shown). The BiP-positive elementsprobably corresponded to the fluorescent spots observed throughoutthe dendritic profiles in confocal sections. Nucleoplasm, Golgiapparatus, mitochondria, and multivesicular bodies in the somatodendriticcompartment were unlabeled. Terminal boutons were always devoidof staining.

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Figure 3. Ultrastructural distribution of elements of the protein synthetic machinery. A₁-A₄, BiP-IR is present in cisternae. A₁, Presence of IR signal in the nuclear envelope (double arrowheads), in cisternae (arrows), and in vesicular elements (arrowheads). A₂, Within dendrites gold particles are present within membrane-bounded organelles in the center (crossed arrow) and close to the plasma membrane (arrow). A₃, A₄, BiP-IR within cisternae (arrows) in front of synaptic boutons. B₁-B₃, Ribosomal P protein-IR can be either associated with cisternae (arrows) or free (arrowheads). B₂ is a higher magnification of b in B₁. B₃, Example from another dendrite. C₁, C₂, Association of eIF-2 $beta$ -IR with postsynaptic cisternae (arrows). Note the presence of coated elements (double-crossed arrow) in the vicinity of labeled cisternae. In all micrographs, Golgi stacks (asterisks), mitochondria, and nucleoplasm (n) are devoid of labeling. Scale bar: A₁, A₂, 1.5 µm; A₃, A₄, 1.1 µm; B₁, 1.9 µm; B₂, B₃, C₁, C₂, 40 µm.

Ribosomes were detected using the antibody directed against ribosomal P proteins. In the soma (data not shown) and withindendrites (Fig. 3B₁) the immunogold signal was foundin the cytosol, probably associated with free ribosomes, as wellas decorating the endoplasmic membranes. More distally, in dendrites,the signal tended to predominate along the plasma membrane. RibosomalP protein-decorated membranous cisternae were frequently locatednear synapses and surrounded by clouds of gold particles (Fig.3B_2,3). In addition, nonmembrane-associated particleswere found over weakly electron-dense material, which likely correspondedto free ribosomes. Accretions of ribosomal P protein-IR were alsofound at dendritic branching points where clusters of Nissl bodiesalso accumulate (data not shown). As expected, axoplasm and Golgicomplexes were devoid oflabeling.
The eIF-2-IR was also present within the somatodendritic compartment as well as near synapses. As for ribosomal P protein-labeling,somatic staining for eIF-2 was observed associated or not withthe RER membranes (data not shown). Beneath postsynaptic differentiationsthe immunogold particles decorated cisternal- and vesicular-shapedcomponents (Fig. 3C_1,2). In some instances, they couldalso be detected in a nonmembrane-associated configuration inthe vicinity of these cisternae (data notshown).

Golgi markers decorate subsynaptic cisternae
Because ER markers were present in the vicinity of synapses, we analyzed the distribution of rab1, a marker of early compartmentsof the secretory pathway, namely the intermediate compartmentand the cis-Golgi cisternae (Saraste et al., 1995). In somata,rab1-associated gold particles were found at the cytoplasmic sideof the fenestrated cis-Golgi cisternae (Fig. 4A₁). TheIR signal was also found associated with more spherical elementsscattered in cytosol and likely belonging to the intermediatecompartment. Nissl bodies were unlabeled. Under synapses, thesignal was mainly associated with cisternous organelles of varioussizes and shapes (Fig. 4A_2-4).

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Figure 4. Dendritic and subsynaptic distribution of the postranslational modification machinery. A₁-A₄, rab1-associated gold particles (arrowheads) are found at the cis-side of the Golgi apparatus in the soma (A₁) and associated with cisternae (arrows) in front of synaptic boutons (A₂-A₄). B₁, B₂, CTR433-IR labels the lumen of central cisternae (between arrowheads) of a Golgi apparatus within a dendrite. A small vesicular element (arrow) adjacent to a synaptic complex is labeled (B₂). C₁-C₃, TGN38-IR stains the lumen of external cisternae of the Golgi apparatus (between arrowheads) and cisternae in front of boutons (arrows). Scale bar: A₁, 1 µm; A₂-A₄, B₂, C₂, C₃, 0.5 µm; B₁, 1.2 µm; C₁, 0.8 µm.

