ABSTRACT
Ca(2+) and synaptotagmin (a Ca(2+)-binding protein that regulates axolemmal fusion of synaptic vesicles) play essential roles in the repair of axolemmal damage in invertebrate giant axons. We now report that neurites of a rat pheochromocytoma (PC12) cell line transected and maintained in a serum medium form a dye barrier (exclude an external hydrophilic fluorescent dye) and survive for 24-hr posttransection (based on morphology and retention of another hydrophilic dye internally loaded at 6-hr posttransection). Some (25%) transected neurites that form a dye barrier regrow. Most (83%) neurites transected in a saline solution containing divalent cations (PBS(++)) also exclude entry of an externally placed hydrophilic fluorescent dye at 15-min posttransection. In contrast, only 14 or 17% of neurites maintained in a divalent cation-free solution (PBS(=)) or in PBS(=) + Mg(2+), respectively, form a dye barrier. Neurites that do not form a dye barrier do not survive for 24 hr. When PC12 neurites are loaded with an antibody to squid synaptotagmin, most (81%) antibody-loaded neurites do not form a dye barrier, whereas most (>/=81%) neurites loaded with heat-inactivated antibody or preimmune IgG do form a barrier. These data show that: 1) transected neurites of PC12 cells have mechanism(s) for plasmalemmal repair (dye barrier formation and survival); 2) Ca(2+) is necessary for dye barrier formation, which occurs minutes after transection and is necessary for survival and regrowth; and 3) synaptotagmin is an essential mediator of barrier formation. The similarity in the requirements for plasmalemmal repair in this mammalian cell preparation with those reported previously for invertebrate axons suggests that mechanisms necessary for plasmalemmal repair have been conserved phylogenetically.
Subject(s)
Calcium-Binding Proteins , Calcium/metabolism , Cell Membrane/metabolism , Cell Survival/physiology , Membrane Glycoproteins/metabolism , Nerve Regeneration/physiology , Nerve Tissue Proteins/metabolism , Neurites/metabolism , PC12 Cells/metabolism , Animals , Axons/drug effects , Axons/metabolism , Axons/ultrastructure , Axotomy/adverse effects , Cell Membrane/drug effects , Cell Membrane/ultrastructure , Cell Survival/drug effects , Dextrans/pharmacology , Fluoresceins/pharmacology , Indicators and Reagents/pharmacology , Nerve Regeneration/drug effects , Neurites/drug effects , Neurites/ultrastructure , PC12 Cells/cytology , PC12 Cells/drug effects , Rats , SynaptotagminsABSTRACT
After axonal severance, a barrier forms at the cut ends to rapidly restrict bulk inflow and outflow. In severed crayfish axons we used the exclusion of hydrophilic, fluorescent dye molecules of different sizes (0.6-70 kDa) and the temporal decline of ionic injury current to levels in intact axons to determine the time course (0-120 min posttransection) of barrier formation and the posttransection time at which an axolemmal ionic seal had formed, as confirmed by the recovery of resting and action potentials. Confocal images showed that the posttransection time of dye exclusion was inversely related to dye molecular size. A barrier to the smallest dye molecule formed more rapidly (<60 min) than did the barrier to ionic entry (>60 min). These data show that axolemmal sealing lacks abrupt, large changes in barrier permeability that would be expected if a seal were to form suddenly, as previously assumed. Rather, these data suggest that a barrier forms gradually and slowly by restricting the movement of molecules of progressively smaller size amid injury-induced vesicles that accumulate, interact, and form junctional complexes with each other and the axolemma at the cut end. This process eventually culminates in an axolemmal ionic seal, and is not complete until ionic injury current returns to baseline levels measured in an undamaged axon.
