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Previous Article | Next Article
Volume 17, Number 2, Issue of January 15, 1997 pp. 646-658
Copyright ©1997 Society for NeuroscienceA Transcription-Dependent Switch Controls Competence of Adult Neurons for Distinct Modes of Axon Growth
Deanna S. Smith1, 2 and J. H. Pate Skene1 Departments of 1 Neurobiology and 2 Genetics, Duke University Medical Center, Durham, North Carolina 27710
ABSTRACT
Although maturing neurons undergo a precipitous decline in the expression of genes associated with developmental axon growth, structural changes in axon arbors occur in the adult nervous system under both normal and pathological conditions. Furthermore, some neurons support extensive regrowth of long axons after nerve injury. Analysis of adult dorsal root ganglion (DRG) neurons in culture now shows that competence for distinct types of axon growth depends on different patterns of gene expression. In the absence of ongoing transcription, newly isolated neurons can extend compact, highly branched arbors during the first day in culture. Neurons subjected to peripheral axon injury 2-7 d before plating support a distinct mode of growth characterized by rapid extension of long, sparsely branched axons. A transition from "arborizing" to "elongating" growth occurs in naive adult neurons after ~24 hr in culture but requires a discrete period of new transcription after removal of the ganglia from the intact animal. Thus, peripheral axotomy
Key words: axon regeneration; sprouting; adult plasticity; growth cone; GAPs; axotomyby nerve crush or during removal of DRGs
INTRODUCTION
Both the nature and the extent of axon growth in the adult nervous system have been subjects of conflicting hypotheses for many years. After contacting their targets, the motile growth cones of developing axons transform over time into mature synaptic terminals with new functions and a distinct complement of proteins (Hall and Sanes, 1993
). For most neurons, this transformation includes a decrease in expression of several prominent growth cone components (Skene and Willard, 1986; Basi et al., 1987
Paradoxically, some forms of axon growth appear to be common in adult nervous systems. Subtle reorganization of terminal arbors is thought to occur throughout life and may underlie some aspects of learning and memory (Purves et al., 1987
There are several possible explanations to reconcile the striking decline in growth and growth-associated proteins with the extensive functional and structural plasticity in the adult nervous system. One proposal has been that axon remodeling in adults is restricted to specific subpopulations of neurons in which expression of major growth cone components persists throughout adult life (Skene and Willard, 1981b
Cultures of dissociated adult rat dorsal root ganglia (DRG) allowed us to determine the growth capabilities of individual adult neurons in the presence and absence of changes in gene expression elicited by nerve injury. These neurons support vigorous axon regeneration and reexpression of several growth-associated genes after peripheral nerve injury (Hoffman, 1989
Here we show that fully mature DRG neurons can support distinct modes of axon extension. Our results provide strong evidence that these modes rely on different patterns of gene expression. DRG neurons are able to extend highly branched arborizing neurites before axotomy-induced changes in gene expression and do so more robustly in response to exogenous neurotrophins and other soluble factors. However, a discrete period of new transcription after peripheral axotomy is critical in order for DRG neurons to support the rapid extension of long, sparsely branched axons. Furthermore, our results indicate that the switch from "arborizing" to "elongating" growth after peripheral axotomy is stimulated by the interruption of retrogradely transported signals activated through interactions of axons with peripheral targets. In addition, we demonstrate that central root injury does not produce the same cellular response.
MATERIALS AND METHODS
Standard DRG cultures. All chemicals were purchased from Sigma (St. Louis, MO) unless indicated otherwise. L4 and L5 ganglia were removed from adult male rats, snipped open with microdissecting scissors, and then placed in ice cold Gibco-BRL F14 medium (Life Technologies, Grand Island, NY) containing N1 additives (as described in Bottenstein and Sato, 1979
Modified DRG cultures. The effect of secreted substances and cell contact on neuritic growth by naive neurons was assayed by plating 2400-4800 neurons per coverslip instead of 800-1200
Sciatic nerve lesions. Adult rats were anesthetized by intraperitoneal injection of 0.15 ml/100 gm ketamine followed by 0.15 ml/100 gm 15% chloral hydrate. The left sciatic nerve was exposed at the hip by blunt dissection and crushed using fine jewelers forceps. This procedure disrupts ~70-80% of the axons emerging from L4 and L5 ganglia (Himes and Tessler, 1989
Colchicine-releasing sciatic nerve cuffs. A 10% solution of Elvax-p40 in methanol (DuPont NEN, Wilmington, DE) containing 3 mg/ml colchicine was poured into 22 × 22 mm molds that had been frozen on dry ice. The thin sheets of quick-frozen Elvax were placed at 80°C overnight to set and then stored at 4°C until used. Strips (3 mm wide) were cut from these sheets and wrapped gently but snugly around the exposed sciatic nerves of anesthetized rats, and the ends were sealed with Superglue. Incisions were closed, and after 2 d DRGs were removed and cultured as described above.
