Cytoskeletal and Morphological Alterations Underlying Axonal Sprouting after Localized Transection of Cortical Neuron Axons In Vitro

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The Journal of Neuroscience, May 1, 2003, 23(9):3715

Cytoskeletal and Morphological Alterations Underlying Axonal Sprouting after Localized Transection of Cortical Neuron Axons In Vitro
Jyoti A. Chuckowree and James C. Vickers
Discipline of Pathology, Faculty of Health Sciences, University of Tasmania, Hobart, Tasmania, 7000, Australia

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

We examined the cytoskeletal dynamics that characterize neurite sprouting after axonal injury to cortical neurons maintainedin culture for several weeks and compared these with initial neuritedevelopment. Cultured neocortical neurons, derived from embryonicday 18 rats, were examined at 3 d in vitro (DIV) and at varioustime points after axotomy at 21 DIV. The postinjury neuritic responsewas highly dynamic, progressing through an initial phase of retraction,followed by substantial axonal sprouting within 4-6 hr. Postinjurysprouts were motile and slender with expanded growth cone-likeend structures. Microtubule markers were localized to sprout shaftsand the proximal regions of putative growth cones and filamentousactin was distributed throughout growth cones, whereas neurofilamentproteins were restricted to sprout shafts. A similar distributionof cytoskeletal proteins was present in developing neurites at3 DIV. Exposure of developing and mature, injured cultures tothe microtubule stabilizing agent taxol (10 µg/ml) caused growthinhibition, process distension, the transformation of growth conesinto bulbous structures, and abnormal neurite directionality.Microtubule and neurofilament segregation occurred after taxolexposure in developing neurites and postinjury sprouts. Exposureto the microtubule destabilizing agent nocodazole (100 µg/ml)resulted in substantial morphological alteration of developingneurons and inhibited neurite growth and postinjury axonal sprouting.Our results indicate that the axons of cortical neurons have anintrinsic ability to sprout after transection, and similar cytoskeletaldynamics underlie neurite development and postinjury axonalsprouting.

Key words: Alzheimer's disease; axonal sprouting; axonal transection; $beta$ III-tubulin; brain trauma; cortical neuron culture; cytoskeleton; growth cone; microtubules; neurite development; posttraumatic epilepsy; neurofilament; tau; taxol

  Introduction

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The axonal cytoskeleton, particularly microfilaments and microtubules, is necessary for axonal outgrowth, elongation, branching,and pathfinding (for review, see Tanaka and Sabry, 1995; Brandt,1998; Gallo and Letourneau, 2000; Korey and Van Vactor, 2000;Suter and Forscher, 2000). The complex interactions between thepolymerization states of these cytoskeletal structures providesthe dynamic driving force underlying axon elongation and growthcone motility (Kalil et al., 2000). In contrast, neurofilaments,the third main polymer constituent of the axonal cytoskeleton,may act in axonal radial growth and provide maturing neurons withstructural support (Hoffman et al., 1984, 1985, 1987; Julien andGrosveld, 1991; Nixon and Sihag, 1991; Lee and Cleveland, 1996)but are not necessary for outgrowth. This is highlighted by theability of developing axons lacking neurofilaments to grow, albeitmore slowly (Walker et al., 2001), and neurofilament deficientanimals to develop relatively normally (Zhu et al., 1997; Levavasseuret al., 1999).

The axonal cytoskeleton also plays an important role in the neuronal response to trauma (Maxwell et al., 1997). Nonpenetrativehead trauma frequently causes cytoskeletal disruption leadingto delayed axotomy (Povlishock and Christman, 1995; Povlishockand Jenkins, 1995; Maxwell et al., 1997). Several studies havedemonstrated a reduction in the levels of microtubules and accumulationsof neurofilaments in areas of axonal disruption (Jafari et al.,1997, 1998; Maxwell and Graham, 1997; Adlard et al., 2000; Dicksonet al., 2000; King et al., 2001).

Traditionally, there has been significant pessimism regarding the potential for regeneration in the mature CNS, attributedprimarily to the inhibitory nature of CNS parenchyma (Berry etal., 1994; Fawcett, 1997; Bandtlow and Schwab, 2000; Goldbergand Barres, 2000; Qiu et al., 2000). However, several reportssuggest that central neurons respond to injury with a complexsequence of morphological, biochemical, and gene expression alterations,directed toward sprouting, regeneration, and synaptogenesis (Christmanet al., 1997; Deller and Frotscher, 1997; Pastor et al., 2000;Vickers et al., 2000; King et al., 2001). Attempted regenerationof mature neurons is associated with substantial cytoskeletalreorganization (Christman et al., 1997; Dickson et al., 2000;King et al., 2001), resulting in the elaboration of fine protrusions(sprouts) into and across lesion sites (McHale et al., 1995; Christmanet al., 1997; Deller and Frotscher, 1997; McKinney et al., 1997;King et al., 2001). However, aberrant axonal sprouting has beenimplicated in the development of posttraumatic epilepsy afterhuman brain trauma (Larner, 1995; McKinney et al., 1997) and thepathogenesis of Alzheimer's disease (Masliah et al., 1991, 1992;Vickers et al., 2000; Arendt, 2001).

We used a novel in vitro model of CNS trauma, involving transection of axonal bundles (Dickson et al., 2000), to characterizethe morphological and cytoskeletal alterations underlying thepostinjury sprouting response of neurons cultured for severalweeks to relative maturity. We compared the sprouting responsewith the cytoskeletal dynamics underlying initial neurite developmentof cultured cortical neurons. Finally, we investigated the consequencesof microtubule stabilization and destabilization, using taxoland nocodazole, respectively, on initial neurite growth and postinjuryaxonalsprouting.

