 |
|||||
|
|||||
|
|||||
|
|||||
|
|||||
Previous Article | Next Article
The Journal of Neuroscience, June 1, 2002, 22(11):4293-4301
Transport of Neuronal BC1 RNA in Mauthner Axons
Ilham A. Muslimov1, Margaret Titmus3, Edward Koenig3, and Henri Tiedge1, 2 Departments of 1 Physiology and Pharmacology and 2 Neurology, State University of New York, Health Science Center at Brooklyn, Brooklyn, New York 11203, and 3 Department of Physiology and Biophysics, State University of New York at Buffalo, Buffalo, New York 14214
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
In neurons, localized RNAs have been identified in dendrites and axons; however, RNA transport in axons remains poorly understood. Here we analyzed axonal RNA transport in goldfish Mauthner neurons in vivo. BC1 RNA, a noncoding RNA polymerase III transcript that is targeted to dendrites in neurons of the rodent nervous system, was used as a probe for axonal RNA transport. Somata of Mauthner neurons were microinjected with various RNAs. Full-length BC1 RNA, but not control RNAs of similar length, was targeted to both axons and dendrites of Mauthner neurons. BC1 RNA was transported in the form of a rapidly advancing wave front that progressed along axons, in a microtubule-dependent manner, at a rate of 2 µm/sec. Whereas a BC1 5' segment of 65 nucleotides was transported to axons and dendrites in a way indistinguishable from full-length BC1 RNA, a BC1 3' segment of 60 nucleotides did not enter Mauthner cell processes to any significant extent. In the wake of the wave advancing through the axon, BC1 RNA was found localized to discrete, spatially delimited domains at the axonal surface. Such demarcated cortical concentrations of BC1 RNA could not be observed after disruption of F-actin organization in the axon. It is concluded that the specific delivery of BC1 RNA to spatially defined axonal target sites is a two-step process that requires the sequential participation of microtubules for long-range axial transport and of actin filaments for local radial transfer and focal accumulation in cortical domains.
Key words: fast axonal transport; RNA localization; targeting element; axons; Mauthner neurons; microinjection
INTRODUCTION
RNA transport and localization have been recognized as important mechanisms for plasticity and pattern formation in various eukaryotic cell types. In neurons, the targeted delivery of RNAs to sites of local translation in dendrites has been implicated in the long-term modulation of synaptic form and function (for review, see Kindler et al., 1997
; Tiedge et al., 1999
Use of diverse experimental systems to investigate axonal RNA localization may have contributed to some of this controversy. In invertebrates (e.g., squid) and lower vertebrates (e.g., fish), RNAs have been identified in various axonal preparations (for review, see van Minnen, 1994
-actin mRNA has been shown to be transported to, and localized at, axonal growth cones in developing mammalian neurons in culture (Bassell et al., 1998
Whereas local protein synthesis has been documented in immature axons (Eng et al., 1999
Despite increasing evidence for the presence of RNAs in the axonal domain, however, little is known about targeted transport of RNAs along axons (Job and Eberwine, 2001
MATERIALS AND METHODS
RNA preparation. RNA was in vitro transcribed in the presence of 35S-UTP. Full-length BC1 RNA [152 nucleotides (nt)] and a 5' segment of BC1 RNA (nt 1-65) were generated from plasmid pBCX607 as described previously (Muslimov et al., 1997
Microinjection of radiolabeled RNAs into Mauthner neurons in vivo. Goldfish (Carassius auratis), 7-12 cm in length, were used for all experiments. Animals were purchased from a commercial supplier and housed in aquaria maintained at 20-22°C on a fixed daily light/dark cycle. In preparation for an experiment, a fish was anesthetized with 0.3 gm/l tricaine methane sulfonate (MS-222), mounted in a chamber, and immobilized with an intramuscular injection of D-tubocurarine (1-3 µg/g body weight) after the lower brainstem was exposed surgically. The fish was respired for the duration of the experiment with a continuous flow of aerated, dechlorinated tap water containing 0.15 gm/l MS-222. Glass filament electrodes, pulled from 1.5 mm tubing, were used for microinjections. Electrode tips were broken, dipped into a solution of 20 µl
-methacryloxypolytriethoxy silane in 2 ml 1-chloronaphtaline, and dried overnight at 100°C. The electrode tip was filled by suction with 35S-labeled RNA, diluted 1:4-1:20 from the transcription reaction in diethyl pyrocarbonate-treated water. Mauthner cells were injected with RNAs in systematically varying concentrations to ensure that resulting labeling profiles were independent of injected amounts. Standard amounts (dilution 1:4) were injected for all time course experiments; low amounts (dilution 1:20) were injected to reveal focal accumulations of radioactive signal in axonal areas from which the wave front had passed (see Results). Electrodes were backfilled with 1.5 M KCl and Fast Green (20 mg/l) and had an electrical resistance of 2.5-8.0 M
when measured in brain tissue.