Dorsal root lesions. The dorsal roots carrying central branches of L4 and L5 DRG neurons were exposed and crushed with fine jewelers forceps ~1 cm from the ganglia. Animals were killed after 48 hr or 1 week. DRGs were dissociated and plated under standard culture conditions for 16 hr. At this time, the cultures were fixed and scored for arborizing and elongating processes as described below.
Visual and quantitative analysis of neurite outgrowth. Cultures were fixed with 4% paraformaldehyde and frequently visualized by immunoperoxidase staining (Vector Laboratories, Burlingame, CA) using monoclonal antibodies to the neuronal markers GAP-43 (Schreyer and Skene, 1991 
Fig. 6. In vitro transition from arborizing to elongating growth by naive neurons. The percentage of naive and pre-axotomized neurons with elongating (A) or arborizing (B) neurites was determined at various times after plating, using visual inspection of all neurons in each culture (circles) or by quantitative analysis of neurite length and branching frequency for randomly selected neurons, as described in Figure 4D (squares). Filled symbols represent cultures from naive ganglia, and open symbols are from pre-axotomized ganglia. Each visually derived time point (circles) represents the mean ± SD of three to seven separate experiments, with duplicate cultures in each experiment. Time points derived from quantitative analysis include 480 randomly selected naive neurons pooled from three separate experiments (squares). The onset of elongating growth is delayed for ~24 hr in naive cultures, but the subsequent emergence of elongating axons parallels the initial outgrowth from pre-axotomized neurons. Arborizing growth plateaus near 20-25% and then declines as more neurons begin to exhibit the elongating morphology.
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Fig. 7. Onset of elongation from naive neurons requires a finite period of new gene transcription after plating. A, Naive DRG cultures were exposed to DRB, a reversible inhibitor of mRNA synthesis for the indicated intervals. Neurons in both DRB-treated and untreated cultures were fixed 40 and 66 hr after plating and visually scored as arborizing (gray bars) and elongating (black bars). Early DRB treatment dramatically reduced the percentage elongating at 40 hr, but not at 66 hr. When transcription was blocked between 12 and 24 hr after plating, the effect was less pronounced, and by 24 hr after plating, neurons were no longer dependent on ongoing transcription to initiate and sustain neurite elongation. Bars represent the mean ± SD from three separate experiments with duplicate cultures in each experiment. B, Estimate of delay produced by transient DRB treatment. The percentage of neurons with elongating neurites was rescored by quantitation of length and branching frequency. Filled circles represent neurons treated with DRB for the first 12 hr; open circles represent control neurons in untreated cultures. Each data point represents the mean ± SD for three separate experiments (30 individual neurons). These data were then compared to the previously determined time course for the onset of elongation under standard conditions (solid curve, from Fig. 6B). To estimate the length of delay produced by transient DRB treatment, we displaced this curve to the right until it intersected with the data points for DRB-treated cultures. The result indicates that an initial exposure to DRB for 12 hr produces a delay in the onset of elongating growth of ~16 hr. C, The delay was not attributable to an overall decrease in protein synthesis, because transient DRB exposure for the first 12 hr after plating did not grossly alter protein synthesis measured 12 hr later, when elongating neurites begin to emerge in control but not in DRB-treated cultures.
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Fig. 4. Neurites of naive and pre-axotomized neurons define two distinct modes of axon growth. Previous axotomy in vivo influenced the growth characteristics of DRG neurons, prompting the extension of longer neurites with fewer branches during the first day in culture. The length and number of branch points were determined for the longest neurite extended by randomly selected DRG neurons from three separate experiments in which cultures had been fixed 16 hr after plating. Open symbols represent individual neurons from naive ganglia; filled symbols those from pre-axotomized ganglia. A, Naive cells plated under standard conditions (circles) or at high density, which promotes outgrowth from a majority of neurons (diamonds). B, Naive neurons cultured in the presence of schwannoma-conditioned medium (triangles) or NGF (squares). C, Pre-axotomized neurons plated under standard conditions. D, Inclusion of the transcription inhibitor DRB during dissociation and plating had no effect on length and branching. E, Data from A-C plotted on a single graph. All neurites extended by naive neurons, regardless of culture conditions, exhibit a branching frequency > 1.5 branches per 100 µm (dotted line). This line, therefore, serves as a simple objective criterion for categorizing neurons. For subsequent quantitative analysis, data points that fall above this line will be scored as "arborizing" and those that fall below the line will be scored as "elongating."