Subject(s)
Axons/physiology , Animals , Astacoidea/physiology , Biophysical Phenomena , Biophysics , Fluorescent Dyes/pharmacokinetics , In Vitro Techniques , Ion Channels/metabolism , Microscopy, Confocal , Nerve Regeneration/physiology , PermeabilityABSTRACT
A damaged cell membrane is repaired by a seal that restricts entry or exit of molecules and ions to that of the level passing through an undamaged membrane. Seal formation requires elevation of intracellular Ca(2+) and, very likely, protein-mediated fusion of membranes. Ca(2+) also regulates the interaction between synaptotagmin (Syt) and syntaxin (Syx), which is thought to mediate fusion of synaptic vesicles with the axolemma, allowing transmitter release at synapses. To determine whether synaptic proteins have a role in sealing axolemmal damage, we injected squid and crayfish giant axons with an antibody that inhibits squid Syt from binding Ca(2+), or with another antibody that inhibits the Ca(2+)-dependent interaction of squid Syx with the Ca(2+)-binding domain of Syt. Axons injected with antibody to Syt did not seal, as assessed at axonal cut ends by the exclusion of extracellular hydrophilic fluorescent dye using confocal microscopy, and by the decay of extracellular injury current compared to levels measured in uninjured axons using a vibrating probe technique. In contrast, axons injected with either denatured antibody to Syt or preimmune IgG did seal. Similarly, axons injected with antibody to Syx did not seal, but did seal when injected with either denatured antibody to Syx or preimmune IgG. These results indicate an essential involvement of Syt and Syx in the repair (sealing) of severed axons. We suggest that vesicles, which accumulate and interact at the injury site, re-establish axolemmal continuity by Ca(2+)-induced fusions mediated by proteins such as those involved in neurotransmitter release.
Subject(s)
Axons/metabolism , Calcium-Binding Proteins , Membrane Fusion/physiology , Membrane Glycoproteins/metabolism , Membrane Proteins/metabolism , Nerve Tissue Proteins/metabolism , Synaptic Vesicles/metabolism , Animals , Antibodies/pharmacology , Antibody Specificity , Astacoidea , Axons/ultrastructure , Axotomy , Cell Membrane/metabolism , Decapodiformes , Fluorescent Dyes , Immunoblotting , In Vitro Techniques , Membrane Fusion/drug effects , Membrane Glycoproteins/antagonists & inhibitors , Membrane Proteins/antagonists & inhibitors , Nerve Tissue Proteins/antagonists & inhibitors , Neurons/drug effects , Neurons/physiology , Neurons/ultrastructure , Qa-SNARE Proteins , SynaptotagminsABSTRACT
We describe structural changes at the cut ends of invertebrate myelinated earthworm giant axons beginning with the formation of a dye barrier (15 minutes posttransection or postcalcium addition) and ending with the formation of a neuritic outgrowth (2-10 days posttransection). The morphology of the cut end, and the location and morphological configuration of the dye barrier, were assessed by time-lapse confocal, fluorescence microscopy and by electron microscopy. During the interval from 15 to 35 minutes postcalcium addition, the dye barrier continuously migrated away from a cut axonal end; the dye barrier then remained stable for up to 5 hours. The size, packing density, and arrangement of membranous structures were correlated with changes in the dye barrier from 15 to 35 minutes postcalcium addition. During this interval, uptake of an externally placed hydrophilic dye by these membranous structures was also variable. After 35 minutes postcalcium addition, the membranous structures remained stable until they completely disappeared between 1 and 2 days posttransection. The disappearance of membranous structures always preceded neuritic outgrowth, which only arose from cut axonal ends. These results demonstrate that the dye barrier and associated membranous structures, which form after transection of earthworm giant axons, are very dynamic in the short term (35 minutes) with respect to their location and morphological configuration and suggest that axolemmal repair must be completed before neuritic outgrowth can occur.
Subject(s)
Axons/physiology , Giant Cells/physiology , Myelin Sheath/physiology , Neurites/physiology , Oligochaeta/ultrastructure , Animals , Axons/ultrastructure , Axotomy , Cell Membrane/physiology , Cell Membrane/ultrastructure , Coloring Agents , Giant Cells/ultrastructure , Myelin Sheath/ultrastructure , Neurites/ultrastructure , Time FactorsABSTRACT
After severance, axons can restore structural barriers that are necessary for recovery of their electrical function. In earthworm myelinated axons, such a barrier to dye entry is mediated by many vesicles and myelin-derived membranous structures. From time-lapse confocal fluorescence and DIC images, we now report that Ca2+ entry and not axonal injury per se initiates the processes that form a dye barrier, as well as the subsequent structural changes in this barrier and associated membranous structures. The time required to restore a dye barrier after transection also depends only on the time of Ca2+ entry.
