 |
|||||
|
|||||
|
|||||
|
|||||
|
|||||
Previous Article | Next Article
Volume 16, Number 19, Issue of October 1, 1996 pp. 5967-5978
Copyright ©1996 Society for NeuroscienceProtein Synthesis within Dendrites: Glycosylation of Newly Synthesized Proteins in Dendrites of Hippocampal Neurons in Culture
Enrique R. Torre and Oswald Steward Department of Neuroscience, University of Virginia School of Medicine, Charlottesville, Virginia 22908
ABSTRACT
There is increasing evidence that certain mRNAs are present in dendrites and can be translated there. The present study uses two strategies to evaluate whether dendrites also possess the machinery for protein glycosylation. First, precursor labeling techniques were used in conjunction with autoradiography to visualize glycosyltransferase activities that are characteristic of the rough endoplasmic reticulum (RER) (mannose) or the Golgi apparatus (GA) (galactose and fucose) in dendrites that had been separated from their cell bodies and in intact neurons treated with brefeldin A or low temperature. Second, immunocytochemical techniques were used to define the subcellular distribution of proteins that are considered markers of the RER (ribophorin I) and GA (p58,
Key words: rough endoplasmic reticulum; Golgi apparatus; TGN; dendrites; glycosylation; hippocampal neurons; dendritic RNA-mannosidase II, galactosyltransferase, and TGN38/41). Autoradiographic analysis revealed that isolated dendrites incorporated sugar precursors in a tunicamycin-sensitive and protein synthesis-dependent manner. Moreover, when intact neurons were pulse-labeled with 3H-labeled sugars at low temperature or after treatment with brefeldin A, labeling was distributed over proximal and sometimes distal dendrites. Immunolabeling for RER markers was predominantly localized in cell bodies but extended for a considerable distance into dendrites of all neurons. Immunolabeling for GA markers was confined to the cell body in ~70% of the neurons, but in 30% of the neurons, the staining extended into proximal and middle dendrites. These results indicate that the machinery for glycosylation extends well into dendrites in many neurons.
INTRODUCTION
The discovery that polyribosomes are selectively localized beneath postsynaptic sites on CNS neurons has led to the hypothesis that some key synaptic proteins are synthesized on site (Steward and Levy, 1982; Steward and Ribak, 1986
The latter findings raise the question of whether any integral membrane proteins are synthesized in dendrites. Recent studies have revealed that mRNA for the 1,4,5-inositol triphosphate receptor (IP3r) is present in the dendrites of Purkinje cells (Furuichi et al., 1993
The goal of the present study was to define whether the machinery for protein glycosylation is present in the dendrites of hippocampal neurons in culture. These are the same cells in which the distribution of particular mRNA species and the distribution of protein synthetic activity have previously been defined (Kleiman et al., 1990
Our results revealed a local incorporation of sugars within proximal and middle dendrites that was blocked by tunicamycin (N-glycosylation inhibitor), and cycloheximide (protein synthesis inhibitor). The distribution of labeling was similar to the distribution of immunostaining for elements of the RER and the GA.
Some of these results were communicated in abstract form (Torre and Steward, 1993
MATERIALS AND METHODS
Cell culture Culture of hippocampal neurons. Cultures of hippocampal neurons were prepared as described by Bartlett and Banker (1984)Preparation of double-surfaced coverslips for the isolation of neurites. The system used to isolate dendrites was prepared as described previously (Torre and Steward, 1992
Hippocampal cell suspensions of 7.5-10 × 104 cells were plated onto the filter surface of the sandwich. Cells were plated at lower densities than described originally (Torre and Steward, 1992
After 10-12 d in culture, the sandwiches were transferred to a dish containing Hank's BSS, and the polycarbonate membranes were peeled off. The matrix on the glass coverslips contained the neurites that had grown through the porous membrane. These coverslips were subsequently used in the pulse-labeling experiments.
Pulse-labeling experiments To maximize sugar incorporation within isolated dendrites or intact neurons, we used the following strategies: (1) Cells and neurites were preincubated and pulse-labeled in a medium in which the glucose concentration was lowered from 7 to 1 gm/l to ensure a higher uptake of the sugar tracer. Complete elimination of glucose from the medium was not tolerated by either hippocampal cells or dissected neurites, even when the medium was supplemented with pyruvate. (2) Neurites were pulse-labeled for 1 hr and with high concentrations of the radioactive sugar precursors to increase the labeling of the endogenous pools of nucleotide-saccharide donors and to promote a more extensive labeling of newly synthesized glycoproteins.Sugar incorporation in isolated neurites. Isolated neurites were preincubated in conditioned N2.1 medium containing low glucose (0.1%) for 1 hr at 37°C and then pulsed for 1 hr with [3H]mannose (500 µCi/ml), [3H]fucose (250 µCi/ml), or [3H]galactose (200 µCi/ml) dissolved in the same medium. The coverslips were chased for 20 min in the presence of 10 mM of the respective unlabeled sugar and washed in BSS solution. In some experiments in which neurons were pulse-labeled in the presence of tunicamycin (Boehringer Mannheim, Indianapolis, IN) (5 µg/ml), the cells were preincubated for 2 hr with the inhibitor before separating the Nucleopore membrane. The preincubation of the isolated neurites was continued for an additional hour before the pulse with the tritiated sugar was initiated. The protein synthesis dependence of the sugar incorporation was evaluated by pulse labeling the neurites in the presence of the protein synthesis inhibitor cycloheximide (Sigma) (50 µg/ml). To evaluate whether any of the labeling of isolated neurites was attributable to the activity of surface galactosyltransferases (Eckstein and Shur, 1989
20°C for 7 min and then treated with methanol/chloroform 1:2 and 2:1 for 15 min each at room temperature. This serves as a histological fixative and simultaneously extracts glycolipids while glycoproteins are retained (Suzuki, 1963
Galactose incorporation in intact neurons treated with brefeldin A or incubated at 20°C. Intact hippocampal neurons were preincubated for 1 hr at 37°C in N2.1 medium containing low glucose (0.1%) either with or without (control) brefeldin A (5 µg/ml). Individual coverslips were labeled with 100 µl of [3H]mannose (500 µCi/ml) for 1 hr and chased in the same medium containing 10 mM unlabeled sugar for an additional hour. Other groups of cells were incubated in N2.1 medium containing 20 mM HEPES, pH 7.4, and 0.1% glucose at either 37°C (control) or 20°C. Individual coverslips were labeled with 100 µl of [3H]galactose (200 µCi/ml) for 1 hr and chased in the same medium containing 10 mM unlabeled sugar for an additional hour. The cells were fixed permeabilized as described above.