Mauthner cell perikarya are located in the rostral medulla, and after decussating, the two large myelinated axons project the full-length of the spinal cord. In its rostral extent in goldfish, the Mauthner cell axon may vary from 40 to 80 µm in diameter (Funch et al., 1981
Local disruption of microtubules and F-actin in axoplasm. Microtubules and F-actin were disrupted by focal pressure microinjection of either 1 µM vinblastine or 10 µM cytochalasin D into one of the two Mauthner axons, ~4 mm distal to the cell body. The disrupting agent was filled at the tip and backfilled with 1.5 M KCl and Fast Green dye to monitor the effectiveness of the injection. Vinblastine, which is effective and specific in the submicromolar range, binds to free tubulin dimers (Wilson et al., 1974
Isolation of Mauthner cell axoplasmic whole mounts. Because of the content and cytoskeletal organization of neurofilaments, native axoplasm behaves as an elastic solid and can be pulled out of its myelin ensheathment as a whole mount from very large fibers (Koenig, 1986
Isolation of Mauthner cell bodies with dendrites. After axoplasmic whole mounts were isolated and attached to a slide, the tissue was transferred to 10 mM ZnOAc and 0.1 M Tris aspartate, pH 5.5, in a dish, and a brainstem slice was prepared from which Mauthner cell bodies with dendrites were isolated by hand microdissection under a stereomicroscope (Koenig and Repasky, 1985
Fixation of isolated specimens. After attachment of Mauthner cell components to the slide, the solution on the latter was drained, and the slide was immersed for 20 min in 3.75% formaldehyde (made from paraformaldehyde) buffered with 0.1 M diethylmalonic acid (Aldrich, Milwaukee, WI), adjusted to pH 7.4 with KOH. The fixative on the slide was drained, the slide was washed in 0.1 M NH4OAc thrice, and either stored in 45 mM NH4OAc (pH 4.5 with acetic acid) in 70% ethanol or immediately drained and dried for autoradiography.
Autoradiography and data evaluation. Emulsion autoradiography was performed as described previously (Tiedge, 1991
For time course experiments, standard amounts of full-length BC1 RNA or the BC1 5' segment were injected. Axonal labeling profiles were established by determining silver grain distribution patterns along axonal extents as follows. Because Mauthner somata were prepared separate from their cognate axoplasmic whole mounts, zero distance was defined as the proximal-most axonal point. The zero-distance point corresponded to the junction between the initial axon segment (which is ensheathed by a dense glial cap) and a greatly enlarged myelinated axon. Zn-denaturation transforms the viscoelastic axoplasm into a plastic solid with considerable tensile strength that retains its in situ shape after isolation of the axoplasmic whole mount. The fluid-suspended whole mount was attached to the slide in a proximal-to-distal manner to ensure consistency of axonal zero-distance points and in situ lengths. To establish labeling profiles as shown in Figure 3, evaluation points were chosen at 1 mm intervals. To establish intensity maxima of wave fronts, evaluation points were set at consecutive 100 µm intervals across the peak. At each evaluation point, silver grains were counted within a 100-µm-wide slab-like cross-section through the axoplasm.
RNA transport rates in Mauthner cell axons were established as follows. For each axon, the position of the intensity maximum of the advancing wave front was determined as described above. For any given time point, the average distance traveled by these peaks was calculated from the combined data obtained from all axons analyzed for that time point. These values were then converted into transport rates. Although the diameter of a Mauthner cell axon is somewhat variable along the axonal extent (see above), distances traveled by wave fronts at given time points were found to be independent of axonal diameter.
RESULTS
Axonal and dendritic transport of BC1 RNA in Mauthner neurons
Perikarya of goldfish Mauthner neurons were injected with full-length radiolabeled BC1 RNA in vivo. Fishes were euthanized after specified periods of time that varied between 0.5 and 4 hr, depending on the type of experiment. Whole mounts of dissected Mauthner cells with dendrites and isolated axoplasm were then attached to slides and processed as described above. Because axons from the pair of Mauthner neurons decussate and cross the midline, left and right axons were aligned with the perikaryon of the contralateral axon. As is shown in Figure 1, soma-injected full-length BC1 RNA was delivered to both dendrites and axons of Mauthner cells. Significant labeling could be observed in the cell body, the dendrites, and along the axon of injected cells. Labeling extended to distal dendrites after a 2 hr post-injection period. Axons were labeled at substantial distances from the cell body, indicating that axonal delivery of BC1 RNA was rapid (see below for details).
View larger version (71K):[in this window]
[in a new window]
Figure 1. Transport and localization of microinjected BC1 RNA in Mauthner neurons. A-D, Full-length radiolabeled BC1 RNA was injected into the perikarya of Mauthner cells in vivo (total number of cells injected: 55). A, Two hours after injection, labeling signal was substantial over cell body (arrowhead) and dendrites, including distal dendritic regions (arrows). B, Significant labeling for BC1 RNA was apparent in the axoplasmic whole mount of the same cell. Photomicrograph was taken at a distance of 10 mm from soma. (The distance at this time point corresponds to the rear slope of the advancing wave, as shown in Fig. 3B.) The appearance of the labeling signal at this position was patchy to uniform. C, D, Focal accumulations of BC1 labeling signal (arrowheads) were revealed in the wake of the advancing front in axons. For these experiments, injection amounts were lowered below the typical amounts by a factor of 5 to ensure that labeling in the trailing part of the advancing wave would not obscure BC1 foci. E-H, Mauthner neurons were injected with an irrelevant-sequence RNA of 144 nt (E, F; number of cells injected: 4) or with nuclear U4 RNA (G, H; number of cells injected: 8). Post-injection intervals were 2 hr. Although injected somata were strongly labeled (E, G, arrowheads), no significant labeling was detected either in dendrites (E, G, arrows), except for a proximal-most region, or in axoplasmic whole mounts (F, H; distance from soma: 10 mm). Arrowheads in F indicate axonal boundaries. Please note that although Mauthner neurons typically have two dendrites, one may be lost during dissection. Scale bar (shown in G): A, E, G, 100 µm; B-D, F, H, 50 µm.
