Neonatal Partial Denervation Results in Nodal But Not Terminal Sprouting and a Decrease in Efficacy of Remaining Neuromuscular Junctions in Rat Soleus Muscle

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The Journal of Neuroscience, October 15, 1999, 19(20):8931-8944

Neonatal Partial Denervation Results in Nodal But Not Terminal Sprouting and a Decrease in Efficacy of Remaining Neuromuscular Junctions in Rat Soleus Muscle
Jane L. Lubischer and Wesley J. Thompson
Section of Neurobiology, School of Biological Sciences, Institute for Neuroscience and Institute for Cellular and Molecular Biology, University of Texas, Austin, Texas 78712

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mature motoneurons respond to partial denervation of their target muscle by sprouting to reinnervate denervated fibers, thusmaintaining muscle strength in the face of motoneuronal loss causedby injury or disease. Neonatal motoneurons, however, do not expandto innervate more muscle fibers. The present work seeks to understandthis developmental change in motoneuron response to partial denervation.It has been suggested that neonatal motor units cannot increasein size because they are already at their maximum size (approximatelyfive times larger than in adulthood). We ruled out this explanationby showing that after partial denervation on postnatal day 14(P14), when motor units have decreased to their adult size, motoneuronsstill did not sprout to reinnervate as many fibers as in adulthood.Instead, we found evidence supporting an alternative explanationinvolving terminal Schwann cells. After partial denervation ofneonatal (but not adult) muscles, terminal Schwann cells at denervatedendplates undergo apoptosis. We found that terminal (but not nodal)sprouting was absent in partially denervated neonatal muscles.This finding suggests that terminal Schwann cells, previouslyreported to guide terminal sprouts to denervated endplates inadult muscles, are necessary for the formation and growth of terminalsprouts. Moreover, partial denervation on P14 severely weakenedthe remaining, uninjured synapses, suggesting that neonatal motoneuronsmay withdraw terminals after the denervation of nearby fibers.These findings have implications for the interpretation of previousstudies on synapse elimination and offer insight into the failureof young motor units to expand after partialdenervation.

Key words: Schwann cells; synapse elimination; NMJ; synaptic strength; development; motoneuron; curare

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The ability of motoneurons to compensate for nerve injury is poor in early postnatal development. After partial denervationof adult muscle, the remaining motoneurons extend sprouts, someof which reinnervate denervated fibers (Hoffman, 1950). This resultsin an expansion of fourfold to fivefold in the number of fibersinnervated by each motoneuron (i.e., an increase in motor unitsize; Thompson and Jansen, 1977; Brown and Ironton, 1978; Gordonet al., 1993). Through this process, muscle strength can be maintainedeven after substantial loss of motoneurons due to injury or disease.In contrast, partial denervation within 7 d of birth results inlittle or no increase in motor unit size (Brown et al., 1976;Thompson and Jansen, 1977; Betz et al., 1980; Fisher et al., 1989).At this time in development, motoneurons have an expanded terminalarbor, and multiple motoneurons innervate each muscle fiber. Duringthe first 2 weeks after birth, synapse elimination removes allbut one synaptic input onto each fiber, and each motor unit becomessmaller (Redfern, 1970; Brown et al., 1976; Jansen and Fladby,1990). Partial denervations shortly after birth were originallyperformed to look for evidence of competition between terminalsduring synapse elimination (Brown et al., 1976; Thompson and Jansen,1977; Betz et al., 1980). The few remaining motoneurons undergolittle or no reduction in unit size in the absence of potentialcompetition. Based on these experiments, it was concluded thatcompetition among motoneurons drives the reduction in motor unitsize during postnatal synapseelimination.

Left unexplained was why neonatal motoneurons do not expand and innervate denervated fibers. One explanation offered was thatthe units were already expanded beyond their adult size and couldnot maintain any more terminals (e.g., Brown et al., 1976; Thompsonand Jansen, 1977). Recent experiments have suggested another possibility.After partial denervation of adult muscle, most (~70%) of theterminal sprouts that innervate denervated fibers grow along processesextended by Schwann cells present at denervated endplates (Sonand Thompson, 1995b). In neonatal muscles, however, terminal Schwanncells quickly die by apoptosis after muscle denervation (Trachtenbergand Thompson, 1996). Thus, these Schwann cells would be unavailableto provide a stimulus or guide for terminal sprouts after neonatalpartialdenervation.

We now report that the inability of young motor units to expand after partial denervation cannot be explained by their alreadyenlarged size but may be related to terminal Schwann cell death.We found that neonatal motoneurons, unlike mature motoneurons,do not extend terminal sprouts after partial denervation. Thereis, however, nodal sprouting in the intramuscular nerves of younganimals, where Schwann cells remain viable. These observationsprovide further evidence for the importance of Schwann cells inthe motoneuronal sprouting response. Finally, we present evidencethat neonatal partial denervation leads to severe morphologicaland physiological disruption of existing motoneuron terminals,a finding that influences the interpretation of previous studiesof partial denervation during developmental synapseelimination.

Portions of this work have been reported previously in abstract form (Lubischer and Thompson, 1997).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

All experiments used rats bred and raised in the Animal Resources Center at the University of Texas at Austin. Surgical procedureswere performed on animals anesthetized with ether. Rats of theAO strain were used because these animals often have a secondnerve supplying the soleus muscle in addition to the soleus nerve.This "aberrant" nerve, derived from the plantar branch of thetibial nerve, is encountered in >50% of soleus muscles in theAO strain but is seen only infrequently in other strains of rats(Thompson and Jansen, 1977). Motor units in the aberrant nervedo not differ from motor units in the soleus nerve in their physiologicalproperties, and soleus muscles in rats with an aberrant nerveare innervated by the same number of motor units as in rats withno aberrant nerve (Thompson and Jansen, 1977). Muscle fibers innervatedby axons in the two nerves intermingle throughout the muscle.Partial denervation of the soleus muscle in AO rats is easilyaccomplished by resection of the lateral gastrocnemius-soleus(LG-S) nerve, leaving the aberrant nerve intact. Resection ofthe LG-S nerve poses no danger of inadvertent injury to eitherthe aberrant nerve or the soleusmuscle.

Surgical procedures
Partial denervation. LG-S nerve resection was performed unilaterally in AO rats on postnatal day 14 (P14) or between postnataldays 25 and 30 (P25-30). By P14, motor units have reached theiradult size (Brown et al., 1976). At P25-30, neuromuscular synapsesare more fully mature, yet soleus muscles are not too large toprevent in vitro studies of synaptic function. The response ofterminal Schwann cells to denervation differs dramatically betweenthese two ages, with extensive terminal Schwann cell death afterdenervation on P14 but not P25-30 (Trachtenberg and Thompson,1996). After exposure of the LG-S nerve in the popliteal fossaat the lateral head of the gastrocnemius muscle, a 3-5 mm segmentof nerve was removed. The incision was closed using 6-0 silk suture.Survival time after partial denervation ranged from 1-3 d (formorphological and physiological assessment of remaining motorterminals) to 2-3 months (for physiological determination of motorunit size). For long survival times, the proximal nerve stumpwas ligated with 6-0 surgical silk to prevent reinnervation byaxons in the LG-Snerve.
Muscle removal. After the specified survival time, partially denervated soleus muscles and their nerves, including the sciaticnerve, were dissected into oxygenated Ringer's solution (in mM:137 NaCl, 4 KCl, 1 MgCl₂ · 6H₂O, 1 KH₂PO₄, 12 NaHCO₃, 2 CaCl₂· 2H₂O, 11 D-glucose; Liley, 1956). Muscles not innervated byan aberrant nerve (and therefore fully denervated by the LG-Snerve resection) were discarded. For experiments in which individualmotor units were isolated, the nerve supply was dissected to includethe L4 and L5 ventral roots, which contain the axons of all soleusmotoneurons (Close, 1967). The contralateral, normally innervatedsoleus muscle from each animal was used as an internal controlin experiments involving short survivaltimes.