Immunohistochemistry To identify dendritic processes, isolated neurites and cells in culture were immunostained for microtubule-associated protein-2 (MAP2). Cells were fixed in 4% paraformaldehyde in PBS containing 0.12 M sucrose. After fixation, processes were permeabilized in 0.1 M morpholino-ethane-sulfonic (MES) buffer, pH 6.8, containing 2 mM MgSO4, 1 mM EGTA (MME buffer), and 0.2% Triton X-100 for 5 min at room temperature. Coverslips were preincubated in MME containing 10% BSA and 1% normal goat serum for 1 hr at 37°C to block nonspecific binding. After blocking, coverslips were incubated overnight at 4°C with the monoclonal antibody AP14 (1:100), which recognizes MAP2, a specific marker of the dendritic compartment (Cáceres et al., 1984Immunohistochemistry for endomembranes. Hippocampal neurons cultured for 14-20 d were rinsed in Mg/Ca-free Hank's balanced salt solution and fixed in periodate-lysine phosphate buffer containing 2% paraformaldehyde (McLean and Nakane, 1974
The markers were detected with biotin-extravidin-FITC as described for MAP2. Most coverslips were double stained with MAP2, in which case, MAP2 was visualized with a rhodamine-conjugated rabbit anti-mouse antibody (Boehringer Mannheim) (1:200).
Histochemistry After immunolabeling, coverslips were stained for 30 min with bisbenzimide (Hoechst 33258, Molecular Probes, Eugene, OR) (5 ng/ml). At neutral pH, bisbenzimide selectively stains DNA, which is detected as blue fluorescence in UV (Hilwig and Grop, 1975
RESULTS
Sugar incorporation in isolated dendrites
To evaluate whether glycosylation of newly synthesized proteins takes place within dendrites, we studied the incorporation of [3H]mannose, [3H]galactose, or [3H]fucose in dendrites that were physically separated from their cell bodies. This was accomplished using a special two-surfaced culture system described previously (Torre and Steward, 1992
Fig. 1. Vitality of isolated dendrites. Hippocampal neurons were cultured for 10 d on a double-surface coverslip (A) as described in Materials and Methods. The Nucleopore membrane containing the cell bodies was peeled off, leaving a mesh of amputated processes on the second surface. Isolated processes were pulse-labeled with 100 µCi/ml [3H]leucine for 1 hr immediately after the isolation (0 hr) or 3, 6, and 12 hr after the isolation. The processes were fixed-stained for MAP2 and DNA and prepared for autoradiography. The graph in B shows the percentage of labeled dendrites at the different survival times. The percentage of living dendrites slowly decreases with time and drops dramatically by 6 and 12 hr after isolation. Dendrites were considered labeled at low levels when they had scattered patches of 2-3 silver grains along their length. Those processes having strings of densely packed silver grains were counted as highly labeled dendrites. The numbers in parentheses represent the number of MAP2-stained processes counted in nine coverslips from three different experiments. The photographs are representative fields showing the incorporation of [3H]leucine by isolated dendrites at different times after the cut. Scale bar, 25 µm.
[View Larger Version of this Image (86K GIF file)]
Survival of isolated dendrites The present experiments required that isolated neurites be maintained under different culture conditions and for longer periods of time than originally reported. To evaluate the time range after the cut within which the dissected dendrites still are viable, dendrites were isolated from 10-d-old cultures and then were pulse-labeled with [3H]leucine (100 µCi/ml) for 1 hr immediately after separation (time 0) and at 3, 6, and 12 hr after separation. The coverslips were prepared for autoradiography, and the viability of the cut dendrites was assessed by the presence of silver grains over processes that stained positively for MAP2.
Approximately 60% of the MAP2-stained neurites incorporated [3H]leucine when pulse-labeled immediately after the cut. Many processes became heavily labeled. Approximately 35% of the MAP2-stained neurites incorporated [3H]leucine when pulse-labeled 3 hr after the cut and ~25% when pulse-labeled 6 hr after the cut (Fig. 1B). By 12 hr, most neurites had degenerated, although in two experiments, a few neurites still were able to incorporate the labeled precursor. Neurites labeled 3 hr after the cut in medium with low glucose (1 gm/l) exhibited leucine incorporation that was similar to that seen in normal medium. These results indicate that isolated dendrites remain viable for several hours and continue to be capable of synthesizing protein for at least 3-4 hr after separation.
Incorporation of [3H]mannose in isolated dendrites Mannose is added to nascent glycoproteins in the RER (Kornfeld and Kornfeld, 1985
Fig. 2. Mannose incorporation in isolated dendrites. Neurites isolated from 10- to 12-d-old cultures were preincubated for 1 hr in low-glucose medium, pulse-labeled with 400 µCi/ml [3H]mannose for 1 hr, rinsed in medium containing 10 mM cold sugar, and fixed and immunostained for MAP2. A-D, Sites of [3H]mannose incorporation evaluated by autoradiography and dark-field microscopy. E-G, MAP2 staining shows colocalization with silver grains. The arrows indicate the location of dendrites. The asterisk indicates the presence of a labeled neuron that was identified by the DNA staining. Scale bar, 25 µm.