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Mixing of naive and pre-axotomized cultures. Approximately one-tenth of the cells from a naive ganglion were incubated for 1 hr in suspension with the lipophilic dye DiI (Molecular Probes, Eugene, OR). Previously axotomized neurons were labeled in a separate tube. Meanwhile, the remainder of the naive and pre-axotomized cells were plated separately under standard conditions. The DiI-labeled, naive neurons were washed several times and then dispersed onto unlabeled pre-axotomized cultures. Similarly, DiI-labeled pre-axotomized neurons were washed and dispersed onto unlabeled naive cultures. After 16 hr, the percentage of labeled neurons exhibiting arborizing or elongating neuritic morphologies was determined.
Transcriptional inhibition. The synthesis of mRNA was inhibited permanently by the addition of -amanitin (Lindell et al., 1970
RESULTS
Genes constitutively expressed in adult neurons can support robust neurite growth
To analyze the growth capabilities of adult neurons, we examined axon outgrowth from DRG neurons acutely isolated from adult rats and cultured under conditions known to support neuritic growth from these cells (Lindsay, 1988
Fig. 1. Distinct time courses of neurite outgrowth from naive and previously axotomized neurons. Neurons from L4 and L5 DRG of adult rats were dissociated and plated under standard conditions, as described in Materials and Methods. Naive neurons from uninjured animals (N) and pre-axotomized neurons the peripheral axons of which had been injured in vivo 1 week earlier (AX) were observed over time in culture. A, Neurons and neurites in typical cultures photographed 6, 16, and 40 hr after plating. Immunoperoxidase staining for GAP-43 labels all neurons and their neurites to varying degrees. Scale bar, 100 µm. B, Time course showing the percentage of neurons in naive cultures (solid line, filled circles) and pre-axotomized cultures (dashed line, open circles) that had extended neurites by the indicated times after plating. Each time point represents the mean ± SD of at least three to seven separate experiments, with duplicate cultures in each experiment.
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What was not anticipated from previous work was the extension of neurites from ~20-25% of naive DRG neurons during the first day in culture (Fig. 1). Genes constitutively expressed in vivo are sufficient to support this early outgrowth, because it was unaltered when cells were cultured in the continuous presence of either DRB (Fig. 2) or 
Fig. 2. Genes commonly expressed in intact adult neurons are sufficient to support robust axon outgrowth. A, The percentage of neurons with neurites 16 hr after plating was determined in transcriptionally active cultures (black bars) and for cultures in which mRNA synthesis was blocked by 80 µM DRB, a potent inhibitor of RNA polymerase II (gray bars). Only 20-25% of naive neurons extended neurites by 16 hr under standard conditions (STD), but the addition of NGF to the medium or use of medium condition by schwannoma cells (not shown) stimulated growth from more neurons during the same interval. Plating at 4× the standard density (HD) had a more pronounced effect. Neuritic growth stimulated by these conditions was not inhibited by continuous exposure to DRB. Neurite extension from neurons axotomized 1 week earlier by sciatic nerve crush in vivo [STD (Ax)] was also unaffected by DRB. Data represent the mean ± SD for four separate experiments with duplicate cultures in each experiment. B, Representative neurite-bearing neurons at 16 hr after plating in the absence (top row) or presence (bottom row) of DRB. C, DRB effectively inhibits mRNA synthesis in DRG cultures. At the doses used in these experiments (80 µM), uptake of [H3]uridine is inhibited >90%.