Physiology
Soleus muscles and nerves were continuously superfused in a bath of oxygenated Ringer's solution at room temperature. Eachmuscle was anchored to a Sylgard-coated dish by an insect pinthrough its proximal tendon and the head of the fibula. The distaltendon was attached to a force transducer (Harvard Apparatus,Holliston, MA; 60-2996; 40 mV/gm; range, 0-50 gm; or CambridgeTechnology, Cambridge, MA; 400A; 80 mV/gm; range, 0-25 gm) forisometric tension measurements. Nerves were stimulated electricallythrough suction electrodes, or muscles were stimulated directlyby current passed between two platinum plates positioned on eitherside of the muscle. At the beginning of each experiment, electricalstimulation of the soleus nerve distal to the resection site verifiedthat no axons had regenerated to the muscle. After determiningthe muscle length at which maximum twitch tension was evoked bysupramaximal stimulation of the nerve with pulses 0.2 msec induration, motor unit number was estimated by counting incrementsin twitch tension upon graded stimulation of the nerve. In someexperiments, individual motor units were isolated by teasing theventral roots into fine filaments until stimulation of a nervefilament resulted in an all-or-nothing twitch of constant amplitude(Close, 1967; Brown et al., 1976; Brown and Ironton, 1978). Datawere collected and analyzed using a MacLab analog-to-digital converterand Macintoshcomputer.
Motor unit expansion. To determine the extent of motor unit expansion after partial denervation on P14, motor unit numberand muscle fiber number were counted 2-3 months after resectionand ligation of the LG-S nerve, sufficient time for the remainingsoleus motor units to fully expand (Thompson and Jansen, 1977).Lack of reinnervation through the soleus nerve was verified, thenmotor unit number and relative sizes were estimated by gradedstimulation of the aberrant nerve. To avoid constraints on motorunit expansion (Thompson and Jansen, 1977), muscles innervatedby more than six units were excluded: if too many motor unitswere present, there would be a ceiling on the number of musclefibers each could innervate, simply because of the limited numberof muscle fibers. Motor unit number also was estimated in normalsoleus muscles innervated through both soleus and aberrant nerves.Muscles were frozen in isopentane (2-methylbutane) cooled to $-$ 60°Cwith liquid nitrogen and sectioned in a cryostat at the levelof the endplate band (verified by $alpha$ -bungarotoxin staining), alevel containing profiles of all fibers in the muscle (Close,1964). Muscle cross-sections 10 µm thick were stained for myosinATPase activity after an alkaline preincubation (modified fromGuth and Samaha, 1970). Stained sections were rinsed in distilledH₂O, dehydrated, cleared, and coverslipped in Permount. Musclefibers were counted, and motor unit size was calculated basedon the percentage of total twitch tension each unit produced.For example, if stimulation of a motor unit produced 25% of thetotal force produced by a muscle, it was assumed to innervate25% of the muscle fibers. Motor units and muscle fibers were countedin eight muscles partially denervated on P14 and in four normalsoleus muscles taken from animals not subjected to any previoussurgery.
Intracellular physiology. Three days after partial denervation on P14, intracellular recordings were made from muscle fibersin the endplate band using glass microelectrodes filled with 3M potassium acetate (50-100 M $Omega$ resistance), and a high input impedancemicroelectrode amplifier (WPI KS-700). The nerve was stimulatedat 100 Hz for 220 msec, and synaptic potentials were recorded.Because muscle contractions were weak (see Results), impalementscould usually be maintained without any pharmacological manipulationto prevent muscle contractions, and intracellular recordings thereforewere made in normal Ringer'ssolution.
Synaptic safety factor. The neuromuscular junction normally has a high safety factor; i.e., much more neurotransmitter isreleased and binds to acetylcholine receptors (AChRs) than isnecessary to bring the postsynaptic muscle fiber to threshold.This is evidenced by the fact that 80-90% of AChRs must be blockedbefore evoked contraction is prevented (Lingle and Steinbach,1988). Two approaches were used to assess synaptic safety factorin muscles partially denervated for 3 d. In the first set of experiments,the AChR antagonist curare was bath-applied at steps of increasingconcentrations (ranging from 1 × 10⁷ to 6.5 × 10⁷ gm/ml). Twitch tension stabilized within 30 min of curare application,at which time the nerve was stimulated and twitch tension wasrecorded as an average of 3 trials separated by about 30 sec.In this manner, we determined the concentration of curare (towithin 0.5 × 10⁷ gm/ml) necessary to completely block evoked muscle contraction(n = 5 at P14; n = 6 at P25-30). Synaptic safety factor also wastested with curare in an additional group of soleus muscles fromnormal (i.e., no surgery) P17 and P26-29 animals (n = 3 at eachage). For each of these experiments, a P17 muscle was paired withan older muscle in the same bath. In a second set of experimentsdesigned to assess synaptic safety factor after partial denervation,calcium concentration in the bath was decreased in the followingsteps: 2 (normal), 1.6, 1.2, 0.8, and 0.4 mM (Jordan et al., 1992).Lowering extracellular calcium levels reduces the driving forceon calcium, resulting in less calcium influx and therefore lessneurotransmitter release in response to each action potential.Evoked twitch tension was recorded as an average of three trialsafter 30 min at each concentration (n = 4 at each age). Experimentswere conducted simultaneously on a partially denervated soleusmuscle and its contralateral control in the same bath so thatboth were exposed to exactly the same concentration of curareor calcium. At the end of each experiment, muscles were processedfor immunohistochemical labeling of neuromuscular junctions asdescribedbelow.