  Materials and Methods

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Cell culture. Primary dissociated cortical neuron cultures were prepared from rat embryos at 18 d of gestation using standardtechniques (Banker and Goslin, 1998) and grown in Neurobasal mediato selectively promote the growth of neuronal cells (Brewer etal., 1993; Brewer, 1995, 1997). Pregnant Hooded Wistar rats werekilled by carbon dioxide exposure. Embryos were rapidly removedusing sterile techniques and placed on ice, and, after removalof the skull and meninges, the neocortical hemispheres were dissectedout and placed in 10 mM HEPES buffer (in 0.01 M PBS), prewarmedto 37°C. Cortical tissue was dissociated by enzymatic digestion(0.025% trypsin) and gentle agitation at 37°C for 20 min. Enzymaticdigestion was halted by rinsing the tissue in fresh 10 mM HEPESbuffer, and dissociation was completed by gentle trituration usinga 1 mlpipette.

Before plating, cell viability was assessed using trypan blue vital dye exclusion. Cells were plated, at a density of 4.5× 10⁵ cells per coverslip, onto circular 19-mm-diameter glass coverslips(Marienfeld, Lauda-Köigshofen, Germany), immersed in an initialplating media, consisting of Neurobasal media, 10% fetal bovineserum, 2% B-27 supplement (all from Invitrogen, Grand Island,NY), 0.5 mM L-glutamine, 25 µM glutamate, and 1 ml/l gentamicin.Coverslips had been previously nitric acid etched and preincubatedin 1 mg/ml L-lysine (Sigma, St. Louis, MO) in borate buffer, pH7.4, overnight, before being placed into individual wells of 12-wellmicroplates (Iwaki, Tokyo, Japan), each containing 2 ml of initialplatingmedia.

Cultures were maintained in a 37°C humidified atmosphere of 5% CO₂ for up to 22 d. After 1 d in vitro (DIV), the initial platingmedia was removed and replaced with a "subsequent," serum-freegrowth media containing Neurobasal media, 2% B-27 supplement,0.5 mM L-glutamine, and 3 ml/l gentamicin. One-half of the volumeof culture media was replenished every 3-4 d with fresh subsequentgrowthmedia.

Axonal injury. Axonal injury was performed as described by Dickson et al. (2000). At 20 DIV, coverslips were transferred toindividual 35 mm sterile plastic Petri dishes (Iwaki) and allowedto reacclimatize to the incubator conditions. At 21 DIV, individualaxonal bundles, interconnecting discrete neuronal aggregates,were transected under microscope guidance using a 12 cm Barkangoniotomy curved-blade diamond knife. Thick axonal bundles, adherentto the underlying substrate, were selected for transection. Theknife blade was carefully pressed on the appropriate axonal bundlesto completely transect the axons and form a cell-free lesion betweentwo previously interconnected neuronal aggregates. Cuts were madeequidistant between neuronal aggregates to produce lesions ~50-150µm wide. Several (10-15) injuries were made per coverslip. Cultureswere removed from the incubator for no longer than 5 min (becauselonger durations compromised neuronal integrity). Cultures werereincubated for 4, 14, or 24 hr afterinjury.

Taxol and nocodazole administration. Taxol powder (Amersham Biosciences, San Francisco, CA) was reconstituted in sterile 0.01M PBS to achieve a concentration of 1 mg/ml and added to the subsequentmedia of cultures at a concentration of 10 µg/ml. Nocodozole (Sigma)was reconstituted in sterile 12% DMSO-0.01 M PBS and added tocultures at a final concentration of 100 µg/ml. Vehicle-treatedcultures (10 µl/ml PBS for taxol studies or 100 µl/ml 12% DMSO-PBSfor nocodozole studies) were processed concurrently to serve ascontrols. To determine the effect of microtubule stabilization(using taxol) on neurite development, cultures were incubatedin taxol for 48 hr, between 3 and 5 DIV. To determine the effectof taxol on postinjury axonal sprouting, taxol was administeredto the subsequent media of cultures immediately after localizedaxotomy at 21 DIV. Cultures were reincubated for 4, 14, or 24hr after injury. Studies into whether the effects of taxol couldbe reversed were performed using 1 µg/ml taxol (because higherconcentrations caused substantial cell death with prolonged exposure).To investigate the permanency of taxol-induced microtubule stabilization,taxol was washed out of developing cultures at 5 DIV, and cultureswere maintained as normal for up to 21 DIV and compared with vehicle-treatedcultures, as well as cultures that were constantly exposed totaxol. For postinjury studies, taxol was washed out of mature,injured cultures 4 hr after injury, and cultures were allowedto recover for an additional 20 hr before fixation. To assay theeffect of microtubule destabilization on developing and mature,injured cultures, cultures were exposed to nocodazole for 48 hrbetween 3 and 5 DIV or for 4 hr immediately after axonal transectioninjury at 21DIV.

Immunohistochemistry. Cultured neurons were fixed in 4% paraformaldehyde at 37°C for 30 min. Indirect double-immunofluorescentlabeling was used to visualize the distribution of specific cytoskeletalcomponents in developing neurites, as well as injured and non-injuredmature axons. Briefly, cultured monolayers were incubated in combinationsof mouse and rabbit primary antibodies (18-20 hr) (Table 1),followed by incubation in secondary antibodies (1 hr). Mouse andrabbit primary antibodies were visualized with goat anti-mouseAlexaFluor 488 and goat anti-rabbit AlexaFluor 594 secondary antibodies(dilution 1:1000; Molecular Probes, Eugene, OR), respectively.To label for filamentous actin (F-actin), cultures were incubatedwith AlexaFluor 488 phalloidin (dilution 1:200; Molecular Probes),for 30 min after immunohistochemistry. After washing, coverslipswere air dried and mounted onto glass slides using Permafluormounting media (Immunotech, Marseille, France). All antibodieswere diluted in diluent (0.3% Triton X-100 in 0.01 M PBS). Controls,omitting the primary antibodies, were processed concurrently andlacked immunoreactivity for the cellular components under investigation.


