Rapid Induction of Functional and Morphological Continuity between Severed Ends of Mammalian or Earthworm Myelinated Axons

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The Journal of Neuroscience, April 1, 1999, 19(7):2442-2454

Rapid Induction of Functional and Morphological Continuity between Severed Ends of Mammalian or Earthworm Myelinated Axons
April B. Lore¹, Jeffery A. Hubbell⁴, David S. Bobb Jr¹, Martis L. Ballinger¹, Keisha L. Loftin¹, Jeffory W. Smith¹, Mark E. Smyers¹, Habacuc D. Garcia¹, and George D. Bittner¹^,²^,³^,⁵
¹ Department of Zoology, ² Institute for Neuroscience, and ³ College of Pharmacy, University of Texas at Austin, Austin, Texas 78712, ⁴ Institute for Biomedical Engineering and Department of Materials, Swiss Federal Institute of Technology and University of Zurich, CH-8044 Zurich, Switzerland, and ⁵ Department of Physiology and Biophysics, University of Texas Medical Branch, Galveston, TX 77555-0641

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
REFERENCES

The inability to rapidly restore the loss of function that results from severance (cutting or crushing) of PNS and CNS axonsis a severe clinical problem. As a novel strategy to help alleviatethis problem, we have developed in vitro procedures using Ca²⁺-free solutions of polyethylene glycol (PEG solutions), whichwithin minutes induce functional and morphological continuity(PEG-induced fusion) between the cut or crushed ends of myelinatedsciatic or spinal axons in rats. Using a PEG-based hydrogel thatbinds to connective tissue to provide mechanical strength at thelesion site and is nontoxic to nerve tissues in earthworms andmammals, we have also developed in vivo procedures that permanentlymaintain earthworm myelinated medial giant axons whose functionaland morphological integrity has been restored by PEG-induced fusionafter axonal severance. In all these in vitro or in vivo procedures,the success of PEG-induced fusion of sciatic or spinal axons andmyelinated medial giant axons is measured by the restored conductionof action potentials through the lesion site, the presence ofintact axonal profiles in electron micrographs taken at the lesionsite, and/or the intra-axonal diffusion of fluorescent dyes acrossthe lesion site. These and other data suggest that the applicationof polymeric fusiogens (such as our PEG solutions), possibly combinedwith a tissue adherent (such as our PEG hydrogels), could leadto in vivo treatments that rapidly and permanently repair cutor crushed axons in the PNS and CNS of adult mammals, includinghumans.

Key words: axotomy; axonal regeneration; membrane fusion; neurotrauma; nerve repair; polyethylene glycol

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
REFERENCES

Various strategies have been used to try to reestablish functional connections after PNS or CNS axons are severed. For PNSaxons, strategies, such as nerve grafts (Jenq and Coggeshall,1986), connective tissue matrices (Herbert et al., 1996), nervegrowth guides (Aebischer et al., 1990), etc. (for review, seeDas and Wallace, 1986; Lundborg, 1990), have been designed toenhance the number of severed axons that regenerate at 1-2 mm/dfrom surviving proximal stumps. However, even if they eventuallyreestablish some functions, these PNS outgrowths usually takefrom months to years to reach denervated target tissues in largermammals, such as humans (Das and Wallace, 1986; Bittner, 1988,1991). To try to reestablish functional connections after severanceof CNS axons (whose proximal stumps normally do not regenerate),strategies have been designed to induce outgrowths from proximalstumps of surviving axons and/or to generate axonal outgrowthsfrom donor tissues. Reestablishment of functional connectionstakes many months and has been difficult to convincingly demonstrateusing such strategies, which include donor transplants of peripheralnerve sheaths (David and Aguayo, 1981) or embryonic tissues (Giovaniniet al., 1997; Miya et al., 1997) and injections of antibodiesto oligodendritic inhibitors of CNS axonal outgrowth (Schnelland Schwab, 1990).

As an alternate strategy to more rapidly reestablish function after severance of PNS or CNS axons in mammals in vivo, we suggestthat solutions of fusiogens, such as polyethylene glycol (PEG),can rapidly (within minutes) and directly reestablish functionaland morphological continuity between severed axonal ends. We alsosuggest that, if necessary, tissue adherents, such as PEG hydrogels,can be used to maintain the integrity of PEG-fused axons whosecut ends have been PEG-fused. To begin to test the efficacy ofthis strategy, we initially developed PEG solutions that couldinduce fusion between the severed ends of a myelinated medialgiant axon (MGA) in the CNS of earthworms (Krause and Bittner,1990; Krause et al., 1991) or unmyelinated MGAs in the CNS ofcrayfish in vitro or mammalian NG 108-15 cells in tissue culture(Bittner et al., 1986). We now report that modified PEG solutionsrapidly fuse both cut and crushed ends of both myelinated mammaliansciatic axons (PNS axons) and spinal axons (CNS axons) in vitroaccording to the measures of functional and morphological continuityoutlined above. We also report that PEG hydrogels that we havedeveloped to adhere tightly to connective and other tissues inmammals and earthworms can be used to maintain the integrity ofPEG-fused axons in vivo. For example, when our PEG-based hydrogelis applied to connective tissue sheaths of PEG-fused MGAs in vivo,MGAs PEG-fused in vivo remain functionally and morphologicallyintact for at least 20 d in nonanesthetized earthworms, and MGA-mediatedbehaviors are permanentlyreestablished.

Given these and other data, we suggest that PEG solutions could be combined with our PEG hydrogel in an efficacious strategyto directly, rapidly, and permanently repair severed axons inthe PNS or CNS of adult mammals in vivo.

  MATERIALS AND METHODS

In vitro preparations. Three centimeter lengths of sciatic nerves with their epineural sheaths intact were dissected fromthe hindlimbs of deeply anesthetized (60-80 mg/kg pentabarbitol)adult male or female rats (250-400 gm; n > 300). Some sciaticnerves (n > 20) were subsequently desheathed by removing the epineuriumwith a coarse-tipped and a fine-tipped Dumont model 5forcep.

Three to five centimeter lengths of spinal cords were dissected free of the spinal column of deeply anesthetized adult rats(250-400 gm; n > 30) as described previously (Shi and Blight,1996, 1997). The spinal cord was divided in half at the midline,and the white matter of the dorsal columns was separated fromthe gray matter with a scalpel blade. Strips of white matter (spinalaxons) 3- to 5-cm-long and several millimeters in diameter weremaintained in oxygenated Krebs' solution at room temperature (~25°C)for at least 1 hr before use. Such spinal axons had no thick epineuralsheaths.

Three to five centimeter lengths (n > 300) of ventral nerve cords (VNCs), the CNS of earthworms, were dissected from the middlebody segments of adult animals anesthetized with 4% (w/v) Chlorotone(Eastman Kodak, Rochester, NY) (Krause and Bittner, 1990; Krauseet al., 1991). As described previously (Günther, 1975, 1976;Roots and Lane, 1983; Okamura et al., 1985; Ballinger et al.,1997), the VNC contains two lateral giant axons (LGAs), each 50-100µm in diameter, and a single MGA, 80-150 µm in diameter, includinga 5- to 10-µm-wide sheath consisting of myelin whose biochemistryis slightly different from that of mammalian myelin and whoselayered structure is somewhat looser than that of mammalian myelin.The MGA typically protrudes ~50 µm from the cut end of each sideof a severed VNC (Krause and Bittner, 1990; Krause et al., 1991,1994; Ballinger et al., 1997), making it particularly easy toappose the two ends. MGA and LGA action potentials (APs) can beuniquely identified in extracellular recordings of transmembranecurrents from the VNC or from the entire animal (Bullock and Horridge,1965; Günther, 1975, 1976; Krause and Bittner, 1990; Krause etal., 1991). That is, the MGA AP typically has the lowest thresholdand fastest conduction velocity in the VNC and the second largest(extracellularly recorded) AP. The two LGAs are connected by gapjunctions and typically exhibit coincident APs, which have thesecond fastest velocity and threshold but largest extracellularlyrecorded AP. All other (nongiant) axons in the VNC generate much(approximately threefold) slower APs with much (approximatelyfivefold) smaller extracellularly recorded APs than MGAs or LGAs.Once activated in vivo by mechanical stimulation of sensory fibersat the rostral end of the earthworm, MGAs evoke a rapid contractionof the caudal end of the earthworm, an escape behavior that iscritical for its survival in its normal environment (Bullock andHorridge, 1965).

