Neuronal Cyclic AMP Controls the Developmental Loss in Ability of Axons to Regenerate

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The Journal of Neuroscience, July 1, 2001, 21(13):4731-4739

Neuronal Cyclic AMP Controls the Developmental Loss in Ability of Axons to Regenerate
Dongming Cai¹, Jin Qiu¹, Zixuan Cao¹, Marietta McAtee², Barbara S. Bregman², and Marie T. Filbin¹
¹ Department of Biological Sciences, Hunter College, City University of New York, New York, New York 10021, and ² Department of Neuroscience, Georgetown University Medical School, Washington, DC 20007

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Unlike neonatal axons, mammalian adult axons do not regenerate after injury. Likewise, myelin, a major factor in preventingregeneration in the adult, inhibits regeneration from older butnot younger neurons. Identification of the molecular events responsiblefor this developmental loss of regenerative capacity is believedkey to devising strategies to encourage regeneration in adultsafter injury. Here, we report that the endogenous levels of thecyclic nucleotide, cAMP, are dramatically higher in young neuronsin which axonal growth is promoted both by myelin in general andby a specific myelin component, myelin-associated glycoprotein(MAG), than in the same types of neurons that, when older, areinhibited by myelin-MAG. Inhibiting a downstream effector of cAMP[protein kinase A (PKA)] prevents myelin-MAG promotion from youngneurons, and elevating cAMP blocks myelin-MAG inhibition of neuriteoutgrowth in older neurons. Importantly, developmental plasticityof spinal tract axons in neonatal rat pups in vivo is dramaticallyreduced by inhibition of PKA. Thus, the switch from promotionto inhibition by myelin-MAG, which marks the developmental lossof regenerative capacity, is mediated by a developmentally regulateddecrease in endogenous neuronal cAMPlevels.

Key words: axonal regeneration; cAMP; protein kinase A; myelin; MAG; development

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The adult mammalian CNS does not regenerate after injury, although young axons do regrow (Bates and Stelzner, 1993; Hasanet al., 1993). Changes in the cellular environment and in theneuronal response to that environment are both responsible forthe absence of regeneration by mature axons (Keirstead et al.,1992; Li and Raisman, 1993; Schwab and Bartholdi, 1996). However,adult CNS neurons have not lost the intrinsic capacity to regrow,because, when provided with a permissive environment, they willextend long processes (Richardson et al., 1980; David and Aguayo,1981; Crutcher, 1989; Schnell and Schwab, 1990; Schwab et al.,1993; Cheng et al., 1996). Therefore, some new component in theadult CNS environment actively inhibits axonal growth after injury.One obvious candidate that appears with late development in theCNS is myelin. Indeed, many studies in vivo and in vitro haveshown that myelin inhibits axonal regeneration in adult neurons(Crutcher, 1989; Schnell and Schwab, 1990; Keirstead et al., 1992;Cheng et al., 1996). Strong evidence that myelin is a major factorin preventing regeneration was presented when extensive regenerationoccurred in mice that had been immunized with myelin before spinalcord transection (Huang et al., 1999). Extensive regenerationoccurred because the myelin antibodies neutralized myelin-specificinhibitors of regrowth, allowing regeneration to commence immediatelyafter injury. On the other hand, myelin does not exert this inhibitoryeffect on embryonic neurons, either in culture (Shewan et al.,1995) or when transplanted in vivo (Li and Raisman, 1993). Identificationof the molecular difference between embryonic and adult neuronsthat is responsible for this change in regenerative capacity haslong been believed to be the key to encouraging adult axons toregrow afterinjury.

Along with a developmental change in axonal response to myelin in general, it has been reported that a number of differentneurons respond to an individual myelin-specific protein, myelin-associatedglycoprotein (MAG), by switching from promotion to inhibitionduring development (McKerracher et al., 1994; Mukhopadhyay etal., 1994; DeBellard et al., 1996). For retinal ganglion (RG)neurons and spinal neurons, the switch has occurred by birth;embryonic RG and spinal neurons are promoted by MAG, whereas postnatalaxonal growth is inhibited (Salzer et al., 1990; DeBellard etal., 1996; Turnley and Bartlett, 1998). For dorsal root ganglion(DRG) neurons, the switch occurs postnatally with a sharp transitionfrom promotion to inhibition by MAG at postnatal day 3-4 (P3-4)(Johnson et al., 1989; Mukhopadhyay et al., 1994; DeBellard etal., 1996). Although the appearance of myelin is an obvious changein the environment with development, the molecular basis for thesignificant developmental shift in the response of neurons toMAG and myelin is not known. However, the response of neuronsto MAG in culture is paralleled by their response to myelin ingeneral, which in turn is indicative of how they regenerate invivo.