CTR433-IR was found within cisternae in the middle of somatic Golgi complexes (data not shown). In the central part of a fewdendrites we also observed profiles of Golgi complexes labeledcentrally with CTR433-associated gold particles (Fig. 4B₁).These profiles were infrequent and might correspond to the threadthat penetrates a few dendrites seen in the immunofluorescentsections (see above). Regardless of the presence of these Golgistacks, cisternae positive for CTR433 were observed in the vicinityof postsynaptic differentiations (Fig. 4B₂).
Within perikarya, gold particles associated with anti-TGN38 antibodies labeled the lumenal side of cisternae located at theedge of Golgi stacks (data not shown). Thus, we assumed that theycorrespond to the trans-most side of the Golgi apparatus. In addition,vesicular elements located near these cisternae and scatteredthroughout the cytoplasm, were immunolabeled. As for the CTR433-IR,TGN38-IR Golgi apparatus were found in few dendrites (exemplifiedin Fig. 4C₁). In the dendrites as well as in the soma,the trans-cisternae were labeled by TGN38-associated particles.Cisternae labeled with TGN38-IR were observed close to the plasmalemmaand quite often underneath synapses (Figs. 4C_1-3).The gold-toned particles associated with subsynaptic cisternaeoften overflowed the boundaries of the organelle. This was probablycaused by the permeabilization and silver-enhancement-gold-toningprocedures.

Morphometrical analysis of BiP-IR and TGN38-IR

The BiP-IR (Fig. 5A) and TGN38-IR (Fig. 5B) were detected even in the smallest dendrites. In some dendrites, the subsynapticorganelles were clearly decorated by the product of the enzymaticreaction, however in most cases, the electron dense reaction productoverflowed over the entire dendritic transversal section. Thisprobably resulted from secondary translocation of oxidized DAB(Fig. 5A,B).

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Figure 5. Morphometrical analysis of BiP- and TGN38-IR. A, B, BiP- and TGN38-IR profiles connected by synaptic boutons. C, Histograms of mean diameters ( $radical$ Ll) of dendritic cross sections obtained from two animals and corresponding to the general population (n = 1673) and BiP-IR (n = 322) or TGN38-IR profiles (n = 393). Values were grouped in classes of mean diameters with a bin of 0.3 µm between 0 and 3.3 µm, the last class (*) represents diameters >3.3 µm. Scale bar: A, B, 0.5 µm.

The extension of BiP- and TGN38-IR was indirectly evaluated by comparing the distribution of the diameter of IR profiles tothat of the general population of dendrites. This approach assumesthat transversal sections of dendrites are of smaller diametereither at distance from the soma or when they are obtained fromdendrites of higher order. This notion, which relies on the taperedstructure of dendrites, is only statistical (Peters et al., 1991;Chen and Wolpaw, 1994). Measurements of the mean diameter of dendritesseen in cross sections (using the formula D = $radical$ Ll, where L andl are the large and small diameter, respectively) gave 1.23 µm± 0.05 (mean ± SEM, n = 322), 0.64 µm ± 0.028 (n = 393), and 0.55µm ± 0.016 (n = 1673) for BiP-IR, TGN38-IR, and the general populationof dendrites, respectively. The latter corresponds to all crosssections of dendrites (labeled and unlabeled, n = 871 for BiP;n = 802 for TGN38) present in micrographs for immunoenzymaticdetection. The general shapes of histograms corresponding to BiP-and TGN38-IRs were comparable to that of the whole population(Fig. 5C). Stained profiles were found in all classes, includingthose accounting for dendrites of smaller diameter. This suggeststhat at least in some cases the synthesis apparatus could extendto the dendritic extremities. Interestingly, we found that thefrequency of observation of TGN38-IR in small profiles (mean diameter,<0.6) was higher that for the BiP-IR, suggesting that the Golgiapparatus extend further away than thereticulum.

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The requirement of protein synthesis during long-lasting forms of synaptic plasticity has highlighted the functional advantagefor a single synapse of accomplishing locally the renewal of itsprotein set (Kang and Schuman, 1996; Mayford et al., 1996; Martinet al., 1997; Schuman, 1997). Until now, apart from ribosomes,the ultrastructural complement for this mechanism was lacking.The notion of synaptic autonomy (Steward and Levy, 1982; Martinet al., 1997) is supported by our demonstration of the presenceof the protein synthetic machinery in the vicinity of the postsynapticdifferentiation.

Dendritic localization of the protein synthetic apparatus and the neuronal endomembranous complex