The BC1 labeling signal was nonuniformly distributed along the axon. Within the extent of the axon that was labeled, the distal-most area exhibited highest relative signal intensities in the form of a peak (attributable to an advancing wave front of transported RNA; see below). In this peak area, the labeling signal was high and appeared in patchy to uniform distribution (Fig. 1B). In more proximal regions, the labeling signal was still significant, but lower than in the peak area. When low concentrations of BC1 RNA (see Materials and Methods) were injected, radioactivity in this proximal-intermediate area (i.e., in the wake of the advancing wave front) was typically restricted to distinct superficial areas (Fig. 1C,D). Such focal concentrations of BC1 labeling indicate that radioactive BC1 RNA had accumulated in discrete, spatially circumscribed cortical domains of the axon.
Dendritic and axonal transport of BC1 RNA in Mauthner neurons was specific. This was demonstrated by injecting Mauthner neurons in vivo with RNAs of similar lengths but irrelevant sequences. A 144 nt RNA of irrelevant polylinker sequence (pSL300) (Brosius, 1989
Taken together, the results show that BC1 RNA is rapidly and selectively transported to axons and dendrites of goldfish Mauthner neurons. The data further indicate that BC1 RNA is specifically recognized by the RNA transport machinery of Mauthner cells, and they prompt the question as to whether BC1 RNA contains a cis-acting element that would mediate such recognition.
A cis-acting axonal and dendritic targeting element in the BC1 5' domain
In rat sympathetic neurons, a BC1 5' segment of no more than 65 nucleotides has been shown previously to be competent to direct dendritic targeting, whereas BC1 3' sequences were found to be targeting-incompetent (Muslimov et al., 1997
View larger version (68K):[in this window]
[in a new window]
Figure 2. Transport competence of the BC1 5' domain in Mauthner neurons. Mauthner cell perikarya were injected in vivo with a BC1 5' segment (A, B; number of cells injected: 46), a BC1 3' segment (C, D; number of cells injected: 27), or a 64 nt irrelevant-sequence RNA (E, F; number of cells injected: 5). Post-injection intervals were 2 hr. A, C, E, Somata/dendrites (arrows indicate dendrites; arrowheads indicate somata); B, D, F, axoplasmic whole mounts (photographed at 10 mm distance from somata). Microinjection of the BC1 5' segment resulted in labeling of somata and dendrites (A) as well as along axoplasmic whole mounts (B). Superficial accumulations of silver grains in cortical axonal domains were revealed after injection of low amounts of the BC1 5' segment (B, inset). After injection of a BC1 3' segment (C, D), no significant labeling was observed along either dendrites (C) or axons (D; arrowheads indicate axonal boundaries). Likewise, injection of a 64 nt irrelevant-sequence RNA did not produce any significant dendritic (E) or axonal labeling (F). Scale bar (shown in E): A, C, E, 100 µm; B, D, F, 50 µm.
View larger version (28K):[in this window]
[in a new window]
Figure 3. Time-dependent proximo-distal translocation of BC1 RNA along Mauthner cell axons. A, Labeling profiles as determined 1 hr after injection into Mauthner somata. Light gray bars indicate full-length BC1 RNA; 24 axons were analyzed. Dark gray bars indicate BC1 5' segment; 15 axons were analyzed. An additional evaluation point (data not shown) was at 0.5 mm, with signal intensities not significantly different from the subsequent three evaluation points. Signal intensities (relative units) were determined at each evaluation point as described in Materials and Methods. From the combined data for full-length BC1 RNA, we calculated the average position of the labeling peak maximum after 1 hr as 7900 ± 789 µm (mean ± SEM). The corresponding average transport velocity was 2.2 ± 0.2 µm/sec. For the BC1 5' segment, the respective numbers were 7817 ± 689 µm, again yielding an average transport velocity of 2.2 ± 0.2 µm/sec. B, Profiles of axonal labeling signals at four additional time points after somatic injection of full-length BC1 RNA. Signal intensities were defined and calculated as in A. C, Synoptic compilation of axonal labeling profiles generated by somatic injection of full-length BC1 RNA. The number of axons analyzed per time point are as follows: 0.5 hr, 2; 1 hr, 24; 1.5 hr, 10; 2 hr, 28; 2.5 hr, 18; 3 hr, 16; 4 hr, 6. Error bars have been omitted for clarity. Transport rates were calculated for four time points and are given in the format mean ± SEM in the inset.