Recently, we showed that elevating endogenous levels of cAMP effectively blocked the inhibition of axonal regeneration byMAG and myelin (Cai et al., 1999). Consistent with this observation,others showed that not only is repulsion of growth cones by MAGdependent on cAMP, but so is the attraction of growth cones toother guidance cues (Ming et al., 1997; Song et al., 1997, 1998).Importantly, it was also shown that for these molecules, inhibitioncould be converted to attraction by elevating neuronal cAMP, andattraction can be converted to inhibition by blocking a downstreameffector of cAMP, protein kinase A (PKA). The question now raisedby all of these studies is whether endogenous levels of cAMP influencethe spontaneous switch in response of neurons to MAG and myelinand the loss of regenerative capacity observed duringdevelopment.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neurite outgrowth on cells or myelin. Rat RG neurons and DRG neurons were isolated as described previously (DeBellard et al.,1996). For raphespinal projecting neurons, the most caudal regionof the raphe nucleus was removed, and the neurons were dissociatedin 0.025% trypsin for 10 min at 37°C. The neurite outgrowth onmyelin or on transfected Chinese hamster ovary (CHO) cells wasas described (Mukhopadhyay et al., 1994; Cai et al., 1999), withthe following modifications. The neurite outgrowth assay was performedby adding 5 × 10⁴ neurons to the immobilized myelin substrate or 2 × 10⁴ neurons to the CHO cell monolayers. Where indicated, db-cAMP(1 mM), db-cGMP (1 mM), H89 (2 µM), KT2750 (200 nM), KT5823 (1µM),Rp-cAMP (20 µM), or Sp-cAMP (50 µM) was added to the cultures.All types of neuron cultures were immunostained for growth-associatedprotein 43 (GAP43) as described before (Mukhopadhyay et al., 1994),but for raphe nuclei neurons, because the cultures were not pure,cultures were also stained for serotonin. A goat serotonin antibody(DiaSorin, Stillwater, MN) was used at 1:1000. For double staining,GAP43 antibody was detected with anti-rabbit Oregon Green-conjugatedsecondary antibody, and serotonin antibody was detected with anti-goatbiotinylated secondary antibody followed by Texas Red-conjugatedstreptavidin. Approximately 98% of the cultures were serotonin-positive.For DRG and RG neurons, the length of the longest neurite foreach GAP43-positive neuron for the first 180-200 neurons encounteredwhen scanning the slide in a systematic manner was determinedusing an Oncor image analysis program. The same effects were obtainedwhen total processes, rather than the longest neurite, were measured.For raphe neurons, only those neurons that were both GAP43- andserotonin- positive were measured. Neurite measurements were comparedbetween groups using a one-wayANOVA.

Immunoassay for cAMP. For each cAMP assay, neurons were dissociated, and cyclic AMP was measured immediately using a competitiveimmunoassay, according to the manufacturer's (Amersham, ArlingtonHeights, IL) instruction . For each assay, 1× 10⁶ RG cells or 2 × 10⁵ DRG or raphe nuclei neurons were plated into each of six wells.Each assay was repeated at least fourtimes.

Immunofluorescence staining for cAMP. cAMP immunostaining was performed on DRG cryosections with a rabbit polyclonal antiserumaccording to Wiemelt et al. (1997). Isolated, intact DRGs werefixed with acrolein for 1 hr at room temperature (RT), incubatedin 20% sucrose until equilibrium, embedded with optimum cuttingtemperature (OCT) matrix (Tissue-Tek; Miles Inc., Elkhart, IN),and cryosectioned at 5 µm. The fixed RG neurons or DRG cryosectionswere washed in a quenching solution containing 1 mg/ml glycinefor 15 min at RT, followed by 1% (w/v) sodium cyanoborohydridefor 15 min. Then the slides were stained by incubating them overnightat 4°C in the anti-cAMP antiserum diluted 1:50 in a solution containing5% goat serum and 0.5% Triton X-100. Then, the binding of theprimary antibody was visualized using the biotin-streptavidinsystem.

Spinal cord lesions and transplants. Pups (2-3 d of age) were anesthetized by hypothermia, and under sterile surgical conditions,a laminectomy was made at the T6 spinal cord level. An overhemisectionlesion was made in all animals (n = 38). The following experimentalgroups were examined: lesion plus H-89 (n = 10), lesion plus saline(n = 10), lesion plus transplant plus H-89 (n = 11), and lesionplus transplant plus saline (n = 7). The saline or H-89 (0.5 mM)was delivered via Gelfoam placed at the lesion or lesion plustransplant site. Transplants of embryonic day 14 spinal cord wereprepared as described previously (Bregman and McAtee, 1993).

Tracing and immunohistochemistry. Two weeks after lesion, the anterograde tracer, biotin dextran amine (BDA, 10,000 molecularweight; Molecular Probes, Eugene, OR), was used to study changesin the descending corticospinal tract fibers. After anesthesia(choral hydrate, 400 mg/kg), the sensorimotor cortex was exposed,and a 10% solution of BDA in sterile saline was injected intothe cortex bilaterally (0.3-0.5 µl per injection, 3 µl total volumeper motor cortex). After the injections, the dura was coveredwith Gelfoam soaked in saline, and the overlaying skin was sutured.Two weeks after the BDA injection, the rats were anesthetizedwith chloral hydrate and perfused transcardially with 0.9% salinefollowed by ice-cold 4% paraformaldehyde in 0.1 M phosphate buffer.Tissue was passed through graded sucrose solutions and preparedfor immunohistochemistry using the modified techniques of Veenmanet al. (1992) and Herzog and Brosamle (1997). Briefly, cryostatsections were washed with phosphate buffer and incubated in anavidin-biotin-peroxidase complex for 90-120 min at room temperature(Vector Elite ABC Kit; Vector Laboratories, Burlingame, CA), andthe BDA-filled axons were visualized using a solution of diaminobenzidinetetrahydrochloride-nickel ammonium sulfate and hydrogen peroxide.Adjacent sections were processed immunocytochemically for visualizationof serotonergic axons (serotonin; DiaSorin) as described previously(Bregman et al., 1997; Diener and Bregman, 1998). Cellular morphologywithin the transplants was evaluated in sections stained withcresyl violet or neutral red. The extent of axonal growth wasevaluated by individuals unaware of the experimental group towhich the animals belonged. The extent of axonal growth withinthe transplants was scored according to a rating scale. No growthwithin the transplant was scored as 0; dense growth throughoutthe transplant equivalent to that observed in previous studieswas rated as +++. Only sections in which the transplant was contiguouswith the host spinal cord and without any intervening glial orcystic barrier were scored. Sections from seven of the transplantplus H89 animals and six of the transplant plus saline-treatedanimals werescored.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Endogenous cAMP levels in DRG neurons decrease with development and parallel the developmental loss of ability to grow on myelin