In vivo preparations. VNCs were completely severed in earthworms (n > 150) anesthetized with 4% Chlorotone, and the cut endsof the MGAs were brought into close apposition with minuten pinsas described below for in vitro preparations. Once the cut endswere closely apposed, in vitro and in vivo procedures were thesame for application of various solutions or PEG hydrogels. APswere recorded from MGAs in vivo as described in Materials andMethods, Electrophysiological techniques. Operated earthwormswere maintained in Petri dishes containing moistened filter paperfor 3 d after surgery and thereafter maintained for up to 20 din Petri dishes containing peat moss and pottingsoil.

Saline solutions. As given in detail in Table 1 for each numbered solution listed below, sheathed or desheathed sciatic nervesor strips of spinal axons were bathed in various solutions: (1)a Ca²⁺-free hypotonic PBS; (2) a physiological "mammalian saline" at~25 or 37°C, as maintained by a Peltier unit; (3) a Ca²⁺-free, slightly hypotonic, mammalian saline formulated as listedin 2, except that CaCl₂ was omitted and 0.5-2 mM EGTA was added;(4) a Ca²⁺-free hypotonic mammalian saline formulated as listed in 3, exceptthat CaCl₂ was omitted, NaCl was reduced by one-half, and 0.5-2mM EGTA was added; (5) a physiological Krebs' solution; and (6)a Ca²⁺-free (isotonic) Krebs' solution formulated as in 5, except forequimolar replacement of CaCl₂ with MgCl₂ plus 0.5-2 mM EGTA.These and other solutions were usually equilibrated with a mixtureof 95% O₂-5% CO₂. We detected no difference in results obtainedwith the mammalian saline versus Krebs' solution or the Ca²⁺-free, slightly hypotonic, mammalian saline versus the Ca²⁺-free (isotonic) Krebs' solution.


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Table 1. Composition of mammalian and earthworm salines

VNCs containing the MGA were bathed at room temperature (~25°C) in either (7) a physiological "earthworm saline" or (8) aCa²⁺-free (slightly) hypotonic earthworm saline formulated as listedabove, except that CaCl₂ was omitted and 0.5-1.0 mM EGTA wasadded.

Electrophysiological techniques. To accomplish conventional extracellular stimulation and recording of either multiple simultaneouslygenerated APs ["compound" APs (CAPs)] from bundles of sciaticaxons or uniquely identifiable APs from a single MGA, sciaticnerves or VNCs were bathed in physiological salines in a single-chambereddevice similar to the one developed to record APs before and afterPEG-induced fusion of MGAs (Krause and Bittner, 1990; Krause etal., 1991). CAPs or APs were led to an extracellular AC amplifier(P-15; Grass Instruments, West Warwick, RI) and displayed on anoscilloscope. APs from MGAs were occasionally extracellularlyrecorded in this apparatus from the entire animal in vivo by usingdamp Kimwipes (Kimberly-Clark, Roswell, GA) to immobilize theentire intact earthworm, positioned so that its ventral surfacewas pressed tightly against the stimulating and recording electrodesin our single-chambered device (Krause et al., 1991, their Fig.1). Sciatic nerves were extracellularly stimulated with voltages(usually 5-15 V) that were supramaximal to elicit a CAP havingthe largest peak amplitude, i.e., voltages that elicited APs inthe maximum number of sciaticaxons.

For double sucrose gap recordings, sciatic nerves, spinal nerves, or VNCs were placed in the central chamber of a five-chamberedrecording device as described previously (Shi and Blight, 1996).CAPs or APs were stimulated or recorded in the end chambers, whichwere filled with 0.12 M KCl. The larger end chambers were eachseparated from the larger central chamber by a smaller chamberthrough which sucrose was perfused. The central chamber was oftencontinuously perfused (except during PEG application) with oxygenated25°C Krebs' solution by gravity flow. Solutions in the centralchamber were continuously removed by vacuum suction. CAPs or APswere led to a DC intracellular amplifier (IE-251; Warner, GrandHaven, MI) to be conventionally displayed on an oscilloscope ora Dell 200 computer to be processed by a data analysis program(C-Scope; RC Electronics, Santa Barbara, CA) whose output wasdisplayed on an x-yplotter.

APs from MGAs were also occasionally recorded intracellularly with glass microelectrodes filled with 3 M KCl. In such cases,the signals were displayed as described for MGA APs in doublesucrose gaprecordings.

Severance of sciatic axons, spinal axons, or MGAs. Sciatic nerves, strips of spinal axons, or VNCs were viewed with a dissectingmicroscope during all experimental procedures, including axonalseverance (cutting or crushing) and subsequent PEG-induced fusion.In all "cut" preparations of sheathed or desheathed sciatic nerves,spinal axons (lacking sheaths), or sheathed VNCs, the nerve bundlewas completely cut between the stimulating and recording electrodeswith a shard of a microknife made from a Gillette (Boston, MA)Blue Blade so that the cut axonal ends always completely separatedby 0.5-1.0 mm. Cut ends were tightly apposed by pushing on thesciatic nerve, spinal axons, or VNC with minuten pins or by lightpressure applied with fine-tipped forceps. A nylon mesh stretchedacross a metal loop (which was not in contact with the nerve tissue)positioned by a micromanipulator was used to keep the tightlyapposed ends in place or to make fine adjustments in the alignmentof the cut ends by gently tugging on the surface axons and nylonmesh strands. In "crushed" preparations of sciatic axons, spinalaxons, or MGAs, the sheathed sciatic nerve or VNC, respectively,was compressed with a dull microknife or fine-tipped forceps toproduce a transparent zone (200- to 500-µm-wide) of axoplasm-freetissue, as viewed with the dissecting microscope. The epineurialsheath surrounding crushed sciatic axons or MGAs did not pullapart, i.e., the connective tissue sheathing the sciatic nerveor VNC was not severed. The completeness of cut or crush severancewas always confirmed by electrically stimulating the sciatic nerve,strip of spinal axons, or VNC and observing that no CAPs fromsciatic axons, spinal axons, or APs from MGAs were transmittedacross the lesion site. Furthermore, most of the morphologicaland electrophysiological data presented in the Results were takenfrom cut (rather than crushed) preparations, thereby eliminatingartifacts or alternate explanations associated with the presenceof an incompletelesion.

Application of PEG solutions. PEG of various molecular weights (in kilodaltons), as specified in the Results, was dissolvedin distilled water, which often contained food coloring to enableus to visualize the location of the PEG solution. PEG was appliedfrom a micropipette positioned using a micromanipulator on oneside of the sciatic nerve, strip of spinal axons, or VNC so thatthe PEG-containing solution flowed in a narrow stream (~500-µm-wide)over the closely apposed cut or crushed axons at the lesion site.The PEG was then removed by continuous suction applied to a glassmicropipette positioned on the opposite side of the sciatic nerve,strip of spinal axons, or VNC as reported previously (Krause andBittner, 1990; Krause et al., 1991).