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Table 1. Primary antibodies

Assay of cell proliferation. To determine the approximate birth dates of cortical neurons in vitro, cultures were incubatedwith 10 µM of the thymadine analog 5-bromo-2'-deoxyuridine (BrdU)(Sigma) for 72 hr at either 7 or 17 DIV. Addition of BrdU (1 or5 µM) to cultures was also attempted at earlier time points (1-3DIV) but resulted in substantial cell death by 21 DIV. Culturesunderwent a complete media change to remove any unincorporatedBrdU and were grown to 21 DIV. After fixation (4% paraformaldehyde),DNA denaturation was performed by incubating cultures in 2 M HClfor 1 hr at 37°C. Dividing cells were visualized by immunolabelingwith an antibody against BrdU (Table 1). To confirm the absenceof neuronal proliferation in cortical cultures, some cultureswere also immunolabeled with an antibody against postmitotic neuronalnuclei (Table 1).

Electron microscopy. For scanning electron microscopy studies, cultures growing on circular glass coverslips were fixed with2.5% glutaraldehyde in 0.1 M phosphate buffer, pH 7.4, for 20min at room temperature, postfixed with 0.1% osmium tetraoxidein phosphate buffer, at room temperature for 15 min, and dehydratedthrough a graded ethanol series. Specimens were critical-pointdried with CO₂, mounted onto copper stubs and sputter coated withgold for observation with a Jeol (Peabody, MA) JSM-840 scanningelectron microscope. For transmission electron microscopy studies,cortical cultures were fixed in 2.5% glutaraldehyde in 0.1 M phosphatebuffer, at 37°C for 10 min. Cultures were postfixed in 1.5% osmiumtetroxide in 0.1 M phosphate buffer at room temperature for 30min, followed by 2% uranyl acetate in 70% ethanol for 5 min. Cultureswere then dehydrated through a graded ethanol series and embeddedin 100% Epon. Specimens were sectioned at 70 nm, stained with5% uranyl acetate (10 min) and Reynolds lead citrate (10 min),and examined on a Philips EM-410 transmission electronmicroscope.

Microscopy and digital imaging. Time-lapse digital imaging was used to investigate the effect of taxol on growth cone motilityand morphology, as well as the dynamic response of neurons tolocalized axotomy. At 1 d before imaging, cultured monolayers,growing on glass coverslips, were transferred to individual 35mm glass Petri dishes. The Neurobasal media, in which the neuronswere growing, was gradually replaced with "imaging buffer" (inmM: 124 NaCl, 5 KCl, 0.2 CaCl₂, 1 MgCl₂, 30 dextrose, and 25 HEPES,pH 7.3) (Zhang and Benson, 2001) over a time course of 1 hr beforeimaging, to promote neuronal survival when imaging over severalhours. Using differential interference contrast (Nomarski) microscopy,a time series of images were captured from a Leica (Nussloch,Germany) DM IRB inverted microscope, equipped with a heating stage.Digital images of immunofluorescence-labeled specimens and livecell images were captured with a Magnifire digital camera (Optronics,Chelmsford, MA), attached to a G4 Macintosh computer (Apple Computers,Cupertino,CA).

Quantitative analysis. The effect of taxol on neurite development was analyzed by determining the proportion of neurites tippedby a growth cone. A growth cone was defined as a fan-shaped structureat the tip of a neurite, with a width three times greater thanits neurite of origin. The effect of taxol treatment on neuritelength was also determined. Digital images of immunofluorescence-labeledspecimens were captured before treatment and after vehicle ortaxol treatment, and the lengths of 100 neurites from each categoryweremeasured.

The effect of taxol on postinjury axonal sprouting was determined in terms of sprout number and sprout length, 4 hr afterinjury. Cultures injured by axonal transection were incubatedin taxol or vehicle for 4 hr immediately after injury, followedby paraformaldehyde fixation and immunofluorescence labeling.Digital images of several individual injury sites were captured.To quantitate the effect of taxol on sprout elongation, the lengthof 100 postinjury axonal sprouts were measured from vehicle- andtaxol-treated fellow cultures. Additionally, to determine theeffect of taxol on sprout elaboration, the number of postinjuryaxonal sprouts was calculated from 15 individual cuts from vehicle-and taxol-treated fellow cultures. This value was expressed asthe number of sprouts per 100 µm of cut sitelength.

For quantitation, taxol-related experiments were repeated five times (i.e., on cultures derived from five individual litters),and studies were performed by an investigator blind to the treatmentof the cultures under investigation. NIH Image (version 1.61)software was used to capture digital images and perform measurements.Statistical analysis was performed using StatView (version 5.0)software (SAS Institute, Cary, NC). As appropriate, paired t testsor ANOVA was performed on quantitative data. Post hoc comparisons(Fisher's test) were performed afterANOVA.

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

In vitro cortical neuron development

In the days after plating, dissociated cortical neurons formed aggregates, adhered to the coverslip substrate, and elaboratedslender neurites. Analysis of the morphological and cytoskeletalcharacteristics of developing cortical neurons was performed at3 DIV. Figure 1 illustrates the localization of specific cytoskeletalcomponents in developing neurites at 3 DIV. The distribution ofmicrotubules within developing neurons was visualized using anantibody with specificity for the neuron-specific $beta$ III-tubulinsubunit of microtubules (Lee et al., 1990) and an antibody againstthe microtubule-associated protein tau. Both $beta$ III-tubulin andtau were localized throughout entire neurons, extending into thetapered extremities of dendrites and splayed extremities of axons,as well as the growth cone remnants (Szebenyi et al., 1998; Kalilet al., 2000), spikes, and small branches located along the lengthsof some neurites. Colocalization analysis demonstrated extensivelabeling of neurites and growth cones for $beta$ III-tubulin (Fig. 1B)and tau (Fig. 1C). Both microtubule markers were more abundantin neurite shafts and the central growth cone domain than in theproximal domain of growth cones. Double labeling for phosphorylatedneurofilaments and tau verified the localization of tau throughoutdeveloping neurites and growth cones (Fig. 1E). Phosphorylatedneurofilaments were, however, only localized in a subset of neurites,and labeling was absent in growth cones (Fig. 1D). $beta$ III-Tubulinwas uniformly distributed throughout neurites (Fig. 1F), whereasF-actin, as visualized with AlexaFluor 488 phalloidin, was moreconfined to growth cones, with punctate labeling in neurite shafts(Fig. 1G).