Previously, we reported that MAG, like many axon guidance molecules (Colamarino and Tessier-Lavigne, 1995; Song et al., 1998)was bifunctional. When cultured on CHO cells that were transfectedto express MAG, the neurite length from rat DRG neurons olderthan P4 and through to adult was, on average, 50% shorter thanthose grown on control CHO cells that were not expressing MAG.In contrast, MAG promoted neurite outgrowth from DRG neurons fromanimals younger than P4, and the transition from promotion toinhibition by MAG occurred sharply at P3-4 (Mukhopadhyay et al.,1994; DeBellard et al., 1996). Now we show that on a substrateof purified myelin, DRG neurons follow a very similar trend inresponse. When cultured on myelin, DRG neurons from P1 animalsextend relatively long processes (longest neurite on average,25 µm), which then show diminished length with age (Figs. 1A,2A). By P5, neurite length is about fivefold shorter than neuritesfrom P1 animals. Extension of short neurites from DRG neuronson myelin persists through to adults. On a control substrate suchas poly-L-lysine or CHO cells not expressing MAG, there is nodecrease in neurite length with age. Therefore, like the age-relatedswitch in response to MAG, DRG neurons grown on myelin at thesame age also switch from extending relatively long neurites atP1 to extending either very short or no neurites by P5 (Figs.1A, 2A). We already know that artificially elevating cAMP in olderneurons blocks inhibition by not only MAG but also myelin in general(Cai et al., 1999). Therefore, it is reasonable to suggest thatthe better growth of young neurons on myelin-MAG is a consequenceof higher endogenous levels of cAMP relative to older neurons.To determine whether this is the case, cAMP levels were measureddirectly in DRG neurons of different ages, immediately after theirremoval from the animal. In concert with the sharp transitionin neurite growth response to myelin and MAG, there is a concomitantsharp drop in the endogenous levels of cAMP in DRG neurons atP3-4 to less than one-tenth the levels at birth (Fig. 1B), wherethey persist to adult. Consistent with this measure of absolutecAMP levels of dissociated DRG neurons, when immunostained insitu with a cAMP antibody (Wiemelt et al., 1997), there is obviouslymuch more cAMP in P0 than in P5 DRG neurons (Fig. 1C).

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Figure 1. Developmental changes in neurite outgrowth of DRG neurons on myelin correlate with changes in endogenous levels of cAMP. Dissociated DRG neurons from P1-P22 animals, as indicated, were cultured overnight on a substrate of purified rat CNS myelin or poly-L-lysine; afterward, they were fixed and immunostained for GAP43. In each experiment, at each DRG age, the mean length of the longest GAP43-positive neurite for 180-200 neurons was measured (±SEM) for at least three separate experiments. Results are presented as percentage of P1 neurite length (A). To measure cAMP, 2 × 10⁵ dissociated DRG neurons from P1-P22 animals, as indicated, were plated into each well, and cAMP was measured using a competitive immunoassay. Results are the mean (±SE) of at least three experiments, each performed in sextuplicate (B). DRG neurons were removed from P0 and P5 animals, fixed immediately, and immunostained for cAMP (C). Scale bar, 50 µm.

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Figure 2. Developmental changes in neurite outgrowth of DRG neurons on myelin and MAG are dependent on changes in endogenous levels of cAMP. Dissociated DRG neurons from P1 or P5 animals, as indicated, were cultured overnight on a substrate of purified rat CNS myelin (A, B), MAG-expressing cells (striped bars), or control cells (black bar) (C). Where indicated, 200 nM KT5720 (+KT), 20 µM Rp-cAMP (+Rp), or 1 µM KT5823 (+PKG Inh.) was added during culture; afterward, they were fixed and immunostained for GAP43. Scale bar (shown in A), 10 µm. In each experiment, at each DRG age, the mean length of the longest GAP43-positive neurite for 180-200 neurons was measured (±SEM) for at least three separate experiments. For neurons grown on myelin, results are presented as percentage of P1 neurite length in the absence of cyclic nucleotides (B). For neurons grown on cells, results are presented as percentage of neurite length on control cells in the absence of cyclic nucleotides (C).

High levels of endogenous cAMP in young DRG neurons account for the promotion of neurite outgrowth by MAG and myelin

To determine whether the high levels of cAMP in newborn DRG neurons are indeed required for promotion of neurite outgrowthby myelin and MAG, the downstream effector of cAMP, PKA, was inhibited.Both the PKA inhibitor, KT5720 (200 nM), and the cAMP antagonist,Rp-cAMP (20 µM), blocked neurite outgrowth on myelin by >50% andcompletely blocked promotion by MAG from P1 DRG neurons in culture;an inhibitor of protein kinase G (PKG), KT5823 (1 µM), had noeffect (Fig. 2A-C). None of these compounds had an effect on neuriteoutgrowth on control cells not expressing MAG or on growth onMAG-expressing cells of DRG neurons older than P4 (data not shown).In addition, the cAMP analog, db-cAMP, had no effect on the goodgrowth of P1 DRG neurons on MAG cells or myelin (data not shown).Together with our previous findings that artificially elevatingcAMP in older DRG neurons blocks inhibition by myelin-MAG, theseresults strongly suggest, first, that promotion and inhibitionof axonal growth by myelin-MAG are each cAMP-dependent and, second,that the endogenous levels of cAMP in DRG neurons dictate thedevelopmental switch of these neurons toinhibition.

Changes in neurite outgrowth of retinal ganglion neurons on myelin and MAG correlate with, and are dependent on, changes in endogenous levels of cAMP

Because many other neurons switch their response to MAG and myelin with development, we now asked whether cAMP dependenceis a general mechanism involved in the switch or if it is restrictedto DRG neurons. Retinal ganglion neurons are also known to switchin response to MAG, but unlike DRG neurons, the switch for RGneurons occurs embryonically (Salzer et al., 1990; DeBellard etal., 1996). Because the endogenous levels of cAMP are likely tochange during the culture period required (days) to isolate RGneurons from other RG cells, cAMP levels were measured for mixedpopulations of RG cells immediately after removal from the animals.We found that the endogenous levels of cAMP in embryonic day 18(E18) RG cells are at least threefold higher than P5 RG cells(Fig. 3A); the cAMP levels remain consistently low in all postnatalRG cells up to adult (data not shown). When grown on myelin asa substrate, embryonic RG neurons (distinguished from other celltypes by their morphology and by staining with a second immunologicalmarker, Thy-1; data not shown) extended relatively long, highlybranched processes after overnight culture, whereas P5 RG neuronsextended neurites that were about fivefold shorter and much lesscomplex (Fig. 3B). When either of the PKA inhibitors, KT5720 orRp-cAMP, was included in the cultures, neurite outgrowth fromE18 RG neurons on myelin was greatly reduced, whereas an inhibitorof PKG had no effect (Fig. 3B,C).

