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Previous Article | Next Article
The Journal of Neuroscience, December 15, 1999, 19(24):10694-10705
The Organization of the Golgi Complex and Microtubules in Skeletal Muscle Is Fiber Type-Dependent
Evelyn Ralston1, Zhuomei Lu1, and Thorkil Ploug2 1 Laboratory of Neurobiology, National Institute of Neurological Disorders and Stroke, National Institutes of Health, Bethesda, Maryland 20892-4062, and 2 Copenhagen Muscle Research Centre, Department of Medical Physiology, The Panum Institute, University of Copenhagen, Copenhagen, DK-2200 Denmark
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Skeletal muscle has a nonconventional Golgi complex (GC), the organization of which has been a subject of controversy in the past. We have now examined the distribution of the GC by immunofluorescence and immunogold electron microscopy in whole fibers from different rat muscles, both innervated and experimentally denervated. The total number of GC elements, small polarized stacks of cisternae, is quite similar in all fibers, but their intracellular distribution is fiber type-dependent. Thus, in slow-twitch, type I fibers, ~75% of all GC elements are located within 1 µm from the plasma membrane, and each nucleus is surrounded by a belt of GC elements. In contrast, in the fast-twitch type IIB fibers, most GC elements are in the fiber core, and most nuclei only have GC elements at their poles. Intermediate, type IIA fibers also have an intermediate distribution of GC elements. Interestingly, the distribution of microtubules, with which GC elements colocalize, is fiber type-dependent as well. At the neuromuscular junction, the distribution of GC elements and microtubules is independent of fiber type, and junctional nuclei are surrounded by GC elements in all fibers. After denervation of the hindlimb muscles, GC elements as well as microtubules converge toward a common pattern, that of the slow-twitch fibers, in all fibers. Our data suggest that innervation regulates the distribution of microtubules, which in turn organize the Golgi complex according to muscle fiber type.
Key words: acetylcholine receptor; endoplasmic reticulum; flexor digitorum brevis; Golgi complex; neuromuscular junction; red gastrocnemius; trans-Golgi network; tensor fascia latae
INTRODUCTION
During development, skeletal muscle fibers diversify into at least four major types (I, IIA, IIB, and IIX) based on the myosin heavy chain isoform they express. They also differ in their speed of contraction, type of metabolism, fatigue resistance, and other properties (Schiaffino and Reggiani, 1996
). Some aspects of this regulation are relatively well understood. For example, it is known that the expression of specific isoforms of several protein families (myosin heavy and light chains, troponins, Ca2+ ATPases) is regulated by activity at the level of transcription (for review, see Buonanno and Fields, 1999
There also are a number of observations regarding fiber type-dependent differences in subcellular organization of mitochondria (Gauthier and Padykula, 1966
In the present study, we asked whether the organization of the Golgi complex is fiber type-dependent. The GC is the strategic cell center for membrane protein trafficking. Its distribution in a giant cell such as a muscle fiber may determine the organization of the subcellular membrane systems. Skeletal muscle is one of several cell types that do not have a conventional GC. In undifferentiated myoblasts, the GC is a compact organelle resembling that of other dividing mammalian cells, but during muscle differentiation, the GC reorganizes into a network of smaller elements (Tassin et al., 1985a
MATERIALS AND METHODS
Antibodies and reagents. A rabbit antibody against the cis-Golgi protein GM130 (Nakamura et al., 1996
-tubulin DM1a was initially received from Dr. S. Doxsey (University of Massachusetts, Worcester, MA) and later purchased from Sigma (St. Louis, MO). Rabbit antibodies against Tyr-, Glu-, and
2-tubulin (Sato et al., 1997
Single muscle fiber preparations. All fibers were prepared from adult Wistar rats (~350 gm) obtained either from Taconic (Germantown, NY) or from the Animal Breeding Facility at the Panum Institute. Muscles were either dissected from animals that had been fixed by perfusion as described in Ploug et al. (1998)
Denervation experiments. A 1 cm section of the sciatic nerve was resected from one hindleg of animals anesthetized with ether. Five days after the operation, the animals were killed and fixed by perfusion. Fibers from the denervated and from the contralateral control muscle were prepared as described above. These experiments were done twice.