Subject(s)
Axons/metabolism , Calcium/metabolism , Calcium/physiology , Coloring Agents/pharmacokinetics , Oligochaeta/metabolism , Animals , Axons/ultrastructure , Dextrans , Fluoresceins , Indicators and Reagents , Microscopy, Confocal , Microscopy, FluorescenceABSTRACT
After axonal injury, dye exclusion is often used as a measure of the re-establishment of a structural barrier. We now report that this use of dye exclusion is equivocal in two situations. (1) When a negatively-charged hydrophilic fluorescent dye (HFD) was placed in the physiological saline (PS) surrounding a crayfish medial giant axon (CMGA) before transection, this dye did not readily diffuse into the cut ends after transection whereas uncharged or neutralized dyes did do so. (2) When axoplasm flowed out of the cut ends of a transected squid giant axon (SGA), this outflow markedly slowed hydrophilic fluorescent dyes from diffusing into the cut ends. These anomalies suggest that dye exclusion by an injured axon does not always indicate that a structural barrier has formed. Therefore, dye assessments of axonal repair require control experiments that rule out anomalous exclusion due to dye interactions (biochemical and fluid dynamics) with components (axoplasm, axolemma, glial sheath, etc.) of the particular axon under study.
Subject(s)
Axonal Transport , Axons/physiology , Fluorescent Dyes/pharmacokinetics , Animals , Anions/pharmacokinetics , Astacoidea , Axonal Transport/drug effects , Axons/drug effects , Axotomy , Calcium/pharmacology , Decapodiformes , Nerve Regeneration/physiology , Time FactorsABSTRACT
Vesicles and/or other membranous structures that form after axolemmal damage have recently been shown to repair (seal) the axolemma of various nerve axons. To determine the origin of such membranous structures, (1) we internally dialyzed isolated intact squid giant axons (GAs) and showed that elevation of intracellular Ca2+ >100 microM produced membranous structures similar to those in axons transected in Ca2+-containing physiological saline; (2) we exposed GA axoplasm to Ca2+-containing salines and observed that membranous structures did not form after removing the axolemma and glial sheath but did form in severed GAs after >99% of their axoplasm was removed by internal perfusion; (3) we examined transected GAs and crayfish medial giant axons (MGAs) with time-lapse confocal fluorescence microscopy and showed that many injury-induced vesicles formed by endocytosis of the axolemma; (4) we examined the cut ends of GAs and MGAs with electron microscopy and showed that most membranous structures were single-walled at short (5-15 min) post-transection times, whereas more were double- and multi-walled and of probable glial origin after longer (30-150 min) post-transection times; and (5) we examined differential interference contrast and confocal images and showed that large and small lesions evoked similar injury responses in which barriers to dye diffusion formed amid an accumulation of vesicles and other membranous structures. These and other data suggest that Ca2+ inflow at large or small axolemmal lesions induces various membranous structures (including endocytotic vesicles) of glial or axonal origin to form, accumulate, and interact with each other, preformed vesicles, and/or the axolemma to repair the axolemmal damage.
Subject(s)
Axons/physiology , Calcium/pharmacology , Endocytosis/physiology , Synaptic Vesicles/physiology , Animals , Astacoidea , Axons/ultrastructure , Axotomy , Cell Communication/physiology , Cell Membrane/physiology , Decapodiformes , Endocytosis/drug effects , Intracellular Membranes/drug effects , Intracellular Membranes/physiology , Membrane Fusion/physiology , Microscopy, Electron , Microscopy, Fluorescence , Microscopy, Video , Neuroglia/physiology , Synaptic Vesicles/drug effects , Synaptic Vesicles/ultrastructureABSTRACT
Transected axons are often assumed to seal by collapse and fusion of the axolemmal leaflets at their cut ends. Using photomicroscopy and electronmicroscopy of fixed tissues and differential interference contrast and confocal fluorescence imaging of living tissues, we examined the proximal and distal cut ends of the pseudomyelinated medial giant axon of the earthworm, Lumbricus terrestris, at 5-60 min post-transection in physiological salines and Ca2+-free salines. In physiological salines, the axolemmal leaflets at the cut ends do not completely collapse, much less fuse, for at least 60 min post-transection. In fact, the axolemma is disrupted for 20-100 microm from the cut end at 5-60 min post-transection. However, a barrier to dye diffusion is observed when hydrophilic or styryl dyes are placed in the bath at 15-30 min post-transection. At 30-60 min post-transection, this barrier to dye diffusion near the cut end is formed amid an accumulation of some single-layered and many multilayered vesicles and other membranous material, much of which resembles delaminated pseudomyelin of the glial sheath. In Ca2+-free salines, this single and multilayered membranous material does not accumulate, and a dye diffusion barrier is not observed. These and other data are consistent with the hypothesis that plasmalemmal damage in eukaryotic cells is repaired by Ca2+-induced vesicles arising from invaginations or evaginations of membranes of various origin which form junctional contacts or fuse with each other and/or the plasmalemma.