[View Larger Version of this Image (68K GIF file)]
Tunicamycin inhibits N-glycosylation by interrupting the formation of the mannose-rich oligosaccharide in the RER (Elbein, 1991
Fig. 4. Labeling of isolated dendrites was depressed by inhibiting the synthesis and N-glycosylation of proteins but not by competing with surface glycosyltransferases. Isolated dendrites were preincubated for 1 hr in low-glucose medium containing 50 µg/ml cycloheximide (C, H), 5 µg/ml tunicamycin (E, I), or 5 mM UDP-galactose (J); control cells (A, G) were incubated with no drugs. Cells were pulse-labeled with [3H]mannose (upper panel) or [3H]galactose (lower panel) for 1 hr, washed in medium containing 10 mM cold sugar, and fixed and immunostained for MAP2 (B, D, F; in G-J, immunofluorescence for MAP2 was combined with dark-field illumination). The arrows indicate the location of dendrites. Scale bar, 25 µm.
[View Larger Version of this Image (117K GIF file)]
Fig. 5. Effect of the inhibition of N-glycosylation, protein synthesis, and surface glycosyltransferases on the labeling of isolated dendrites with the tritiated sugar precursors mannose, galactose, and fucose. Neurites isolated as described in Materials and Methods were treated with tunicamycin (5 µg/ml), cycloheximide (50 µg/ml), or the impermeant sugar precursors UDP-galactose (5 mM) and pulse-labeled for 1 hr with tritiated sugars. The bars represent the proportion of labeled and unlabeled MAP2-stained processes ± SEM after the different treatments. The numbers in parentheses indicate the number of dendrites evaluated in at least two different experiments. Controls were compared with the incorporation of [3H]leucine by isolated dendrites in similar conditions.
[View Larger Version of this Image (23K GIF file)]
Galactose and fucose incorporation in isolated dendrites Galactose and fucose are incorporated into complex oligosaccharides of membrane and secretory glycoproteins in the GA (Kornfeld and Kornfeld, 1985
The label over the isolated dendrites was rather patchy but was higher than that seen with mannose. Labeling was highest over the thicker (proximal) end of the isolated dendrite (Fig. 3A,C for galactose, E,G for fucose). Thin processes (presumed distal dendrites) generally were not labeled, although the most heavily labeled processes were labeled throughout their extent. As was the case with mannose incorporation, axons remained unlabeled.
Fig. 3. Galactose and fucose incorporation in isolated dendrites. Neurites isolated from 10- to 12-d-old cultures were preincubated for 1 hr in low-glucose medium, pulse-labeled with 200 µCi/ml [3H]fucose or 100 µCi/ml [3H]galactose for 1 hr, rinsed in medium containing 10 mM cold sugar, and fixed and immunostained for MAP2. A, C, Autoradiographic localization of the sites of [3H]galactose incorporation. E, G, Autoradiographic localization of [3H]fucose incorporation. B, D, F, H, The parts show that the sugar incorporation is localized over MAP2-stained processes. The arrows indicate the localization of dendrites identified by MAP2 staining. The asterisk indicates the presence of a labeled neuron that was identified by the DNA staining. Scale bar, 25 µm.
[View Larger Version of this Image (91K GIF file)]
The fact that galactosyltransferases may be found on the cell surface (Shur, 1989
In contrast, the dendritic incorporation of galactose and fucose was drastically reduced by tunicamycin (Figs. 4E,I, 5). Only a few dendrites showed some scattered silver grains. These observations underline the intracellular locus of the sugar incorporation.
Incorporation of sugars in dendrites is dependent on protein synthesis The labeling of membrane and secretory proteins depends on the continued availability of newly synthesized precursors (Kornfeld and Kornfeld, 1985Taken together, the results suggest that there is a compartment within dendrites that is able to glycosylate recently synthesized proteins in a way similar to that for the RER-GA complex.
Pulse labeling of intact neurons at low temperature and in the presence of brefeldin A
To corroborate the results obtained with isolated dendrites, we wished to evaluate the distribution of glycosyltransferase activities in intact neurons using autoradiography to visualize sites of sugar incorporation. However, this approach is complicated by the fact that neurons are capable of very rapid transport of glycoproteins after their synthesis (Hammerschlag et al., 1982Incubation of cells in the presence of brefeldin A induces the rapid fusion of the GA with the ER (Lippincott Schwartz et al., 1989
Fig. 8. Dendritic localization of different Golgi compartments in hippocampal neurons in culture. Fourteen-day-old cultures were stained for p58 (A),-galactosyltransferase (
[View Larger Version of this Image (58K GIF file)]
Distribution of newly synthesized glycoproteins in brefeldin A-treated neurons Autoradiographs of control cells that have been incubated for 1 hr in [3H]mannose or galactose revealed silver grains densely packed over the cell body and extending into all processes, including axons (Fig. 6A for mannose, C for galactose). This is consistent with a rapid transport of recently synthesized glycoproteins. [3H]mannose labeling of axons was reduced by ~96% with brefeldin A (0.59 ± 0.02 grains/µm in control cells to 0.021 ± 0.003 grains/µm after brefeldin A; n = 40), demonstrating the expected blockade of rapid axonal transport. In contrast, dendrites still were heavily labeled when cells were pulse-labeled with mannose in the presence of brefeldin A (Fig. 6B), consistent with local mannose incorporation within dendrites. Dendritic labeling decreased in a proximo-distal manner and generally was absent in distal dendritic branches. Silver grains were not evenly distributed in all dendrites. Thus, in a given cell, some dendrites were densely labeled, whereas others were lightly labeled or unlabeled (Fig. 6B).
Fig. 6. Effects of brefeldin A and temperature on the localization of newly synthesized glycoproteins in hippocampal neurons. Fifteen-day-old neurons were pulse-labeled for 1 hr with [3H]mannose at 37°C with or without (control) brefeldin A (5 µg/ml) to block the exit of newly synthesized glycoproteins from the ER. Another group of cells was pulse-labeled with [3H]galactose at 37°C (control) or 20°C to block the exit of proteins from the trans-Golgi compartment. The distribution of newly synthesized glycoproteins was evaluated by autoradiography. A, Control cells pulse-labeled with [3H]mannose. B, Cells labeled with [3H]mannose in the presence of brefeldin A. C, Control cells pulse-labeled with [3H]galactose at 37°C. D, E, Cells labeled with [3H]galactose at 20°C. In control cells, newly synthesized glycoproteins were localized in the cell body, dendrites (large arrows), and axons (small arrows). In cells treated with brefeldin A or at 20° C, silver grains concentrate in the cell body and proximal or medial dendrites that were identified by their morphology (B, D) or MAP2 staining (E). The label was significantly reduced in axons. Scale bar, 50 µm.