Synthesis of PEG hydrogels. As described previously (Pathak et al., 1992; Sawhney et al., 1993), our PEG hydrogel was synthesizedby photochemically inducing the polymerization of a precursorsolution to form a cross-linked hydrogel directly on the tissuebeing treated in situ. The precursor solution consisted of 23%8 kDa PEG diacrylate (see below), 1 mM eosin Y (Sigma, St. Louis,MO), 100 mM triethanolamine (Sigma), and 1500 ppm N-vinylpyrrolidone(Aldrich, Milwaukee, WI) dissolved in PBS at a final pH of 7.4.The 8 kDa PEG diacrylate was formed from 8 kDa PEG, which hasan alcohol at both ends, by reacting the terminal alcohols withacryloyl chloride to form the $alpha$ , $omega$ -diacrylate of PEG (Pathak etal., 1992). This precursor polymer is soluble in the aqueous precursorsolution, but polymerization of the material (because it has anacrylate at both ends) forms a cross-linked polymer network thatis highly swollen with water (~90% of its mass is water). Thispolymerization was induced by exposing the precursor solutionbriefly (15-30 sec) to visible light at intensities and frequenciesthat are noncytotoxic, even for exposures lasting manyhours.

In brief, the PEG-based hydrogel we developed has several valuable properties. (1) The hydrogel transforms within 30 sec froma liquid precursor into a solid gel that adheres strongly to theVNC and sciatic nerve tissues. PEG-based diacrylate precursorswere polymerized in situ from aqueous solution to form materialsthat adhered tightly to VNCs (n > 20) and sciatic nerves (n >20) and remained there during degradation as reported for theperitoneal cavity (Hubbell et al., 1994; Chowdhury and Hubbell,1996) and the carotid artery (West and Hubbell, 1996). The PEGdiacrylate penetrates the biological macromolecular network inthe extracellular matrix of the tissue. Conversion into a solidcross-linked hydrogel results in permanent interpenetration andthus adhesion. The PEG diacrylate is the precursor polymer thatis further polymerized and cross-linked, the eosin Y and triethanolamineform a photoinitiation system, and the N-vinylpyrrolidone servesas a polymerization accelerator. (2) Our hydrogel transforms froma liquid precursor to a solid hydrogel on the surface of VNCs,sciatic nerves, or spinal cords without cytotoxicity as reportedfor other tissues (West and Hubbell, 1996). The PEG diacrylateprecursor has essentially the same biocompatibility (lack of cytotoxicity)as native PEG of the same molecular weight, eosin Y is a commondrug colorant, triethanolamine is commonly used in pharmaceuticalformulations, and N-vinylpyrrolidone is acceptable as a contaminantin the medical polymer Povidone at much higher concentrationsthan used herein (Sawhney et al., 1993). (3) The hydrogel is biocompatibleand noninflammatory in vivo. The transformed PEG hydrogel is highlybiocompatible, in a large part because of the favorable interactionsof PEG with proteins. PEG is very hydrophilic and nonionic, andit blocks interactions with cell-surface receptors, thus producinglow levels of protein adsorption and inflammatory cell adhesion(West and Hubbell, 1996). (4) Our hydrogel can be designed todegrade over a few days to several months by incorporating ester(e.g., glycolic, lactic, caproic acid) linkages to provide sitesfor nonenzymatic hydrolysis (Sawhney et al., 1993; West and Hubbell,1996). In the present case, biostable hydrogels, lacking suchdegradation sites, were usually selected for these studies. (5)Our hydrogel does not affect axonal structure or function (seeResults).

Application of PEG hydrogels. PEG hydrogels were applied from microsyringe needles in vitro or in vivo to sciatic nerves ofrats anesthetized with pentabarbitol as described above. Afterrecovery from anesthesia, the animals were kept in individualcages. Wounds were closed with 7-0 or 8-0 sutures (Ethicon, Somerville,NJ). Topical anesthetics were applied to the wound site, whichwas examined daily forinfection.

PEG hydrogels were applied to the VNC of earthworms maintained in 10-cm-diameter Petri dishes, sometimes containing filterpaper or soil moistened with 0.1% Chlorotone to anesthetize theanimal. The lesion site was sometimes closed with 7-0 or 8-0 sutures.MGA APs were occasionally recorded in vivo from the outer surfaceof earthworms as described in Materials and Methods, Electrophysiologicaltechniques.

Histological-ultrastructural procedures. After recording CAPs, control (n = 2) or PEG-fused (n = 5) sciatic nerves were carefullyfixed in place in the recording chamber (which was then discarded)with a solution of 3% paraformaldehyde, 3% glutaraldehyde, and0.1% picric acid in 0.1 M cacodylate buffer, pH 7.4. The tissuewas post-fixed in 2% osmium tetroxide in 0.1 M cacodylate buffer,pH 7.4, dehydrated in a graded alcohol series, and embedded inSpurrs's plastic as described previously (Sunio and Bittner, 1997).The sciatic nerve was sectioned longitudinally approximately halfwaythrough the fusion site, taking both thick (0.5 µm) sections forimaging at lower magnifications to identify the original siteof apposed cut ends and thin (silver or gold) sections for imagingat higher magnifications. To construct a better three-dimensionalimage of the fusion site, we sometimes remounted the remainingtissue and took thick and thin cross sections at the site of PEG-inducedfusion (see Ballinger et al., 1997, for a description of thissectioningprocedure).

Confocal or epifluorescence microscopy of dye-filled axons. The following fluorescent dyes taken up by sciatic axons wereobtained from Molecular Probes (Eugene, Oregon): sulforhodamine101 (548 nm excitation wavelength, 605 nm emission wavelength),sulforhodamine B-dextran (565 nm excitation wavelength, 586 nmemission wavelength), and Texas Red (584 nm excitation wavelength,605 nm emission wavelength). Dye-labeled desheathed sciatic axonswere viewed with confocal and differential interference contrast(DIC) microscopy using a Leica (Nussloch, Germany) TCS-4D fittedwith two water immersion lenses [40×, 0.75 numerical aperture;63×, 0.90 numerical aperture; both from Zeiss (Oberkochen, Germany)]and a 10×, 0.30 numerical aperture lens from Leica. (Sciatic axonswere much more difficult to image confocally in sheathed sciaticnerves.) Digitized DIC and confocal images were stored and analyzedon a Macintosh 7200/90 equipped with NIH Image 1.6 and Adobe Systems(San Jose, CA) Photoshop 4.0 software. Dyes were extracellularlyapplied to sciatic or spinal nerve bundles by using a 26 gaugeneedle to inject ~1 µl of a 15% solution of a fluorescent dyefrom a microsyringe into these nerve bundles at 3-6 mm from thelesion site. The injected sciatic nerves were maintained at 25°Cfor 6-14 hr to allow diffusion of the dyes through the entirelength of control or PEG-fused sciatic axons. To ensure that thedye did not travel by an extracellular diffusion path, we continuouslyperfused oxygenated Krebs' through the chamber containing thelesion site to remove any dye that may have leaked into the bathsaline.

MGAs (n > 15) were iontophoretically injected (Krause and Bittner, 1990) on one side of the lesion site with micropipettesfilled with Lucifer yellow CH (Molecular Probes). Sciatic axons,spinal axons, or MGAs filled with fluorescent dyes were also examinedusing an inverted Zeiss ICM-35 with the ability to image for epifluorescenceand enhanced video microscopy of whole mounts cleared in methylsalicylate.