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Competence for this early growth is not restricted to a subset of DRG neurons that maintain persistent expression of any unique set of genes, because plating at higher cell density (increasing the number of neurons, Schwann cells, and fibroblasts) stimulated early neurite outgrowth from nearly 70% of naive neurons, even in the continued presence of DRB (Fig. 2). Similarly, exuberant neuritic growth could be induced by soluble factors. Medium conditioned by a schwannoma cell line (Pfeiffer and Wechler, 1972) elicited acute outgrowth from >40% of naive cells, as did the addition of NGF, one of several neurotrophins and cytokines produced by Schwann cells (Kimura et al., 1990 Altered outgrowth after axon injury in vivo
Although acutely cultured naive DRG neurons have the capacity to support neurite extension, previous peripheral axotomy dramatically alters the type of neurites these cells extend during the first day in culture. In contrast to the extensive branching and modest length of neurites extended by naive neurons (Fig. 3A), neurites extended by previously axotomized neurons tended to be very long, and they branched rarely (Fig. 3B). These long neurites often fasciculated with one another (Fig. 1A), a behavior rarely observed in naive cultures during the first day after plating. The growth cones were typically tapered, with few filopodia (Fig. 3B), and advanced rapidly over the laminin substrate. The rate of advance for individual growth cones varied over time but could reach 1.0 mm/hr (Hess et al., 1993
Fig. 3. Naive and pre-axotomized neurons extend different types of neurites in acute cultures. A, Naive adult DRG neurons after 16 hr under standard plating conditions extend neurites that are highly branched and extend over a limited radius, terminating in large, palmate growth cones with numerous filopodia. B, Neurites in 16 hr cultures from previously axotomized rats (1, 2, 4, 5) or in 40 hr cultures from naive rats (3) branch much less frequently, often exceed 1-2 mm in length, and tend to fasciculate with other processes. Growth cones are typically tapered with few filopodia (5). Immunoperoxidase labeling with antibodies to major neuronal proteins stained all neurons to varying degrees and were often used to facilitate counting: GAP-43 (A: 1, 2, 5, 6; B: 1-3), NF-H (A: 4; B: 4), or MAP-2 (A: 3). Scale bar, 75 µm.
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Quantitation of the length and branching of individual neurites shows that the processes extended by naive neurons and pre-axotomized neurons during the early phase of outgrowth define two distinct modes of axon growth (Fig. 4A,C). For this analysis, we scored only neurites that could be traced over their entire length. Because very long neurites in pre-axotomized cultures overlap and fasciculate with other processes, the longest processes in these cultures are under-represented in the quantitative analysis. Nonetheless, quantitation of individual neurites shows a profound difference in the characteristics of growth by naive and pre-axotomized neurons. Those processes of pre-axotomized neurons that could be traced were frequently >500 µm in length, with very few if any branches per neurite. In contrast, individual neurites extended by a subset of naive neurons under standard conditions branched an average of seven times but rarely exceeded 100 µm in length.
To examine the characteristics of neurites extended by the majority of naive neurons, we analyzed processes induced by high-density plating (Fig. 4A) and addition of NGF or schwannoma-conditioned medium (Fig. 4B). Neurites extended under those conditions were somewhat longer than in the absence of exogenous growth factors, but they remained shorter than the long axons characteristic of pre-axotomized cells. Moreover, the absolute number of branch points per neurite remained high. The number of branch points and length of neurites 16 hr after plating were not affected by continuous exposure to the transcription inhibitor DRB (Fig. 4D).
Although the arborizing and elongating neurites differ in several characteristics (see above), the spatial frequency of branching provides a simple and objective measurement for distinguishing the arborizing outgrowth characteristic of naive DRG neurons from the elongating outgrowth induced after axon injury in vivo. Graphic analysis shows that all neurites extended during the first 16 hr by naive DRG neurons, under any culture conditions tested, cluster above a line corresponding to a branching frequency of 1.5 branch points per 100 µm. Neurites with a much lower frequency of branching arise only from cells that have responded to a previous nerve injury (Fig. 4E). It is notable that a small number of neurons from these pre-axotomized ganglia extend neurites that overlap in branch frequency with those of naive neurons (Fig. 4E). This may reflect the fact that the sciatic nerve lesions used for these studies interrupts the axons of only 70-80% of neurons in the L4 and L5 DRG (Himes and Tessler, 1989
To determine whether an unspecified factor in pre-axotomized cultures or an intrinsic change in injured neurons was prompting the growth of elongating neurites, a small number of naive neurons were labeled with the fluorescent dye DiI and then dispersed onto a bed of newly plated cells from pre-axotomized DRG harvested at the same time. By 16 hr after plating, <10% of the labeled neurons had elongating neurites, demonstrating that the environment of a pre-axotomized culture was not sufficient to elicit an elongating mode of growth from naive neurons. In the converse experiment, DiI-labeled neurons from pre-axotomized ganglia readily extended elongating axons in the environment of naive DRG cultures. Furthermore, the distinction between arborizing and elongating modes of growth does not lie simply in the responsiveness of cells to the laminin substrate. Even after being plated for 16 hr on a confluent layer of schwannoma cells (Pfeiffer and Wechsler, 1972 In vitro transition produces competence for elongation by naive neurons
Removal and dissociation of naive adult DRG axotomize neurons, and we found that by the second day in culture, cells from naive DRG also began to extend processes that resembled the elongating axons of pre-axotomized neurons (Fig. 5). To follow the emergence of this elongating type of growth in naive cultures, neurons at various times after plating were scored for arborizing and elongating growth in two assays. Quantitation of a sample of neurons from each culture was used to determine the percentage of cells with arborizing and elongating processes on the basis of branching frequency. To avoid any effects of sample bias, we also used visual inspection to score all cells in each culture dish on the basis of neurite length, branching frequency of all processes, growth cone morphology, and fasciculation. Both visual inspection (Figs. 1, 3) and quantitative analysis (Figs. 5, 6) show that neurites with a characteristic elongating morphology first emerge in naive DRG cultures beginning ~24 hr after cells are dissociated and plated. The percentage of neurons with elongating axons increases sharply, followed by a slow decline in the number of arborizing cells. By 48 hr after plating, a majority of neurites are of the elongating type. Figure 6A shows that the curve representing the onset of elongation in naive cultures is similar to that derived from pre-axotomized cultures but is shifted to the right by ~20 hr.