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Figure 1. Cultured cortical neurons at 3 DIV. A shows a typical neuronal aggregate (arrow), from which several neurites were elaborated (arrowheads). B and C illustrate neurites double labeled for $beta$ III-tubulin and tau, respectively. Both proteins were distributed throughout neurite shafts and growth cones. D and E illustrate the same cell double labeled for phosphorylated neurofilaments and tau, respectively. The former were restricted to neurite shafts (arrow in D) and were not localized in growth cones (arrows in E). Figures F and G demonstrate neurites double labeled for $beta$ III-tubulin and F-actin, respectively. F-actin was most abundant in growth cones (arrows in F and G), with punctate distribution along some axons. Scale bars: A, 60 µm; B, C, 15 µm; D, E, 30 µm, F, G, 10 µm.

Microtubule stabilization and destabilization during development

To determine the effect of microtubule stabilization on neuronal development, developing cultures were exposed to taxol (10µg/ml) and examined for morphological and cytoskeletal alterations.Taxol was administered to cultures immediately before imaging,and a series of digital images were captured at 1 min intervalsusing differential interference contrast microscopy. Initially,characteristically splayed growth cones existed at the tips ofneurites; however, in the presence of taxol, the neurites rapidlyformed bulbous end structures, many of which lacked the filopodialprotrusions characteristic of growth cones (Fig. 2A).

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Figure 2. Effect of taxol exposure (10 µg/ml) on neurite morphology and cytoarchitecture. A shows a selection of images from a time-lapse series. Times shown on each image indicate minutes after taxol administration. In the presence of taxol, the originally splayed tips of neurites take on a bulbous morphology (arrows). Immunofluorescence labeling for $beta$ III-tubulin demonstrated that neurites elaborated from vehicle-treated cultures (3-5 DIV) were slender and extended radially, often in defined bundles (arrows in B), whereas neurites from taxol-treated cultures (3-5 DIV) were distended, particularly in their distal domains (arrow in C) and often demonstrated a curled morphology (arrowheads in C). D, $beta$ III-Tubulin labeling of vehicle-treated cultures demonstrating examples of growth cones (exhibiting defined filopodia) located at the distal tips of developing axons (arrows). In the distal tips of taxol-treated developing neurites, $beta$ III-tubulin was localized to club-like (arrows) and loop-like (arrowhead) structures (E). Phosphorylated neurofilaments accumulated into club-like (long arrow), ball-like (short arrow), or loop-like (arrowhead) structures (F). Tau was localized throughout distended neurites and in the filopodial-like protrusions emanating from their distal tips (arrow in G), whereas F-actin was most abundant in neurite tips, forming bulb-like accumulations (H). Scanning EM images of growth cones from vehicle-treated (I) and taxol-treated (J, K) neurons (3-5 DIV). Vehicle-treated growth cones had an elaborate three-dimensional structure (H), whereas taxol-treated growth cones were bulbous, with few remaining filopodia (I, J). Double-labeling analysis demonstrated that some neurites regained growth cones after taxol washout (M, F-actin labeling) and underwent more neurite growth than cultures continually exposed to taxol; however, neurites often remained distended (L, $beta$ III-tubulin). Scale bars: A, D-H, L-M, 20 µm; B, C, 60 µm; I-K, 1 µm.

Developing cultures, incubated in taxol between 3 and 5 DIV, demonstrated substantially altered morphology compared with vehicle-treatedcontrols. Vehicle-treated neuronal aggregates elaborated numerousslender neurites, which extended radially and often in definedbundles. These neurite bundles splayed out distally into individualneurites, many of which were tipped by a growth cone (Fig. 2B,I).In contrast, the neurites of taxol-treated neurons remained localizedaround their neuronal aggregates, often curling and looping backtoward the aggregates from which they originated (Fig. 2C). Comparedwith vehicle-treated neurites (Fig. 2D), taxol-treated neuriteswere thickened and often swollen into bulbous structures at theirdistal tips (Fig. 2E-H,J,K). Furthermore, some neurites retainedaberrant growth cones with filopodial-like protrusions distally,whereas others completely lacked protuberances at their distaltips. Neuron-specific $beta$ III-tubulin was localized to club- andloop-like structures in the distal tips of taxol-treated neurites(Fig. 2E), whereas phosphorylated neurofilaments (Fig. 2F) andtau (Fig. 2G) were evenly distributed throughout the distendedneurites. Additionally, accumulations of phosphorylated neurofilamentsinto ring- or ball-like structures were present in some neuritetips after taxol treatment (Fig. 2F). F-actin was most abundantin neurite tips. Figure 2H illustrates an example of a phalloidin-labeledneuron in which tight ball-like structures of F-actin have formedwithin neurite tips and filopodia have been completely eliminated.F-actin, $beta$ III-tubulin, and tau were distributed throughout thefilopodial-like structures emanating from the swollen tips ofsome taxol-treated neurites; presumably these structures correspondto growth cones, in which normal morphology has been retardedby microtubule stabilization. Taxol washout demonstrated thatthe effects of taxol were long lasting, with stunted neuronalmorphology persistent at 21 DIV. However, the effects of taxolwere partially reversible because increased neurite growth wasobserved in cultures from which taxol was washed out comparedwith cultures grown in the presence of taxol (cell death was highin the latter cultures). Moreover, some of the neurites from whichtaxol was removed regained their growthcones.