Subject(s)
Axons/physiology , Myelin Sheath/physiology , Animals , Coloring Agents , Myelin Sheath/ultrastructure , Neuroglia/ultrastructure , Oligochaeta , Solubility , Styrene , Styrenes , Water/chemistryABSTRACT
A barrier (seal) must form at the cut ends of a severed axon if a neuron is to survive and eventually regenerate. Following severance of crayfish medial giant axons in physiological saline, vesicles accumulate at the cut end and form a barrier (seal) to ion and dye diffusion. In contrast, squid giant axons do not seal, even though injury-induced vesicles form after axonal transection and accumulate at cut axonal ends. Neither axon seals in Ca2+-free salines. The addition of calpain to the bath saline induces the sealing of squid giant axons, whereas the addition of inhibitors of calpain activity inhibits the sealing of crayfish medial giant axons. These complementary effects involving calpain in two different axons suggest that endogenous calpain activity promotes plasmalemmal repair by vesicles or other membranes which form a plug or a continuous membrane barrier to seal cut axonal ends.
Subject(s)
Axons/physiology , Calpain/pharmacology , Cell Membrane/physiology , Membrane Fusion/drug effects , Animals , Astacoidea , Axons/drug effects , Cell Membrane/drug effects , Cysteine Proteinase Inhibitors/pharmacology , Decapodiformes , Electric Conductivity , Membrane Potentials , Species SpecificityABSTRACT
Crayfish medial giant axons (MGAs) transected in physiological saline form vesicles which interact with each other, pre-existing vesicles, and/or with the plasmalemma to form an electrical and a physical barrier that seals a cut axonal end within 60 min. The formation of this barrier (seal) was assessed by measuring the decay of injury current at the cut end; its location at the cut end was determined by the exclusion of fluorescent hydrophilic dye at the cut end. When a membrane-incorporating styryl dye was placed in the bath prior to axonal transection and a hydrophilic dye was placed in the bath just after axonal transection, many vesicles near the barrier at the cut axonal end had their limiting membrane labeled with the styryl dye and their contents labeled with the hydrophilic dye, indicating that these vesicles originated from the axolemma by endocytosis. This barrier does not form in Ca2+-free salines. Similar collections of vesicles have been observed at regions of plasmalemmal damage in many cell types. From these and other data, we propose that plasmalemmal lesions in most eukaryotic cells (including axons) are repaired by vesicles, at least some of which arise by endocytosis induced by Ca2+ inflow resulting from the plasmalemmal damage. We describe several models by which vesicles could interact with each other and/or with intact or damaged regions of the plasmalemma to repair small (1-30 microm) plasmalemmal holes or a complete transection of the plasmalemma.
Subject(s)
Axons/physiology , Cell Membrane/physiology , Animals , Astacoidea , Axons/ultrastructure , Calcium/metabolism , Cell Membrane/ultrastructure , Coloring Agents/metabolism , Endocytosis , Microscopy, Confocal , Microscopy, Interference , Models, BiologicalABSTRACT
A steady, spontaneous current oscillation (1 nA p-p) occurs in voltage-clamped, isolated ampullary organs (canal, ampulla, and nerve) from skates (Raja). Spectral analysis showed that energy in the oscillation was confined to a narrow band of frequencies (3 Hz) about a fundamental frequency (32 Hz at 20 degrees C) and in harmonics. The frequency of the oscillation was temperature dependent (increasing from 21 to 33 Hz for increases in temperature from 13 degrees C to 21 degrees C). The addition of 0.5 microM tetrodotoxin to the basal side of the ampullary epithelium eliminated afferent nerve activity but had no effect on the epithelial oscillation, indicating that the oscillation is not generated or induced by afferent nerve activity. Nitrendipine (2 microM) added to the solution bathing the basal side of the ampullary epithelium abolished the oscillation rapidly (within minutes), but a steady-state negative conductance (i.e., real part of the complex admittance < 0) generated by the preparation remained for 36 min. Conversely, nitrendipine (50 microM) added to the perfusate (artificial sea water) of the apical side eliminated the negative conductance rapidly (18.5 min) but had no effect on the spontaneous oscillation for more than 1 h. The effect and the elapsed time for an effect of nitrendipine after separate applications to the basal and apical membrane surfaces of ampullary epithelium suggest that 1) the negative conductance and the oscillation are generated independently in apical and basal membranes, respectively, and 2) both processes involve L-type Ca channels. Furthermore, the addition of tetraethylammonium (2 mM) to the basal side eliminated both the oscillation and the postsynaptic response to voltage clamps (< or = 100 microV) of the ampullary epithelium in the operational voltage range of the afferent nerve. This result suggests that the basal membrane oscillation functions in neurotransmitter release from presynaptic (basal) membranes.