The subcellular distributions of RER and Golgi apparatus have been described in vivo in many neuronal types and were shownto extend into dendrites (Broadwell and Cataldo 1983; Peters etal., 1991). The distributions of markers of synthetic machineryhave been studied by immunocytochemistry in neurons kept in vitro(De Camilli et al., 1986; Lowenstein et al., 1994; Krijnse-Lockeret al., 1995; Tiedge and Brosius, 1996). Interestingly, the distributionof the constitutive elements of the machinery seems to dependon cell types and experimental procedures. Our work is the firstthat combines in vivo confocal and electron microscopic immunocytochemistryto approach the organization of the synthetic apparatus withinneurons maintained in their actual network. We have focused ouranalysis on neurons of the ventromedial laminae of the rat spinalcord, where we previously found a dendritic and postsynaptic localizationof GlyR $alpha$ subunits mRNAs (Racca et al., 1997a, 1998). We foundthat ribosomes, an initiation factor of protein synthesis (eIF-2),as well as BiP, a chaperone residing in the ER, were somatodendriticallydistributed. Therefore, in spinal cord neurons, the distributionof ribosomal P proteins and eIF-2 IRs was comparable to that foundin cultured hippocampal neurons (Tiedge and Brosius, 1996). Ribophorin(Torre and Steward, 1996) was also detected in proximal to middendrites, whereas another ER marker (TRAP/SSR) was found in somataand proximal dendrites (Krijnse-Locker et al., 1995) and occasionallymore distally (Tiedge and Brosius, 1996). Our EM morphometricalanalysis suggests that ER extend over the whole length of somedendrites. The Golgi apparatus identified with antibodies againstTGN38 (trans-most cisternae and trans-Golgi network) and CTR433(medial cisternae) shows the same somatodendritic pattern. Othersfound that TGN38-IR Golgi tubules are confined to the cell bodies(Krijnse-Locker et al., 1995) or detected in proximal and, infrequently,in distal dendrites (Torre and Steward, 1996). Our EM measurementsindicate that TGN38 labeling could extend into distaldendrites.

Like other authors (Dotti and Simons 1990; Lowenstein et al., 1994; Torre and Steward, 1996), we found that the Golgi elementsconnected with the somatic ones penetrated only few dendrites(two or three in 96% of the neurons). The strongest dendriticER and mRNA signals were present within the principal dendriteswhere the Golgi apparatus had the classical thread-like structure.This association suggests that this distribution may have a physiologicalmeaning. In addition to this dendritic central thread-shaped Golgiconnected with its somatic counterpart, discontinuous punctateTGN38- and CTR433-IR elements were observed not only in the principaldendrite(s) but also in others. In double-labeling experiments(anti-TGN-38 and anti-synaptophysin; CTR433 and anti-synapsyn),these Golgi elements, defined by their immunoreactivities, werepresent under synapses. Therefore, the Golgi apparatus could displaya thread-like structure connected with the somatic network andpresent in few dendrites, or a vesicular structure present inmany more dendrites often in front of synaptic contacts. Yet theGolgi apparatus is a highly dynamic structure (Sciaky et al.,1997). In muscular cells, dramatic changes in Golgi distributionsare observed during synaptogenesis and denervation (Jasmin etal., 1989, 1995). We, therefore, suggest that the tubular-shapedGolgi apparatus could move into some dendrites in which high levelsof synthesis are required. The vesicular-shaped CTR433 and TGN38-IRstructures could then correspond to elements of the Golgi complexthat would have remained at specific sites after the withdrawalof the main thread-shaped Golgiapparatus.

Subsynaptic cisternae and receptor synthesis

Subsurface and hypolemmal cisternae have been described in several types of central neurons, including spinal neurons (Rosenbluth,1962; Bodian, 1965; Kaiserman-Abramof and Palay, 1969; Peterset al., 1991). The morphology and localization of these elementsvaries within and from one neuronal type to another. These morphologicaldifferences could be associated with different functions. Bodian(1965) was the first to postulate a "trophic" (protein synthesis)function for them. In the spinal cord, most of the postsynapticsites display a complex array of cisternae. We found in spinalcord neurons that some subsynaptic cisternae are BiP-positive.The presence of BiP indicates that these cisternae are compartmentswhere neosynthesized proteins can be properly translocated andfolded (Haas and Wabl, 1983; Bole et al., 1986; Gething and Sambrook,1992). We have also detected ribosomal P protein-IR around thesecisternae. The presence of pericisternal ribosomes and initiationfactors (both detected by immunocytochemistry) support the notionthat some of these cisternae correspond to RER and could achievethe synthesis of transmembrane proteins. Ribosomes and initiationfactors not associated with cisternae could participate in thesynthesis of cytosolic and perisynaptic proteins involved in othersynaptic functions for which the presence of the correspondingmRNAs was reported in dendrites (e.g., MAP2, Davis et al., 1987;Garner et al., 1988; the $alpha$ subunit of the calcium/calmodulin-dependentkinase, Burgin et al., 1990; Arc, Link et al., 1995, Lyford etal., 1995; for review, see Steward et al., 1996). Cisternae werealso labeled by markers of the medial-Golgi (CTR433) and the trans-Golginetwork and cisternae (anti-TGN38). Rab1, a member of the rabfamily involved in the routing between cisternae that synthesizeproteins and cis-Golgi, was also found near synapses. The questionremained whether or not the postsynaptic cisternae stained forthe various antibodies were distinct elements. It is generallyaccepted that the synthetic transport pathway for membrane proteinsis the same in all eukaryotes. It is composed of distinct compartments,and the vectorized routing passes sequentially from RER to Golgiand then to plasma membrane (Pelham and Munro, 1993). This generalscheme of organization probably also holds for the postsynapticsynthetic machinery. None of the antibodies labeled all of thepostsynaptic membrane-limited structures. Moreover, as seen withdouble immunofluorescence experiments, TGN38- and BiP-IRs werenot colocalized but rather juxtalocalized. This indicates thatsubsynaptic cisternae stained by each antibody were differententities. Therefore, we postulate that the collection of postsynapticcisternal elements form a local synthetic/secretion machineryconstituted by adjacent compartments with defined functions locatednearsynapses.