Fig. 5. Neurites observed at later times in cultures from naive animals resemble those extended early by previously axotomized neurons. Randomly selected naive neurons from three separate naive cultures at different times were analyzed for length and number of branch points of their longest neurite. High frequency of branching and limited length persisted through 16 and 22 hr (A, B), but by 48 hr (C) neurites were typically longer with fewer branches, resembling neurites in 16 hr cultures from pre-axotomized ganglia. When plotted together (D), the data segregate on either side of the same line used in Figure 4, with neurites from 16 and 22 hr cultures falling above the line and the majority of those from 48 hr cultures falling below the line.
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Analysis of individual neurons from naive ganglia over time in culture demonstrated that change in the percentage of neurons with arborizing and elongating processes does not reflect differential cell survival or death (Table 1). To follow the fates of individual cells, we located and photographed 60 neurons in naive DRG cultures 12 hr after plating and then incubated the cultures for an additional 24 hr. Of 25 cells with no discernible neurites at 12 hr after plating, all but 7 (28%) could be relocated after 36 hr in culture. Of the relocated cells, 56% had extended axons with an elongating morphology, 5% had extended arborizing neurites, and the remaining cells (39%) appeared viable but had not yet extended processes. Of 35 cells with arborizing neurites at 12 hr after plating, all but 6 (17%) could be relocated after 36 hr in culture. Of these, 45% had extended elongating axons and 10% retained typical arborizing neurites. The remaining 45% retained some neurites with an arborizing morphology but also displayed one or more sparsely branched processes that extended beyond the halo of highly branched neurites. These cells may represent an intermediate stage in a transition from arborizing to elongating growth. These results indicate that the emergence of elongating axons from naive DRG neurons, beginning 24 hr after dissociation and plating, reflects a transition in the growth characteristics of individual neurons rather than differential survival of a subpopulation of cells competent for elongation. Elongation, furthermore, occurs both from the subset of neurons that extend arborizing neurites during the first 12 hr under standard culture conditions and from the majority of cells that initially fail to extend processes under those conditions.
Table 1. Neurons that had not extended neurites by 12 hr after plating, as well as those that had extended arborizing neurites, exhibited elongating neurites by 36 hr
Status 12 hr after plating Percent relocated 36 hr after plating Status 36 hr after plating No neurites Arborizing Elongating No neurites 72% 39% 5% 56% Arborizing 83% 0% 55% 45% Elongating axon growth requires a period of gene transcription after axotomy
The ability of naive DRG neurons to carry out in vitro the transition between growth modes induced by sciatic nerve lesion provides an experimentally accessible system for analyzing the critical molecular events in that transition. We used DRB, the reversible inhibitor of RNA polymerase II, to determine whether the onset of neuronal competence for elongating growth requires new gene transcription after axotomy. Naive DRG neurons were plated under standard culture conditions and exposed transiently to DRB for the first 12 hr after plating. The percentage of neurons with elongating axons was then determined at 40 and 66 hr after plating by visual categorization of all of the neurons in each culture (Fig. 7A) and by quantitative analysis of a sample of the cells (Fig. 7B). When transcription was prevented during the first 12 hr in culture, the emergence of elongating axons was delayed dramatically. The number of neurons with elongating axons remained low until at least 40 hr after plating and then increased to near control levels by 66 hr (Fig. 7A). As illustrated in Figure 7B, this transient inhibition of axon elongation can be accounted for by a simple displacement in the onset of elongation by ~16 hr. Biochemical analysis indicated that cells treated with DRB for the first 12 hr in culture showed no gross alterations in protein synthesis by 24 hr after plating, just before the onset of elongation in control cultures (Fig. 7C).