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Figure 3. Developmental changes in neurite outgrowth of RG neurons on myelin correlate with, and are dependent on, changes in endogenous levels of cAMP. Dissociated RG cells from E18 or P5 animals were measured for cAMP (1 × 10⁶ cells per well) using a competitive immunoassay. Results are the mean (±SE) of at least three experiments, each performed in sextuplicate (A). E18 or P5 RG neurons were cultured overnight on a substrate of purified myelin (B, C). Where indicated, 200 nM KT5720 (+KT), 20 µM Rp-cAMP (+Rp), 1 µM KT5823 (+PKG Inh.), 1 mM db-cAMP, 50 µM Sp-cAMP, or 1 mM db-cGMP was added during culture as described in Figure 2, after which the neurons were fixed and immunostained for GAP43. Scale bar, 10 µm. Neurite length was measured for 180-200 neurons (±SEM) in each experiment, and results are from at least three experiments. Results are presented as percentage of E18 neurite length, in the absence of cyclic nucleotides. C, Stippled bars represent E18 neurons; white bars represent P5 neurons. *p < 0.05.

In a similar fashion, the promotion of neurite outgrowth by MAG from E18 RG neurons was blocked by the same PKA inhibitorsand not by inhibitors of PKG (Fig. 4A). Furthermore, as with DRGneurons older than P5, inhibition of neurite outgrowth from postnatalRG neurons grown on myelin or MAG was blocked if either db-cAMPor Sp-cAMP, but not db-cGMP, was included in the cultures (Figs.3B,C, 4B). None of the compounds used had any effect on neuriteoutgrowth on control cells (data not shown). Together, these resultssuggest that cAMP levels of RG neurons are initially high in embryonicneurons and drop to low levels by birth, consistent with the developmentalchange measured for the RG cell population as a whole. Therefore,like DRG neurons, both the promotion and the inhibition of regenerationby myelin and MAG of RG neurons is cAMP dependent, and the developmentalswitch in response to myelin-MAG is dictated by the endogenouslevels of cAMP in the neuron.

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Figure 4. Developmental changes in neurite outgrowth of RG neurons on MAG are dependent on changes in endogenous levels of cAMP. Dissociated RG neurons from E18 (A) or P5 (B) animals were cultured overnight on a substrate of MAG-expressing cells (striped bars) or control cells (black bars). Where indicated, 200 nM KT5720 (+KT), 20 µM Rp-cAMP (+Rp), 1 µM KT5823 (+PKG Inh.), 1 mM db-cAMP, 50 µM Sp-cAMP (+Sp), or 1 mM db-cGMP was added during culture; afterward, they were fixed and immunostained for GAP43. In each experiment, the mean length of the longest GAP43-positive neurite for 180-200 neurons was measured (±SEM) for at least three separate experiments. Results are presented as a percentage of neurite length on control cells in the absence of cyclic nucleotides. **p < 0.001.

Regeneration of neonatal spinal tract axons in vivo and in culture is cAMP dependent

After spinal cord injury in neonatal animals, there is considerable anatomical reorganization of immature pathways and recoveryof function (Bregman and Goldberger, 1982, 1983). Depending onthe species and the precise timing of the injury, axons of thespinal tracts are at different stages of maturity; some have alreadyreached their target, and others are still in the process of elongatingthroughout the cord. Regeneration of those more mature axons thathave been severed, aberrant rerouting of late-developing axons,and sprouting from undamaged axons all contribute to the recovery(Bregman et al., 1989, 1993; Bernstein-Goral and Bregman, 1993).In the rat at P1, corticospinal tract axons are still elongatingthrough the spinal cord, whereas for raphespinal axons, most havereached their targets at all spinal cord levels but continue toincrease their projections within the gray matter throughout thenext several weeks (Bregman, 1987a,b; Bregman et al., 1989). Furthermore,at this time in the rat spinal cord, depending on the level andthe particular tract, myelination has begun, and, of the putativemyelin inhibitors, at least MAG is expressed, because it is expressedat the initial stages of myelination (Quarles, 1983). There isa critical period for developmental plasticity; the lesion-inducedgrowth seen at P1 is dramatically decreased by P5 and abolishedby the end of the first week of age (Bregman et al., 1989). Consistentwith this developmental loss in ability to regenerate in vivo,when raphe nucleus neurons are grown in culture, at P1 they arenot inhibited by myelin and MAG, but their ability to grow isinhibited by the PKA inhibitor, H89 (Fig. 5 A,C). In contrast,at P5, raphe neurons are inhibited from extending processes onboth myelin and MAG, and inhibition is blocked by elevating cAMP(Fig. 5B,C). As for DRG and RG neurons, the switch of raphe neuronsto inhibition by myelin-MAG is paralleled by a significant dropin endogenous cAMP levels of about threefold between P0 and P5(Fig. 5D). Therefore, like DRG and RG axons, raphespinal axonsswitch their response to myelin-MAG during development, and thisswitch is closely matched with a decrease in their endogenouscAMP levels.