Quantitative analysis demonstrated that taxol significantly (p < 0.05) reduced the proportion of neurites tipped by a growthcone from 53.2 ± 7.8% (mean ± SE throughout) in vehicle-treatedcontrols to 18.2 ± 3.7% after taxol treatment (Fig. 3A). Additionally,taxol inhibited neurite elongation between 3 and 5 DIV (Fig. 3B).At 3 DIV, mean neurite length for untreated cultures was 64.0± 3.9 µm. By 5 DIV, vehicle-treated neurites had elongated significantly(p < 0.05) to 90.9 ± 2.1 µm; however, taxol-treated neurites didnot extend significantly (p > 0.05) from pretreatment and weresignificantly shorter (p < 0.05) than vehicle-treated controls,with a mean neurite length of 59.8 ± 1.4 µm.

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Figure 3. Bar graphs showing the effect of exposing developing cortical cultures to vehicle or taxol for 48 hr between 3 and 5 DIV. A, Proportion of neurites tipped by a growth cone after 48 hr vehicle or taxol treatment. B, Mean neurite length before treatment and after vehicle or taxol treatment. *p < 0.05. Error bars are SEMs.

Preliminary investigations were performed to determine the effect of microtubule destabilization on neurite development usingnocodazole. Nocodazole exposure for 48 hr between 3 and 5 DIVresulted in profound morphological alteration compared with controlcultures (Fig. 4A). Neurite growth was clearly stunted, neuronalcell bodies and neurites were often bordered by sections of lamellipodial-likemembrane, which were not observed in vehicle-treated culturesby this stage of development (Fig. 4B), whereas many growth coneslacked obvious lamellipodia (Fig. 4C).

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Figure 4. Effect of nocodazole (100 µg/ml) on neuronal morphology in developing cortical cultures. Vehicle-treated neurons (3-5 DIV, 1.2%DMSO-PBS) had defined cell bodies, axons were slender and tipped by growth cones, and future axonal branch points were indicated by growth cone "remnants" (A). Nocodozole-treated cultures had vastly altered morphology: neurites were stunted and often existed as thick protrusions of the cell, cell bodies were often bordered by a lamellipodial-like fringe (B), and large axonal growth cones often lacked lamellipodia (C). Scale bars, A, 20 µm; B, C, 10 µm.

Response of mature cortical neurons to localized axonal transection

Relatively mature (21 DIV) cultures were characterized by large, multicellular aggregates, from which elaborate networks andbundles of neuronal processes extended, forming interconnectionswith other aggregates. Even by this stage of development, somegrowth cones (with similar morphology and cytoskeletal constitutionto developmental growth cones) were present in more sparsely populatedregions of the cultured monolayers. The nuclei of neurons culturedfor 21 d lacked immunoreactivity for BrdU (applied at either 7or 17 DIV) (Fig. 5A-D) but were immunoreactive for a marker ofNeuN (neuronal-specific postmitotic nuclear protein) (Fig. 5E,F).Additionally aggregated neurons were immunoreactive for othermarkers of mature neurons, such as MAP2 (microtubule-associatedprotein 2) and neurofilament triplet proteins. Electron microscopycombined with immunohistochemistry (for synaptophysin immunoreactivity)confirmed the presence of substantial synaptic contacts throughoutthe cultures (Fig. 5G-I); however, axons in axonal bundles werenot myelinated (Fig. 5J). Collectively, these results demonstratethat cortical neurons cultured for 21 d were postmitotic, wereat least 14 d old, and were relatively mature.

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Figure 5. Confirmation of cortical neuron maturity. BrdU was administered to cultures at 7 (A, B) or 17 (C, D) DIV, for cell proliferation assays, and cultures were grown to 21 DIV. Neuron-specific enolase (NSE) immunopositive neurons (arrows in A and C) lacked BrdU-immunoreactive nuclei (B, D) in double-labeling studies, indicating that they were not proliferating. Double labeling for tau (E) and postmitotic neuronal nuclei (F) at 21 DIV demonstrated that aggregated neurons were not dividing. NSE-labeled neuron (G) in apposition with a profile of synaptophysin-immunoreactive puncta (arrows depict examples in H), demonstrating that neurons had abundant synaptic connections. The presence of synapses was confirmed with electron microscopy (I). J, Electron microscopy demonstrating that axons within axonal bundles were not myelinated (arrows depict examples). Scale bars: A-H, 30 µm; I, 2 µm; J, 1 µm.

Cultured cortical neurons were injured by local neurite transection at 21 DIV. Time-lapse digital imaging demonstrated thatneurons respond to transection with a specific, highly dynamicsequence of changes. Immediately after injury, neuronal processesbegan to retract away from the site of injury (Fig. 6A). Thisretraction response persisted for up to 4-6 hr after injury. Within2-6 hr after injury, an extensive axonal sprouting response wasinitiated (Fig. 6B).

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Figure 6. Time course of the posttransection response. A, Time-lapse imaging of a cut site immediately after injury, demonstrating retraction away from the injury site (note retraction in relation to the asterisk in each image). B, Time-lapse imaging of a cut site imaged from 2 hr after injury, with sprout growth indicated by arrows at each time point. Time course of postinjury axonal sprouting in cultures immunofluorescence labeled for $beta$ III-tubulin (C), tau (D), and phosphorylated neurofilaments (E). Arrows in each image depict examples of sprouts. By 24 hr after injury, sprouting was extensive and several sprouts had crossed the lesion sites. Times shown on each image indicate postinjury interval in hours. Double labeling for $beta$ III-tubulin and F-actin (F, G, respectively), as well as tau and phosphorylated neurofilaments (H, I, respectively), demonstrated that $beta$ III-tubulin and tau were distributed throughout postinjury sprouts and proximal growth cones, whereas F-actin was most abundant in sprout growth cones and phosphorylated neurofilament were restricted to sprout shafts. Scale bars: A, B, 40 µm; C-E, 60 µm; F-I, 30 µm.