Interestingly, when naive DRG neurons were allowed to synthesize new mRNA for 12 hr after plating, and then exposed to DRB for 12 hr, there was a less dramatic reduction in the number of elongating neurites at the 40 hr time point; by 24 hr after plating, cells no longer required ongoing transcription to support axon elongation (Fig. 7A,B). Similarly, neurons pre-axotomized in vivo are able to support elongating axon outgrowth in the continuous presence of DRB for 16 hr after plating (Fig. 2). The results indicate that a finite period of new transcription after axotomy is essential in order for naive DRG neurons to gain competence for the elongating mode of axon growth. Regulation of growth mode by target-dependent retrograde signals
The transition from arborizing to elongating growth can be triggered in DRG neurons by axon interruptions resulting from removal and dissociation of a ganglion or from peripheral nerve injury in vivo. This implies that signals conveyed along axons to neuron cell bodies can regulate the growth mode supported by DRG neurons. To explore the nature of these signals, we used the microtubule-depolymerizing agent colchicine to block axonal transport in DRG axons. Colchicine was applied to the sciatic nerve by encircling the nerve with a permeable plastic cuff impregnated with the drug. Two days later, DRG neurons were removed and assayed for their ability to support arborizing and elongating outgrowth in our standard culture assay (16 hr after dissociation and plating).
Electron microscopy confirmed that axons in the nerve segment surrounded by the plastic cuff remained intact, although the depolymerization of microtubules produced a characteristic eccentricity in the shape of the axons (Fig. 8A). Application of colchicine to the sciatic nerve 1 hr before a nerve crush had no effect on the ability of nerve injury to induce the in vivo transition to elongating growth (Fig. 8B). On the other hand, disruption of axonal transport in the absence of nerve injury was sufficient to induce a dramatic increase in the number of DRG neurons able to support axon elongation in vitro. Quantitative analysis of individual cells showed that the length and branching frequencies of axons from the colchicine pretreated neurons closely resembled the elongating axons from pre-axotomized cells (Fig. 8C). The proportion of DRG neurons extending elongating axons after colchicine treatment in vivo was slightly lower than after sciatic nerve crush. This could result from incomplete or delayed inhibition of axonal transport in some axons in the interior of the sciatic nerve, or it could indicate that signals in addition to the disruption of axonal transport contribute to the regulation of elongating growth after nerve injury. The results show, however, that disruption of ongoing retrograde transport of signals in intact axons is sufficient to induce competence for elongating growth in many DRG neurons. This, in turn, implies that competence for elongation is chronically suppressed in the intact adult neurons by signals conveyed by retrograde axonal transport in peripheral axons. 
Fig. 8. Disruption of axonal transport induces competence for elongating growth. Pliable plastic cuffs impregnated with colchicine or vehicle control were placed around sciatic nerves of anesthetized rats. Assays were performed after 48 hr. A, Electron microscopy confirmed that axons in the nerve segment surrounded by the plastic cuff remained intact. Colchicine produces an increase in irregular profiles of myelinated axons compared to vehicle controls, consistent with its disruption of microtubules. In contrast, sciatic nerve crush produces dramatic degeneration of axons just proximal to the crush site. B, The percentage of elongating (black bars) and arborizing cells (gray bars) after 16 hr in culture. Colchicine did not block the induction of elongating growth after peripheral axotomy (Ax./Colch.), but in the absence of sciatic nerve crush, the drug induced competence for elongating growth in otherwise uninjured neurons (Colch.). Data from naive (N.) and pre-axotomized (Ax.) untreated animals are provided for comparison. Application of cuffs containing vehicle alone (Veh.) had no effect on the onset of axon elongation (compare to 16 hr time points in Fig. 5A,B). Each bar represents the mean ± SD of four separate experiments with duplicate cultures in each experiment. C, Quantitative analysis of neurite branching and length shows that neurites extended in three separate experiments by neurons from colchicine-treated animals (filled squares) resemble the elongating axons of pre-axotomized neurons and are clearly segregated from the arborizing neurites extended after application of vehicle-containing cuff (open circles).