Cryostat sections and staining. A piece from the middle part of a muscle was mounted in Tissue Tek (Miles, Elkhart, IN) and rapidly frozen by immersion in liquid nitrogen-cooled isopentane. Ten-micrometer-thick transverse or longitudinal sections cut at
22°C were placed on glass slides. Blocking of nonspecific binding was done by incubating with 50 mM glycine and 0.25% bovine serum albumin in PBS for 15 min followed by primary antibody incubation in the same buffer for 90 min. After three washes, sections were incubated for 45 min with fluorescein isothiocyanate (FITC)-conjugated goat anti-rabbit F(ab)2 fragments (Sigma) diluted 1:250 in blocking buffer. Sections were mounted in Vectashield (Vector Laboratories, Burlingame, CA).
Staining whole fibers for immunofluorescence and immunogold EM. Fibers were transferred to 50 mM glycine, 0.25% bovine serum albumin, 0.04% saponin, and 0.05% sodium azide in PBS for blocking and permeabilization for 30 min, after which they were incubated overnight with the primary antibody diluted in blocking buffer supplemented with 200 µg/ml goat IgG. After three washes of 30 min each in PBS-0.04% saponin, they were incubated for 2 hr with FITC-conjugated goat anti-rabbit F(ab)2 fragments (Sigma) diluted 1:250 in blocking buffer. For double-labeling, biotin-coupled goat anti-mouse IgG was added (1:500) followed, after three washes, by Texas Red-conjugated streptavidin and Hoechst 33342 (0.5 µg/ml) in blocking buffer. Fibers were mounted in Vectashield on a glass slide.
A detailed protocol for the immunogold staining has been given in Ploug et al. (1998)
Microscopy and image analysis. Conventional microscopy was done with a Leica (Deerfield, IL) DMRD microscope. Photographs were taken on Kodak (Eastman Kodak, Rochester, NY) T-Max 400 film, and the negatives were scanned with an Agfa Arcus II flatbed scanner. Digital images were collected with a Sensys CCD camera (Photometrics, Tucson, AZ). Images were adjusted for contrast with Photoshop 5.0 and printed from a Power MacIntosh computer on a Pictrography 3000 digital printer (Fuji, Elmsford, NY). Confocal images were obtained on a Zeiss LSM 410 at the NINDS Light Imaging Facility. Images were transferred to a MacIntosh computer and analyzed with NIH Image (written by W. Rasband at the United States National Institutes of Health and available from the Internet at http://rsb.info.nih.gov/nih-image/).
To calculate the distribution of Golgi elements between the surface and the core of the fibers (Table 1), Z-series of 10 optical sections, 500 pixels long by 300 pixels wide and 1 µm apart, were recorded with a 63× NA 1.4 lens. At this magnification, each section has an area of 6000 µm2 or a volume of 6000 µm3. The first image was focused on the nuclei at the surface of the fiber and was stored on its own (surface image). The subsequent images, each 1 µm deeper inside the fiber, were combined by maximal projection, and the resultant single image (core image) was stored. We verified that this sampling and projection scheme, in which the brightest (maximum) value is kept for each pixel of the image were adequate to include all the surface and core elements. Each image, surface or core, was inverted, thresholded, binarized, and measured in two ways: (1) the number of particles was calculated to determine the number the Golgi elements and (2) the total surface of black pixels was calculated to measure the total surface of the Golgi elements. The results for the core images were divided by the number of sections that had been projected. For both surface and core, the results were divided by the volume of the optical section expressed in cubic micrometers to obtain the unit staining density. To measure the dimensions of the fiber, focus was moved from the top to the bottom surface of the fiber, identified by the immunofluorescent staining pattern, and the Z displacement, corresponding to the thickness of the fiber, was noted. Focus was then moved to the midbelly position, and the width of the fiber was measured with the functions/measure menu item of the Zeiss LSM software. We assumed that the fiber section was elliptical. The total volume, Vt, of a segment of fiber was calculated as Vt =
t w l, where t is the thickness of the fiber divided by 2, w is its width divided by 2, and l is the length of fiber (arbitrarily 100 µm). To calculate the core volume, Vc, we subtracted 1 µm from t and w, because we had observed that for most fibers the surface pattern was entirely contained in the first 1-µm-thick optical section. The surface volume,Vs, was calculated as Vs = Vt
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Table 1. Distribution of Golgi complex elements between surface and core of fibers from the soleus (SOL) and tensor fascia latae (TFL) muscles To calculate the number of myonuclei per fiber length unit, fibers stained for GLUT4 and counterstained with Hoechst 33342 were observed with a 25× objective in the Leica DMRD. Each field of view, measured with a graticule, was 440-µm-wide. Hoechst staining shows all the nuclei, whereas GLUT4 labels myonuclei only. The microscope filter magazine was switched from blue (Hoechst) to green (GLUT4) to ensure that only myonuclei were counted in a total of 20 fields per fiber type.