[View Larger Version of this Image (98K GIF file)]
Distribution of newly synthesized glycoproteins in neurons maintained at 20°C The sites of accumulation of recently synthesized glycoproteins in cells incubated at 20°C provide an estimate of the distribution of the GA in intact hippocampal neurons. Cells that were pulse-labeled with galactose at 20°C exhibited labeling that was more tightly concentrated over the region of the cell body than was the case in cells incubated at 37°C [compare Fig. 6C (galactose at 37°C) with D (galactose at 20°C)]. Axons exhibited little, if any, labeling (0.09 ± 0.005 grains/µm at 20°C, n = 40 vs 0.75 ± 0.002 grains/µm at 37°C), consistent with the expected blockade of rapid transport.
Although axonal labeling was greatly reduced or eliminated, labeling was clearly present over dendrites (Fig. 6D,E). However, in contrast to the cells that were pulse-labeled at 37°C, the labeling was concentrated over proximal dendrites, decreasing to near background levels over middle and distal dendrites (Fig. 6D). Many cells were labeled only in the cell body and very proximal dendrites. Dendritic labeling after galactose exposure was detected in 43.78 ± 8.03% of the cells.
Immunolocalization of markers of the endomembrane system
The localization of the glycosyltransferase activities was compared with the distribution of organelles of the RER and GA, visualized by immunofluorescence microscopy of cultured hippocampal cells using antibodies against proteins localized in different compartments of the RER and GA. Endoplasmic reticulum The distribution of the RER in cultured hippocampal cells was assessed by using antibodies that recognize ribophorin I. Immunolabeling for ribophorin I was very intense in the perinuclear region of the cell body and extended from 50 to 120 µm into the dendritic shaft of most neurons. Distal dendrites and axons appeared unstained (Fig. 7A). These results were consistent with the autoradiographic distribution of mannose labeling in isolated dendrites and intact neurons and provided the background against which the subcellular distribution of the GA can be compared (Fig. 7B).
Fig. 7. Immunofluorescent localization of the endomembrane system in hippocampal neurons in culture. Fourteen-day-old neurons were fixed and stained for markers of the ER and GA. A, Localization of the rough ER protein ribophorin I. Note the accumulation of stained ER structures at branch points (asterisks) as well as the absence of label in some dendritic branches (open circles). Axons (open triangles) remained unlabeled. g indicates glial cell. C, Distribution of the medial cisterns of the GA as revealed by
[View Larger Version of this Image (51K GIF file)]
Golgi apparatus The organization of the Golgi complex in hippocampal neurons in culture was assessed by immunodetection of proteins specifically localized in the different compartments of the GA. Immunostaining for these markers (Fig. 8A-D) was localized in the cell body in all neurons and in the dendrites of ~30% of the cells (Fig. 8E). In contrast, axons were always devoid of label (Figs. 7, 8). The immunostaining pattern for each Golgi marker is illustrated in Figure 8A-D. The distribution of the cis-most region of the Golgi complex was evaluated using an antibody that recognizes a protein of 58K (p58) that has been shown to be enriched in the intermediate or salvage compartment and the cis-cisterns of the GA (Saraste and Svensson, 1991
The antibody against
To evaluate the distribution of staining in different cellular compartments, cells present in each coverslip were counted and classified as follows: (1) cells showing positive staining for Golgi markers only in the cell body, (2) cells showing positive staining for Golgi markers in only one dendrite, or (3) cells showing staining for Golgi organelles that extended for at least one cell diameter into several dendrites. Figure 8E shows that Golgi elements stained by different antibodies were restricted to the cell body of ~70% of the neurons. Approximately 20% of the cells also showed stained structures in one dendrite between 30 and 100 µm from the cell body. In 10% of the cells, staining was observed in all the dendrites. A similar distribution of staining was found with all the GA antibodies.
Treatment with brefeldin A led to a rapid alteration in the immunostaining pattern for elements of the GA. After a 10 min treatment, most cells exhibited a diffuse staining pattern for
DISCUSSION
Our results provide evidence that elements that function like the RER and GA extend into dendrites of hippocampal neurons in culture. This conclusion is based on the following: (1) a tunicamycin-sensitive and protein synthesis-dependent incorporation of tritiated sugar precursors by amputated dendrites; (2) the somatodendritic localization of newly synthesized glycoproteins in neurons treated with brefeldin A or at 20°C; and (3) the immunolocalization of the RER and GA markers in proximal and middle dendrites.RER-associated glycosyltransferase activity
Translation of secretory and membrane proteins and the initial step in glycosylation (i.e., mannosylation) take place in the RER (Kornfeld and Kornfeld, 1985The autoradiographic and immunochemical observations in intact hippocampal neurons in culture yielded consistent evidence regarding the distribution of RER in dendrites. Specifically, labeling after exposure to [3H]mannose in brefeldin A-treated neurons was distributed over the cell body and proximal dendrites in a pattern that resembled that of ribophorin I. This distribution is consistent with electron microscopic observations showing membrane-bound ribosomes along dendrites of the dentate gyrus and pyramidal neurons of the hippocampus (Steward and Levy, 1982
Golgi-associated glycosyltransferase activities
Our interpretation that the GA is present in dendrites is based on the finding that in amputated dendrites, the labeling after exposure to sugar precursors was inhibited by tunicamycin and cycloheximide but not by cold UDP-galactose in the incubation medium. Thus, the results suggest that within dendrites, sugars are linked to newly synthesized N-glycoproteins in a Golgi-like compartment rather than in the cytosol or on the dendrite surface.In general, autoradiographic studies of the distribution of glycosyltransferase activities as well as immunocytochemical studies of the distribution of markers of the distinct compartments of the GA in intact neurons provided consistent data. Both approaches revealed the presence of GA markers or glycosyltransferase activity characteristic of the GA in ~30-40% of the dendrites in intact neurons. The only inconsistency was that the spatial distribution of glycosyltransferase activity revealed by pulse chase experiments in intact neurons was somewhat more extensive than the distribution of the GA markers as revealed by immunocytochemistry. There are several possible explanations for this difference. First, it is possible that the immunocytochemical approach is not sufficiently sensitive to detect small elements of the GA that, nevertheless, possess sufficient glycosyltransferase activity to be detectable using autoradiographic techniques. Second, we cannot rule out the possibility that some of the distal labeling in cells treated with brefeldin A or low temperature is the result of somatodendritic transport of cytosolic glycoproteins (Dong et al., 1993
The autoradiographic studies of sites of glycosyltransferase activity in amputated dendrites confirm the presence of this activity in at least the proximal portions of the dendrites. However, there are some inconsistencies in the proportion of dendrites exhibiting glycosyltransferase activity. Given that only ~30% of the neurons exhibit immunostaining for the GA, it is surprising that 30-40% of the isolated dendrites exhibited labeling after pulse labeling with galactose or fucose. The reason is that only ~35% of the total number of MAP2-stained dendrites remain viable (as evidenced by an ability to incorporate leucine). If dendrite survival was random, one would expect 30% of this surviving population to contain elements of the GA detectable by immunostaining. Thus, one would expect only ~10% of the isolated dendrites to exhibit glycosylation activity. The three possible explanations for this discrepancy are: (1) There may be glycosylation activity in the absence of a GA that is detectable by immunostaining; (2) A greater number of dendrites may possess GA in the sandwich culture conditions; and (3) Dendrites that have a well-developed endomembrane system may be better able to survive the isolation.