Morphology of the neuromuscular junction
Terminal morphology and sprouting. Muscles were fixed in 4% buffered paraformaldehyde (10-30 min), permeabilized in absoluteMeOH cooled to $-$ 20°C (5-10 min), blocked for 30 min (0.3% TritonX-100, 0.2% BSA, 0.1% sodium azide in PBS), and incubated overnightin the primary antibodies of interest, diluted in blocker. Thefollowing primary antibodies were used: a polyclonal antibodyto S100 to visualize Schwann cells (1:400; Dako, Glostrup, Denmark;Z0311), a monoclonal antibody to neurofilament (2H3) to visualizeaxons (1:200; Developmental Studies Hybridoma Bank, Universityof Iowa, Department of Biological Sciences, Iowa City, IA), amonoclonal antibody to synaptophysin (1:400; Sigma, St. Louis,MO; S5768) or the synaptic vesicle protein SV2 (1:400; DevelopmentalStudies Hybridoma Bank) to visualize nerve terminals, a monoclonalantibody to protein zero (P07) to visualize myelin sheaths (1:200;courtesy of Dr. J. J. Archelos, University of Wurzburg, Wurzburg,Germany), and a monoclonal antibody (G3G4) to 5-bromo-2'-deoxyuridine(BrdU) to visualize mitotically active cells (1:5; DevelopmentalStudies Hybridoma Bank). When the protein zero antibody was used,paraformaldehyde fixation was omitted; when G3G4 was used, muscleswere incubated in 2N HCl and 0.3% Triton for 30 min before blocking.Primary antibodies were visualized with the following fluorochrome-conjugatedsecondary antibodies: fluorescein isothiocyanate-conjugated sheepanti-mouse (1:100; Sigma; F2266) and tetramethylrhodamine isothiocyanate-conjugatedgoat anti-rabbit (1:400; Cappel, West Chester, PA; 55671) or Cy5-conjugatedgoat anti-rabbit (1:100; Jackson ImmunoResearch, West Grove, PA).AChRs were visualized using rhodamine- or Cy5-conjugated $alpha$ -bungarotoxin.After staining, a thin layer of muscle fibers was dissected offeach side of the muscle and mounted in fluorescence mounting medium(0.1 M ethanolamine, 0.01 M p-phenylenediamine in 90% glycerol,pH 9.5; modified from Johnson and Nogueira Araujo, 1981). Analyseswere conducted using a 63×, 1.32 numerical aperture (NA) or a100×, 1.30 NA objective, an integrated, cooled CCD camera (CarlZeiss, Thornwood, NY), and NIH Image software (available on theInternet at nih.gov).
Hoffman (1950) described two types of motoneuronal sprouts: those that originate from the terminal (terminal sprouts) andthose that originate from nodes of Ranvier (nodal sprouts). Inthe present study, terminal sprouts were defined as nerve processesextending from a terminal beyond the boundary of AChR label, aliberal definition that included even the shortest of sprouts(as short as 1 µm). Nodal sprouts were identified as thin axonalbranches that reached a synaptic site (i.e., an AChR plaque) butdid not originate from a terminal branch. These nodal sproutswere associated with Schwann cell processes and may have reachedthe denervated site by growing along the endoneurial tube thatremained after axonal degeneration or by following new Schwanncell processes extending from the intramuscular nerve. Each endplatewas first categorized as being (1) innervated by an axon ("axon-derived"),(2) fully denervated (i.e., not contacted by a neuronal processof any sort), (3) denervated but contacted by a terminal sprout,or (4) denervated but contacted by a nodal sprout. Axon-derivedterminals were further divided based on whether they had extendedterminalsprouts.
Schwann cell mitosis. To determine whether partial denervation on P14 caused mitotic activity in terminal Schwann cells, cellsactively synthesizing DNA were labeled with BrdU (Calbiochem,La Jolla, CA; 203806). Soleus muscles (n = 3) were partially denervatedon P14, and animals were given intraperitoneal BrdU injections(0.1 mg/gm body weight, dissolved in 0.9% NaCl containing 0.007NNaOH; Love and Thompson, 1998) twice daily for 3 d (P15-17). Thirtyminutes after a final BrdU injection on P18 (4 d after partialdenervation), muscles were removed and processed for immunohistochemicallabeling using antibodies to BrdU, neurofilament, and S100 (seeabove).

Statistical analyses
Statistical analyses were performed using StatView (SAS Institute Inc., Cary, NC), typically as two-way ANOVAs, with age asa between-group factor (P14 vs P25-30) and partial denervationas a within-group factor (partially denervated muscle vs contralateralcontrol muscle). Significant two-way interactions were followedby hypothesis-driven post hoc comparisons using Fisher's PLSD.Data are presented as mean ±SEM.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Partial denervation of adult muscle results in an expansion of approximately fourfold to fivefold in motor unit size (Thompsonand Jansen, 1977; Brown and Ironton, 1978). Such an expansiondoes not occur after partial denervation shortly after birth (Brownet al., 1976; Thompson and Jansen, 1977; Betz et al., 1980), whenmotoneurons have not completed synapse elimination and thereforealready have an enlarged terminal arbor. By P14, synapse eliminationis essentially complete, and each motoneuron innervates the samenumber of muscle fibers as in adulthood (Brown et al., 1976).In addition, after complete denervation of muscles at this age,most terminal Schwann cells die (Trachtenberg and Thompson, 1996).Because these cells appear to play a critical role in inducingand guiding terminal sprouts to reinnervate denervated sites afterpartial denervation of mature muscles (Son and Thompson, 1995b),we were interested in the behavior of motor terminals after partialdenervation at an age at which terminal Schwann cells at denervatedsites die. Finally, previous studies of motor unit expansion afterpartial denervation considered only relatively long survival times(weeks to months), and there is a dearth of information aboutthe anatomy and physiology of nerve terminals in the time shortlyafter partial denervation. We therefore examined morphologicaland functional characteristics of the neuromuscular junction shortlyafter partialdenervation.

P14 motoneurons show only limited increases in motor unit size after partial denervation

The soleus muscle was partially denervated on P14, and 2-3 months later motor units and muscle fibers were counted to estimatemotor unit size. Normal adult soleus muscles (n = 4) contained3365 ± 115 fibers and were innervated by 31 ± 0.7 motoneurons.Thus, each soleus motoneuron would be expected to innervate 109fibers, on average. These numbers are consistent with previousestimates (Close, 1967; Brown et al., 1976; Kugelberg, 1976; Thompsonand Jansen, 1977). Partial denervation on P14 resulted in motorunits that were larger than those seen after partial denervationearlier in development, on P1-5 (Fig. 1). However, after partialdenervation on P14, motor unit expansion was less than that seenafter partial denervation in adulthood. The mean size of 39 motorunits in eight muscles partially denervated on P14 was 355 fibers,compared with 524 fibers in muscles partially denervated in adulthood(Thompson and Jansen, 1977). Some units in muscles partially denervatedin adulthood were larger than any seen after partial denervationat younger ages (Fig. 1, Adult, dark bars), and some units inmuscles partially denervated on P14 were smaller than any foundafter partial denervation in adulthood (Fig. 1, P14, dark bars).Thus, even though motor units had achieved their adult size byP14, they still were deficient in expanding to reinnervate denervatedfibers.

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Figure 1. Motor unit expansion is impaired after partial denervation on P14, at the end of synapse elimination. Soleus muscles were partially denervated at the indicated age, and motor unit size was determined 2-3 months later (see Materials and Methods). After partial denervation in adulthood (bottom), motor units expand from their normal size of 100-150 fibers to an average of 524 fibers. After partial denervation on P1-5 (top), average motor unit size is only 227 fibers. Normal motor units at P1-5 are ~700 fibers large; therefore some developmental synapse elimination appears to continue even after partial denervation at this age. After partial denervation on P14 (middle), motor units expanded to an average of 355 fibers (dotted line), smaller than in adult muscles. After partial denervation on P14, some units (middle, dark bars) were smaller than any seen after partial denervation in adulthood, whereas after partial denervation in adulthood, some units (bottom, dark bars) are larger than any seen after partial denervation in development. Data on partial denervations on P1-5 and in adults were taken from Thompson and Jansen (1977).

P14 motoneurons extend nodal sprouts but not terminal sprouts in response to partial denervation

As a first step toward understanding why young motoneurons do not expand to the same extent as their adult counterparts afterpartial denervation, we looked for evidence of the initial sproutingresponse 3 d after partial denervation. Partial denervation ofP25-30 muscles resulted in terminal sprouting by almost all terminals3 d later (Fig. 2A,B), but in muscles partially denervated onP14 there was no increase in the percentage of terminals withsprouts compared with normally innervated, contralateral controls(Fig. 2C). The mean number of sprouts per terminal was also higherin muscles partially denervated on P25-30 than in any other group(Fig. 2D). The only effect of P14 partial denervation on terminalsprouts was an increase in sprout length compared with contralateralcontrols, and terminal sprouts were even longer in muscles partiallydenervated on P25-30 (Fig. 2E). Importantly, denervated endplateswere more likely to be contacted by terminal sprouts in oldermuscles than in muscles partially denervated on P14 (Fig. 3A-C).Three days after partial denervation on P25-30, 6.1% of endplateshad been contacted by a terminal sprout. This is consistent withthe finding of Son and Thompson (1995b) that 3 d after partialdenervation, reactive Schwann cell processes at ~7% of denervatedendplates had made contact with adjacent, innervated endplates.Differences in terminal sprouting were not attributable to differencesin the extent of denervation: there were 5.8 ± 0.84 motor unitsstill innervating the partially denervated P14 muscles and 6.1± 0.86 units still innervating the partially denervated P25-30muscles (p > 0.70). In addition, Brown and colleagues (1980) foundno relationship between the amount of nodal or terminal sproutingby soleus motoneurons and the extent of partial denervation.