In contrast to full-length BC1 RNA or the BC1 5' segment, somatic injection of a BC1 3' segment (60 nt) did not result in any significant axonal labeling (Fig. 2D), although the soma was strongly labeled (Fig. 2C). Dendrites were not labeled, except for a low-level signal in dendritic segments immediately proximal to the soma. The central region of BC1 RNA, a stretch of 22 consecutive A-residues, was not analyzed for targeting competence. It should be noted that the subcellular labeling patterns after BC1 and control injections were independent of the amounts injected. For instance, injection of low amounts of the BC1 5' segment still resulted in significant axonal labeling (Fig. 2B). On the other hand, injection of standard amounts of a BC1 3' segment did not result in any noticeable "spillover" into dendritic (Fig. 2C) or axonal (Fig. 2D) compartments. Injected control RNAs, such as a 64 nt RNA of irrelevant sequence or nuclear U6 RNA, did not produce any significant dendritic or axonal signal at standard-level injection routines that resulted in strongly labeled cell bodies (Fig. 2E,F) (and data not shown).
We conclude from these results that BC1 RNA contains, within a 5' segment of no more than 65 nt, a cis-acting targeting element that is sufficient to specify both axonal and dendritic BC1 transport in goldfish Mauthner neurons. The same 5' segment has been shown previously to contain a targeting element that is responsible for dendritic BC1 transport in rat sympathetic neurons (Muslimov et al., 1997
High velocity of axonal BC1 transport in Mauthner neurons
To determine the velocity of BC1 transport in Mauthner cell axons, we adopted a modified classical pulse-labeling paradigm used to measure rapid axonal transport in the cat (Ochs, 1972
The distribution profile 1 hr after injection showed an advancing wave front at ~8 mm distal from the soma (Fig. 3A). The signal distribution produced by injection of the BC1 5' segment was very similar to that obtained after injection of full-length BC1 RNA. The labeling profiles suggest that injected BC1 RNA, and the BC1 5' segment, leave the soma and are translocated along the axon in the form of a wave with a diminishing disto-proximal gradient trailing the peak. It was in such regions proximal to the peak that labeling could be observed in the form of spatially restricted focal domains, after low-level injections as described above (Figs. 1, 2). The data thus indicate that these domains are in a region of the axon from which the mobile radioactive front had been cleared, thereby revealing the focal accumulations of the RNA in cortical periaxoplasmic domains.
The axonal BC1 labeling pattern was typical, as is apparent from a compilation of axonal labeling profiles taken at various time points (Fig. 3B,C). The wave front, in particular the trailing slope, becomes broader as it advances along the axon and its height decreases. From the data shown in Figure 3, we calculated the average velocity of the wave front advancing along the axon as 2 µm/sec (Fig. 3C). This rate was found to be identical for full-length BC1 RNA and for the BC1 5' segment. Transport of BC1 RNA along Mauthner cell axons can therefore be classified as rapid, with rates comparable to those of fast axonal transport in mammals.
Axonal transport and localization of BC1 RNA: roles of cytoskeletal systems
A simple interpretation of the above data would suggest that BC1 RNA is rapidly transported along Mauthner axons and concurrently localized (i.e., "docked") in distinct cortical domains along the axonal extent. The high velocity of anterograde BC1 translocation suggests a role for fast, microtubule-based molecular motors in axonal BC1 transport. To test this hypothesis, we investigated which cytoskeletal components were requisite for such transport. We addressed this question by direct focal microinjection of selective cytoskeletal disrupting drugs into Mauthner axons.
We first examined whether axonal BC1 transport depended on intact microtubules. Vinblastine, a microtubule-disrupting agent that is specific and effective in the submicromolar range, was microinjected intra-axonally at a distance of 4 mm from the soma. BC1 RNA was microinjected into the soma of the same cell before intra-axonal vinblastine injection (time differential 20 ± 5 min). Axons as well as somata with dendrites were isolated and fixed 1 hr after BC1 injections. In these experiments (Fig. 4A-C), BC1 RNA was detected at substantial levels in the area of the axon that was proximal to the vinblastine injection site (Fig. 4B). In sharp contrast, only negligible labeling was observed at a point 8 mm distal from the soma (Fig. 4C), an area where the advancing peak of radioactivity was ordinarily detected under standard non-vinblastine conditions after 1 hr. Quantitative analysis revealed that BC1 signal intensities were significant along the axonal extent up to ~3-4 mm distal from the cell body, at which point the signal decreased precipitously (Fig. 5A,B). This result contrasted with the situation in control injections (Fig. 3A) in which the peak of the wave front had progressed to ~8 mm after 1 hr. The data thus indicate that intra-axonal microinjection of vinblastine effectively creates a barrier through which soma-injected BC1 RNA cannot traverse.