Measurements of the average length of Golgi cisternae were done from photographic prints of electron micrographs resulting from at least four independent experiments.
RESULTS
The immunofluorescence pattern of proteins of the Golgi complex is fiber type-specific
When fibers from the soleus muscle are stained for GM130, a bona fide protein of the cis-Golgi, we observe, at the surface of the fibers (Fig. 1A, left panel), a perinuclear belt around each nucleus plus dots between the nuclei. In the core of the fibers (right panel), we observe stretches of dots. This is the same pattern as we previously reported for the glucose transporter GLUT4 (Ploug et al., 1998
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Figure 1. Different staining patterns are observed in different fibers of a mixed muscle stained with an antibody to a Golgi complex protein. Single fibers were prepared from rat soleus (a) or red gastrocnemius (b-d) and stained with anti-GM130. Images, focused at the surface of the fibers (left panels) or 5- to 6-µm-deep in the core of the fibers (right panels) were collected with a conventional fluorescence microscope. Insets give an enlarged view of a single nucleus (left) or of an equivalent area in the core (right). Arrows point to the position of nuclei (a-c) or of nuclear poles (d). Filled arrowheads point to the Golgi complex of nonmuscle cells, and open arrowheads to stretches of staining in the core of fibers. The dark channels that can be seen at the surface of the fibers in a and c correspond to the position of blood vessels. Notice that the RG fiber shown in b has a pattern very similar to that in the soleus, both at the surface and in the core of the fiber. Fibers shown in c and d present a different pattern in which nuclei are not highlighted by the staining. Scale bar, 50 µm.
The total length of the teased fibers reaches 1 cm. We find that the staining pattern is constant from one end of the fiber to the other, with the exception of the NMJ, which will be discussed separately. However, there are some subtle variations along the fiber, as seen in higher magnification photographs of type I fibers (Fig. 2): the number of elements surrounding each nucleus is variable, and ~44% of the nuclei (n = 163) show some staining immediately above and below the nucleus (Fig. 2, top panel), whereas others just show a belt in a plane parallel to the fiber surface. Finally, staining resembling the compact Golgi complex of nonmuscle cells is occasionally found next to a nucleus at the surface of the fibers (Fig. 1a,c, arrowheads). These nuclei are not stained with anti-GLUT4 (Fig. 2, bottom panel). Because GLUT4 is only expressed in muscle, whereas the other Golgi markers are present in all cell types, these results show that the compact staining belongs to nonmuscle nuclei (fibroblasts, endothelial cells, Schwann cells, etc.), which remain associated with the muscle fibers during their preparation.
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Figure 2. At higher magnification, variability in the Golgi complex staining pattern can be observed. Fibers from soleus muscles were double-stained with MG160 (mg) and GLUT4 (gt) and observed with a conventional fluorescence microscope. Top panel shows the MG160 staining at the surface of a fiber. Notice that some nuclei only show staining in the equatorial plane, whereas others (arrows) show staining above and below as well. In the bottom panel, also focused on the surface of a fiber, we observe three nuclei, visualized by Hoechst staining (h). Two of them (arrowheads) show perinuclear staining for both MG160 and GLUT4. The third nucleus (arrow), has a very localized and strong MG160 labeling, but no GLUT4 labeling, which identifies it as a nonmuscle nucleus, associated with, but outside of the muscle fiber. Scale bars, 10 µm.
It seems likely that those fibers in the RG with a soleus-like pattern are type I, as are the majority of soleus fibers. Fibers were stained for the sarcoplasmic reticulum Ca2+-ATPase of type II fibers (SERCAI) (Wu and Lytton, 1993
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Figure 3. The red gastrocnemius fibers with distinct perinuclear Golgi complex staining are type I. RG fibers were double-stained for GLUT4 (gt) and SERCA1 (srca), the Ca2+ ATPase of type II fibers. Two fibers are shown. One (arrow) is positive for SERCA1, which identifies it as a type II fiber. It has no distinct perinuclear pattern for GLUT4 on its surface. The other fiber (arrowhead), which is negative for SERCA, shows a distinct perinuclear GLUT4 staining. Scale bar, 50 µm.