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Figure 2. Terminal sprouting is robust in more mature muscles (P25-30) but deficient in younger muscles (P14) 3 d after partial denervation (PD). A, B, Confocal photomicrographs of an endplate 3 d after partial denervation on P35. Nerve processes (A) were labeled with antibodies to neurofilament and synaptophysin, and AChRs (B) were labeled with $alpha$ -bungarotoxin. Terminal sprouts can be seen extending well beyond the AChR plaque. C, The percentage of terminals with sprouts is much higher in muscles partially denervated on P25-30 than in younger muscles or in contralateral control muscles (contra). Two-way interaction, p < 0.0001; n = 8 at P14; n = 7 at P25-30. D, The mean number of terminal sprouts per endplate (excluding endplates with no sprouts) is higher in mature muscles than in neonatal muscles or contralateral controls. Two-way interaction, p < 0.01; n = 5 at P14; n = 4 at P25-30. E, Terminal sprouts are longer in partially denervated muscles than in contralateral controls and longer in older muscles than in immature muscles after partial denervation. Two-way interaction, p < 0.05; n = 5 at P14; n = 4 at P25-30.

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Figure 3. Terminal sprouts are less likely to contact denervated endplates in muscles partially denervated on P14 than in muscles partially denervated on P25-30. A, The percentage of denervated endplates contacted by terminal sprouts was determined 3 d after partial denervation by labeling nerve terminals, axons, and AChRs for fluorescence microscopy. One-way ANOVA, p < 0.01; n = 8 at P14; n = 7 at P25-30. B-E, Confocal photomicrographs of a terminal sprout (B, C) and a nodal sprout (D, E) in contact with denervated endplates. Nerve processes (B, D) were labeled with antibodies to neurofilament and synaptophysin, and AChRs (C, E) were labeled with $alpha$ -bungarotoxin. In both examples, the denervated endplate site is outlined, and an arrow shows where the sprout branches from a terminal (B) or from an axon (D). These photomicrographs were taken 3 d after partial denervation on P30 (B, C) or P14 (D, E). At this time, there is little arborization by sprouts in contact with denervated endplates. Scale bars, 10 µm.

In contrast to terminal sprouting, nodal sprouting by immature motoneurons did not appear to be impaired (Fig. 3D,E). Althoughdifficult to quantify, there looked to be extensive growth ofnodal sprouts in muscles partially denervated on P14. One indicationof such growth was our finding in one muscle of sprouts that hadstarted to grow back up the distal stump of the soleus nerve,as has been described previously (Thompson, 1978). We did not,however, look for this in a systematic manner. Based on the percentageof endplates contacted by nodal sprouts, nodal sprouting afterpartial denervation was apparently more robust in younger muscles(16.9 ± 4.02%) than in more mature muscles (6.1 ± 1.47%; p < 0.05).It is important to note, however, that axons in the process ofwithdrawing from contact with the muscle fiber might have a morphology(Gan and Lichtman, 1998) similar to those defined herein as nodalsprouts. In normal P14 muscles labeled with our immunohistochemicaltechnique (n = 4), 10.6 ± 1.59% of endplates were still contactedboth by an axon and by a second, fine process, not yet withdrawn.If these were maintained in partially denervated muscles, thenthe actual percentage of endplates contacted by nodal sproutswould be lower than 16.9%, closer to that seen in older musclesafter partial denervation. Although we may, therefore, have overestimatedthe extent of nodal sprouting in neonatal muscles, there is noevidence for an impairment of nodal sprouting after partial denervationon P14 relative to that seen after partial denervation on P25-30.

Schwann cells react to partial denervation in an age-dependent manner

Terminal Schwann cells die after full denervation of neonatal muscles (Trachtenberg and Thompson, 1996). To determine whetherSchwann cell death also results from partial denervation, we labeledSchwann cells either 1 or 3 d after partial denervation on P14with an antibody to S100, in combination with fluorescent labelingof nerve processes and AChRs. Partial denervation on P14 resultedin an extensive loss of Schwann cells at denervated but not innervatedendplates. One day after partial denervation on P14 (n = 2 muscles),many denervated endplates were found to have cells with S100-positivecytoplasm condensed around an S100-negative nucleus and/or werefragmented into small, S100-positive pieces, features characteristicof apoptosis in these cells (Trachtenberg and Thompson, 1996).Apoptotic Schwann cells were not seen over innervated endplates.Three days after partial denervation on P14 (n = 5 muscles), most(67.5 ± 8.68%) denervated endplates were completely devoid ofSchwann cell coverage. Of the denervated endplates that stillhad Schwann cells present, almost all (44 of 45) were only partiallycovered by Schwann cells and their processes. The Schwann cellsthat remained at denervated sites extended processes away fromthe endplate in only 42% of cases. In contrast, in muscles partiallydenervated on P25-30 (n = 4), <1% were completely devoid of Schwanncells 3 d after partial denervation, and 75% were fully coveredby Schwann cells and their processes. In these older muscles,Schwann cells at denervated sites extended processes away fromthe endplate in 91% of cases. Thus, after partial denervationon P14, most denervated endplates had lost all of their terminalSchwann cells; the rest appeared to have lost a portion of theirSchwann cells, and the Schwann cells that remained were less likelyto extend processes than their counterparts in more maturemuscles.

Consistent with previous work (Son and Thompson, 1995a,b), Schwann cell processes accompanied almost all terminal and nodalsprouts. Although we did see instances (~10%) of terminal sproutsin which Schwann cell coverage did not extend fully to the tipof the sprout, these were extremely subtle and were independentof partial denervation and of the age of the animal. Such casesmay not have been seen by Son and Thompson (1995a,b) because theystained nerve processes with antibodies only to neurofilamentand not to synaptophysin. We also observed a few examples of nodalsprouts that were not fully covered by Schwann cells 3 d afterpartial denervation on P14 but not after partial denervation onP25-30 (Fig. 4). These sprouts usually had a punctate appearance,morphology not typical of nodal sprouts. Although these data arebased on static images and consist of only a few observations,it is tempting to speculate that these cases of varicose sproutsnot fully covered by Schwann cells, as well as the terminal sproutsnot fully covered, represent dynamic interrelationships betweenSchwann cell and nerve process extension and retraction. Sucha dynamic relationship is suggested for terminal sprouts by preliminaryobservations that many of the short sprouts present 3 d afterpartial denervation have disappeared a few days later (F. M. Loveand W. J. Thompson, unpublished observations).

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Figure 4. In muscles partially denervated on P14, nodal sprouts were occasionally found that were not fully covered by Schwann cell processes. Three days after partial denervation on P14, this muscle was processed immunohistochemically with antibodies to neurofilament, synaptophysin, and SV2 to label nerve processes (top panel) and antibodies to S100 to label Schwann cells (bottom panel). In this photomontage, a nodal sprout enters the field of view from the left and branches several times. Arrows indicate the distal end of one branch of this sprout that is not accompanied by a Schwann cell process. Note the spotty appearance of this branch of the sprout. No endplate was seen in the vicinity of this branch (data not shown).