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Figure 5. Developmental changes in neurite outgrowth of raphespinal neurons on MAG and myelin are dependent on changes in endogenous levels of cAMP. Raphe nucleus neurons were dissociated from P0-P1 and P4-P8 rat pups and grown on either MAG-expressing (striped bars) or control CHO cells (black bars) (A, B) or purified myelin (C). Where indicated, H89 (2 µM), KT5720 (200 nM), db-cAMP (1 mM), Sp-cAMP (50 µM), or inhibitors-agonists of cGMP were added. Results represent the average neurite length of 180-200 GAP43-positive neurites per experiment from three separate experiments. For neurons grown on myelin, results are presented as percentage of P0-P1 neurite length, and for neurons grown on cells, results are presented as a percentage of neurite length on control cells, each in the absence of cyclic nucleotides. D, Dissociated raphe cells from P0-P1 or P3-8 animals were measured for cAMP (2 × 10⁵ cells per well) using a competitive immunoassay. Results are the mean (±SE) of at least three experiments, each performed in sextuplicate. *p < 0.05; **p < 0.001.

Next, we tested whether spontaneous regeneration and growth of neonatal rat spinal cord is cAMP dependent. P2-3 rat spinalcords were lesioned by overhemisection (all axons in one halfof the spinal cord are lesioned along with all dorsal column axons),and the PKA inhibitor, H89, was applied. We have shown previouslythat implantation of embryonic spinal cord tissue into the lesionsite enhances both survival and regeneration at P3 and P8 butdoes not alter the general outcome; at P3, spinal axons grow intoand through the implanted tissue, whereas at P8 axons grow onlya short distance into the implanted tissue and never out intothe distant host tissue (Bregman, 1987a; Bregman et al., 1989;Bernstein-Goral and Bregman, 1993). Therefore, the H89 was appliedeither directly to the lesion site via Gelfoam or to the embryonicgrafted tissue, also via Gelfoam. After 2 weeks, corticospinalaxons were labeled by anterograde tracing methods, and raphespinaltract axons were labeled by immunostaining for serotonin. Thetreatment with H89 did not alter the survival of the transplantsor their apposition with the host tissue. Also, the morphology,as assessed by staining with cresyl violet, of the transplantedcells was unchanged by H89 treatment (data not shown). Healthytransplants with areas of good apposition in the host spinal cordwere identified in 5 of 7 lesion plus transplant animals treatedwith saline (71%) and in 8 of 11 lesion plus transplant animalstreated with H89 (73%). This rate of survival was equivalent tothat observed in earlier studies from this laboratory and wassimilar in H89- and saline-treated groups. The axonal growth inthe H89-treated animals was compared with animals treated withsaline. In most of the animals treated with H89 (n = 21), a visualdifference from control (n = 17) was immediately apparent, inboth the length and the number of corticospinal and raphespinalaxons at the lesion or lesion plus transplant site. Results froma typical experiment for corticospinal axons are shown in Figure6. In the H89-treated animals, the axonal growth characteristicof developmental plasticity was greatly attenuated in both thelesion only and lesion plus transplant animals. The dense axonalgrowth characteristic of early lesions was decreased markedlyin 18 of the 21 H89-treated animals (Fig. 6A--D; arrows in D pointto the little regeneration that is apparent in the H89-treatedanimals). Similar results were obtained for the raphespinal tractaxons that were stained for serotonin (data not shown). The extentof axonal growth within the transplants was scored for the saline-and H89-treated groups (Table 1). These results clearly showthat the spontaneous regeneration and continued growth of youngspinal cord axons in vivo is cAMP dependent.

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Figure 6. Regeneration of neonatal spinal axons in vivo is cAMP-dependent. P2-3 rat pups were subjected to overhemisection lesion of their spinal cords at T6. Embryonic spinal cord transplants were placed into the lesion site without (A, B) or with H89 (0.5 mM) (C, D). Corticospinal axons were labeled anterogradely with BDA, and animals were killed at 4 weeks after transplantation. Dashed lines (A, C) indicate the approximate border between host and transplant (TP) tissue, and the boxed areas in A and C are shown at higher magnification in B and D, respectively. Corticospinal axon growth within the transplant is dramatically decreased in the presence of H89. Arrows in C indicate the few axons that regenerated into the TP in the H89-treated animal. A similar decrease in axonal growth by H89 was also seen for serotonergic axons (data not shown). Scale bars, 100 µm.


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Table 1. Scoring axonal growth within transplant

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study represents the first step toward a molecular understanding of the switch during development that results in theinhibition of axonal regeneration by myelin and consequently theinability to regenerate in vivo. Here, we show that the endogenouslevel of cAMP in three different types of neuron drops dramaticallywith development and that this spontaneous decrease in cAMP coincideswith a switch to the inhibition of regeneration by myelin-MAG.We also show that inhibition in older neurons can be preventedby elevating cAMP and that inhibiting a signal downstream of cAMPactivation (inhibition of PKA) can block early developmental promotionof axonal regeneration by myelin-MAG. Consistent with their relativelyhigh levels of cAMP and ability to grow well on myelin and MAGin culture, the ability of young axons to spontaneously regenerateafter injury in vivo is also dependent on activation of PKA. Theseresults are important for two reasons. First, they identify forthe first time a molecular difference between young and adultneurons that determines their response to inhibitors in myelinand consequently their ability to regenerate. The strong implicationis that artificially adjusting cAMP levels or manipulating PKAactivity in adult neurons may offer a means to support regenerationafter injury. Second, the results demonstrate that the physiologicallevels of cAMP change sufficiently with development to the pointat which they can effect the switch from promotion to inhibitionin response to myelin-MAG. Others have shown in vitro that alteringcAMP levels can reverse the turning of Xenopus growth cones inresponse to a number of different guidance cues (Ming et al.,1997; Song et al., 1997, 1998). The relevance of those observationsto events in vivo was not demonstrated previously. In addition,neither was it shown that the changes in cAMP necessary for suchdramatic switches in guidance response were inside the physiologicalrange in vivo. Here, we show, at least for myelin and MAG, thatthese changes are well within physiological ranges. Therefore,it is highly likely that endogenous cAMP levels determine theguidance response to other molecules in vivo.