Glycosylation in dendrites

The presence of mRNAs encoding receptors in dendrites (Furuichi et al., 1993; Miyashiro et al., 1994; Racca et al., 1997a),has pointed to the requirement for machinery allowing translocationand glycosylation of the corresponding proteins. Autoradiographicanalysis of synaptosomes (Rao and Steward, 1991) and isolateddendrites (Torre and Steward, 1992) has shown an incorporationof radiolabeled amino acids, thus indicating translational activityperformed by nonsomatic compartments. Using the same system (i.e.,dendrites isolated from neuronal cultures), Torre and Steward(1996) have shown that dendrites may also undergo glycosylation.Indeed, they found that the percentage of dendrites incorporatingradiolabeled glycosylation precursors was greater than the percentageof dendrites immunopositive for Golgi markers. They conclude thatthis underestimation could be caused by either culture differencesor the existence of a population of dendrites exhibiting glycosylationactivity without detectable Golgi apparatus immunoreactivity.Our results support the latter hypothesis. The Golgi-like cisternaethat we found with a punctate fluorescent staining under synapseswere present in many dendrites where the thread-like Golgi apparatuscould not be detected. At the EM level, some of these elementscorrespond to cisternae that do not display the classical conformationof Golgi stacks. We hypothesize that the cisternae immunopositivefor these Golgi markers could be responsible for dendritic andsubsynapticglycosylation.

Conclusions

Long-term potentiation at single synapses in hippocampal slices has been shown to be dependent on exocytosis in the postsynapticcell (Lledo et al., 1998). This secretion-dependent plasticitycould result from (1) exocytosis of retrograde messengers or (2)delivery of receptor that could be stored and/or synthesized underthe synapse. The nature of the signal that could trigger theselocal modifications is unknown. Within dendrites some cisternaeare involved in the sequestration (Villa et al., 1991; Takei etal., 1992) and regulation of the cytosolic concentration (Llanoet al., 1994) of calcium. Local modifications of the concentrationof calcium, before or during its storage in subsynaptic cisternae(Pozzo-Miller et al., 1997), may be the first step in a signalingcascade leading to the insertion of newly synthesized molecules.After "activation" of synaptically localized silent mRNAs, theprotein synthesis of specific proteins may be restricted to thesingle previous-activated synapse. The cisternae that we havecharacterized and which are likely to be involved in local proteinsynthesis and insertion may be different from those involved incalcium storage (Pozzo-Miller et al., 1997). Therefore, the subpostsynapticregion may include a complex array of organelles ensuring thefunctional autonomy of thesynapse.

  FOOTNOTES

Received June 26, 1998; revised Oct. 15, 1998; accepted Oct. 15, 1998.

This work was supported by grants from Institut de Recherche sur la Moelle Epinière and from Direction des Recherches Etudeset Techniques (95-126). C.R. was supported by a European CommunityTraining and Mobility of Researchers Marie Curie Research Grantand A.G. by a Ministère de l'Education Nationale, de l'EnseignementSupérieur et de la Recherche Fellowship. We thank A. Dumoulin,M. T. Loones, A. Trembleau, and C. Vannier for their helpful comments,suggestions, and discussion. We also acknowledge C. Antony, U.Bommer, M. Bornens, P. De Camilli, K. Elkon, and B. Goud for generouslysupplyingantibodies.
Correspondence should be addressed to Antoine Triller, Laboratoire de Biologie Cellulaire de la Synapse Normale et Pathologique,Institut National de la Santé et de la Recherche Médicale U497,Ecole Normale Supérieure, 46 rue d'Ulm, F-75005 Paris,France.

Dr. Raccas's present address: Medical Research Council Anatomical Neuropharmacology Unit, Oxford University, Mansfield Road,Oxford OX1 3TH,UK.

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