After partial denervation of soleus muscles at 5 weeks of age, Love and Thompson (1998) found BrdU-positive Schwann cellsat 27% of innervated endplates. In these muscles, BrdU-positiveSchwann cells are most common at innervated endplates that havebeen contacted by reactive Schwann cell processes from nearbydenervated sites. Following the same protocol, we found BrdU-positiveSchwann cells at only 7.1 ± 0.60% of innervated endplate sitesafter partial denervation on P14 (10 of 150 endplates in threemuscles). Thus, after partial denervation on P14, in the absenceof Schwann cell processes from denervated endplates, Schwann cellsat innervated endplates are less likely to become mitotic. Thisis consistent with the idea that Schwann cell processes growingfrom denervated endplates play a role in inducing Schwann cellmitosis at innervatedendplates.

Motor units produce less tension shortly after partial denervation on P14

Schwann cells made reactive by denervation or (in neonates) by application of glial growth factor can alter synaptic morphologyand function (Trachtenberg and Thompson, 1997). We therefore lookedfor evidence of functional synaptic changes after partial denervationby studying the ability of the nerve to evoke muscle contraction.Soleus muscles were partially denervated on P14 or P25-30, and3 d later the muscle tension evoked by stimulation of the sciaticnerve was recorded. Repetitive stimulation revealed an inabilityof muscles partially denervated on P14 to maintain tension throughout1500 msec of stimulation (Fig. 5A), even at a stimulation frequencyas low as 2 Hz. The fifth stimulus delivered at 2 Hz produced75.6 ± 3.85% as much tension as the first stimulus, whereas inmuscles partially denervated on P25-30, the fifth stimulus produced93.9 ± 1.00% as much tension as the first. When muscles partiallydenervated on P14 were stimulated by direct activation of themuscle fibers at 100 Hz for 1500 msec, there was no decline intension (i.e., fade). These observations suggest a deficiencyin synaptic transmission rather than in the ability of the muscleto generate or maintain tension.

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Figure 5. Muscles partially denervated on P14 do not maintain tension during high-frequency nerve stimulation. A, Control muscles (contra) and muscles partially denervated (PD) on P25-30 maintained 95-100% tension during the 1500 msec of nerve stimulation at 100 Hz, whereas tension produced by muscles partially denervated on P14 dropped by almost half. Two-way interaction, p < 0.0001; n = 9 at P14; n = 10 at P25-30. B, This fade during high-frequency stimulation was independent of the number of units still innervating the muscle within the range of units considered (3-13): P14, r² = 0.023, p = 0.70; P25-30, r² = 0.285, p = 0.11.

Differences between young and older muscles could not be accounted for by differences in the extent of partial denervation.In these experiments, partially denervated P14 muscles were innervatedby 6.4 ± 0.71 (range, 3-9) motor units, and partially denervatedP25-30 muscles were innervated by 8.3 ± 0.90 (range, 5-13) units(p > 0.1). Within this range of motor unit number, there was noclear relationship between the number of units innervating a partiallydenervated muscle and the severity of the effects (Fig. 5B) eitherat P14 (r² = 0.023; p = 0.70) or at P25-30 (r² = 0.285; p = 0.11).

We confirmed these deficits in synaptic transmission by examining single motor units. Soleus muscles partially denervatedon P14 (n = 4 animals) were dissected 2-3 d later with their contralateralcontrol muscles so that motor units could be isolated from theventral roots and stimulated individually (3-11 units sampledper muscle). Partially denervated muscles in this group remainedinnervated by three to seven motor units. The amplitude of thetwitches evoked by stimulating these units tended to be smallerthan those evoked in contralateral control muscles, although thisdid not reach statistical significance (Table 1). However, themaximum tetanic forces produced by single motor units were, onaverage, less than half the size of those in the contralateralcontrol muscle (p < 0.05; Table 1, Fig. 6A). Moreover, as wasseen after whole nerve stimulation, isolated units in musclespartially denervated on P14 failed to maintain peak tension throughouta 1500 msec train of stimuli at frequencies from 10 to 100 Hz(Fig. 6B). On average, tension at the end of 1500 msec of 100Hz stimulation of a motor unit was less than half of the peaktension (Table 1). Units from contralateral control muscles showedno such drop (Table 1). As evidenced by decreased tetanic tensionand the failure to maintain tension during repetitive stimulation,partial denervation on P14 lessened the ability of the remainingmotoneurons to evoke contraction in muscle fibers they innervatedat the time of partial denervation.


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Table 1. Motor unit tension 3 d after partial denervation (PD) on P14

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Figure 6. Motor units produce less tension 3 d after partial denervation on P14. A, Frequency-tension curves for motor units isolated from muscles partially denervated 3 d earlier on P14 (filled circles) and contralateral controls (open circles). Motor unit twitch tension (2 Hz stimulation) is slightly lower in experimental muscles. Stimulation of motor units at higher frequencies reveals a more dramatic decrease in the ability to generate tension after partial denervation (n = 4 animals). B, Stimulation at 100 Hz for 1500 msec of a motor unit from a muscle partially denervated on P14 (PD P14) and its contralateral control muscle (contra). Stimulation of the unit in the partially denervated muscle produced less tension, and maximum tension was not maintained for the duration of the stimulus. The arrow indicates stimulus onset. The dashed lines mark 220 and 600 msec after stimulus onset, intervals during which intracellular recording was used to examine branch point failure (see Results).

Branch point failure cannot account for the decreased tetanic tension or the fade seen during repetitive stimulation after partial denervation on P14

Extensive nodal sprouting might result in the failure of action potential conduction at axonal branch points, particularlyduring repetitive stimulation (Krnjevic and Miledi, 1957). Ifthis were occurring, one would expect to see a frequency-dependentincrease in failures to evoke an excitatory junctional potential(EJP) by nerve stimulation. We tested this by recording intracellularlyin muscle fibers during 100 Hz stimulation of the nerve for 220msec. Consistent with other evidence of weakened synapses, muscleresponses to nerve stimulation 3 d after partial denervation onP14 were usually weak enough that electrode impalements couldbe maintained without any pharmacological manipulation to preventmuscle contraction. A total of 58 innervated muscle fibers weresampled in three muscles partially denervated 3 d earlier on P14(13-26 fibers per muscle). Each muscle was innervated by two tosix motoneurons. After 220 msec of 100 Hz stimulation (Fig. 6B,dashed line on left), units in contralateral muscles produced0.42 ± 0.037 gm force and had not yet reached peak tension. Incontrast, units in muscles partially denervated on P14 producedonly 0.15 ± 0.046 gm force and were already losing tension. Despitethis dramatic inability to produce tension, only 14% (8 of 58)of innervated fibers exhibited failures during 100 Hz nerve stimulation,and half of these exhibited only one failure during the trainof 20 stimuli. If the stimulation was extended to 600 msec (Fig.6B, dashed line on right), failures were seen in only 18% (5 of28) of innervated fibers. Whether stimulation lasted for 220 or600 msec, <2% of the stimuli resulted in failures. Although failureswere rare, EJPs were often subthreshold, consistent with weakenedsynaptic transmission relative to normal muscles. In addition,there was usually (72% of fibers) a decrease in EJP amplitudeduring the 220 msec train of stimuli (Fig. 7). This synaptic depressionis consistent with a general depression of synaptic transmission,rather than intermittent failure of action potential conduction.

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Figure 7. Conduction failure does not account for muscle tension deficits 3 d after partial denervation on P14. This intracellular muscle fiber recording was made in a muscle that had been partially denervated 3 d earlier on P14. EJPs were evoked by 100 Hz nerve stimulation. No failures to evoke an EJP were seen in this fiber, but EJPs were subthreshold, and their amplitude decreased during the 220 msec stimulation.