View larger version (64K):[in this window]
[in a new window]
Figure 4. Cytoskeletal systems implicated in the transport and localization of BC1 RNA in Mauthner axons. Radiolabeled BC1 RNA was microinjected into the Mauthner cell body, followed by microinjection of a cytoskeletal disrupting agent at a distance of 4 mm from the soma (time differential: 20 ± 5 min). The tissue was fixed 1 hr after injection of BC1 RNA, a time when the peak of the wave front was normally located at 8 mm distal to the soma. Axons and perikaryra were then isolated and processed as described in Materials and Methods. A-C, Vinblastine (1 µM), which disrupts microtubules, was injected into the axon (7 axons analyzed). A robust labeling signal was observed in dendrites (A) and in the axonal segment proximal to the vinblastine injection site (B; showing an area at a distance of 3.5 mm from the soma). No significant labeling was observed distal to the vinblastine injection site (C; showing an area at a distance of 8 mm from the soma). D-F, Cytochalasin D (10 µM), a specific F-actin depolymerizing agent, was injected intra-axonally (7 axons analyzed). Dendrites were again labeled (D). In the axon, BC1 labeling appeared in form of a peak at 8 mm (F) where it was restricted to the axoplasmic core (F, arrows). At times, labeling in this peak area was "trail-like" in appearance (F, inset). No significant labeling was observed in axonal areas proximal to the peak (E; distance from soma is 1 mm). Arrows in A and D indicate labeled dendrites. Arrowheads indicate axonal circumferences. Scale bar (shown in A): A, D, 100 µm; B, C, E, F, 50 µm. G, Schematic diagram depicts the approximate location of the Mauthner cells (M-cell) in the rostral medulla and the distribution of their axons (M-axon) in the spinal cord. The corresponding diagram (H) shows the injection sites of vinblastine (vinbl) and cytochalasin D (cyt D), as well as the relative locations of regions illustrated in photomicrographs A-F.
View larger version (23K):[in this window]
[in a new window]
Figure 5. Inhibition by vinblastine of anterograde BC1 translocation in Mauthner axons. Cells were fixed 1 hr after injection of BC1 RNA. A, B, Intrasomatic injection of BC1 RNA was followed after 20 min (±5 min) by intra-axonal injection of vinblastine at a distance of 4 mm from the soma (arrowheads). Two examples (of 7 experiments) are shown. Results were not averaged in these experiments because time intervals between intrasomatic and intra-axonal injections could not be controlled precisely and were therefore variable. C, Intrasomatic injection of BC1 RNA was followed after 20 min (±5 min) by intra-axonal injection of cytochalasin D at a distance of 4 mm from the soma (arrowheads). In three of seven cases, a low but significant signal was observed in the extreme proximal axonal area, directly adjacent to the soma. D, Intra-axonal injection of BC1 RNA (4 mm distal from cell body; arrowhead) produced a wave-like labeling pattern with a peak at 11 mm, indicating an anterograde translocation of the RNA at a velocity comparable to the rates observed in Figure 3.
As a control, and to probe for any involvement of actin filaments in axonal BC1 transport or localization, parallel experiments were performed with cytochalasin D. Cytochalasin D has been used extensively to disrupt actin filaments in living cells, a process that involves an energy-dependent and myosin-driven collapse of the actin network into focal aggregates (Schliwa, 1982
Notwithstanding such similarity of axonal labeling profiles, comparison of intra-axonal signal distribution revealed clear differences between cytochalasin D experiments (Fig. 4D-F) and standard experiments (Fig. 1). In standard experiments, BC1 labeling signal was observed in discrete cortical domains of the axon in areas posterior to the advancing wave front. In contrast, no such cortical concentrations of BC1 labeling were observed in cytochalasin D experiments. Indeed, the axonal extent posterior to the advancing wave was devoid of any significant BC1 labeling in the latter case (Figs. 4E, 5C). These results indicate that BC1 RNA fails to localize to cortical domains in the presence of cytochalasin D. In further support for this view, we observed that in the peak area representing the advancing wave, BC1 labeling signal remained concentrated in the central domain of the whole mount and was mostly excluded from the cortical regions (Fig. 4F). At times, such central axoplasmic BC1 labeling had a distinctive trail-like appearance (Fig. 4F, inset). It thus appears that in the presence of cytochalasin D, BC1 RNA is rapidly transported along the axonal extent but fails to reach cortical axonal domains.
In additional control experiments, BC1 RNA was microinjected intra-axonally at a distance of 4 mm from the cell body. Again, this produced an anterogradely directed wave front, which now peaked at a distance of ~11 mm after 1 hr (Fig. 5D). These experiments demonstrate that intra-axonal microinjection, as such, does not compromise the transport capacity of the axon. Remarkably, both full-length BC1 RNA and the BC1 5' domain, injected intra-axonally, were transported anterogradely at the same rate; in contrast, the BC1 3' domain was not transported after intra-axonal injection (data not shown). The results also suggest that trans-acting factors of the microtubule-based molecular transport machinery are ubiquitously available in the Mauthner axon for functional interactions with BC1 RNA.
On the basis of the foregoing experiments, we conclude that fast axonal transport of BC1 RNA in Mauthner neurons is dependent on the integrity of microtubules. Actin filaments, in contrast, although not required for proximo-distal axonal transport of BC1 RNA, appear to be necessary for radial transport of the RNA and for its localization to cortical periaxoplasmic domains.