Immunofluorescent labeling was used to determine the distribution of cytoskeletal components in postinjury neurite sproutsat 4, 14, and 24 hr after injury. Postinjury analysis demonstratedthat the alterations occurring in response to axonal transectionwere consistent across all cultures at each time point investigated.Double-labeling studies demonstrated that MAP2 labeled processes(dendrites) only extended short distances from the neuronal aggregatesand were rarely transected during neuronal injury. $beta$ III-Tubulin(Fig. 6C) and tau (Fig. 6D) were consistently distributed throughoutpostinjury axonal sprouts at all time points investigated. At4 hr after injury, numerous axonal sprouts had extended into theinjury sites. By 14 hr after injury, sprouts had continued toelongate and were extending toward the opposite side of the injurysited from their origin. At 24 hr after injury, sprouting wasextensive, and many sprouts had crossed the injury site. Phosphorylatedneurofilaments became distributed in postinjury axonal sproutsat 14 and 24 hr after injury, as opposed to either $beta$ III-tubulinor tau, which were distributed throughout sprouts at all postinjurytime points examined (Fig. 6E).

Postinjury axonal sprouts were generally characterized by slender sprout shafts tipped by expanded growth cone-like end structures,although some sprouts tapered distally. Both $beta$ III-tubulin andtau were uniformly distributed throughout sprout shafts and theirsplayed end structures (Fig. 6B,H, respectively). F-actin wasabundant in sprout growth cones (Fig. 6G); however, phosphorylatedneurofilaments were restricted to the sprout shafts (Fig. 6I).A prominent feature marking the injury site border was the accumulationof phosphorylated neurofilaments into ring- and bulb-like structuresas we described previously in in vivo and in vitro models of neuronalinjury (King et al., 1997, 2000, 2001; Dickson et al., 2000).Ring- and bulb-like structures lacked immunoreactivity for $beta$ III-tubulinand tau and were apparent at all time points examined, existingeither in isolation or as a continuum of the severed axonaltips.

Microtubule stabilization and destabilization after axonal transection

The effect of microtubule stabilization on postinjury axonal sprouting was investigated by exposing cultures, grown for 21DIV, to taxol (10 µg/ml culture media) immediately after axonaltransection. Taxol exposure had a substantial effect on postinjuryaxonal sprouting. In vehicle-treated control cultures, the degreeof sprouting increased as time progressed, resulting in extensivesprout growth across the injury sites by 24 hr after injury (Fig.7A,B). However, postinjury axonal sprouting was comparably limitedin taxol-treated cultures (Fig. 7D,E). In addition, taxol exposureresulted in substantial alteration in sprout morphology. Injured,vehicle-treated cultures elaborated sprouts that were generallytipped by expanded growth cone-like structures (Fig. 7C). Conversely,injured taxol-treated cultures elaborated sprouts tipped by bulbousend structures (Fig. 7F). Taxol washout at least partially reversedthe effects of microtubule stabilization on sprout growth inhibition,with increased sprouting observed in cultures in which taxol hadbeen removed compared with those continually exposed to taxolafter injury at 21 DIV. Additionally, some sprouts regained growthcone-like structures at their tips after taxol washout (Fig. 7G).

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Figure 7. Immunofluorescence labeling for tau, demonstrating the effect of taxol exposure on postinjury axonal sprouting. Times shown on each image indicate hours of vehicle or taxol exposure after injury. Vehicle-treated cultures demonstrated an extensive and progressive sprouting response after axonal transection, with several sprouts crossing the lesion site by 24 hr after injury (A, B). Postinjury sprouts elaborated from vehicle-treated cultures were typically slender with expanded growth cone-like distal domains (arrows in C). Limited postinjury axonal sprouting was demonstrated in taxol-treated cultures up to 24 hr after injury (D, E), and bulb-like structures formed at the tips of sprouts (arrows in F). Arrows in A, B, D, and E depict examples of postinjury sprouts. C and F were captured at 4 and 14 hr after injury, respectively. Taxol washout, after 4 hr of postinjury taxol exposure, resulted in increased sprout growth across injury sites, and some sprouts gained growth cone-like structures at their tips (arrows in G). Scale bars: A, B, D, E, 60 µm; C, F, 20 µm; G, 10 µm.

Quantitative analysis demonstrated that taxol substantially influenced sprout outgrowth and elongation. Sprout outgrowth wassignificantly (p < 0.05) inhibited by taxol, with vehicle-treatedcultures elaborating an average of 14.7 ± 1.6 sprouts per 100µm of cut site length compared with taxol-treated cultures, whichhad elaborated on average only 6.6 ± 1.5 sprouts per 100 µm ofcut site length, 4 hr after injury (Fig. 8A). Similarly, statisticalanalysis indicated a significant (p < 0.05) difference betweenmean sprout length in injured, taxol-treated (21.6 ± 0.8 µm) andvehicle-treated (42.6 ± 0.5 µm) cultures at 4 hr after injury,demonstrating that taxol profoundly inhibited sprout elongation(Fig. 8B). Cell death analysis, using the vital dye propridiumiodide, demonstrated the localization of dead and dying cellsalong injury site boarders. Taxol exposure did not affect thelevel of cell death up to 24 hr after axotomy. However increasedcell death was observed when cultures were exposed to taxol for>72 hr.

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Figure 8. Bar graphs demonstrating the effect of exposing cultures to taxol for 4 hr after axonal transection. A, Mean sprout length. B, Mean number of sprouts per 100 µm of injury site length. *p < 0.05. Error bars are SEMs.

Exposure to the microtubule destabilizing agent nocodazole (100 µg/ml) substantially inhibited postinjury axonal sprouting,with little evidence of sprouting observed by 4 hr after injury(Fig. 9).