Synaptic safety factor is reduced 3 d after partial denervation on P14

Our findings thus suggested a weakening of remaining synapses 3 d after partial denervation on P14. Although not examinedin detail, other reports have hinted that such changes might occurafter partial denervation in neonates (Brown et al., 1976; Gatesand Ridge, 1992) as well as in adults (Thompson and Jansen, 1977;Slack and Hopkins, 1982; Ridge and Rowlerson, 1990) and in agedanimals (Jacob and Robbins, 1990). The changes seen in twitchand tetanic tension and in EJPs after partial denervation on P14could reflect decreases in synaptic safety factor. We assessedsynaptic safety factor 3 d after partial denervation by (1) blockingAChRs using increasing concentrations of curare or (2) decreasingevoked acetylcholine release by lowering extracellular calciumconcentration in a stepwisemanner.

Synapses in partially denervated muscles are more sensitive to curare block
Synapses in muscles partially denervated on P14 were much more sensitive to curare block than were those in contralateralcontrol muscles, suggesting a decreased safety factor (Fig. 8A).On average, the concentration of curare necessary to completelyblock evoked muscle contraction in muscles partially denervationon P14 was half that of contralateral controls (Fig. 8A, Table2). Thus, there did not appear to be a subpopulation of synapsesin partially denervated P14 muscles with normal safety factor.In contrast, although muscles partially denervated on P25-30 showedsome increase in sensitivity to curare, it was less severe thanin the younger muscles (Fig. 8B, Table 2).

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Figure 8. Curare block provides evidence of weakened synapses after partial denervation, especially in younger muscles. Twitch tension was recorded in the presence of increasing concentrations of curare 3 d after partial denervation on P14 (A; n = 5) or on P25-30 (B; n = 6). At both ages, synapses in partially denervated muscles (filled circles) were more sensitive to curare than synapses in contralateral control muscles (open circles). Synapses in muscles partially denervated on P14 (A) were more severely affected than were synapses in muscles partially denervated on P25-30 (B).


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Table 2. Synaptic strength after partial denervation (PD) on P14 or P25-30

To our surprise, curare sensitivity of contralateral control muscles also differed between the two age groups. A higher concentrationof curare was necessary for complete block of evoked contractionin P17 contralateral muscles than in older contralateral muscles(p < 0.001; Table 2). These data are consistent with reportsthat curare acts as a partial agonist on the embryonic form ofAChR (Steinbach and Chen, 1995) and can actually depolarize musclefibers in late embryonic life (Ziskind and Dennis, 1978), althoughone might have expected to see little evidence of these complexeffects of curare as late as P17. To determine whether this apparentage dependence of curare sensitivity was attributable to contralateraleffects of the partial denervation, we tested normal P17 and P26-29soleus muscles taken from animals that had not been subjectedto any previous surgery (n = 3 per age group). As was true formuscles contralateral to partial denervation, normal P17 soleusmuscles were less sensitive to curare than were normal P26-29muscles. The curare concentration (×10⁷ gm/ml) required for complete block of evoked muscle contractionwas 6.67 ± 0.44 for P17 muscles and 4.83 ± 0.17 for P26-29 muscles(p < 0.02). These data indicate that developmental changes inthe pharmacological effects of curare are still occurring as lateas P17 and are not caused by partial denervation of the contralateralmuscle.

Synapses in partially denervated muscles are more sensitive to reductions in extracellular calcium
In addition to its effects on postsynaptic AChRs, curare might also act on presynaptic AChRs, blocking feedback effects ofacetylcholine on its own release (Bowman et al., 1988; Fu andLiu, 1997). Because of the complexity of curare effects and thedevelopmental changes that are still taking place at P17, we useda second method of assessing synaptic safety factor. By decreasingextracellular calcium concentration in a step-wise manner (Jordanet al., 1992), we confirmed the decrease in synaptic safety factorseen in our curare experiments in a separate set of animals. Synapsesin muscles partially denervated 3 d earlier were more sensitiveto lowering extracellular calcium than were contralateral controls,and this was more striking after partial denervation on P14 thanafter partial denervation on P25-30 (Fig. 9, Table 2). For eachdecrease in calcium concentration (except the last), muscles partiallydenervated on P14 exhibited at least a twofold greater decreasein twitch tension than muscles partially denervated on P25-30(Fig. 9). Together, these studies of the sensitivity of neurotransmissionto curare and extracellular calcium levels provide strong evidenceof weakened synapses in muscles partially denervated on P14. Theydo not, however, offer insight into the changes underlying thisdecreased synaptic safety factor.

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Figure 9. Lowering calcium levels provides evidence of decreased synaptic safety factor after partial denervation, especially in younger muscles. Twitch tension was recorded in the presence of decreasing levels of calcium 3 d after partial denervation on P14 (A; n = 4) or on P25-30 (B; n = 4). At both ages, synapses in partially denervated muscles (filled circles) were more sensitive to lowering calcium levels than synapses in contralateral control muscles (open circles). Synapses in muscles partially denervated on P14 (A) were more severely affected than were synapses in muscles partially denervated on P25-30 (B).

Synaptic weakening after partial denervation on P14 may be due to loss of terminal branches

One factor underlying decreased synaptic strength could be a loss of synaptic release sites. A loss of some terminals afterpartial denervation has been suggested previously, based on glycogendepletion studies of adult rat lumbrical muscle (Ridge and Rowlerson,1990). We assessed the physical relationship between nerve terminalsand AChRs in whole mounts 3 d after partial denervation on P14or P25-30 and in contralateral control muscles (n = 7-8 animalsper group). Endplates contacted by terminal or nodal sprouts werenot included in this analysis. The normal neuromuscular junctiondisplays a close apposition of presynaptic nerve terminal branchesand postsynaptic AChRs (Rich and Lichtman, 1989; Balice-Gordonand Lichtman, 1993; Fig. 10E,F,O,P). In contrast, after partialdenervation on P14, more than half of all innervated junctionsshowed a severe mismatch between nerve terminal and AChRs (Figs.10A-D, 11), characterized by regions of AChRs without any overlyingterminal branches. Although not quantified, typically at leastone-fourth of the AChR plaque was apparently devoid of terminalbranches. This occurred at a lower frequency in muscles partiallydenervated on P25-30 and was rare in contralateral control muscles(Fig. 11). Only 10.6% of endplates had any sign of polyneuronalinnervation at the time of partial denervation on P14, and weexcluded terminals supplied by thin axons (characterizing nodalsprouts or inputs in the process of withdrawal); therefore, theseabnormal terminals (52.7% of all innervated sites) cannot be attributableto partial denervation of individual endplates. Morphologicaldisruption of terminals also was seen when terminals were labeledwith an antibody to SV2 rather than synaptophysin (Fig. 10I-K).Because we stained terminals using antibodies against synapticvesicle proteins, it is possible that the terminal branches werestill present, but their synaptic machinery had been dismantled.We have not yet distinguished between these two possibilities,but either would suggest that a presynaptic change accompaniesthe synaptic weakening seen after partial denervation on P14.Schwann cells at disrupted junctions typically covered the remainingterminal but not the entire AChR plaque (Fig. 10A-D).