Further confirmation was obtained by staining fibers prepared from the TFL, a muscle in which ~90% of the fibers are type IIB (Armstrong and Phelps, 1984
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Figure 4. Golgi complex elements are differentially distributed in type I fibers from the soleus and type II B fibers from the tensor fascia latae. Z-series of confocal images were collected from soleus and TFL fibers stained for MG160. The focus of the first image was at the surface of the fibers and is shown in the top panel. Nine additional images were recorded at 1 µm intervals. The projections of the 10 images were pseudocolored according to a depth scale (bottom panels). Notice the dominant contribution of the surface staining (red) in the soleus and the arrangement of the core staining in long stretches at different depths, compared to the much more random distribution of the staining in the TFL. Scale bar, 10 µm.
Electron microscopy shows stacks of Golgi cisternae both at the surface and in the core of all muscle fibers
When rat muscles (soleus and red gastrocnemius) are examined in the electron microscope, small stacks of three to four cisternae are observed in all parts of the muscle (Fig. 5): around the nuclei, especially at the poles, along the plasma membrane in regions devoid of nuclei, and in the myofibrillar core. The stacks are short (0.71 ± 0.3 µm; mean ± SD; n = 46 in the soleus) compared to the long ribbons found in dividing cells, which is consistent with the immunofluorescent pattern of dots and dashes. When the fibers are immunolabeled for MG160, the grains are clearly limited to the medial/trans-cisternae. In contrast, they extend to the last cisternae and beyond for TGN38 and GLUT4. This distribution shows that the stacks are polarized, with the cis-Golgi facing the nuclear membrane. Thus, each of the Golgi elements observed in light microscopy represents a small stack of cisternae.
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Figure 5. EM immunogold labeling of Golgi complex proteins in skeletal muscle. Typical stacks of cisternae (arrows) are found at the nuclear poles (a, c-e), in the myofibrillar core of the fibers (b, d), and elsewhere in the cytoplasm (e, f) of soleus (a-d) and RG fibers (e, f). Immunogold labeling for MG160 (a, b) is confined to the middle to trans-cisternae, whereas TGN38 (c) and GLUT4 (d-f) are found in the TGN area. N, Nuclei; M, mitochondria; I, I-band; A, A-band. Scale bars: a-d, 200 nm; e, f, 500 nm.
The organization of the microtubule cytoskeleton is fiber type-dependent as well
What distributes the Golgi complex elements throughout the fibers? In other mammalian cell types, the Golgi complex is positioned by the microtubule-linked motors dynein and kinesin (for review, see Burkhardt, 1998
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Figure 6. Microtubule patterns are fiber type-dependent. Soleus and TFL fibers were double-stained for
Although it is clear that the Golgi elements in type IIB fibers are positioned at the microtubule nucleation points, for type I fibers, the observation of the microtubules provides no clue as to the position of the Golgi elements, except that they are found along the densest bundles. To examine whether stable microtubules may be involved in the positioning of the Golgi elements and determine whether their organization is fiber type-dependent, soleus and TFL fibers were stained with anti-MG160 antibodies, together with antibodies specific for either tyr-tubulin, glu-tubulin, or
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Figure 7. Golgi complex elements colocalize with stable microtubules. Soleus fibers were double-stained for MG160 (red) and glutamylated tubulin (green) and observed with a confocal microscope. The top panel shows a view at the surface of a fiber. A nucleus (arrows) is surrounded by microtubules and Golgi elements. Notice that all Golgi elements are associated with stable microtubules. The bottom panel shows a view from inside the fiber. The rows of Golgi elements are associated with stretches of stable microtubules. Scale bar, 10 µm.