In a recent study, Krijnse-Locker et al. (1995)
Possible role of the dendritic endomembrane system in protein synthesis
The present results reveal the presence of glycosylation activity (implying functional RER and GA) in proximal and even middle dendritic regions, from which all but a few mRNAs are excluded (for review, see Steward, 1995At this point, it is not known whether mRNAs for glycoproteins are present in the dendrites of hippocampal neurons in culture. Thus, it is not possible to compare the distribution of RER and GA markers with the distribution of particular mRNAs. The only mRNA for a glycoprotein that has been shown to be present in dendrites at relatively high levels is the mRNA for the IP3r, and this conclusion is based exclusively on studies of mRNA distribution in brain sections (Furuichi et al., 1993
Whether mRNAs for other glycoproteins are present in dendrites remains to be established. In this regard, there is evidence that mRNAs for subunits of neurotransmitter receptors are present in dendrites at some level (Miyashiro et al., 1994
The present observations raise a number of new questions about the nature and significance of dendritic protein synthetic machinery. The distribution of endomembrane organelles in dendrites suggests that membrane and secretory proteins can be produced in broad regions of the dendrite. However, these proteins could be fully glycosylated only in proximal segments. This raises the interesting possibility that glycoproteins synthesized in distal dendrites are mostly of the high mannose type that could be produced in the RER. Further characterization of the protein synthetic machinery will likely help to reveal the role of local protein synthesis and processing in dendritic function.
FOOTNOTES
Received June 5, 1996; revised July 9, 1996; accepted July 11, 1996.
This work was supported by National Institutes of Health Grant NS 12333 to O.S. We gratefully acknowledge Dr. David Castle for his critical review of this manuscript. We thank also Dr. David Meyer for his antibody against Ribophorin I, Drs. Kelly Moremen and Marilyn Farquar for the antibody against
Correspondence should be addressed to Dr. Enrique R. Torre, Department of Neuroscience, University of Virginia School of Medicine, Box 5148 MR4 Annex, Charlottesville, VA 22908.
REFERENCES
- Bartlett WP, Banker GA (1984) An electron microscopic study of the development of axons and dendrites by hippocampal neurons in culture. II. Synaptic relationships. J Neurosci 4:1954-1965 . [Abstract]
- Begovac PC, Shur BD (1990) Cell surface galactosyltransferase mediates the initiation of neurite outgrowth from PC12 cells on laminin. J Cell Biol 110:461-470 .
[Abstract/Free Full Text] - Bonatti S, Torrisi MR (1993) The intermediate compartment between endoplasmic reticulum and Golgi complex in mammalian cells. In: The endoplasmic reticulum. Subcellular biochemistry 21 (Borgese, N, Harris, JR, eds) , p. 121. New York: Plenum.
- Bottenstein JE, Sato GH (1979) Growth of a rat neuroblastoma cell line in serum-free supplemented medium. Proc Natl Acad Sci USA 76:514-519 .
[Abstract/Free Full Text] - Broadwell RD, Cataldo AM (1983) The neuronal endoplasmic reticulum: its cytochemistry and contribution to the endomembrane system. J Histochem Cytochem 31:1077-1088 . [Abstract]
- Cáceres A, Banker G, Steward O, Binder L, Payne M (1984) MAP2 is localized to the dendrites of hippocampal neurons which develop in culture. Dev Brain Res 13:314-318.
- De Camilli P, Moretti M, Denis Donini S, Walter U, Lohmann S (1986) Heterogeneous distribution of the cAMP receptor protein RII in the nervous system. J Cell Biol 103:189-203 .
[Abstract/Free Full Text] - Dong DL, Xu ZS, Chevrier MR, Cotter RJ, Cleveland DW, Hart GW (1993) Glycosylation of mammalian neurofilaments. Localization of multiple O-linked N-acetylglucosamine moieties on neurofilament polypeptides L and M. J Biol Chem 268:16679-16687 .
[Abstract/Free Full Text] - Eckstein DJ, Shur BD (1989) Laminin induces the stable expression of surface galactosyltransferase on lamellipodia of migrating cells. J Cell Biol 108:2507-2517 .