It should be noted that a second group of guidance cues, although independent of cAMP, are dependent on the cyclic nucleotidecGMP for dictating the response of the neuron (Ming et al., 1997).Importantly, Polleux et al. (2000) showed recently that axonsof pyramidal neurons are repelled by the guidance molecule, Sem3A,whereas dendrites of the same neuron are attracted by Sem3A. Asymmetricdistribution of the cGMP synthesizing enzyme, guanylate cyclase,and hence, presumably, of cGMP, is responsible for the oppositeeffects of Sema3A on axons and dendrites; cGMP is high in dendritesand low in the axon. Our findings here indicate that inhibitionnot only by MAG but also by myelin inhibitors in general, whichmust include the recently described inhibitor Nogo (Chen et al.,2000; GrandPre et al., 2000), are largely cAMP dependent. Recently,it was shown that inactivation of the small GTPase, Rho, not onlyblocked inhibition by MAG and myelin but also allowed regenerationin vivo (Lehmann et al., 1999). It is possible that cAMP-dependentactivation of PKA has a direct effect on Rho signaling. In addition,because all neuronal types tested to date respond by either inhibitionor promotion, depending on age, we can conclude that they allexpress the myelin-MAG receptor(s). Because cAMP levels are sufficientto determine whether inhibition or promotion of neurite outgrowthoccurs, the myelin-MAG neuronal receptor(s) is likely to be identicalfor each effect and in each type of neuron. For other guidancecues that are reversed by altering cAMP signaling, the importanceof the cytoplasmic domains of certain receptors in determiningthe response to those cues has been demonstrated (Bashaw and Goodman,1999; Hong et al., 1999). However, it is possible that signalingthrough particular receptors directly alters cyclic nucleotidelevels and so influences whether there is an attractive or repulsiveeffect. Indeed, a coreceptor for one such bifunctional guidancecue, Netrin, is the A2b adenosine receptor that, when activated,directly affects cellular cAMP levels (Corset et al., 2000).

In addition to inhibitors in myelin, other factors also affect regeneration in vivo (Schwab and Bartholdi, 1996). The formationof the glial scar is a major obstacle to regrowth. However, theglial scar takes time to form, and the recent report of regenerationin myelin-immunized mice clearly shows that myelin componentsstop growth immediately after injury; their neutralization withantibodies allows growth before the scar forms (Huang et al.,1999). In addition, adult neurons have been shown to extend longaxons when they are transplanted into the adult CNS with suchcare that no scar forms (Davies et al., 1997, 1999). Importantly,under these conditions, myelin is not damaged. Consequently, theseaxons grow on the outer surface of undamaged myelin, which containsmolecules shown to be permissive for growth (Turnley and Bartlett,1998). Myelin inhibitors, therefore, are only exposed afterdamage.

What causes the decline in the endogenous levels of cAMP in neurons with development? There could be some developmental switchin enzymes that synthesize or degrade cAMP. Isoforms of PKA maychange with development. This could affect the "free" levels ofcAMP and the threshold level of cAMP required for PKA activation.Alternatively, we showed previously that the inhibition of axonalregeneration by myelin-MAG could be blocked if neurons were exposedto various neurotrophins before their exposure to the inhibitor,a process we termed "priming with neurotrophin" (Cai et al., 1999).Furthermore, the block of inhibition by priming with neurotrophinwas cAMP dependent, and the neurotrophins used were shown to elevateneuronal cAMP levels. Coupled with the demonstration that expressionin vivo of both neurotrophins and their receptors (along withpeptides and hormones more traditionally regarded as cAMP activators)declines with development (Jelsma and Aguayo, 1994), these observationsraise the likelihood that neurotrophins and growth factors inthe environment regulate the cAMP levels of neurons. The samemolecules can then be seen to dictate the response to myelin-MAG.Because there is strong evidence implicating cAMP-dependent eventsin plasticity (Bailey et al., 1996), it is notable that the switchin response of neurons to myelin-MAG accompanies, at about essentiallythe same time, the developmental loss of neuronal plasticity.One possibility is that the spontaneous decrease in neuronal cAMPnot only mediates the switch from promotion to inhibition of axonalregeneration by myelin-MAG but also leads to the loss of neuronalplasticity. Interestingly, the physiological function of inhibitionby myelin-MAG is suggested to control sprouting (Schwegler etal., 1995), a phenomenon closely associated with neuronal plasticity.Endogenous cAMP levels may also affect neuronal survival becauseelevating cAMP has been shown to potentiate the effects of a numberof neurotrophins (Meyer-Franke et al., 1995; Hanson et al., 1998;Shen et al., 1999). However, the ability of elevated cAMP to overcomeinhibition by myelin-MAG is not purely a consequence of improvedsurvival because elevated cAMP does not affect axonal growth oncontrol cells. In addition, for RG neurons at least, elevatedcAMP alone is insufficient to improve survival (Shen et al., 1999).It is also of note that mice overexpressing the anti-apoptoticprotein, bcl-2, show improved survival but no improved regenerativecapacity (Chierzi et al., 1999). Finally, all of these cAMP-affectedphenomena (regeneration, plasticity, and survival) are connectedin that they switch with development, are likely to share similarmechanisms, and are all required for functional recovery afterinjury.

  FOOTNOTES

Received Jan. 16, 2001; revised March 21, 2001; accepted April 17, 2001.

This work was supported by grants from the National Multiple Sclerosis Society (NMSS), the National Institutes of Health (NIH)(NS 37060 to M.T.F. and NS19259 to B.S.B.), and a core facilitygrant from the Research Centers for Minorities Institute-NIH.J.Q. is a fellow of the NMSS. We thank Dr. Arthur McMorris andDr. Anthony Weimelt for providing the cAMP antibody, Dr. RogerPersell for critically reading this manuscript, and Dr. LloydWilliams for his assistance with the imageanalysis.
D.C. and J.Q. contributed equally to thisstudy.