The organization of the Golgi complex at the NMJ is independent of fiber type
There has been some debate as to whether there is a special organization of the GC at the NMJ (Jasmin et al., 1989
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Figure 8. The Golgi complex pattern at the NMJ is consistently perinuclear independently of fiber type. The NMJ of single fibers from different muscles was stained with different combinations of markers. To localize the NMJ along the fibers, we used either staining with Texas Red-labeled bungarotoxin (a) or the unique appearance of the clustered endplate nuclei (b) stained with Hoechst (blue channel). The insets show extrajunctional nuclei from the same fiber. a shows a single confocal image at the NMJ of a soleus fiber stained with bungarotoxin (red) and MG160 (green). Each myonucleus is surrounded by a belt of Golgi complex elements but, because the nuclei are not all in the same orientation, the staining is distinct around a few nuclei only (arrows). The arrowhead points to the Golgi complex of a nonmuscle nucleus. b shows the NMJ of a red gatrocnemius fiber stained for MG160 (red) and GLUT4 (green). The inset shows an extrajunctional nucleus, the staining of which identifies the fiber as type IIB. The junctional nuclei, however, are surrounded by GLUT4 (green) and MG160 (red) staining. Nonmuscle nuclei (arrowheads) can be identified by the compact MG160 staining and the absence of GLUT4 staining. c shows the NMJ of a soleus fiber stained with
If the distribution of microtubules is to explain the distribution of GC elements, we should expect the distribution of microtubules at the NMJ to be fiber type-independent as well. Examination of tubulin staining at the NMJ of a soleus fiber (Fig. 8c) demonstrates a denser labeling than elsewhere, as was shown by Rahkila et al. (1997)
The effects of fiber type on the organization of the Golgi complex are reversed by denervation
To observe whether the effects of muscle activity on Golgi complex organization are reversible, as suggested by the data of Jasmin et al. (1989)
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Figure 9. After denervation, the Golgi complex pattern is similar at the surface of type I and type II fibers. Five days after denervation, fibers from both denervated and contralateral control hindlegs of soleus and RG muscles were stained for MG160. The staining in the control fibers was similar to what is shown in Figure 1. In denervated soleus fibers (a-d), the perinuclear pattern is maintained. In RG fibers (e-j), all fibers have a perinuclear pattern that resembles that of the soleus (e, h-j). In some fibers, Golgi elements are still more concentrated at the nuclear poles (f). The perinuclear pattern is not as tight (arrowheads) as in the control fibers. d and g show aggregated nuclei, marked with an asterisk. Such aggregates are frequently encountered in the denervated but not in the control fibers (see Results). The bright Golgi complex of a nonmuscle cell is marked by a small arrow in i. Scale bar, 10 µm.
A novel observation, in denervated fibers, was an increase in the proportion of clustered nuclei (Fig. 9d,g). In control fibers, few nuclei (11.8%, n = 228 for the soleus; 2.3%, n = 258 for the RG) form clusters (two or more muscle nuclei close enough that their membranes appear to touch in light microscopy). After denervation, there is a 3.9-fold increase in the proportion of clustered nuclei in the soleus fibers and a 4.3-fold increase in the RG fibers (46.3%, n = 214; 9.8%, n = 255, respectively). In addition, clusters of three nuclei or more (Fig. 9d,g) are frequent, whereas they are very rare in control fibers.
The images shown in Figure 9 were taken without attention to the relative intensity of the staining. To quantitate the effects of denervation, 12 Z-series of confocal images were collected from all samples under identical recording conditions, and NIH Image was used to quantitate the staining associated with the immediate perinuclear belt of the nuclei as well as the surface and core staining. Results are summarized in Table 2. They show that Golgi complex staining decreases by a factor of ~2 in the soleus, with a large contribution from the surface staining, although the perinuclear labeling remains unchanged. In contrast, the staining in the RG fibers increases nearly twofold, with contributions from both surface (40%) and core (30%). After denervation, all fibers atrophy to the same degree, as shown by a 30% reduction in their cross-sectional area. The absolute numbers (data not shown) indicate that the control soleus has, per nucleus, 1.6 times as much Golgi as the control RG, which is slightly higher than the difference between soleus and TFL (Table 1). After denervation, however, the RG has about the same amount of GC as the control soleus. Therefore, it appears that innervation reversibly modulates the organization of the Golgi complex in muscle fibers.
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Table 2. Changes in the distribution of Golgi complex elements after denervation of soleus (SOL) and red gastrocnemius (RG) muscles Denervation affected microtubules as well. The density of labeling appeared generally lower throughout the fibers, but all nuclei, independent of fiber type, showed a continuous perinuclear staining (Fig. 10). The staining pattern at the NMJ for both GC markers and microtubules appeared largely unchanged after denervation. In the soleus, it was less attenuated than that of the extrajunctional nuclei (data not shown). All results, therefore, are consistent with a model in which the Golgi complex organization is regulated by the fiber type-dependent organization of microtubules.
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Figure 10. After denervation, the microtubule pattern is similar at the surface of type I and type II fibers. Distribution of the microtubules in denervated soleus (SOL) and red gastrocnemius (RG) fibers. Notice the strong perinuclear staining and the longitudinal microtubules in both. Scale bar, 10 µm.