[Abstract/Free Full Text] - Elbein AD (1991) Glycosidase inhibitors: inhibitors of N-linked oligosaccharide processing. FASEB J 5:3055-3063 . [Abstract]
- Furuichi T, Simon-Chazottes D, Fujino I, Yamada N, Hasegawa M, Miyawaki A, Yoshikawa S, Guénet J-L, Mikoshiba K (1993) Widespread expression of inositol 1.4.5-triphosphate receptor type 1 gene (Insp3r1) in the mouse central nervous system. Receptors Channels 1:11-24 . [Web of Science][Medline]
- Gething M-J, Sambrook J (1992) Protein folding in the cell. Nature 355:33-45 . [Medline]
- Gonatas JO, Mezitis SGE, Stieber A, Fleicher B, Gonatas NK (1989) A novel sialoglycoprotein of the medial cisternae of the Golgi apparatus. J Biol Chem 264:646-653 .
[Abstract/Free Full Text] - Haltiwanger RS, Kelly WG, Roquemore EP, Blomberg MA, Dong L-YD, Kreppel L, Chou TY, Hart GW (1992) Glycosylation of nuclear and cytoplasmic proteins is ubiquitous and dynamic. Biochem Soc Trans 20:264-269 . [Web of Science][Medline]
- Hammerschlag R, Stone GC, Bolen FA, Lindsey JD (1982) Evidence that all newly synthesized proteins destined for fast axonal transport pass through the Golgi apparatus. J Cell Biol 93:568-575 .
[Abstract/Free Full Text] - Hammond C, Braakman I, Helenius A (1994) Role of N-linked oligosaccharide recognition, glucose trimming, and calnexin in glycoprotein folding and quality control. Proc Natl Acad Sci USA 91:913-917 .
[Abstract/Free Full Text] - Hilwig I, Grop A (1975) pH-dependent fluorescence of DNA and RNA in cytologic staining with ``Hoechst 33258.'' Exp Cell Res 91:457-460.
- Hortsch M, Meyer DL (1985) Immunochemical analysis of rough and smooth microsomes from rat liver. Segregation of docking protein in rough membranes. Eur J Biochem 150:559-564 . [Web of Science][Medline]
- Kleiman R, Banker GA, Steward O (1990) Differential subcellular localization of particular mRNAs in hippocampal neurons in culture. Neuron 5:821-830 . [Web of Science][Medline]
- Kleiman R, Banker G, Steward O (1993) Subcellular distribution of rRNA and poly(A) RNA in hippocampal neurons in culture. Mol Brain Res 20:305-312 . [Medline]
- Kornfeld R, Kornfeld S (1985) Assembly of asparagine-linked oligosaccharides. Annu Rev Biochem 54:631-664 . [Web of Science][Medline]
- Krijnse-Locker J, Parton RG, Fuller SD, Griffiths G, Dotti CG (1995) The organization of the endoplasmic reticulum and the intermediate compartment in cultured rat hippocampal neurons. Mol Biol Cell 6:1315-1332 . [Abstract]
- Kuismanen E, Saraste J (1989) Low temperature-induced transport blocks as tools to manipulate membrane traffic. Methods Cell Biol 32:257-274 . [Web of Science][Medline]
- Lippincott Schwartz J, Yuan LC, Bonifacino JS, Klausner RD (1989) Rapid redistribution of Golgi proteins into the ER in cells treated with Brefeldin A: evidence for membrane cycling from Golgi to ER. Cell 56:801-813. [Web of Science][Medline]
- Lopez LC, Maillet CM, Oleszkowicz K, Shur BD (1989) Cell surface and Golgi pools of
[Abstract/Free Full Text] - Lowenstein PR, Morrison EE, Bain D, Shering AF, Banting G, Douglas P, Castro MG (1994) Polarized distribution of the trans-Golgi network marker TGN38 during the in vitro development of neocortical neurons: effects of Nocodazole and Brefeldin A. Eur J Neurosci 6:1453-1465 . [Web of Science][Medline]
- Luzio JP, Brake B, Banting G, Howell KE, Braghetta P, Stanley KK (1990) TGN 38: Identification, sequencing and expression of an integral membrane protein of the trans-Golgi network. Biochem J 270:97-102 . [Web of Science][Medline]
- Martone ME, Zhang Y, Simpliciano V, Carragher BO, Ellisman MH (1993) Three-dimensional visualization of the smooth endoplasmic reticulum in Purkinje cell dendrites. J Neurosci 13:4636-4646 . [Abstract]
- McLean I, Nakane PK (1974) Periodate-lysine paraformaldehyde fixative. A new fixative for immunoelectron microscopy. J Histochem Cytochem 22:1077-1083 . [Abstract]
- Miyashiro K, Dichter M, Eberwine J (1994) On the nature and differential distribution of mRNAs in hippocampal neurites: implications for neuronal functioning. Proc Natl Acad Sci USA 91:10766-10768.
[Free Full Text] - Moremen KW, Touster O (1986) Topology of mannosidase II in rat liver Golgi membranes and release of the catalytic domain by selective proteolysis. J Biol Chem 261:10945-10951 .
[Abstract/Free Full Text] - Moremen KW, Touster O, Robins PW (1991) Novel purification of the catalytic domain of Golgi
[Abstract/Free Full Text] - Morré DJ, Kartenbeck J, Franke W (1979) Membrane flow and interconversions among endomembranes. Biochim Biophys Acta 559:71-152 . [Medline]
- Rao A, Steward O (1991) Evidence that protein constituents of postsynaptic membrane specializations are locally synthesized: analysis of proteins synthesized within synaptosomes. J Neurosci 11:2881-2995 . [Abstract]
- Saraste J, Svensson K (1991) Distribution of the intermediate elements operating in ER to Golgi transport. J Cell Sci 100:415-430 .