  RESULTS

Development of our protocol for PEG-induced fusion of sciatic axons in vitro

In an initial series of experiments (n > 250 sciatic nerves) to devise a protocol to fuse the cut or crushed ends of mammalianaxons, we first extracellularly recorded control CAPs generatedby 1 Hz maximal stimulation of intact sciatic axons in sheathedsciatic nerves (Fig. 1A,B, i) bathed in mammalian saline (seeMaterials and Methods). Sciatic nerves were then bathed in a Ca²⁺-free saline (Materials and Methods; Tables 1, 2) before completelycutting (n > 50) or crushing (n > 200) the sciatic nerves halfwaybetween the stimulating and recording electrodes (see Materialsand Methods). CAPs were usually slightly smaller in Ca²⁺-free salines in these initial (data not shown) and later (Fig.1D,E) experiments. CAPs always completely disappeared after sciaticaxons were completely transected by cutting or crushing (Fig.1A,B, t). The 1 Hz electrical stimulation was temporarily haltedafter the sciatic axons were severed, and a PEG solution was appliedto the lesion site. After 0.2-2 min, the Ca²⁺-free saline was replaced with a physiological saline containingCa²⁺. CAPs were counted as conducting through the lesion site (successfulfusion) only if a CAP reappeared after PEG-induced fusion (Fig.1A,B, f) and then completely disappeared after the sciatic axonswere retransected (Fig. 1A,B, rt), i.e., transected so that thecut ends were completely separated by a gap of at least 0.5 mm.In brief, we applied the same electrophysiological criteria toCAPs to define a successful fusion event for mammalian sciaticaxons (Fig. 1A,B; Table 2) that we applied in previous (Krauseet al., 1991) or current (Fig. 1F; Table 2) reports of successfulfusion of earthworm MGAs; conduction of MGA APs across the stimulatingand recording electrodes must be present before severance, completelyeliminated by severance, restored by PEG, and completely eliminatedby resevering.

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Figure 1. CAPs from sciatic (A-D, I) or spinal (E) axons or APs from MGAs (F-H) in intact and PEG-fused preparations extracellularly recorded using conventional (A-C, F-I) or double sucrose gap techniques (C-E). A-E, Individual CAPs recorded conventionally (A-C) or with double sucrose gap (C, E) from control rat sciatic or spinal axons (i traces) before replacing the Krebs' (Table 1, solution 5) in the central chamber with Ca²⁺-free Krebs' (Table 1, solution 6) containing 1 mM EGTA (OCa²⁺ traces) at ~25°C. The sciatic or spinal axons were then transected to eliminate the CAP (t traces). PEG was applied to the apposed cut ends, and the central chamber was again perfused with Krebs' (Table 1, solution 5). Within 10 min, the CAP again appeared in fused sciatic or spinal axons (f traces) and remained for $>=$ 30 min. The CAP was again eliminated when the sciatic or spinal axons were retransected at the original lesion site (rt traces). C illustrates the increase in signal-to-noise ratios achieved using sucrose gap recordings (sr trace) compared with conventional recordings (cr trace) of an intact sciatic nerve. The sciatic nerve or strip of spinal axons was always extracellularly stimulated by a maximal voltage (e.g., ~6 V in D and 10 V in E) that reliably produced a CAP with the greatest peak amplitude. F, Individual MGA and LGA APs recorded conventionally using the single-chamber device of Krause et al. (1991). Control (intact) MGA (m) and LGA (L) APs (trace 1) placed in physiological earthworm saline (Table 1, solution 7) stimulated by a rostral electrode and recorded from rostrally (r) and caudally (c) placed electrodes before cutting the axons between the two recording electrodes to eliminate the APs from the caudal electrode (trace 2). The VNC was placed in Ca²⁺-free earthworm saline (Table 1, solution 8), and PEG was applied to the apposed cut ends of the MGA, but not the LGA, to induce PEG-fusion only of the MGA, and the central chamber was again perfused with earthworm saline (Table 1, solution 7). PEG hydrogel was then applied to the lesion site. Within 10 min, the MGA (but not LGA) AP was again recorded for 1-24 hr on the caudal side of the lesion site (trace 3). G, MGA and LGA APs recorded in vitro from a VNC before (trace 1) and after (trace 2) it was surrounded by our PEG-based hydrogel for 1 hr. H, MGA APs recorded from a VNC in which MGAs PEG fused in vivo by our PEG solution were surrounded by our PEG-based hydrogel and then maintained in vivo for 15 d. The VNC was then dissected from the animal. When the VNC was extracellularly stimulated rostral to the lesion site and extracellularly recorded rostrally and caudally to the site of PEG-induced fusion and hydrogel application, the rostral electrodes recorded MGA and LGA APs, and the caudal electrode recorded only MGA APs. That is, the MGA, but not the LGA, had been PEG-fused. The MGA was then injected with Lucifer yellow CH, which diffused through the site of PEG-induced fusion (Fig. 3D). I, CAPs conventionally recorded in vitro from a sciatic nerve exposed to PEG-based hydrogel for 10 d in vivo. The sciatic nerve was extracellularly stimulated with 0.1 (subthreshold), 3, 6, and 10 (maximal) V pulses. Calibration: A, B, F-I, 0.5 mV, 1 msec; C-E, 1 mV, 0.5 msec.


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Table 2. Percent of PEG-fused CAPs observed within 60 min after severing sciatic axons

We observed no instances of PEG-induced fusion (as measured by reappearance of a CAP) of cut or crushed sciatic axons withmost of our initial attempts (Table 2) to modify the protocolthat had been most successful in PEG-fusing earthworm giant axons:4 kDa PEG at 50% w/w (in double-distilled water) applied for 30-60sec to the lesion site, which was bathed in Ca²⁺-free salines of 70-90% tonicity with 1 mM EGTA (Krause and Bittner,1990). For example, CAPs were not conducted across a crush siteafter application of 50% (w/w) PEG of 1.5 kDa or 60% PEG of 1-1.5kDa (J. T. Baker Chemical Company, Phillipsburg, NJ) applied for30-60 sec in Ca²⁺-free hypotonic PBS with 0.5 mM EGTA (Table 2, protocols 1, 2).No cases of successful fusion were noted when 50% 4 kDa PEG (J.T. Baker Chemical Company) was applied in Ca²⁺-free mammalian salines or Ca²⁺-free hypotonic mammalian salines for shorter times, e.g., <15sec (Table 2, protocols 3-5). No cases of successful CAP conductionacross a crush site were noted after 30-60 sec applications of50% 1.5 kDa PEG in Ca²⁺-free, slightly hypotonic, mammalian saline when <1.0 mM EGTAwas used, even if 0.1 or 1% DMSO was added (Table 2, protocols6-8). Only one successful fusion of crushed sciatic axons wasobserved when PEG with a somewhat higher molecular weight wasapplied (Table 2, protocol 9). No cases of successful fusionof crushed sciatic axons were noted when lower concentrations(1-10%) of 2 kDa PEG (Aldrich) were applied in Ca²⁺-free, slightly hypotonic, mammalian saline containing 1.0 mMEGTA (Table 2, protocols 10,11).

In contrast to these earlier trials, PEG-induced fusion was consistently observed in subsequent sets of trials using a 50%(w/w) solution of 2 kDa PEG (Aldrich) applied once or twice for60-120 sec in Ca²⁺-free, slightly hypotonic, salines containing 1-2 mM EGTA. Forexample, cut or crushed sheathed sciatic axons exhibited fusionwhen 50% 2 kDa PEG was applied for 60 sec once or twice in a Ca²⁺-free, slightly hypotonic, mammalian saline containing 1 mM EGTA(Table 2, protocols 12-19). The percentage of sciatic nerve preparationsexhibiting electrophysiological evidence of successful PEG-inducedfusion ranged from 10 to 71% in different sets of trials (Table2) performed by different personnel. In general, the rate ofsuccess increased with practice by eachcollaborator.

The addition of 100 µg/ml calpain to 50% 2 kDa PEG slightly increased the frequency of preparations exhibiting successfulPEG-induced fusion of crushed sciatic axons, whereas the additionof 100 µg/ml leupeptin greatly decreased the frequency of successfulPEG-induced fusion (Table 2, paradigms 20, 21, respectively).We also noted (Table 2, paradigms 22, 23) that sheathed sciaticaxon preparations were much easier to fuse with PEG than desheathedpreparations (used for confocal viewing because the sciatic nervesheath distorts confocalimaging).