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Figure 10. Terminal morphology is disrupted 3 d after partial denervation (PD). A-H, Fluorescent photomicrographs of neuromuscular junctions from a muscle partially denervated 3 d earlier on P14 (A-D) and from the contralateral control muscle (P17 contra; E-H). Junctions were triple-labeled with anti-neurofilament (NF) and anti-synaptophysin (syn) to visualize nerve processes (A, E), $alpha$ -bungarotoxin to visualize AChRs (B, F), and anti-S100 to visualize Schwann cells (C, G). In the color montages (D, H), nerve processes are green, AChRs are red, and Schwann cells are blue. In control muscles, terminal branches fully covered AChR plaques, whereas in partially denervated muscles, there were often regions of AChR without apposed terminal branches (A-D, arrows). Schwann cells (only partially in focus in this photomicrograph) at disrupted junctions maintained coverage of the nerve terminal but not of the entire endplate (C, D). I, J, Disrupted terminal morphology was also apparent with anti-SV2 labeling, as seen in this confocal image of a junction from a muscle partially denervated 3 d earlier on P14. Junctions were labeled with anti-neurofilament (NF) and anti-SV2 to visualize nerve processes (I) and $alpha$ -bungarotoxin to visualize AChRs (J). In the color montage (K), nerve processes are green, and AChRs are red. L-Q, In muscles partially denervated on P25-30, a myelin-specific antibody showed that myelinated axons supplied the disrupted terminals that were occasionally seen. L-N, Confocal image of a junction from a muscle partially denervated 3 d earlier on P26. O-Q, Confocal image of a junction from the contralateral control muscle (P29 contra). Junctions were labeled with anti-synaptophysin and anti-protein zero to visualize nerve terminals and myelin sheaths (L, O) and $alpha$ -bungarotoxin to visualize AChRs (M, P). In the color montages (N, Q), terminal branches and myelin are green, and AChRs are red. Scale bars, 10 µm.

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Figure 11. Immature nerve terminals are morphologically disrupted by denervation of neighboring fibers in the muscle. Muscles were processed immunohistochemically (see Materials and Methods) 3 d after partial denervation (PD) on P14 (n = 8) or on P25-30 (n = 7). Endplates in which extensive regions of AChRs were not covered by terminal branches (see Fig. 10) were categorized as being severely disrupted. Typically, at least one-fourth of the AChR plaque had no apposing terminal branches. This analysis excluded endplate sites contacted by a nodal or terminal sprout. In muscles partially denervated on P14, more than half of all terminals were severely disrupted. Severely disrupted terminals were less common in muscles partially denervated on P25-30 and were extremely rare in contralateral control muscles (contra). No bar is seen for contralateral muscles at P25-30, because values were all zero. Two-way interaction, p < 0.0001.

It is formally possible that the disrupted synapses seen after partial denervation are new synapses being formed by nodalsprouts (although with unexpectedly thick axons), which are thereforeimmature in structure and in strength. This would be consistentwith the fade seen during high-frequency stimulation but can beruled out by a number of observations. First, if terminals newlyformed by sprouts were weak, but terminals present at the timeof partial denervation were unaffected, one would expect a componentof the twitch tension in curare or lowered calcium to behave likenormally innervated muscle (Rochel and Robbins, 1988). We didnot see evidence of such a subpopulation of normal terminals inmuscles partially denervated on P14. Second, if existing terminalswere unaffected, we would expect no decrease in twitch or tetanictension, but a slight increase reflecting the contribution ofnew, albeit weaker, synapses. Instead, we saw a trend toward decreasedtwitch tension and a striking decrease in tetanic tension afterpartial denervation on P14. Third, in an additional group of partiallydenervated P25-30 muscles, we used an antibody to protein zero,a myelin-specific protein, instead of labeling neurofilament.In these muscles, we observed examples of severely disrupted terminalsinnervated by myelinated axons (Fig. 10L-N), clearly ruling outthe possibility that all disrupted terminals were newly formingterminals at the end of misidentified nodal sprouts. In summary,neonatal partial denervation sets in motion processes that disruptuninjured terminals present in the muscle at the time of partialdenervation. A loss of potential release sites may underlie thedecreased synaptic efficacy of motor terminals in partially denervatedmuscles.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present studies shed light on the relatively poor response of neonatal motoneurons to partial denervation of their targetmuscle and have implications for our understanding of developmentalsynapse elimination. Our results are consistent with the hypothesisthat the death of terminal Schwann cells at denervated endplatesin neonates removes a critical stimulus for terminal sprouting,which is the primary means by which fibers are reinnervated inpartially denervated adult soleus muscles (Brown and Ironton,1978). We also found evidence of severe synaptic disruption afterpartial denervation on P14, suggesting that some terminals retractafter partial denervation indevelopment.

The limited expansion of neonatal motor units after partial denervation is not attributable to their already enlarged size

In the initial studies of neonatal partial denervation, muscles were partially denervated before P7, when motor units aresubstantially larger than in adulthood. It has been suggestedthat neonatal motoneurons are less able to reinnervate denervatedfibers because they are already maintaining a large number ofterminals. The present data argue strongly against this hypothesis.We partially denervated the soleus muscle at the end of developmentalsynapse elimination (Brown et al., 1976), when soleus motor unitshave decreased to their adult size. Motor units in muscles partiallydenervated on P14 did not expand as much as units in partiallydenervated adult muscles. Studied in a different context, Fisheret al. (1989) found no difference in motor unit expansion afterpartial denervation (by ventral rhizotomy) of the soleus on P4-6or on P17-19. Thus, immature motoneurons fail to reinnervate denervatedfibers as effectively as mature motoneurons even if they startat the same motor unitsize.

Death of terminal Schwann cells after partial denervation may underlie the limited expansion of neonatal motor units

Schwann cells are necessary for axonal regeneration in peripheral nerve (Enver and Hall, 1994). Previous work also suggestedthat terminal Schwann cells at denervated endplates are importantin motoneuron sprouting after partial denervation (Son and Thompson,1995b; Trachtenberg and Thompson, 1997). Three days after partialdenervation of adult soleus muscles, most (~70%) of the terminalsprouts that reach denervated endplate sites are found in associationwith processes extended only by Schwann cells at the denervatedsite (Son and Thompson, 1995b). However, partial denervation duringearly postnatal life caused the death of terminal Schwann cellsat denervated endplates. If these cells are important in the motoneuronsprouting response, one would expect to see a deficit in terminalsprouting by neonatalmotoneurons.

As expected (Brown and Ironton, 1978), partial denervation of the soleus muscle on P25-30 resulted in robust terminal sprouting,but terminal sprouting was absent in muscles partially denervatedon P14. Young motoneurons did not appear to be less competentthan mature motoneurons at sprouting, because they were capableof extending nodal sprouts. An appealing explanation for the differencein terminal and nodal sprouting after partial denervation on P14arises from the observation that after neonatal denervation, Schwanncell death is more severe at endplates than in the intramuscularnerves (Trachtenberg and Thompson, 1996). After partial denervationon P14, reactive Schwann cells are present to induce sprouts fromaxons at nodes of Ranvier but are not present to induce sproutsfrom terminals, which could explain the difference in nodal andterminal sprouting by immature motoneurons. Because terminal sproutingis the primary means by which motor unit expansion occurs in thesoleus muscle (Brown and Ironton, 1978), the lack of Schwann cell-inducedterminal sprouting may account for the failure of immature motorunits to expand after partialdenervation.