DISCUSSION
In this paper, we show, for the first time, that the organization of the Golgi complex and of the microtubules in muscle is fiber type-dependent. The most striking difference in GC organization between different fiber types seems to be the relative accumulation of GC elements at the surface of the type I fibers, especially as a perinuclear belt, compared to a more even distribution between surface and core in type II fibers. We have observed this difference with several antibodies that label different compartments of the GC: GM130 for the cis-Golgi, MG160 for the medial/trans-Golgi, and TGN38 and GLUT4 for the TGN. In addition, we have observed by EM a higher frequency of cisternae around the nuclei of soleus fibers than of red gatrocnemius fibers. We therefore feel confident that our observations truly reflect a different organization of the GC rather than the local upregulation or downregulation of one of its proteins.
The present work establishes in unequivocal terms that the Golgi complex is present throughout the whole fiber of all muscle types, and it suggests that the controversy on the existence of the GC in extrajunctional areas of muscle (Jasmin et al., 1989
Each GC element in muscle is very small compared to the GC of dividing cells. However, we must keep in mind the gigantic size of muscle fibers. To estimate the total amount of GC in muscle, we have quantitated optical sections of whole fibers. Regardless of fiber type, we find an average of ~100 Golgi elements per nucleus. EM shows that each element is a small stack of cisternae, of similar size to those found in mammalian cells treated with microtubule-disrupting agents. Cole et al. (1996)
The proposal that microtubules are responsible for the differential distribution of the GC throughout the muscle fibers is based on two observations: the colocalization of GC elements with microtubules, previously reported in other muscles as well (Rahkila et al., 1997
In type IIB fibers, Golgi elements are localized at microtubule nucleation points, marked by a microtubule aster. This is similar to the gathering of the GC around the centrosome of dividing cells. In type I fibers, however, there are very few distinct microtubule nucleating sites, and it is not clear what determines the exact position of the Golgi elements along the microtubules, assuming they are stationary. During myogenesis, the nucleation site of microtubules changes from a unique centrosome to multiple sites, some of which are along the outer nuclear membrane, which is part of the endoplasmic reticulum (ER) (Tassin et al., 1985a
The fiber type-dependent organization of the microtubules, in turn, may be caused by a differential organization of microtubule-organizing proteins such as pericentrin (Doxsey et al., 1994
Our observations definitely show that innervation does not suppress the extrajunctional Golgi complex as had been proposed (Jasmin et al., 1989
At the neuromuscular junction, we observe, in all fiber types, a perinuclear staining of the junctional nuclei with GC markers and an increased density of microtubules. Such a pattern was also demonstrated by Simon et al. (1992)
The fiber type-dependent distribution of the Golgi complex has functional consequences: the capacity for glycosylation, transmembrane protein, and lipid synthesis, all functions of the GC, are more concentrated in the core of the fast than of the slow fibers. It may therefore be responsible for the larger amount of T-tubules in the faster fibers. Another consequence is an increased capacity for glucose uptake in the core of fast fibers, because the TGN is an important storage site for the glucose transporter GLUT4 (Ploug et al., 1998
FOOTNOTES Received July 14, 1999; revised Sept. 20, 1999; accepted Sept. 27, 1999.
This work was supported by the National Institutes of Health Intramural Program, by a grant from the Danish National Research Foundation (504-14) to T. Ploug, and by a NATO Collaborative Research Grant to T. Ploug and E. Ralston. We are grateful to Tom S. Reese for support throughout this project, to Carolyn Smith [National Institute of Neurological Disorders and Stroke (NINDS) Light Imaging Facility] for help with the confocal microscopy, to Jung-Hwa Tao-Cheng, and V. Tanner-Crocker [NINDS electron microscopy (EM) facility] for help with the EM work, and to Gerda Hau (Panum Institute) for skillful technical help. We thank all those, cited in the text, who provided us with reagents. We are also grateful to Jung-Hwa Tao-Cheng, Matt Daniels (National Heart, Lung, and Blood Institute), and Andres Buonanno (National Institute of Child Health and Human Development) for useful comments on this manuscript.
Correspondence should be addressed to Evelyn Ralston, Laboratory of Neurobiology, National Institute of Neurological Disorders and Stroke, National Institutes of Health, Building 36, Room 2A-21, Bethesda, MD 20892-4062. E-mail: esr{at}codon.nih.gov.
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