Given these data and our observations that (1) hypotonic salines were not necessary to fuse cut spinal axons and (2) Ca²⁺-free Krebs' solutions containing 1-2 mM EGTA produced resultssimilar to slightly hypotonic mammalian salines containing 1-2mM EGTA, we performed almost all subsequent sucrose gap-recordedfusions of cut sciatic or spinal axons using a 50% solution of2 kDa PEG (Aldrich) applied once or twice for 60-120 sec in anisotonic Ca²⁺-free Krebs' solution (sciatic axons) containing 1-2 mMEGTA.

Sucrose gap assessment of sciatic axons and MGAs fused with PEG in vitro

To enhance the signal-to-noise ratio of CAPs recorded from PEG-fused sciatic (Fig. 1C,D) or spinal (Fig. 1E) axons, we placedsheathed or desheathed sciatic nerves or strips of spinal axonsfrom rats in a five-chambered device (Shi and Blight, 1996) forsingle or double sucrose gap recordings (see Materials and Methods).The ability of intact (control), severed, or fused sciatic orspinal axons to conduct CAPs through the central chamber was assessedin the following manner. Control CAPs generated by maximum stimulationof intact axons in one end chamber were conducted across the centralchamber containing Krebs' solution (Table 1, solution 5) andrecorded in the opposite end chamber(Fig. 1D,E, i). The axonsin the central chamber were then immersed in the Ca²⁺-free Krebs' solution containing 1 mM EGTA (Table 1, solution6). Although CAP amplitude usually declined by 10-30%, this calcium-freesolution did not eliminate the conduction of CAPs across the centralchamber (n > 20 sciatic nerves) (Fig. 1D,E, OCa²⁺). The sciatic or spinal axons were then cut completely at theirmidpoint in the central chamber, as assessed by visual inspectionand by the complete elimination of CAP conduction across the lesionsite in the central chamber (Fig. 1D,E, t).

To induce severed axonal ends to fuse, the cut surfaces of sciatic or spinal axons bathed in the Ca²⁺-free Krebs' were first tightly apposed, and a continuous streamof 50% 2 kDa PEG was applied to the lesion site for 60-120 sec.The Ca²⁺-free solution in the central chamber bathing the PEG-exposedaxons was replaced by oxygenated Krebs' (Table 1, solution 5).CAPs often conducted across the lesion site within 2-15 min afterPEG application and continued up to 120 min thereafter (Fig. 1D,E,f), at which time recordings were discontinued. The peak amplitudeof CAPs after PEG fusion ranged from 1 to 25% (usually 5-15%)of the amplitude of control CAPs recorded from the same sciaticor spinal axons before severance. The latency of the CAP oftenincreased slightly, and the peak broadened after PEG-induced fusion.The peak amplitude of the CAP after PEG fusion was reduced, probablybecause PEG reestablished continuity between only a fraction ofthe total number of severed sciatic axons, as suggested by photomicrographsor electronmicrographs (Figs. 2, 3A) or confocal images (Fig.4) of such lesion sites after the application of PEG solutions.The increased latency and/or broadening of the peak of the CAPafter PEG-induced fusion might result from a slowed conductionvelocity through the fusion site, possibly because of a decreasedinput resistance of PEG-fused membranes as reported for PEG-fusedearthworm giant axons (Krause et al., 1991), or from a tendencyfor fusion to occur in smaller-diameter fibers in a bundle ofPNS or CNS axons.

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Figure 2. Photomicrographs (A-C) and electron micrographs (D-F) of longitudinal (A, B, D, E) and cross (C, F) sections of PEG-fused sciatic nerves after a complete cut (A, D, E) or crush (B, C, F). Vertical dashed lines in A-C show the site of severance and subsequent PEG application. Note that B and C are longitudinal and cross sections, respectively, taken through the site of PEG-induced fusion of a crushed sciatic nerve, of which a portion (box in C) is shown at higher magnification in F. As described in Materials and Methods and by Ballinger et al. (1997), the crushed sciatic axon was first sampled in longitudinal section (B) until a portion of the fusion site was detected (dashed line). The tissue was then remounted, and cross sections (C) were taken through another portion of the fusion site (dashed line). D and E are higher-magnification images of a portion of the cross section (box in A) of the entire sciatic nerve at the site of PEG-induced fusion. Axons exposed to PEG at the lesion site were in some disarray, and hence some individual axons were in transverse (D) or longitudinal (E) planes with respect to the long axis of an axon. Ax*, An axon with myelin or other membranes seriously delaminated, damaged, or dissolved by PEG; Ax , an axon with relatively intact axoplasm, myelin, and other membranes at the plane of PEG-induced fusion; Ax?, an axon with slightly damaged axoplasm, myelin, and other membranes at the plane of PEG-induced fusion; apposed arrowheads, the extent of myelin sheaths (My). For the cut axon shown in A, D, and E, the peak amplitude of the control CAP was 20 mV before the axons were transected. The CAP amplitude was 0 mV after the axons were cut in Ca²⁺-free hypotonic mammalian saline with 1.0 mM EGTA. A thin stream of 50% PEG 2000 kDa (Aldrich) was applied to the lesion site for 2 min. The preparation was then bathed in Krebs' saline. Within 2 min after PEG application, the CAP was 0.5 mV, suggesting that PEG had induced fusion in a small fraction (2-5%) of crushed axonal ends. The CAP grew to 5 mV after the PEG-fused axons were maintained in Krebs' for 1 hr, suggesting that as many as 20-30% of axons were now conducting through the lesion site. The sciatic nerve was then fixed as described in Materials and Methods. For the crushed sciatic nerve shown in B, C, and F, the peak amplitude of the control CAP was 14 mV before the axons were crushed. The CAP amplitude was 0 mV after the axons were crushed in Ca²⁺-free hypotonic mammalian saline with 1.0 mM EGTA. A thin stream of 50% PEG 2000 kDa (Aldrich) was applied to the lesion site for 1 min. The preparation was then bathed in the mammalian saline. Within 5 min after PEG application, the peak amplitude of the CAP was 1.0 mV, suggesting that PEG had induced fusion in a fraction (5-10%) of crushed axonal ends. The sciatic nerve was then fixed as described in Materials and Methods. Scale bar: A-C, 75 µm; D, 2 µm; E, F, 4 µm.

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Figure 3. Photomicrographs of sciatic axons (A, E, F) and MGAs showing PEG fusion in vitro (A) or in vivo (C, D) and that the PEG hydrogel does no obvious morphological damage to MGAs (B-D) or sciatic axons (E, F). A, Photomicrograph of a longitudinal section taken through a cut sciatic axon that had been PEG-fused as described in Materials and Methods. Asterisk identifies a myelinated axon that could be traced through the lesion site. Arrowheads mark the site of PEG-induced fusion. B, Lucifer yellow fill of an MGA surrounded by PEG-based hydrogel for 15 d. The hydrogel was appled to the VNC in the region bounded by the two arrows. C, Lucifer yellow fill of an MGA fused with the PEG solution and then surrounded by the PEG-based hydrogel for 5 d in vivo. Arrows show location of hydrogel. D, Lucifer yellow fill of a PEG-fused MGA surrounded by PEG-based hydrogel maintained for 15 d in vivo. Arrows show location of hydrogel. cb, The dye-filled cell body of the MGA. Data from same animal shown in Figure 1G. E, Photomicrograph of rat sciatic axon surrounded by PEG-based hydrogel for 24 hr. F, Enlargement of boxed area in E. bv, Blood vessel. Scale bar: A, F, 25 µm; B, 100 µm; C, D, 150 µm; E, 200 µm.