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To identify the source of these retrogradely transported signals, we first performed crush lesions of the sciatic nerve at varying distances from neuronal cell bodies (Fig. 9A). The more proximal lesions (1.0-1.5 cm from the ganglia) remove a large part of the axon and disconnect cell bodies from signals arising along the length of the nerve and from peripheral targets. More distal lesions (5.0-5.5 cm from the ganglia) remove the influence of peripheral targets but leave a large portion of the axon and its associated Schwann cells in communication with the cell body. After 24, 48, or 72 hr, neurons were cultured as usual and assayed for elongating neurites 16 hr after plating. We found that both proximal and distal lesions elicit competence for elongating growth in the majority of DRG neurons by 48 hr after injury (Fig. 9A). The slightly lower number of elongating cells resulting from the more distal lesion is consistent with previous evidence that only 70% of neurons in the lumbar ganglia project axons to the more distal lesion site (Himes and Tessler, 1989 
Fig. 9. Competence for elongating growth is regulated by a retrograde signaling pathway(s) activated by contact with peripheral targets. A, The length of the proximal nerve stump affects the timing, but not the extent, of the transition to elongating growth competence. Sciatic nerve crush was performed either 1.0-1.5 cm (black bars) or 5.0-5.5 cm (gray bars) from neuronal cell bodies, and neurons were removed and transferred to tissue culture 24, 48, or 72 hr later. By 48 hr after injury, both proximal and distal lesions produced a large increase in the number of neurons able to extend elongating axons by 16 hr after plating (fewer neurons are injured by the distal lesion, so the maximal response is lower than after proximal injury). The response to proximal crush reaches 45% of the maximum response by 24 hr after injury. In contrast, the response to a more distal lesion by 24 hr is only 12% of the maximum. This may reflect time required for the depletion of retrogradely transported inhibitory molecules in longer proximal nerve segments. Each bar represents the mean ± SD of three separate experiments with duplicate cultures in each experiment. B, Sciatic nerves were subjected to a crush lesion, which permits effective regeneration of axons, or complete transection or resection of a 0.5 cm nerve segment, both of which delay or prevent reinnervation of peripheral targets. DRG neurons were removed 1 week (shaded bars) or 8 weeks (black bars) after injury, and plated for 16 hr in vitro. By 1 week after injury, all three types of lesion had stimulated competence for elongating growth. By 8 weeks after injury, competence for elongation had declined in neurons with crush lesion but remained elevated after nerve transection or resection. Each bar represents the mean ± SD of three separate experiments with duplicate cultures in each experiment.
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When DRG axons are allowed to regenerate and restore contact with peripheral targets, their ability to support elongating growth in the 16 hr tissue culture assay declines by 8 weeks after peripheral nerve injury (Fig. 9B). When regeneration and target reinnervation are disrupted, by transecting the nerve or by resecting a 5 mm segment of nerve, DRG neurons maintain competence for elongating growth at least 8 weeks after the injury (Fig. 9B). Together, the results indicate that competence for the elongating mode of axon growth is chronically suppressed in uninjured adult DRG neurons by retrogradely transported signals activated by interactions of axons with peripheral targets. Central and peripheral axotomy differentially affect growth competence
In addition to its peripherally projecting branch, the axon of each DRG neuron extends a second branch through the dorsal root to innervate targets in the spinal cord or brainstem. Previous studies have shown that interruption of these centrally projecting axons induces only limited expression of some genes activated by peripheral injury (Wong and Oblinger, 1990
Fig. 10. Central and peripheral axotomy affect the growth characteristics of DRG neurons differently. DRG neurons subjected to central axotomy displayed growth characteristics intermediate between naive and peripherally axotomized neurons. A, Fewer neurons were able to elongate (black bars) 2 or 7 d after a central root crush than 2 d after a peripheral crush. In addition, more neurons extended arborizing neurites (gray bars) after the central root lesions. Each bar represents the mean ± SD of three separate experiments with duplicate cultures in each experiment. B, Analysis of neurite length and branching revealed that the neurites in these cultures did not fall into distinct groups but, instead, covered a wide range of intermediate morphologies. Filled circles, Neurites measured in 16 hr cultures from ganglia removed 2 d after dorsal root crushes were performed in vivo. Open circles, Neurites measured in 16 hr cultures from ganglia removed 7 d after dorsal root crushes were performed.
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Quantitative analysis of individual cells showed the axons extended by these centrally axotomized neurons did not segregate into two distinct populations corresponding to arborizing and elongating neurites. Rather, the distribution of growth characteristics for centrally axotomized neurons is intermediate between those of naive and peripherally axotomized cells (Fig. 10B). For the population as a whole, central axotomy produces a substantial reduction in branching and an increase in neurite length. Nonetheless, branching remains much more extensive than after peripheral axotomy, and a majority of neurons fail to extend processes longer than 300 µm. It is not yet clear whether those centrally lesioned cells that extend much longer axons represent a discrete subpopulation of DRG neurons or stochastic variation within a single population of cells. It is clear, however, that interruption of centrally projecting axons does produce a general shift in the growth capabilities of DRG neurons but fails to elicit the same competence for elongating growth induced by peripheral lesions.