Correspondence should be addressed to Dr. Marie T. Filbin, Biology Department, Hunter College, 695 Park Avenue, New York,NY 10021. E-mail: filbin{at}genectr.hunter.cuny.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Bailey CH, Bartsch D, Kandel ER (1996) Toward a molecular definition of long-term memory storage. Proc Natl Acad Sci USA 93:13445-13452[Abstract/Free Full Text].
Bashaw GJ, Goodman CS (1999) Chimeric axon guidance receptors: the cytoplasmic domains of slit and netrin receptors specify attraction versus repulsion. Cell 97:917-926[ISI][Medline].
Bates CA, Stelzner DJ (1993) Extension and regeneration of corticospinal axons after early spinal injury and the maintenance of corticospinal topography. Exp Neurol 123:106-117[ISI][Medline].
Bernstein-Goral H, Bregman BS (1993) Spinal cord transplants support the regeneration of axotomized neurons after spinal cord lesions at birth: a quantitative double-labeling study. Exp Neurol 123:118-132[ISI][Medline].
Bregman BS (1987a) Spinal cord transplants permit the growth of serotonergic axons across the site of neonatal spinal cord transection. Brain Res 431:265-279[Medline].
Bregman BS (1987b) Development of serotonin immunoreactivity in the rat spinal cord and its plasticity after neonatal spinal cord lesions. Brain Res 431:245-263[Medline].
Bregman BS, Goldberger ME (1982) Anatomical plasticity and sparing of function after spinal cord damage in neonatal cats. Science 217:553-555[Abstract/Free Full Text].
Bregman BS, Goldberger ME (1983) Infant lesion effect: III. Anatomical correlates of sparing and recovery of function after spinal cord damage in newborn and adult cats. Brain Res 285:137-154[Medline].
Bregman BS, McAtee M (1993) Embryonic CNS tissue transplantation for studies of development and regeneration. Neuroprotocols 3:17-27.
Bregman BS, Kunkel-Bagden E, McAtee M, O'Neill A (1989) Extension of the critical period for developmental plasticity of the corticospinal pathway. J Comp Neurol 282:355-370[ISI][Medline].
Bregman BS, Kunkel-Bagden E, Reier PJ, Dai HN, McAtee M, Gao D (1993) Recovery of function after spinal cord injury: mechanisms underlying transplant-mediated recovery of function differ after spinal cord injury in newborn and adult rats. Exp Neurol 123:3-16[ISI][Medline].
Bregman BS, McAtee M, Dai HN, Kuhn PL (1997) Neurotrophic factors increase axonal growth after spinal cord injury and transplantation in the adult rat. Exp Neurol 148:475-494[ISI][Medline].
Cai D, Shen Y, De Bellard M, Tang S, Filbin MT (1999) Prior exposure to neurotrophins blocks inhibition of axonal regeneration by MAG and myelin via a cAMP-dependent mechanism. Neuron 22:89-101[ISI][Medline].
Chen MS, Huber AB, van der Haar ME, Frank M, Schnell L, Spillmann AA, Christ F, Schwab ME (2000) Nogo-A is a myelin-associated neurite outgrowth inhibitor and an antigen for monoclonal antibody IN-1. Nature 403:434-439[Medline].
Cheng H, Cao Y, Olson L (1996) Spinal cord repair in adult paraplegic rats: partial restoration of hind limb function. Science 273:510-513[Abstract].
Chierzi S, Strettoi E, Cenni MC, Maffei L (1999) Optic nerve crush: axonal responses in wild-type and bcl-2 transgenic mice. J Neurosci 19:8367-8376[Abstract/Free Full Text].
Colamarino SA, Tessier-Lavigne M (1995) The axonal chemoattractant netrin-1 is also a chemorepellent for trochlear motor axons. Cell 81:621-629[ISI][Medline].
Corset V, Nguyen-Ba-Charvet KT, Forcet C, Moyse E, Chedotal A, Mehlen P (2000) Netrin-1-mediated axon outgrowth and cAMP production requires interaction with adenosine A2b receptor. Nature 407:747-750[Medline].
Crutcher KA (1989) Tissue sections from the mature rat brain and spinal cord as substrates for neurite outgrowth in vitro: extensive growth on gray matter but little growth on white matter. Exp Neurol 104:39-54[ISI][Medline].
David S, Aguayo AJ (1981) Axonal elongation into peripheral nervous system "bridges" after central nervous system injury in adult rats. Science 214:931-933[Abstract/Free Full Text].
Davies SJ, Fitch MT, Memberg SP, Hall AK, Raisman G, Silver J (1997) Regeneration of adult axons in white matter tracts of the central nervous system. Nature 390:680-683[Medline].
Davies SJ, Goucher DR, Doller C, Silver J (1999) Robust regeneration of adult sensory axons in degenerating white matter of the adult rat spinal cord. J Neurosci 19:5810-5822[Abstract/Free Full Text].
DeBellard ME, Tang S, Mukhopadhyay G, Shen YJ, Filbin MT (1996) Myelin-associated glycoprotein inhibits axonal regeneration from a variety of neurons via interaction with a sialoglycoprotein. Mol Cell Neurosci 7:89-101[ISI][Medline].
Diener PS, Bregman BS (1998) Fetal spinal cord transplants support growth of supraspinal and segmental projections after cervical spinal cord hemisection in the neonatal rat. J Neurosci 18:779-793[Abstract/Free Full Text].
GrandPre T, Nakamura F, Vartanian T, Strittmatter SM (2000) Identification of the Nogo inhibitor of axon regeneration as a Reticulon protein. Nature 403:439-444[Medline].