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Figure 4. Confocal fluorescence images (photomicrographs) of control (A) and cut sciatic axons subsequently PEG-fused (B, C) and injected with sulforhodamine 101 24 hr before viewing. All figures are oriented so that the injected segment is at the bottom of each panel and the injection site is ~3 mm from the lesion site. A, Lower-magnification image using a 10× Leica lens, showing control sciatic axon that was transected and closely apposed to the injected segment, but PEG was not applied to the lesion site (see Materials and Methods). The gap at lesion site is denoted by G and a double-headed arrow. Arrow points to the uptake of dye by connective tissue elements at the lesion site of the noninjected segment. B, Lower-magnification image using a 10× Leica lens of the lesion site (bracket) showing some dye-filled axons traversing the lesion site. C, Higher-magnification image using a 40× Zeiss lens showing dye-filled axons traversing the lesion site. For the cut sciatic nerve shown in B and C, the peak amplitude of the CAP was 6.2 mV before transection, 4.0 mV in Ca²⁺-free saline with 1.0 mM EGTA, 0 mV after transection, 1.9 mV within 10 min after PEG-induced fusion, and 0 mV when retransected. Scale bar: A, B, 110 µm; C, 25 µm.

We performed a series of control procedures using conventional or sucrose gap recordings to ensure that restored CAP conductionof PEG-fused sciatic and/or spinal axons represented a restorationof their axolemmal integrity at the lesion site rather than anartifactual conduction of electrical signals through the lesionsite (Krause and Bittner, 1990; Krause et al., 1991). For example,CAPs did not conduct through the lesion site if the following:(1) PEG-fused sciatic or spinal axons were stimulated with subthresholdvoltages (n > 40); (2) sciatic or spinal axons at the originalfusion site were retransected (n > 50) (Fig. 1D,E, rt); (3) Ca²⁺-free Krebs' (or Ca²⁺-free mammalian saline), but not PEG, was applied to the closelyabutted ends of cut (n > 20) or crushed sciatic (n > 10) or spinal(n > 10) axons; and (4) Ca²⁺-free Krebs' (or Ca²⁺-free mammalian saline) and PEG were applied to loosely abuttedends of cut sciatic (n > 20) or spinal (n > 10) axons. As furthercontrols for artifacts that might somehow be idiosyncratic tothe five-chambered device or the sucrose gap technique, we showedthat electrophysiological evidence that our PEG solutions fusedthe cut ends of MGAs could be obtained in three different ways:(1) double sucrose gap recordings using the five-chambered device;(2) conventional recordings using the five-chambered device inwhich all chambers were filled with earthworm saline; and (3)conventional recordings using the single-chambered device (Fig.1F) from which APs from PEG-fused MGAs have already been published(Krause et al., 1991).

Ultrastructural assessments of sciatic axons fused with PEG in vitro

The anatomical continuity of sheathed sciatic axons was examined in electron micrographs of thin and thick sections of cut(n = 2) or crushed (n = 3) sciatic nerves that demonstrated PEG-inducedfusion by restoration of CAP conduction using conventional orsucrose gap recording techniques (Fig. 1A,B,D). Sciatic axonswere often in disarray when viewed in longitudinal (Fig. 2A,B,D,E)or cross (Fig. 2C,F) sections taken at many points through thelesion site. The myelin sheaths of most sciatic axons exposedto PEG showed extensive delamination and vesiculation in longitudinal(Fig. 2D,E, Ax*) or cross (Fig. 2F, Ax*) sections. The myelinsheaths of other sciatic axons exposed to PEG exhibited intermediateamounts of delamination and vesiculation (Fig. 2F, Ax?). Onlysome sciatic axons had tightly packed laminar membranes in theirmyelin sheaths (Fig. 2D-F, Ax ), similar to those reported previously(Sunio and Bittner, 1997) for intact sciatic axons. Only thosePEG-treated sciatic axons that did not have severe myelin delaminationsor other damage typically exhibited a continuous axoplasm, sheath,and (possibly) axolemma at the lesion site when viewed in longitudinal(Fig. 2D,E, Ax ) or cross (Fig. 2F) sections. That is, PEG appearedto affect the myelin and other membranes of many sciatic axonsat the fusion site but appeared to restore axonal and cytoplasmiccontinuity to only a relatively small fraction (usually 1-20%)of myelinated sciatic axons. (Individual unmyelinated sciaticaxons were too small for us to detect in photomicrographs or toreliably examine the effects of PEG in low-power electronmicrographs.)The extent of repair of myelinated sciatic axons assessed ultrastructurallygenerally correlated with the extent of sciatic axon repair assessedelectrophysiologically. For example, a greater percentage of myelinatedsciatic axons appeared to be PEG-fused in the cut shown in Figure2A compared with the crush shown in B and C, a result consistentwith the CAP data taken from these same preparations before fixationin which ~25% of the peak amplitude of the control CAP was restoredfor the cut sciatic axons and ~7% of the peak amplitude was restoredfor the crushed sciatic axons (Fig. 2). In longitudinal sectionstaken through a lesion site, myelinated axons could occasionallybe traced through a site of PEG fusion (Fig. 3A, asterisk).

Confocal and epifluorescence assessments of sciatic axons fused with PEG in vitro

In another protocol to examine anatomical continuity of PEG-fused sciatic axons, desheathed sciatic nerves that conductedCAPs across the lesion site were evaluated by noting the diffusionacross the lesion site of hydrophilic fluorescent dyes containedwithin individual sciatic axons. The lesion site was readily visibleas a distinct gap in low-power fluorescence images of controlpreparations in which the two cut ends of a bundle of sciaticaxons (n = 5) were closely apposed but PEG was not applied tothe lesion site (Fig. 4A). In these control preparations, a dyeinjected into a segment on one side of the lesion did not transferto axons in the segment on the opposite side of the lesion site(Fig. 4A), although small amounts of dye did label connectivetissue elements at the cut edges (Fig. 4A, arrow). The lesionsite was identifiable as a series of gaps in low-power fluorescenceimages of PEG-fused preparations (Fig. 4B, bracket). In contrastto control preparations, a small fraction of dye-filled sciaticaxons did traverse the lesion site (Fig. 4B,C) in preparations(n = 5) of cut sciatic axons that also showed electrophysiologicalevidence of PEG-induced fusion as assessed by the reappearanceof a CAP after PEGapplication.

Functional and morphological measures in vitro and in vivo for nontoxicity of PEG hydrogels in control axons

We first examined how different formulations of PEG hydrogels affected the function (e.g., AP peak amplitude, threshold, and/orconduction velocity or CAP peak amplitude) or morphology (e.g.,light microscopic or ultrastructural appearance) of MGAs or sciaticaxons in vitro and in vivo. As one example of an initial seriesof in vitro functional tests on over 200 MGAs, MGA (n > 20) APswere hyperexcitable (fired repetitively to a standard stimuluspulse of 0.5 msec in duration) when exposed to a 23% concentrationof the PEG hydrogel with one eosin Y initiator but were indistinguishablefrom control APs with a second eosin initiator compared with controlMGA APs (n > 20). Conversely, MGA (n > 20) APs were hypoexcitableand difficult to generate with a 28% concentration of the PEGhydrogel with either eosin initiator. Based on the results ofsuch tests, we used the following formulation of the PEG hydrogel(see Materials and Methods) for all of the protocols describedbelow: 23% w/v of 8 kDa PEG diacrylate dissolved in PBS, pH 7.4,containing 1 mM eosin Y, 100 mM triethanolamine, and 1500 ppmN-vinylpyrrolidone.