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Figure 9. Effect of nocodazole on postinjury axonal sprouting. Nocodazole (100 µg/ml) exposure for 4 hr immediately after axonal transection injuries at 21 DIV markedly inhibited sprouting from transacted axonal bundles (arrow in B) compared with vehicle-treated controls (1.2%DMSO-PBS) in which short sprouts, tipped by growth cones, were elaborated into cut sites (arrows in A).

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Using live digital imaging and immunofluorescence-labeling techniques, we compared initial neurite development with the sproutingresponse exhibited by relatively mature neurons after localizedaxonal transection in vitro. After injury, a substantial regenerativeattempt was indicated by the elaboration of sprout-like protuberancesinto injury sites. The overall morphology, motility, and cytoskeletalcomposition of axonal sprouts were highly homologous with developingneurites. Exposure to the microtubule stabilizing agent taxoland microtubule destabilizing agent nocodazole inhibited neuritedevelopment and postinjury axonal sprouting, demonstrating thatsimilar microtubule dynamics may underlie bothprocesses.

In vitro neuronal development

Both $beta$ III-tubulin and tau were distributed throughout neurite shafts and the central domain of growth cones, with less abundantlabeling exhibited in peripheral growth cone regions. F-actinwas punctately distributed along some neurites and abundant indevelopmental growth cones. Conversely, phosphorylated neurofilamentswere only localized in a subset of developing neurites (presumablythose destined to become axons), and immunoreactivity was absentin growth cones. The distributions of these cytoskeletal componentsmay reflect their relative importance in axonal growth. For instance,microtubules have been demonstrated to be essential in axonaloutgrowth (Okabe and Hirokawa, 1990; Walker et al., 2001), whereasaxonal growth can proceed in the absence of neurofilaments (Jianget al., 1996; Zhu et al., 1997; Levavasseur et al., 1999), albeitat a slower rate (Walker et al., 2001).

Microtubule stabilization and destabilization inhibits neurite growth

Early-stage cultures (3 DIV) were exposed to taxol to investigate the effects of microtubule stabilization on neurite development.Taxol, widely used in the treatment of various cancers, promotesthe polymerization of tubulin monomers and the formation of stable,nonfunctional microtubules (Gotaskie and Andreassi, 1994). Themicrotubule network is a particularly motile component of theaxonal cytoskeleton within developing neurites (for review, seeBrandt, 1998; Kalil et al., 2000). Exposure of cortical neuronsto taxol in the current study resulted in neurite distension,cessation of neurite elongation, and a significant reduction ingrowth cone formation. Similar effects of taxol have been observedin cultured chick sensory neurons (Letourneau and Ressler, 1984;George et al., 1988). We also demonstrated that, after taxol treatment,loops of tubulin immunoreactivity were localized within the deformedend structures that replaced developmental growth cones at neuritetips, with ring- and bulb-like accumulations of phosphorylatedneurofilaments often observed within the central core of the microtubuleloops. The segregation of microtubules and neurofilaments is unusualbecause these cytoskeletal components are normally intermixed(Letourneau and Ressler, 1984). The dilated bulbous structuresthat formed at neurite tips after taxol exposure frequently lackedfilopodia and lamellipodia and thus probably lacked the abilityto effectively transduce guidance cues, which is a factor likelyto account for the curling and looping of neurites around theiraggregates oforigin.

Abnormalities occurring after taxol exposure are likely to reflect the bundling and proliferation of microtubules within neurites,as well as altered microtubule spacing and interaction with microtubule-associatedproteins (Black, 1987). Taxol-promoted microtubule proliferationmay exhaust the local pool of tubulin monomers available for usein neurite elongation and presumably causes steric hindrance ofaxonal transport, which may prevent the delivery of constituentsnecessary for neurite extension. Indeed, Theiss and Meller (2000)demonstrated that taxol inhibits anterograde axonal transport.Furthermore, we demonstrated that, although some taxol-treatedneurites regained growth cones and neurite growth increased aftertaxol washout, many neurites remained distended, indicating thattaxol-induced microtubule stabilization is relativelypermanent.

Nocodazole binds to tubulin and causes microtubule depolymerization (Dinter and Berger, 1998). Exposure of developing corticalcultures to nocodozole inhibited neurite growth and caused substantialmorphological reorganization, which differed from the morphologicalaberrations induced by taxol exposure. Nocodazole-exposed neuritesdeveloped growth cones that lacked lamellipodia, as reported previouslyby Gallo (1998), and some neurons were bordered by lamellipodial-likefringes, phenomena that were not observed in taxol-treatedcultures.

Axons respond to transection by retraction and sprouting

Using an in vitro model of axonal trauma capable of eliciting a substantial axonal sprouting response, we demonstrated thattransection of the axonal bundles and networks interconnectingneuronal aggregates induced a characteristic and highly dynamicresponse. Time-lapse imaging verified that axons retract awayfrom injury sites, toward their aggregate of origin, immediatelyafter transection. Postinjury axonal retraction has been reportedpreviously after lamprey spinal cord transection (McHale et al.,1995). The retraction response was accompanied by other reactivealterations, including swelling in the distal region of severedaxons and the accumulation of neurofilaments into ring- and bulb-likestructures, as reported previously (Meller et al., 1993: Kinget al., 1997, 2000, 2001; Dickson et al., 2000).

Extensive neurite sprouting was initiated by 4-6 hr after injury. Time course immunofluorescence-labeling studies confirmedthat, by 4 hr after injury, several fine $beta$ III-tubulin and tauimmunoreactive sprouts emanated into injury sites. By 24 hr afterinjury, several sprouts had traversed the lesion sites. Severalof the postinjury sprouts exhibited small growth cone-like structuresat their tips, indicating the sprouting response was possiblya guided mechanism and not simple elongation along randompathways.