Subject(s)
Sensory Receptor Cells/physiology , Afferent Pathways/physiology , Animals , Cell Membrane/drug effects , Cell Membrane/physiology , Electric Conductivity , Epithelium/drug effects , Epithelium/physiology , In Vitro Techniques , Membrane Potentials , Nitrendipine/pharmacology , Oscillometry , Patch-Clamp Techniques , Sensory Receptor Cells/drug effects , Skates, Fish , Tetrodotoxin/pharmacologyABSTRACT
Two ampullary epithelial properties necessary for electroreception were used to identify the types of ion channels and transporters found in apical and basal membranes of ampullary receptor cells of skates and to assess their individual role under voltage-clamp conditions. The two essential properties are (1) a steady-state negative conductance generated in apical membranes and (2) a small, spontaneous current oscillation originating in basal membranes (Lu and Fishman, 1995). The effects of pharmacological agents and ion substitutions on these properties were evaluated from transorgan or transepithelial complex admittance determinations in the frequency range 0.125 to 50 Hz measured in individual, isolated ampullary organs. In apical membranes, L-type Ca channels were found to be responsible for generation of the steady-state negative conductance. In basal membranes, K and Ca-dependent Cl (Cl(Ca)) channels were demonstrated to contribute to a net positive membrane conductance. L-type Ca channels were also evident in basal membranes and are thought to function in synaptic transmission from the electroreceptive epithelium to the primary afferent nerve. In addition to ion channels in basal membranes, two transporters (Na+/K+ pump and Na(+)-Ca+ exchanger) were apparent. Rapid (minutes) cessation of the current oscillation after blockage of any of the basal ion channels (Ca, Cl(Ca), K) suggests critical involvement of each of these channel types in the generation of the oscillation. Suppression of either Na+/K+ transport or Na(+)-Ca2+ exchange also eliminated the oscillation but at a slower rate, indicating an indirect effect.
Subject(s)
Carrier Proteins/physiology , Ion Channels/physiology , Mechanoreceptors/physiology , Animals , Calcium Channel Blockers/pharmacology , Calcium Channels/physiology , Cell Membrane/drug effects , Cell Membrane/physiology , Charybdotoxin/pharmacology , Electric Conductivity , Epithelium/drug effects , Epithelium/physiology , In Vitro Techniques , Ion Channels/drug effects , Kinetics , Patch-Clamp Techniques , Potassium Channels/drug effects , Potassium Channels/physiology , Skates, Fish , Sodium Channels/analysis , Sodium-Potassium-Exchanging ATPase/analysis , Time FactorsSubject(s)
Axons , Fluoresceins , Fluorescent Dyes , Neuroglia/cytology , Animals , Astacoidea , Axons/metabolism , Decapodiformes , Nerve Fibers/metabolism , Neuroglia/metabolismABSTRACT
For many years, membrane potential (Vm) and input resistance have been used to characterize the electrophysiological nature of a seal (barrier) that forms at the cut end of a transected axon or other extended cytoplasmic structure. Data from a mathematical and an analog model of a transected axon and other theoretical considerations show that steady-state values of Vm and input resistance measured from any cable-like structure provide a very equivocal assessment of the electrical barrier (seal) at the cut end. Extracellular assessments of injury currents almost certainly provide a better electrophysiological measure of the status of plasma membrane sealing because measurements of these currents do not depend on the cable properties of extended cytoplasmic processes after transection.