DISCUSSION
Our findings indicate that most, if not all, adult sensory neurons are constitutively competent to support arborizing axon growth, characterized by a high frequency of branching and a concomitantly limited linear extension of individual processes. We find, however, that these cells are unable to initiate or sustain rapid, linear extension of axons
Although clearly distinct from elongating processes, the arborizing neurites extended by naive DRG neurons actually encompass a broad range of individual morphologies (see Fig. 3A), and subpopulations of DRG neurons differ in their propensity to extend arborizing processes under various conditions. DRG cells are a heterogeneous population of neurons that innervate distinct targets and, in the absence of injury, express different neurotrophin receptors, synaptic components, and growth-associated proteins (Schreyer and Skene, 1991
In contrast to arborizing growth, the genes constitutively expressed in naive adult neurons are not adequate for these cells to initiate or sustain the more rapid, elongating mode of axon extension. Successful nerve regeneration requires the rapid, linear extension of individual axonal processes for distances on the order of millimeters to centimeters (McQuarrie et al., 1978
The most parsimonious interpretation of these findings is that DRB blocks the onset of elongating growth by preventing a selective, axotomy-induced increase in expression of one or more genes above the levels characteristic of uninjured adult neurons in vivo. Although DRB inhibition of RNA polymerase II produces a nonselective blockade of all mRNA synthesis, the earliest and most pronounced effect of this inhibition will be to prevent any increase in mRNA species induced in response to axotomy. For genes expressed at relatively high levels in adult neurons before explantation, preexisting pools of mRNA should permit continued production of protein for several hours during transient disruption of transcription. This would explain why DRB no longer interferes with the onset of elongating growth once neurons have been permitted 12-24 hr to transcribe new mRNAs after axotomy. This period of active transcription would allow the cells to establish a critical pool of mRNA species required for the transition to elongating growth.
Extensive biochemical analysis has shown that interruption of peripheral axons does in fact induce selective accumulation of several specific mRNA species, including those coding for prominent components of axonal growth cones (Basi et al., 1987
One alternative possibility is that a critical molecule(s) involved in triggering the cell body transition to elongation is encoded by a constitutively expressed, but very rapidly degraded, mRNA. If both the mRNA and the protein it encodes were very rapidly degraded, ongoing transcription would be required to maintain effective levels of the relevant triggering component(s) for a defined period after axotomy. For such a model, the critical mRNA would need to carry out an irreversible or self-perpetuating step in triggering competence for elongating growth, rather than having a continuing role in maintaining the cell's competence for elongation, because interruption of transcription beginning 12-24 hr after axotomy no longer prevents the onset of elongating growth. Similarly, neurons axotomized in vivo 2-7 d before explantation are able to initiate and sustain elongating growth in the continuous presence of the transcription inhibitor for up to 16 hr (Fig. 1). With either model, our results indicate that regenerative growth depends on a molecular apparatus distinct from that underlying common forms of growth and remodeling in the normal adult nervous system.
Numerous studies have shown previously that various types of neurite outgrowth can be supported by embryonic neurons, as well as by neuronal tumor cell lines, in vitro (Gunning et al., 1981
In the mammalian CNS, axon injury often fails to induce the changes in gene expression typically elicited by peripheral axotomy (Skene, 1989
The effect of dorsal root lesions on the growth properties of DRG neurons indicates that the transition from arborizing to elongating growth does not always occur in a single, coordinated step and that intermediate states can be maintained in vivo.
One explanation for such intermediate states is the induction, or persistent expression, of a subset of genes required for elongating growth. The transcription factor c-jun, for example, is induced in a small and variable number of DRG neurons after dorsal rhizotomy (Jenkins, 1993). Expression of major cytoskeletal proteins occurs but is attenuated compared to peripheral lesions (Wong and Oblinger, 1990
Characterization of the transition between distinct growth modes in vitro now provides an experimentally accessible framework for investigating how individual genes, known or previously unidentified, alter specific features of axonal growth and for determining which combinations of these proteins are required for effective axon elongation.
FOOTNOTES
Received Aug. 6, 1996; revised Sept. 23, 1996; accepted Oct. 22, 1996.
This work was supported by National Institutes of Health Grant NS20178/EY11475.
Correspondence should be addressed to Pate Skene, Department of Neurobiology, Box 3209, Duke University Medical Center, Durham, NC 27710.
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