Analysis of the morphology, cytoskeletal composition, and dynamic properties of postinjury sprouts indicated some notablesimilarities with developing neurites. Developing neurites andsprouting axons were motile, slender structures. Additionally,a majority of sprouts were tipped by expanded growth cone-likestructures, which exhibited immunoreactivity for $beta$ III-tubulin,tau, and F-actin, although they were generally smaller than developmentalgrowth cones. Phosphorylated neurofilaments were restricted tosprout shafts and appeared at later time points than observedfor the microtubule markers. In a similar manner, it has beensuggested that the sequence of cytoskeletal gene expression occurringduring neuronal regenerative attempts recapitulates the developmentalpattern (Hoffman and Cleveland, 1988; Lee and Cleveland, 1996).The delay in the appearance of phosphorylated neurofilaments insprout shafts may indicate they are not required for initial sproutoutgrowth. Similarly, neurite outgrowth proceeds in the absenceof neurofilaments (Zhu et al., 1997; Levavasseur et al., 1999).Neurofilaments, however, may play an important role in sproutelongation. In this regard, reduced regenerative ability of theperipheral nervous system has been reported in neurofilament-deficientanimals (Jiang et al., 1996; Zhu et al., 1997). Furthermore, Melleret al. (1993) speculates that neurofilaments may provide the propulsiveforce underlying sproutgrowth.

Microtubule stabilization and destabilization inhibits postinjury sprouting

Administration of taxol immediately after axonal transection at 21 DIV resulted in distinct morphological changes similarto those observed in developing taxol-treated neurites. Taxolexposure substantially inhibited postinjury axonal sprouting,causing a significant reduction in both sprout length and numberat 4 hr after injury. Interestingly, postinjury sprouting wasnot completely inhibited by taxol but rather reduced by approximatelyone-half. This indicates that either the concentration of, orexposure time to, taxol was insufficient to stabilize all microtubules.Conversely, mechanisms other than microtubule dynamics may beresponsible for sprout formation and growth. For instance, theactin and microtubule cytoskeletons may act in a synergistic andcoordinated manner to dictate the cytoskeletal response underlyingsprout growth, as is the case during neurite development (Letourneauet al., 1987), with disruption of one component affecting thedynamics of the other (Dent and Kalil, 2001). Unlike the limitedsprouting observed in taxol-treated cultures, postinjury nococazoleexposure completely abolished axonalsprouting.

Our results indicate some of the notable similarities between developing and sprouting axons and verify that the dynamic propertiesof microtubules are fundamental to the processes of sprout outgrowthand elongation. The effects of taxol on postinjury axonal sproutingwere partially reversible, with increased sprouting observed aftertaxol washout in addition to the formation of growth-cone likestructures at the tips of somesprouts.

Taxol has been demonstrated to reduce $beta$ -amyloid toxicity in Alzheimer's disease (Michaelis et al., 1998), as well as to inhibitdetrimental alterations in intracellular calcium levels that mayresult in neuronal death (Burke et al., 1994), aberrant changesin tau antigenicity (Mattson, 1992), and excitotoxicity (Furukawaand Mattson, 1995). At low doses, taxol has also been demonstratedto promote recovery of function after spinal cord injury (Perez-Espejoet al., 1996). However, Figueroa-Masot et al. (2001) have reportedthat taxol potently induces apoptosis in cultured cortical neuronsin a dose-dependent and exposure-time-dependent manner. Accordingly,although we recorded relatively little cell death after taxolexposure for 24 hr, cell death was substantially increased after72 hr of taxol treatment. Using an in vivo model of brain trauma,Adlard et al. (2000) demonstrated that taxol inhibits microtubuleloss and neurofilamentous accumulation. However, taxol exposuremay also delay the resolution of reactive axonal alterations afterinjury, which may not be helpful for the adaptive response totrauma (Adlard et al., 2000).

Conclusion

The inability of axons to successfully regenerate after brain trauma has been attributed to several factors within the CNSmilieu (Berry et al., 1994; Fawcett, 1997; Bandtlow and Schwab,2000; Goldberg and Barres, 2000; Qiu et al., 2000), as well asan intrinsic incapacity for regeneration by the damaged neurons(Fawcett, 1997). The current study shows that the axons of relativelymature neurons can respond rapidly to injury by adaptive sprouting,and the cytoskeletal dynamics that underlie this attempt at regenerationare similar to the mechanisms underlying initial neurite development.The microtubule disrupting agents taxol and nocadazole effectivelyinhibited both initial neurite development and the regenerativesprouting response after injury, indicating the importance ofcytoskeletal, particularly microtubule dynamics, in neurite growthand the neuronal response to injury. Although taxol and nocodazolehave opposing effects on microtubule structure (polymerizationand depolymerization, respectively), both agents essentially actto suppress microtubule dynamics, which, as our studies have demonstrated,are crucial to normal neurite growth and postinjury axonal sprouting.Cytoskeletal disrupting agents, such as taxol, could potentiallybe useful for preventing the maladaptive regenerative sproutingresponse that may underlie posttrauma epilepsy (Larner, 1995;McKinney et al., 1997) and Alzheimer's disease (Masliah et al.,1991, 1992; Vickers et al., 2000; Arendt, 2001).

  FOOTNOTES

Received July 25, 2002; revised Feb. 24, 2003; accepted Feb. 24, 2003.

This research was supported by the National Health and Medical Research Council, the Royal Hobart Hospital Research Foundation,and the Tasmanian Masonic Centenary Medical Research Foundation.We thank Sandrine Chopin, Graeme McCormack, Marian Quilty, andIrene Jacobs for their technical assistance in completing thiswork.

Correspondence should be addressed to Prof. James C. Vickers, Discipline of Pathology, Faculty of Health Sciences, Universityof Tasmania, 43 Collins Street, Hobart, Tasmania, 7000, Australia,E-mail: james.vickers{at}utas.edu.au.

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