Subject(s)
Axons/physiology , Animals , Axons/ultrastructure , Biophysical Phenomena , Biophysics , Electric Impedance , Membrane Potentials , Models, NeurologicalABSTRACT
Transected axons are often assumed to seal at their cut ends by the formation of continuous membrane barriers that allow for the restoration of function in the axonal stumps. We have used several electrophysiological measures (membrane potential, input resistance, injury current density) and several morphological measures (phase-contrast, video-enhanced differential interference contrast, light, and electron microscopies) of living and fixed material to assess the extent and mechanism of sealing within hours after transecting giant axons of squid (Loligo pealei and Sepioteuthis lessoniana) and earthworms (Lumbricus terrestris). Our electrophysiological data suggest that the proximal and distal ends of transected squid giant axons do not completely seal within 2.5 hr in physiological saline. In contrast, the same set of measures suggest that proximal and distal ends of transected earthworm giant axons seal within 1 hr in physiological saline. Our morphological data show that the cut ends of both squid and earthworm axons constrict, but that a 20-70-microns-diameter opening always remains at the cut end that is filled with vesicles. Axonal transection induces the formation of vesicles that are observed in the axoplasm within minutes in standard salines and that rapidly migrate to the cut ends. These injury-induced vesicles are loosely packed near the cut ends of squid giant axons, which do not functionally seal within 2.5 hr of transection. In contrast, vesicles formed a tightly packed plug at the cut ends of earthworm medial giant axons, which do functionally seal within 1 hr of transection in physiological saline. Since we detect no single continuous membrane that spans the cut end, sealing does not appear to occur by the fusion of constricted axolemmal membrane or the formation of a membranous partition at the cut end. Rather, our data are consistent with the hypothesis that a tightly packed vesicular plug is responsible for sealing of earthworm giant axons.
Subject(s)
Axons/physiology , Denervation , Wound Healing/physiology , Animals , Axons/ultrastructure , Decapodiformes , Fixatives , OligochaetaABSTRACT
The exquisite sensitivity of elasmobranch fishes to electric fields is thought to reside in electroreceptive organs called ampullae of Lorenzini. We measured the stimulus-response behavior of ampullary organs excised from skates. Under open-circuit conditions, the ampullary organ showed three distinct response states: spontaneous repetitive spikes, evoked spikes, and small, damped oscillatory responses. Under short-circuit conditions, the amplitude range for a linear current response to a sinusoidal (0.5 Hz) voltage clamp of an organ (assessed by spectral analysis of the harmonics generated) was 7-200 microV rms. Changes in the spike firing rate of the afferent nerve innervating the organ were evident for voltage clamps of the ampullary epithelium of 3 microV and the spike rate saturated for clamp steps exceeding 100 microV. Thus, the linear response range of the ampullary epithelium exceeded the range in spike firing rate of the afferent nerve. The steady-state transorgan electrical properties under voltage clamp conditions were obtained by analysis of complex admittance determinations in the frequency range 0.05-20 Hz for perturbations (< 100 microV rms) in the linear range. Admittance functions were distinctly related to the preparation states observed under open-circuit conditions. A negative real part in the organ admittance (i.e., a steady-state negative conductance generated by the preparation) was a common characteristic of the two (open-circuit) excitable states. The negative conductance was also confirmed by the direction of current flow through the ampullary epithelium in response to step voltage clamps. We conclude that the steady state-negative conductance is an essential property of the ampullary epithelium,and we suggest that the interplay of negative and positive conductances generated by ion channels in apical and basal membranes of receptor cells results in signal amplification that may contribute significantly to the electric field sensitivity of ampullary organs.
Subject(s)
Cell Membrane/physiology , Electric Organ/physiology , Ion Channels/physiology , Mechanoreceptors/physiology , Afferent Pathways/physiology , Animals , Electric Conductivity , Electric Stimulation , Electrophysiology/instrumentation , Electrophysiology/methods , Epithelium/physiology , In Vitro Techniques , Membrane Potentials , Oscillometry , Skates, FishABSTRACT
The shortening of severed squid giant axons (GAs) in vitro was analyzed using video light microscopy. Axonal shortening occurred in two temporal phases along the length of the GA: a rapid initial phase during the first 3.5 min after severance followed by a slower phase lasting at least 30 min. The rate of shortening was greatest near the cut end and declined with distance from the cut end for at least 30 min after transection. Axonal shortening may help pack injury-induced vesicles [3] which facilitate sealing of the cut end [7] and/or retard the entry of various substances.