In a subsequent series of in vitro tests, we determined that this formulation of a PEG hydrogel was nontoxic to control MGAsand sciatic axons. For example, when this PEG hydrogel was appliedto VNCs (n = 10) for 1-24 hr in vitro, we were able to conventionallyrecord extracellular APs from MGAs in 90% of all animals tested(Fig. 1H). (The MGA is occasionally damaged in dissecting theVNC from an earthworm, and MGA APs cannot be recorded from 5-10%of dissected VNCs in control preparations.) Furthermore, thisability to extracellularly record an MGA AP and the peak amplitudeof intracellularly recorded APs (67 ± 4 mV) or their conductionvelocity (13 ± 3 m/sec) were not significantly different (p >0.1%) compared with MGAs (n = 10) taken from paired intact (control)regions of the VNC from the same animal (90%; 65 ± 3 mV; 14 ±3 m/sec,respectively).

Similar data were obtained from VNCs dissected from earthworms to which PEG hydrogel was applied in vivo for 1-30 d and sampledat the postoperative times given in Table 3. For example, anability to elicit MGA APs and their conduction velocity were notsignificantly different (p > 0.1%) from data obtained from controlMGAs (see above) or from sham-operated worms (Table 3). In thisprotocol, hydrogel-treated and sham-operated animals were anesthetizedfor 1 d at 16°C on Chlorotone-soaked filter paper and then placedin anesthetic-free soil. After recovery from anesthesia, the earthwormsexhibited behaviors normally elicited by MGA activation, includinga rapid contraction of the caudal end of the earthworm when therostral end was mechanically stimulated.


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Table 3. Conduction of MGA APs in intact or PEG-fused MGAs versus postoperative time

Morphological examinations of VNCs (Fig. 3B-D) confirmed data from these functional tests showing that the hydrogel "did noharm" to intact MGAs in vivo. For example, the diameter of MGAsor LGAs filled with Lucifer yellow CH were unaffected, or onlyslightly decreased, by application of the PEG hydrogel for 5 or15 d (Fig. 3B). Video-enhanced microscopic or ultrastructuralexamination showed only minor exfoliation at the site of hydrogelapplication (data not shown). The portion of VNC exposed to thePEG hydrogel often showed an accumulation of connective tissuethat adhered to the VNC. Sham-operated worms showed similar accumulationsof connective tissue, although these structures were usually lessextensive and less frequent compared with PEG hydrogel-treatedVNCs maintained in vivo forweeks.

This formulation of a PEG hydrogel was also nontoxic to rat sciatic axons in vitro and in vivo according to various functionaland structural tests. For example, when this PEG hydrogel wasapplied to rat sciatic nerves (n = 20) in vitro, the amplitudeand conduction velocity of CAPs did not decrease compared withintact (control) sciatic axons taken from the same animal. WhenPEG hydrogel was applied to rat sciatic nerves (n > 20) in vivo,sciatic axons continued to conduct normal CAPs for days to weeksafter application when the sciatic axons were removed from theanimal and recorded in vitro (Fig. 1I). The sciatic functionalindex, an in vivo measure of rat sciatic function (de Medinaceliet al., 1982), was not obviously affected by application of PEGhydrogel to sciatic nerves for 1-30 d compared with control orsham-operated rats (A. Lore, K. Loftin, and G. Bittner, unpublishedobservations). Finally, rat sciatic axons surrounded by this PEGhydrogel for weeks in vivo exhibited normal morphology (Fig. 3E,F)compared with control sciatic axons (Sunio and Bittner, 1997).In brief, our PEG hydrogels adhered tightly (see Materials andMethods) and were nontoxic to intact MGAs and rat sciatic axonstested in vitro and in vivo.

Use of the PEG hydrogel to maintain PEG-fused MGAs in vitro and in vivo

We first applied this PEG hydrogel to PEG-fused MGAs in vitro and in vivo to ensure that the PEG hydrogel was nontoxic toPEG-fused MGAs. For example, the application of PEG hydrogelsto VNCs containing an MGA fused with our PEG solution in vitrodid not decrease our probability of observing PEG-fused MGAs whenthe VNC was examined for conduction of MGA APs through the lesionsite from 0.5 to 24 hr (Table 3, PEG-fused MGAs in vitro). Infact, the PEG hydrogel may even have enhanced our ability to observePEG-fused MGAs, which varied from 8 to 71%, in different in vitrotrials that did not use the PEG hydrogel (Tables 2, 3).

If our PEG hydrogel was not applied to PEG-fused MGAs in vivo, those MGAs remained PEG-fused for 24 hr (Table 3, PEG-fusedMGAs in vivo) only if the earthworm was immobilized by maintainingit on filter paper or soil moistened with an anesthetic (0.05-0.1%Chlorotone). That is, once the earthworm was no longer immobilizedby the anesthetic, the VNC of PEG-fused MGAs quickly pulled apartat the site of fusion induced by application of the PEG solution.By applying our PEG hydrogel to the site where cut ends of anMGA had been induced to fuse in vivo, APs in PEG-fused MGAs couldbe maintained in nonanesthetized animals (Fig. 1H) sampled at1, 5-15, or 20 d after transection (Table 3, PEG-fused MGAs invivo), i.e., postfusion times that almost certainly equate toa permanent reestablishment of structural and functional continuityfor earthworm axons. Other data were consistent with this hypothesis.For example, tactile stimulation of the rostral ends of theseanimals with PEG-fused MGAs elicited a rapid contraction of thecaudal end of the earthworm. Furthermore, before sampling formicroscopy, MGA APs traversed the lesion site in whole animalrecordings (see Materials and Methods). When the VNCs were removedfrom these earthworms (n = 14) and recorded in vitro, MGA APsconducted across the site of PEG-induced fusion (Fig. 1H). WhenLucifer yellow CH was injected into some (n = 4) of these PEG-fusedMGAs ~1 mm caudal to the lesion site at the time of sampling (5-15d after transection) (Fig. 3C,D), the dye remained within theinjected MGA and diffused across the lesion site within minutes.All of these data suggest that PEG solutions combined with PEGhydrogels can reestablish and permanently maintain morphologicaland functional continuity in vivo between the previously severedhalves of PEG-fused earthworm MGAs, a myelinated invertebrateCNS axon that mediates behaviors important to the survival ofthe animal. Because there has been a rather conservative evolutionof the structural and functional properties of invertebrate andvertebrate (including mammalian) axons, these data from rats andearthworms also suggest that mammalian axons might be repairedin vivo by PEG solutions and, if need be, that the integrity ofPEG-fused axons could be maintained in vivo by PEGhydrogels.

  DISCUSSION

Our in vitro data show that PEG solutions can rapidly (within minutes) establish functional (Fig. 1A-E; Table 2) and morphological(Figs. 2A-F, 3A,E,F, 4A-C) continuity between the cut or crushedends of myelinated mammalian PNS and/or CNS axons. Our in vitroand in vivo data also show that PEG hydrogels adhere tightly (seeMaterials and Methods) and are nontoxic to intact earthworm MGAs(Figs. 1G, 3B; Table 3) and rat sciatic axons (Figs. 1I, 3E,F).Finally, our in vivo data show that PEG solutions combined withPEG hydrogels can rapidly and permanently repair severed earthwormmyelinated axons (MGAs) according to functional (Fig. 1H; Table3) and morphological (Fig. 3C,D) criteria. These data suggestthat PEG solutions, possibly combined with a PEG hydrogel, mightalso permanently reestablish functional and morphological continuityin vivo between the cut or crushed (severed) ends of myelinatedmammalian PNS and CNSaxons.