DISCUSSION
Although RNA transport in dendrites has been the subject of a number of studies in recent years, RNA transport in axons has received little attention and remains poorly understood. The fact that axonal RNA transport has so far not been examined directly reflects to a large extent the problem of studying an inaccessible, small-diameter neuronal compartment that is obscured by its ensheathment. This problem has been overcome in selected model systems, such as the squid giant axon and the goldfish Mauthner cell axon, in which it is possible to isolate axoplasm. For the purpose of this work, we elected to use the Mauthner cell, which has been used as a favorable vertebrate neuronal model system for a wide range of studies over the years. Although proximal regions of many invertebrate axons serve dendrite-like functions in providing postsynaptic junctional domains to afferents (for review, see Mohr, 1999
The data presented here show that neuronal BC1 RNA introduced into goldfish Mauthner neurons is rapidly and specifically transported to both axons and dendrites. BC1 transport in Mauthner axons is characterized by a rapidly advancing wave front, reminiscent of similarly advancing waves of radiolabeled proteins in earlier reports of fast axonal transport in mammalian nerve fibers (Ochs, 1972
The high velocity of axonal BC1 transport in Mauthner neurons led us to conjecture that fast molecular motors mediate translocation of the RNA along microtubules. This hypothesis was tested in experiments using cytoskeletal disrupting agents. Microtubules were locally disrupted in the axon by microinjections of submicromolar concentrations of vinblastine to test whether the BC1 wave front would be arrested in its advance along the axon. Indeed, as BC1 was transported into the axon, it accumulated proximal to the vinblastine injection region. The action of vinblastine thus produced a blockade of axonal BC1 transport, a result consistent with the assumption that long-range transport of BC1 RNA in Mauthner axons is dependent on intact microtubules. Intra-axonal microinjection of cytochalasin D, in contrast, did not block BC1 transport; however, localization of the RNA to discrete cortical periaxoplasmic domains was eliminated.
On the basis of these results, we suggest that the targeted delivery of BC1 RNA to local axonal sites is a two-step process. In the first step, long-range fast axial transport of the RNA is mediated by microtubules. Given that axonal microtubules are uniformly oriented with their plus ends distal to the soma (Heidemann et al., 1981
A BC1 5' domain of no more than 65 nucleotides, previously shown to be responsible for dendritic BC1 transport in mammalian neurons (Muslimov et al., 1997
The results also support the conjecture that the cis-acting targeting element that is contained within the BC1 5' domain is recognized by molecular RNA delivery systems in both axons and dendrites. BC1 RNA has been shown previously to be transported along axons of hypothalamic neurons to the posterior lobe of the pituitary (Tiedge et al., 1993b
BC1 RNA is transported along Mauthner axons to be localized to discrete, spatially restricted domains at the axonal surface. Dimensions, contours, and in particular the typical location of such BC1 target domains at the axoplasmic surface are of striking resemblance to ribosomal periaxoplasmic plaque domains (Koenig and Martin, 1996
A role in translational regulation is also entertained in mammalian dendrites (Brosius and Tiedge, 2001
We conclude by paying homage to A. Goldscheider, who more than 100 years ago first proposed that there is "an actual transport of a material" from the cell body "along the whole course of the axone to its extremity" [as quoted by Barker (1899)
FOOTNOTES Received Jan. 14, 2002; revised March 4, 2002; accepted March 12, 2002.
This work was supported in part by a grant from the New York City Council Speaker's Fund For Biomedical Research (I.A.M.), by National Science Foundation Grants IBN 9604841 and IBN 0118368 (E.K.), and by National Institutes of Health Grant NS34158 (H.T.).
Correspondence should be addressed to Henri Tiedge, Department of Physiology and Pharmacology, State University of New York, Health Science Center at Brooklyn, 450 Clarkson Avenue, Brooklyn, NY 11203. E-mail: tiedge{at}hscbklyn.edu.
REFERENCES
- Alvarez J, Giuditta A, Koenig E (2000) Protein synthesis in axons and terminals: significance for maintenance, plasticity and regulation of phenotype. With a critique of slow transport theory. Prog Neurobiol 62:1-62[Web of Science][Medline].
- Baas PW, Ahmad FJ (1993) The transport properties of axonal microtubules establish their polarity orientation. J Cell Biol 120:1427-1437
[Abstract/Free Full Text] .- Banker K, Goslin K (1998) In: Culturing nerve Cells. Cambridge, MA: MIT.
- Barker LF (1899) In: The nervous system and its constituent neurons. New York: D. Appleton and Company.
- Bassell GJ, Zhang H, Byrd AL, Femino AM, Singer RH, Taneja KL, Lifshitz LM, Herman IM, Kosik KS (1998) Sorting of
[Abstract/Free Full Text] .- Bleher R, Martin R (2001) Ribosomes in the squid giant axon. Neuroscience 107:527-534[Web of Science][Medline].
- Brosius J (1989) Superpolylinkers in cloning and expression vectors. DNA 8:759-777[Web of Science][Medline].
- Brosius J, Tiedge H (2001) Dendritic BC1 RNA: intracellular transport and activity-dependent expression. In: Cell polarity and subcellular RNA localization (Richter D, ed), pp 129-138. Berlin: Springer.
- Brown SS (1999) Cooperation between microtubule- and actin-based motor proteins. Annu Rev Cell Dev Biol 15:63-80[Web of Science][Medline].
- Campbell DS, Holt CE (2001) Chemotropic responses of retinal growth cones mediated by rapid local protein synthesis and degradation. Neuron 32:1013-1026[Web of Science][Medline].
- Chartrand P, Singer RH, Long RM (2001) RNP localization and transport in yeast. Annu Rev Cell Dev Biol 17:297-310[Web of Science][Medline].
- Chicurel ME, Terrian DM, Potter H (1993) mRNA at the synapse: analysis of a preparation enriched in hippocampal dendritic spines. J Neurosci 13:4054-4063[Abstract].