[Abstract/Free Full Text] - Shur B (1989) Expression and function of cell surface galactosyltransferase. Biochim Biophys Acta 988:389-409 . [Medline]
- Spacek J (1985) Three-dimensional analysis of dendritic spines. II. Spine apparatus and other cytoplasmic components. Anat Embryol 171:235-243 . [Medline]
- Steward O (1995) Targeting of mRNAs to subsynaptic microdomains in dendrites. Curr Opin Neurobiol 5:55-61 . [Medline]
- Steward O, Levy WB (1982) Preferential localization of polyribosomes under the base of dendritic spines in granule cells of the dentate gyrus. J Neurosci 2:284-291 . [Abstract]
- Steward O, Reeves TM (1988) Protein synthetic machinery beneath postsynaptic sites on CNS neurons: association between polyribosomes and other organelles at the synaptic site. J Neurosci 8:176-184 . [Abstract]
- Steward O, Ribak CE (1986) Polyribosomes associated with synaptic specializations on axon initial segments: localization of protein-synthetic machinery at inhibitory synapses. J Neurosci 6:3079-3085 . [Abstract]
- Suzuki (1963) The pattern of mammalian brain gangliosides. II. Evalua-tion of the extraction procedures, postmortem changes, and the effect of formalin preservation. J Neurochem 12:629-638. [Web of Science][Medline]
- Takei K, Stukembrok H, Metcalf A, Mignery GA, Südhof TC, Volpe P, Camilli PD (1992) Ca+ stores in Purkinje neurons: endoplasmic reticulum subcompartments demonstrated by heterogeneous distribution of Insp3 receptor, Ca2+-ATPase, and Calsequestrin. J Neurosci 12:489-505 . [Abstract]
- Terasaki M, Slater NT, Fein A, Schmidek A, Reese TS (1994) Continuous network of endoplasmic reticulum in cerebellar Purkinje neurons. Proc Natl Acad Sci USA 91:7510-7514 .
[Abstract/Free Full Text] - Torre ER, Steward O (1992) Demonstration of local protein synthesis within dendrites using a new culture system that permits the isolation of living axons and dendrites from their cell bodies. J Neurosci 12:762-772 . [Abstract]
- Torre ER, Steward O (1993) Post translational modifications of proteins within dendrites: evaluation of sugar incorporation in isolated dendrites from neurons in culture. Soc Neurosci Abstr 19:63.
- Torre ER, Steward O (1995) Immunochemical localization of the Golgi apparatus (GA) within dendrites of hippocampal neurons in culture and in situ. Mol Biol Cell [Suppl] 6:100a.
- Varki A, Freeze HH (1994) The major glycosylation pathways of mammalian membranes. A summary. Subcell Biochem 22:71-100 . [Medline]
- Villa A, Sharp AH, Racchetti G, Podini P, Bole DG, Dunn WA, Pozzan T, Snyder SH, Meldolesi J (1992) The endoplasmic reticulum of Purkinje neuron body and dendrites: molecular identity and specializations for Ca2+. Neuroscience 49:467-477 . [Web of Science][Medline]
Copyright ©1996 Society for Neuroscience 0270-6474/1996/165967-12$05.00/0
This article has been cited by other articles:
M. Shi, J. Bradner, T. K. Bammler, D. L. Eaton, J. Zhang, Z. Ye, A. M. Wilson, T. J. Montine, C. Pan, and J. Zhang
Identification of Glutathione S-Transferase Pi as a Protein Involved in Parkinson Disease Progression
Am. J. Pathol., July 1, 2009; 175(1): 54 - 65.
[Abstract] [Full Text] [PDF]
H. Wang, A. Iacoangeli, D. Lin, K. Williams, R. B. Denman, C. U.T. Hellen, and H. Tiedge
Dendritic BC1 RNA in translational control mechanisms
J. Cell Biol., December 5, 2005; 171(5): 811 - 821.
[Abstract] [Full Text] [PDF]
J. Glanzer, K. Y. Miyashiro, J.-Y. Sul, L. Barrett, B. Belt, P. Haydon, and J. Eberwine
RNA splicing capability of live neuronal dendrites
PNAS, November 15, 2005; 102(46): 16859 - 16864.
[Abstract] [Full Text] [PDF]
C. A. Farah, D. Liazoghli, S. Perreault, M. Desjardins, A. Guimont, A. Anton, M. Lauzon, G. Kreibich, J. Paiement, and N. Leclerc
Interaction of Microtubule-associated Protein-2 and p63: A NEW LINK BETWEEN MICROTUBULES AND ROUGH ENDOPLASMIC RETICULUM MEMBRANES IN NEURONS
J. Biol. Chem., March 11, 2005; 280(10): 9439 - 9449.
[Abstract] [Full Text] [PDF]
H. Bannai, K. Fukatsu, A. Mizutani, T. Natsume, S.-i. Iemura, T. Ikegami, T. Inoue, and K. Mikoshiba
An RNA-interacting Protein, SYNCRIP (Heterogeneous Nuclear Ribonuclear Protein Q1/NSAP1) Is a Component of mRNA Granule Transported with Inositol 1,4,5-Trisphosphate Receptor Type 1 mRNA in Neuronal Dendrites
J. Biol. Chem., December 17, 2004; 279(51): 53427 - 53434.
[Abstract] [Full Text] [PDF]
R. Lu, H. Wang, Z. Liang, L. Ku, W. T. O'Donnell, W. Li, S. T. Warren, and Y. Feng
The fragile X protein controls microtubule-associated protein 1B translation and microtubule stability in brain neuron development
PNAS, October 19, 2004; 101(42): 15201 - 15206.
[Abstract] [Full Text] [PDF]
H. Wang and H. Tiedge
Translational Control at the Synapse
Neuroscientist, October 1, 2004; 10(5): 456 - 466.
[Abstract] [PDF]
M. Aridor, A. K. Guzik, A. Bielli, and K. N. Fish
Endoplasmic Reticulum Export Site Formation and Function in Dendrites
J. Neurosci., April 14, 2004; 24(15): 3770 - 3776.
[Abstract] [Full Text] [PDF]
Z. Ren, N. J. Riley, L. A. Needleman, J. M. Sanders, G. T. Swanson, and J. Marshall
Cell Surface Expression of GluR5 Kainate Receptors Is Regulated by an Endoplasmic Reticulum Retention Signal
J. Biol. Chem., December 26, 2003; 278(52): 52700 - 52709.
[Abstract] [Full Text] [PDF]
J. Shan, T. P. Munro, E. Barbarese, J. H. Carson, and R. Smith
A Molecular Mechanism for mRNA Trafficking in Neuronal Dendrites
J. Neurosci., October 1, 2003; 23(26): 8859 - 8866.
[Abstract] [Full Text] [PDF]
J. Bi, X. Hu, H. H. Loh, and L.-N. Wei
Mouse {kappa}-Opioid Receptor mRNA Differential Transport in Neurons
Mol. Pharmacol., September 1, 2003; 64(3): 594 - 599.