Possible mechanisms by which PEG solutions induce axonal fusion

We propose the following model to explain how PEG-induced fusion restores functional and morphological continuity betweenthe ends of cut or crushed axons. PEG is a polymeric fusiogenthat removes water from hydrophilic groups on the plasmalemmalsurface, thereby inducing closely apposed cell membranes to fuse(Sowers, 1987; Lee and Lentz, 1997). Ca²⁺-free salines containing EGTA prevent the cut ends of unmyelinated(Eddleman et al., 1997, 1998; Godell et al., 1997) and myelinated(Krause and Bittner, 1990; Krause et al., 1991, 1994; Ballingeret al., 1997) axons from sealing by preventing the formation ofCa²⁺-induced vesicles, which normally seal a somewhat constrictedcut end. That is, a much greater area can be more closely apposedbetween the interface of two open axonal ends than between theinterface of two constricted ends filled with a mass of vesicles.[Myelin membranes may also fuse with the axolemma. Slightly hypotonicsalines produce axoplasmic swellings that open cut and crushedaxonal ends and may facilitate PEG-induced fusion by allowingcloser apposition of crushed axonal ends within unsevered perineuralor epineural sheaths (Krause and Bittner, 1990; Krause et al.,1991).] However, even open ends of closely apposed axons are incompletelyfused by PEG, and those PEG-fused axons initially have many plasmalemmaldiscontinuities. When such axons are subsequently placed in aCa²⁺-containing physiological saline, Ca²⁺ inflow at the plasmalemmal discontinuities induces the formationof endocytotic vesicles and other membranous structures, which,in turn, seal those discontinuities (Krause et al., 1994; Ballingeret al., 1997; Eddleman et al., 1997, 1998). This repair of plasmalemmallesions takes from several seconds to an hour, depending on thesize and type of membrane lesion (Krause et al., 1994; Steinhardtet al., 1994; Ballinger et al., 1997; Eddleman et al., 1997, 1998).Calpain enhances the ability of cut axonal ends to constrict andseal (Xie and Barrett, 1991; Eddleman et al., 1997; Godell etal., 1997), thereby inhibiting PEG-fusion between severed ends.In contrast, leupeptin (an inhibitor of calpain) inhibits constrictionand sealing of severed axonal ends (Eddleman et al., 1997; Godellet al., 1997), thereby enhancing PEG-inducedfusion.

Agents other than PEG might also be used to induce the fusion of severed axonal ends in mammals. For example, closely apposedends of severed earthworm MGAs have been fused by laser beams(Yogev et al., 1991) and electric fields (Todorov et al., 1992).Similarly, agents other than our PEG-based hydrogel might be usedto add mechanical strength to the sheaths of axons repaired byPEGsolutions.

Possible clinical applicability of PEG solutions and PEG hydrogels

We have considered four problems that need to be resolved for successful implementation of our strategy to use PEG solutionsto rapidly and permanently reestablish the function of severedPNS or CNS axons in mammals in vivo.

First, the restoration of all original functions requires that, in a bundle of PNS or CNS axons, the cut nerve ends be perfectlyaligned and all axons successfully PEG-fused. This problem isobserved clinically in accidents that cut PNS axons, after whichthe amount and specificity of naturally occurring axonal regenerationis not high unless the ends of severed fascicles are carefullyaligned by microsurgery (Lundborg, 1990; Seckel, 1990). [Thisproblem is somewhat less severe for crush-type lesions to CNSor PNS axons because crushed ends often remain aligned (Blight,1989; Lundborg, 1990; Seckel, 1990).]

Second, PEG solutions do not induce axonal fusion unless the severed axonal ends are tightly apposed. Axonal ends usuallyseparate somewhat after cut lesions, and an obvious gap oftenoccurs between crushed axonal ends after many CNS (especiallyspinal) and some PNS contusion injuries (Blight, 1989).

Third, the mechanical strength at the lesion site is low when severed PNS or CNS axons are induced to fuse by PEG solutionsapplied in vitro or in vivo. PEG solutions do not reconnect severedconnective tissue elements (e.g., collagen) that provide mechanicalstrength to nervebundles.

Fourth, the distal stumps of severed mammalian axons usually degenerate within hours to a few days after severance (Ramony Cajal, 1928; Das and Wallace, 1986; Bittner, 1991). Withoutintervention to lengthen the survival times of severed distalaxonal processes, the time window for PEG-induced fusion wouldbe limited to several hours afterinjury.

We believe that each of these four problems can be at least partiallyresolved.

First, if the goal is partial restoration of function rather than complete recovery, then the survival or regeneration ofonly 10% of CNS axons in mammals produces significant behavioralrecovery (Eidelberg et al., 1977; Das and Wallace, 1986). Hence,the successful PEG-induced fusion of only 10% of axons in a CNSbundle whose ends are carefully (but not perfectly) aligned couldproduce rapid return of some functions that otherwise would neverbe restored. Furthermore, successful PEG-induced fusion of carefullyaligned PNS axons would restore function much more rapidly (withinminutes) compared with regeneration by growth cone outgrowth at1-2 mm/d. (We have observed that mammalian sciatic axons or earthwormMGAs that are not successfully PEG-fused are not prevented fromregenerating at 1-2 mm/day.)

Second, cut CNS or PNS nerve ends can be brought into close apposition by various surgical procedures (Das and Wallace, 1986).Furthermore, our current in vitro data from crushed rat sciaticaxons and our current and published (Krause and Bittner, 1990;Krause et al., 1991) in vitro data from crushed earthworm MGAsshow that the success rate for PEG-induced fusion of crushed myelinatedaxons is rather high when their axonal ends are opened and broughtinto close apposition in Ca²⁺-free, slightly hypotonic, salines containing 1-2 mMEGTA.

Third, our PEG hydrogel provides high mechanical strength at the lesion site and allows MGAs fused by PEG solutions to transmitAPs across the lesion site for many posttransection days in nonanesthetizedanimals. Because this hydrogel exhibits similar properties onmany invertebrate and mammalian soft tissues, it should providesufficient mechanical strength to nerve sheaths in vivo to allowPEG-fused PNS and CNS axons in mammals to remain fused once theanimal recovers fromanesthesia.

Fourth, the rapid Wallerian degeneration of mammalian myelinated axons can now be greatly retarded via procedures that arenot technically demanding. For example, we have recently shownthat in vivo cooling to 13°C (Sea et al., 1995) or injection ofcyclosporin A (Sunio and Bittner, 1997) allows the distal stumpsof many myelinated axons to survive for at least 6-10 d in rats,as does injection of antibodies to complement three receptors(Lunn et al., 1989).

In summary, we expect that our in vitro protocols to PEG fuse mammalian myelinated axons might be combined with our PEG hydrogeltechniques to greatly decrease the time in vivo required for returnof function after cut or crush lesions to PNS or CNS axons inmammals (including humans). These PEG-induced fusion techniquesmight also be combined with microsurgery, nerve growth guides(Jenq and Coggeshall, 1986; Aebischer et al., 1990; Herbert etal., 1996), or other strategies to increase the speed, amount,or specificity of regeneration of severed PNS axons in mammals.Our PEG-fusion techniques might also be combined with transplantsof peripheral nerve sheaths (David and Aguayo, 1981), embryonictissues (Giovanini et al., 1997; Miya et al., 1997), or injectionsof antibodies to oligodendritic inhibitors of CNS axonal outgrowth(Schnell and Schwab, 1990) to restore function to severed mammalianCNSaxons.

  FOOTNOTES

Received July 22, 1998; revised Jan. 11, 1999; accepted Jan. 14, 1999.

These studies were funded by National Institutes of Health Grants NS31256 and HD31484, a Texas Advanced Technology grant toG.D.B., personal funds of G.D.B., and National Science FoundationGrant BES-9696020 to J.A.H. We thank Dr. Riyi Shi (Center forParalysis Research, Purdue University, West Lafayette, IN) fordemonstrating the use of a three-chambered device for double sucrosegap recordings. We also thank Dr. Jennifer L. West for demonstratinghow to apply PEG-based hydrogeladhesives.
Correspondence should be addressed to Dr. George D. Bittner, Department of Zoology, University of Texas, Austin, TX 78712-1064.

  REFERENCES

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ABSTRACT
INTRODUCTION
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