- Crispino M, Kaplan BB, Martin R, Alvarez J, Chun JT, Benech JC, Giuditta A (1997) Active polysomes are present in the large presynaptic endings of the synaptosomal fraction from squid brain. J Neurosci 17:7694-7702
[Abstract/Free Full Text] .- Deininger PL, Tiedge H, Kim J, Brosius J (1996) Evolution, expression, and possible function of a master gene for amplification of an interspersed repeated DNA family in rodents. In: Progress in nucleic acid research and molecular biology, Vol 52 (Cohn W, Moldave K, eds), pp 67-88. San Diego: Academic.
- Eberwine J (2001) Molecular biology of axons. "A turning point." Neuron 32:959-960[Medline].
- Edmonds BT, Koenig E (1990) ATP and calmodulin dependent actomyosin aggregates induced by cytochalasin D in goldfish retinal ganglion cell axons in vitro. J Neurobiol 21:555-566[Medline].
- Eng H, Lund K, Campenot RB (1999) Synthesis of
[Abstract/Free Full Text] .- Funch PG, Kinsman SL, Faber DS, Koenig E, Zottoli SJ (1981) Mauthner axon diameter and impulse conduction velocity decrease with growth of goldfish. Neurosci Lett 27:159-164[Medline].
- Goode BL, Drubin DG, Barnes G (2000) Functional cooperation between the microtubule and actin cytoskeletons. Curr Opin Cell Biol 12:63-71[Web of Science][Medline].
- Hausner TP, Giglio LM, Weiner AM (1990) Evidence for base-pairing between mammalian U2 and U6 small nuclear ribonucleoprotein particles. Genes Dev 4:2146-2156
[Abstract/Free Full Text] .- Heidemann SR, Landers JM, Hamborg MA (1981) Polarity orientation of axonal microtubules. J Cell Biol 91:661-665
[Abstract/Free Full Text] .- Himes RH (1991) Interactions of the catharanthus (Vinca) alkaloids with tubulin and microtubules. Pharmacol Ther 51:257-267[Web of Science][Medline].
- Job C, Eberwine J (2001) Localization and translation of mRNA in dendrites and axons. Nat Rev Neurosci 2:889-898[Web of Science][Medline].
- Kindler S, Mohr E, Richter D (1997) Quo vadis: extrasomatic targeting of neuronal mRNAs in mammals. Mol Cell Endocrinol 128:7-10[Web of Science][Medline].
- Koenig E (1986) Isolation of native Mauthner cell axoplasm and an analysis of organelle movement in non-aqueous and aqueous media. Brain Res 398:288-297[Web of Science][Medline].
- Koenig E (1991) Evaluation of local synthesis of axonal proteins in the goldfish Mauthner cell axon and axons of dorsal and ventral roots of the rat in vitro. Mol Cell Neurosci 2:384-394.
- Koenig E, Adams P (1982) Local protein synthesizing activity in axonal fields regenerating in vitro. J Neurochem 39:386-400[Web of Science][Medline].
- Koenig E, Giuditta A (1999) Protein-synthesizing machinery in the axon compartment. Neuroscience 89:5-15[Web of Science][Medline].
- Koenig E, Martin R (1996) Cortical plaque-like structures identify ribosome-containing domains in the Mauthner cell axon. J Neurosci 15:1400-1411.
- Koenig E, Repasky EA (1985) A regional analysis of
-spectrin in the isolated Mauthner neuron and in isolated axons of the goldfish and rabbit. J Neurosci 5:705-714[Abstract].
- Koenig E, Martin R, Titmus M, Sotelo-Silveira JR (2000) Cryptic peripheral ribosomal domains distributed intermittently along mammalian myelinated axons. J Neurosci 20:8390-8400
[Abstract/Free Full Text] .- Lin Y, Brosius J, Tiedge H (2001) Neuronal BC1 RNA: co-expression with growth-associated protein-43 messenger RNA. Neuroscience 103:465-479[Web of Science][Medline].
- MacLean-Fletcher S, Pollard TD (1980) Mechanism of action of cytochalasin B on actin. Cell 20:329-341[Web of Science][Medline].
- Martin R, Vaida B, Bleher R, Crispino M, Giuditta A (1998) Protein synthesizing units in presynaptic and postsynaptic domains of squid neurons. J Cell Sci 111:3157-3166[Abstract].
- Mohr E (1999) Subcellular RNA compartmentalization. Prog Neurobiol 57:507-525[Web of Science][Medline].
- Muslimov IA, Santi E, Homel P, Perini S, Higgins D, Tiedge H (1997) RNA transport in dendrites: a cis-acting targeting element is contained within neuronal BC1 RNA. J Neurosci 17:4722-4733
[Abstract/Free Full Text] .- Muslimov IA, Banker G, Brosius J, Tiedge H (1998) Activity-dependent regulation of dendritic BC1 RNA in hippocampal neurons in culture. J Cell Biol 141:1601-1611
[Abstract/Free Full Text] .- Ochs S (1972) Rate of fast axoplasmic transport in mammalian nerve fibres. J Physiol (Lond) 227:627-645
[Abstract/Free Full Text] .- Rand K, Yisraeli J (2001) RNA localization in Xenopus oocytes. In: Cell polarity and subcellular RNA localization (Richter D, ed), pp 157-173. Berlin: Springer.