[Abstract] [Full Text] [PDF]
A. C. Horton and M. D. Ehlers
Dual Modes of Endoplasmic Reticulum-to-Golgi Transport in Dendrites Revealed by Live-Cell Imaging
J. Neurosci., July 16, 2003; 23(15): 6188 - 6199.
[Abstract] [Full Text] [PDF]
H. Wang, A. Iacoangeli, S. Popp, I. A. Muslimov, H. Imataka, N. Sonenberg, I. B. Lomakin, and H. Tiedge
Dendritic BC1 RNA: Functional Role in Regulation of Translation Initiation
J. Neurosci., December 1, 2002; 22(23): 10232 - 10241.
[Abstract] [Full Text] [PDF]
E. Mohr, N. Prakash, K. Vieluf, C. Fuhrmann, F. Buck, and D. Richter
Vasopressin mRNA localization in nerve cells: Characterization of cis-acting elements and trans-acting factors
PNAS, June 19, 2001; 98(13): 7072 - 7079.
[Abstract] [Full Text] [PDF]
J. Eberwine, K. Miyashiro, J. E. Kacharmina, and C. Job
Local translation of classes of mRNAs that are targeted to neuronal dendrites
PNAS, June 19, 2001; 98(13): 7080 - 7085.
[Abstract] [Full Text] [PDF]
I. S. Moon, I. S. Park, L. T. Schenker, M. B. Kennedy, J.-I. Moon, and I. Jin
Presence of both Constitutive and Inducible Forms of Heat Shock Protein 70 in the Cerebral Cortex and Hippocampal Synapses
Cereb Cortex, March 1, 2001; 11(3): 238 - 248.
[Abstract] [Full Text] [PDF]
E. Koenig, R. Martin, M. Titmus, and J. R. Sotelo-Silveira
Cryptic Peripheral Ribosomal Domains Distributed Intermittently along Mammalian Myelinated Axons
J. Neurosci., November 15, 2000; 20(22): 8390 - 8400.
[Abstract] [Full Text] [PDF]
J. E. Kacharmina, C. Job, P. Crino, and J. Eberwine
Stimulation of glutamate receptor protein synthesis and membrane insertion within isolated neuronal dendrites
PNAS, October 10, 2000; 97(21): 11545 - 11550.
[Abstract] [Full Text] [PDF]
C. R. Raymond, V. L. Thompson, W. P. Tate, and W. C. Abraham
Metabotropic Glutamate Receptors Trigger Homosynaptic Protein Synthesis to Prolong Long-Term Potentiation
J. Neurosci., February 1, 2000; 20(3): 969 - 976.
[Abstract] [Full Text] [PDF]
Y. Ouyang, A. Rosenstein, G. Kreiman, E. M. Schuman, and M. B. Kennedy
Tetanic Stimulation Leads to Increased Accumulation of Ca2+/Calmodulin-Dependent Protein Kinase II via Dendritic Protein Synthesis in Hippocampal Neurons
J. Neurosci., September 15, 1999; 19(18): 7823 - 7833.
[Abstract] [Full Text] [PDF]
M. E. Rubio and R. J. Wenthold
Differential Distribution of Intracellular Glutamate Receptors in Dendrites
J. Neurosci., July 1, 1999; 19(13): 5549 - 5562.
[Abstract] [Full Text] [PDF]
A. Gardiol, C. Racca, and A. Triller
Dendritic and Postsynaptic Protein Synthetic Machinery
J. Neurosci., January 1, 1999; 19(1): 168 - 179.
[Abstract] [Full Text] [PDF]
F. Angenstein, W. T. Greenough, and I. J. Weiler
Metabotropic glutamate receptor-initiated translocation of protein kinase p90rsk to polyribosomes: A possible factor regulating synaptic protein synthesis
PNAS, December 8, 1998; 95(25): 15078 - 15083.
[Abstract] [Full Text] [PDF]
I. A. Muslimov, G. Banker, J. Brosius, and H. Tiedge
Activity-dependent Regulation of Dendritic BC1 RNA in Hippocampal Neurons in Culture
J. Cell Biol., June 29, 1998; 141(7): 1601 - 1611.
[Abstract] [Full Text] [PDF]
E. Tongiorgi, M. Righi, and A. Cattaneo
Activity-Dependent Dendritic Targeting of BDNF and TrkB mRNAs in Hippocampal Neurons
J. Neurosci., December 15, 1997; 17(24): 9492 - 9505.
[Abstract] [Full Text] [PDF]
A. H. Gazzaley, D. L. Benson, G. W. Huntley, and J. H. Morrison
Differential Subcellular Regulation of NMDAR1 Protein and mRNA in Dendrites of Dentate Gyrus Granule Cells after Perforant Path Transection
J. Neurosci., March 15, 1997; 17(6): 2006 - 2017.
[Abstract] [Full Text] [PDF]
C. Racca, A. Gardiol, and A. Triller
Dendritic and Postsynaptic Localizations of Glycine Receptor alpha Subunit mRNAs
J. Neurosci., March 1, 1997; 17(5): 1691 - 1700.
[Abstract] [Full Text] [PDF]
C. Job and J. Eberwine
From the Cover: Identification of sites for exponential translation in living dendrites
PNAS, November 6, 2001; 98(23): 13037 - 13042.
[Abstract] [Full Text] [PDF]
This Article Abstract 
Full Text (PDF) Submit an eLetter Alert me when this article is cited Alert me when eLetters are posted Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in Web of Science Similar articles in PubMed Alert me to new issues of the journal Download to citation manager 
Citing Articles Citing Articles via HighWire Citing Articles via Web of Science (109) Citing Articles via Google Scholar Google Scholar Articles by Torre, E. R. Articles by Steward, O. Search for Related Content PubMed PubMed Citation Articles by Torre, E. R. Articles by Steward, O. Pubmed/NCBI databases
Compound via MeSH
Hazardous Substances DB
ABSTRACT
|
|
|
|
 |
|