Hanson MG, Shen Jr S, Wiemelt AP, McMorris FA, Barres BA (1998) Cyclic AMP elevation is sufficient to promote the survival of spinal motor neurons in vitro. J Neurosci 18:7361-7371[Abstract/Free Full Text].
Hasan SJ, Keirstead HS, Muir GD, Steeves JD (1993) Axonal regeneration contributes to repair of injured brainstem-spinal neurons in embryonic chick. J Neurosci 13:492-507[Abstract].
Herzog A, Brosamle C (1997) 'Semifree-floating' treatment: a simple and fast method to process consecutive sections for immunohistochemistry and neuronal tracing. J Neurosci Methods 72:57-63[ISI][Medline].
Hong K, Hinck L, Nishiyama M, Poo MM, Tessier-Lavigne M, Stein E (1999) A ligand-gated association between cytoplasmic domains of UNC5 and DCC family receptors converts netrin-induced growth cone attraction to repulsion. Cell 97:927-941[ISI][Medline].
Huang DW, McKerracher L, Braun PE, David S (1999) A therapeutic vaccine approach to stimulate axon regeneration in the adult mammalian spinal cord. Neuron 24:639-647[ISI][Medline].
Jelsma TN, Aguayo AJ (1994) Trophic factors. Curr Opin Neurobiol 4:717-725[Medline].
Johnson PW, Abramow-Newerly W, Seilheimer B, Sadoul R, Tropak MB, Arquint M, Dunn RJ, Schachner M, Roder JC (1989) Recombinant myelin-associated glycoprotein confers neural adhesion and neurite outgrowth function. Neuron 3:377-385[ISI][Medline].
Keirstead HS, Hasan SJ, Muir GD, Steeves JD (1992) Suppression of the onset of myelination extends the permissive period for the functional repair of embryonic spinal cord. Proc Natl Acad Sci USA 89:11664-11668[Abstract/Free Full Text].
Lehmann M, Fournier A, Selles-Navarro I, Dergham P, Sebok A, Leclerc N, Tigyi G, McKerracher L (1999) Inactivation of rho signaling pathway promotes CNS axon regeneration. J Neurosci 19:7537-7547[Abstract/Free Full Text].
Li Y, Raisman G (1993) Long axon growth from embryonic neurons transplanted into myelinated tracts of the adult rat spinal cord. Brain Res 629:115-127[ISI][Medline].
McKerracher L, David S, Jackson DL, Kottis V, Dunn RJ, Braun PE (1994) Identification of myelin-associated glycoprotein as a major myelin-derived inhibitor of neurite growth. Neuron 13:805-811[ISI][Medline].
Meyer-Franke A, Kaplan MR, Pfrieger FW, Barres BA (1995) Characterization of the signaling interactions that promote the survival and growth of developing retinal ganglion cells in culture. Neuron 15:805-819[ISI][Medline].
Ming GL, Song HJ, Berninger B, Holt CE, Tessier-Lavigne M, Poo MM (1997) cAMP-dependent growth cone guidance by netrin-1. Neuron 19:1225-1235[ISI][Medline].
Mukhopadhyay G, Doherty P, Walsh FS, Crocker PR, Filbin MT (1994) A novel role for myelin-associated glycoprotein as an inhibitor of axonal regeneration. Neuron 13:757-767[ISI][Medline].
Polleux F, Morrow T, Ghosh A (2000) Semaphorin 3A is a chemoattractant for cortical apical dendrites. Nature 404:567-573[Medline].
Quarles RH (1983) Myelin-associated glycoprotein in development and disease. Dev Neurosci 6:285-303[Medline].
Richardson PM, McGuinness UM, Aguayo AJ (1980) Axons from CNS neurons regenerate into PNS grafts. Nature 284:264-265[Medline].
Salzer JL, Pedraza L, Brown M, Struyk A, Afar D, Bell J (1990) Structure and function of the myelin-associated glycoproteins. Ann N Y Acad Sci 605:302-312[ISI][Medline].
Schnell L, Schwab ME (1990) Axonal regeneration in the rat spinal cord produced by an antibody against myelin-associated neurite growth inhibitors. Nature 343:269-272[Medline].
Schwab ME, Bartholdi D (1996) Degeneration and regeneration of axons in the lesioned spinal cord. Physiol Rev 76:319-370[Abstract/Free Full Text].
Schwab ME, Kapfhammer JP, Bandtlow CE (1993) Inhibitors of neurite growth. Annu Rev Neurosci 16:565-595[ISI][Medline].
Schwegler G, Schwab ME, Kapfhammer JP (1995) Increased collateral sprouting of primary afferents in the myelin-free spinal cord. J Neurosci 15:2756-2767[Abstract].
Shen S, Wiemelt AP, McMorris FA, Barres BA (1999) Retinal ganglion cells lose trophic responsiveness after axotomy. Neuron 23:285-295[ISI][Medline].
Shewan D, Berry M, Cohen J (1995) Extensive regeneration in vitro by early embryonic neurons on immature and adult CNS tissue. J Neurosci 15:2057-2062[Abstract].
Song H, Ming G, He Z, Lehmann M, McKerracher L, Tessier-Lavigne M, Poo M (1998) Conversion of neuronal growth cone responses from repulsion to attraction by cyclic nucleotides. Science 281:1515-1518[Abstract/Free Full Text].
Song HJ, Ming GL, Poo MM (1997) cAMP-induced switching in turning direction of nerve growth cones. Nature 388:275-279[Medline]. [Erratum (1997) 389:412]
Turnley AM, Bartlett PF (1998) MAG and MOG enhance neurite outgrowth of embryonic mouse spinal cord neurons. NeuroReport 9:1987-1990[Medline].
Veenman CL, Reiner A, Honig MG (1992) Biotinylated dextran amine as an anterograde tracer for single- and double-labeling studies. J Neurosci Methods 41:239-254[ISI][Medline].
Wiemelt AP, Engleka MJ, Skorupa AF, McMorris FA (1997) Immunochemical visualization and quantitation of cyclic AMP in single cells. J Biol Chem 272:31489-31495[Abstract/Free Full Text].

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