- Rao A, Steward O (1993) Evaluation of RNAs present in synaptodendrosomes: dendritic, glial, and neuronal cell body contribution. J Neurochem 61:835-844[Web of Science][Medline].
- Rozhdestvensky T, Kopylov A, Brosius J, Hüttenhofer A (2001) Neuronal BC1 RNA structure: evolutionary conversion of a tRNAAla domain into an extended stem-loop structure. RNA 7:1-9[Medline].
- Schliwa M (1982) Action of cytochalasin D on cytoskeletal networks. J Cell Biol 92:79-91
[Abstract/Free Full Text] .- Silveira-Sotelo JR, Koenig E (2000) Localization of
- Tiedge H (1991) The use of UV light as a cross-linking agent for cells and tissue sections in in situ hybridization. DNA Cell Biol 10:143-147[Web of Science][Medline].
- Tiedge H, Fremeau Jr RT, Weinstock PH, Arancio O, Brosius J (1991) Dendritic location of neural BC1 RNA. Proc Natl Acad Sci USA 88:2093-2097
[Abstract/Free Full Text] .- Tiedge H, Chen W, Brosius J (1993a) Primary structure, neural-specific expression, and dendritic location of human BC200 RNA. J Neurosci 13:2382-2390[Abstract].
- Tiedge H, Zhou A, Thorn NA, Brosius J (1993b) Transport of BC1 RNA in hypothalamo-neurohypophyseal axons. J Neurosci 13:4114-4219[Abstract].
- Tiedge H, Bloom FE, Richter D (1999) RNA, wither goest thou? Science 283:186-187
[Free Full Text] .- Trembleau A, Melia KR, Bloom FE (1995) BC1 RNA and vasopressin mRNA in rat neurohypophysis: axonal compartmentalization and differential regulation during dehydration and rehydration. Eur J Neurosci 7:2249-2260[Web of Science][Medline].
- van Minnen J (1994) RNA in the axonal domain: a new dimension in neuronal functioning? Histochem J 26:377-391[Web of Science][Medline].
- Wilson L, Bamburg JR, Mizel SB, Grisham LM, Creswell KM (1974) Interaction of drugs with microtubule proteins. Fed Proc 33:158-166[Web of Science][Medline].
- Yisraeli JK, Sokol S, Melton DA (1990) A two-step model for the localization of maternal mRNA in Xenopus oocytes: involvement of microtubules and microfilaments in the translocation and anchoring of Vg1 mRNA. Development 108:289-298[Abstract].
- Zhang HL, Eom T, Oleynikov Y, Shenoy SM, Liebelt DA, Dictenberg JB, Singer RH, Bassell GJ (2001) Neurotrophin-induced transport of a
- Zheng JQ, Kelly TK, Chang B, Ryazantsev S, Rajasekaran AK, Martin KC, Twiss JL (2001) A functional role for intra-axonal protein synthesis during axonal regeneration from adult sensory neurons. J Neurosci 21:9291-9303
[Abstract/Free Full Text] .- Zottoli SJ (1978) Comparative morphology of the Mauthner cell in fish and amphibians. In: Neurobiology of the Mauthner cell (Faber DS, Korn H, eds), pp 13-45. New York: Raven.
Copyright © 2002 Society for Neuroscience 0270-6474/02/22114293-09$05.00/0
This article has been cited by other articles:
A. Giuditta, J. Tai Chun, M. Eyman, C. Cefaliello, A. P. Bruno, and M. Crispino
Local Gene Expression in Axons and Nerve Endings: The Glia-Neuron Unit
Physiol Rev, April 1, 2008; 88(2): 515 - 555.
[Abstract] [Full Text] [PDF]
I. A. Muslimov, V. Nimmrich, A. I. Hernandez, A. Tcherepanov, T. C. Sacktor, and H. Tiedge
Dendritic Transport and Localization of Protein Kinase M{zeta} mRNA: IMPLICATIONS FOR MOLECULAR MEMORY CONSOLIDATION
J. Biol. Chem., December 10, 2004; 279(50): 52613 - 52622.
[Abstract] [Full Text] [PDF]
S.-K. Lee and P. J. Hollenbeck
Organization and translation of mRNA in sympathetic axons
J. Cell Sci., November 1, 2003; 116(21): 4467 - 4478.
[Abstract] [Full Text] [PDF]
J.-Y. Hu, X. Meng, and S. Schacher
Redistribution of Syntaxin mRNA in Neuronal Cell Bodies Regulates Protein Expression and Transport during Synapse Formation and Long-Term Synaptic Plasticity
J. Neurosci., March 1, 2003; 23(5): 1804 - 1815.
[Abstract] [Full Text] [PDF]
W. Ge, J. Wu, J. Zhai, Z. Nie, H. Lin, W. W. Schlaepfer, and R. Canete-Soler
Binding of p190RhoGEF to a Destabilizing Element on the Light Neurofilament mRNA Is Competed by BC1 RNA
J. Biol. Chem., November 1, 2002; 277(45): 42701 - 42705.
[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 (24) Citing Articles via Google Scholar Google Scholar Articles by Muslimov, I. A. Articles by Tiedge, H. Search for Related Content PubMed PubMed Citation Articles by Muslimov, I. A. Articles by Tiedge, H.
|
|
|
|
 |
|