Extensive nodal sprouting may contribute to the disruption of existing terminals

Motor units in muscles partially denervated on P14 do not increase in size as much as mature motor units. This indicates thatnodal sprouts do not fully compensate for the lack of terminalsprouts. One possible explanation is that nodal sprouts are moremetabolically costly to the motoneuron than are terminal sprouts,which predominate in more mature muscles. The extensive nodalsprouting seen 3 d after partial denervation therefore may notbe maintained. In addition, metabolic support of existing terminalsmay be compromised by extensive nodal sprouting. If so, a greaterprofusion of nodal sprouts in immature muscles might explain thegreater synaptic disruption seen after partial denervation onP14. Another contributing factor could be that synapses are inherentlyless stable during and shortly after the period of synapse eliminationthan in adulthood. This is consistent with the greater sensitivityof developing neuromuscular junctions to disruption by neuregulintreatment (Trachtenberg and Thompson, 1997) and is attractivein light of the dynamic nature of neuromuscular junctions duringearly postnatal development (Gan and Lichtman, 1998). In addition,reactive Schwann cells can cause similar disruption of otherwisenormal neuromuscular junctions (Trachtenberg and Thompson, 1997).However, the fact that we saw greater terminal disruption afterpartial denervation on P14 (when most Schwann cells die) thanon P25-30 (when Schwann cells become reactive) argues againsta direct role for reactive Schwann cells in the changes seen afterneonatal partialdenervation.

Presynaptic changes that occur after partial denervation on P14 result in decreased synaptic safety factor

We found striking decreases in synaptic efficacy after partial denervation in development, with lesser effects after partialdenervation on P25-30. Three days after partial denervation onP14, stimulation of isolated motor units produced decreased tetanictension. The tension evoked by repetitive nerve stimulation alsodiminished, or faded, during the 1500 msec stimulus. This fade,especially striking during high-frequency stimulation, and thedecreased tetanic tension were not due to muscle fatigue or conductionblock but appeared instead to be due to decreased synaptic safetyfactor. Synapses in muscles partially denervated 3 d earlier onP14 were much more sensitive to curare block and to lowered calciumlevels than were synapses in muscles partially denervated on P25-30.Thus, synapses formed by immature motoneurons became weaker 3d after partial denervation of their target muscle. This was attributable,at least in part, to the loss of functional release sites evidencedby decreased labeling with antibodies to the synaptic vesicleproteins synaptophysin and SV2. Although a significant portionof terminals looked normal morphologically, our physiologicalstudies suggested that all terminals in muscles partially denervatedon P14 were functionally impaired. Thus, there may have been otherchanges that also affected synapticfunction.

Implications for understanding developmental synapse elimination

Early studies of neonatal partial denervation were designed to test the hypothesis that competition between motor terminalsdrives developmental synapse elimination (Brown et al., 1976;Thompson and Jansen, 1977; Betz et al., 1980; Fladby and Jansen,1987; Gates and Ridge, 1992). These experiments led to two majorconclusions. First, competition between motor terminals is animportant component of developmental synapse elimination. Second,something intrinsic to motoneurons (not competition-based) alsocontributes to synapse elimination. Our findings suggest thatthe latter conclusion is not justified. We found that the terminalsof immature motoneurons that continue to innervate the soleusmuscle after partial denervation do not remain normal. Thus, whatwas seen as an intrinsic tendency of motoneurons to withdraw synapsesmay instead be a process secondary to the denervation of neighboringmuscle fibers. The present findings also raise more general concernsabout the use of partial denervation in development to study synapseelimination. Although not directly injured, motoneurons remainingafter partial denervation are not completely normal. The synapseelimination that occurs after partial denervation may not be preciselythe same as normal developmental synapseelimination.

Although the changes seen in terminals after partial denervation on P14 are reminiscent of those seen in terminals being lostduring developmental synapse elimination, there are critical differences.During normal development and after reinnervation, synapses becomeweaker before being eliminated (Colman et al., 1997), but evidencesuggests that this is attributable primarily to a decrease inpostsynaptic AChR density (Rich and Lichtman, 1989; Balice-Gordonand Lichtman, 1993; Colman et al., 1997). We did not observe anyobvious changes in AChR labeling 3 d after partial denervation,but this was not studied in a quantitative manner. Nevertheless,it is possible that although the factors triggering these eventsdiffer, the mechanisms underlying the apparent loss of terminalbranches after partial denervation on P14 may be related to thoseunderlying the loss of terminal branches that occurs during synapseelimination (Gan and Lichtman, 1998). Our results are consistentwith the hypothesis that increased nerve growth at some sitesalong an axon can cause the loss of terminal branches at othersites. Perhaps after partial denervation on P14, we observe anexaggerated version of what normally occurs during developmentalsynapse elimination, namely that the growth of some terminalsof a motoneuron weakens other terminals, placing them at a competitivedisadvantage (Colman et al., 1997) and resulting in theirelimination.

  FOOTNOTES

Received May 17, 1999; revised July 13, 1999; accepted Aug. 6, 1999.

This work was supported by National Institutes of Health National Research Service Award F32 NS09687 (J.L.L.) and NationalInstitutes of Health Grant NS20480 (WJT). Antibody 2H3, developedby T. M. Jessell and J. Dodd, antibody SV2, developed by K. M.Buckley, and antibody G3G4, developed by S. J. Kaufman, were obtainedfrom the Developmental Studies Hybridoma Bank maintained by theUniversity of Iowa, Department of Biological Sciences, under contractN01-HD-7-3263 from the National Institute of Child Health andHuman Development. Antibody P07 was kindly provided by Dr. JuanJ. Archelos (University of Wurzburg). We thank L. A. Sutton forexcellent technical assistance, G. E. Gage for help with graphics,and L. M. Hurley and G. T. Smith for helpful comments on thismanuscript.
Correspondence should be addressed to Jane L. Lubischer, Section of Neurobiology, C0920, 140 Patterson Laboratory Building,University of Texas, Austin, TX78712.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Balice-Gordon RJ, Lichtman JW (1993) In vivo visualization of the growth of pre- and postsynaptic elements of neuromuscular junctions in the mouse. J Neurosci 10:894-908[Abstract].
Betz WJ, Caldwell JH, Ribchester RR (1980) The effects of partial denervation at birth on the development of muscle fibres and motor units in rat lumbrical muscle. J Physiol (Lond) 303:265-279[Abstract/Free Full Text].
Bowman WC, Marshall IG, Gibb AJ, Harborne AJ (1988) Feedback control of transmitter release at the neuromuscular junction. Trends Pharmacol Sci 9:16-20[Medline].
Brown MC, Ironton R (1978) Sprouting and regression of neuromuscular synapses in partially denervated mammalian muscles. J Physiol (Lond) 278:325-348[Abstract/Free Full Text].
Brown MC, Jansen JKS, Van Essen D (1976) Polyneuronal innervation of skeletal muscle in new-born rats and its elimination during development. J Physiol (Lond) 261:387-422[Abstract/Free Full Text].
Brown MC, Holland RL, Ironton R (1980) Nodal and terminal sprouting from motor nerves in fast and slow muscles of the mouse. J Physiol (Lond) 306:493-510[Abstract/Free Full Text].
Close R (1964) Dynamic properties of fast and slow skeletal muscles of the rat during development. J Physiol (Lond) 173:74-95.
Close R (1967) Properties of motor units in fast and slow skeletal muscles of the rat. J Physiol (Lond) 193:45-55[Web of Science][Medline].
Colman H, Nabekura J, Lichtman JW (1997) Alterations in synaptic strength preceding axon withdrawal. Science 275:356-361[Abstract/Free Full Text].
Enver MK, Hall SM (1994) Are Schwann cells essential for axonal regeneration into muscle autografts? Neuropathol Appl Neurobiol 20:587-598[Web of Science][Medline].
Fisher TJ, Vrbová G, Wijetunge A (1989) Partial denervation of the rat soleus muscle at two different developmental stages. Neuroscience 28:755-763[Web of Science][Medline].
Fu WM, Liu JJ (1997) Regulation of acetylcholine release by presynaptic nicotinic receptors at developing neuromuscular synapses. Mol Pharmacol 51:390-398[Abstract/Free Full Text].
Gan W-B, Lichtman JW (1998) Synaptic segregation at the developing neuromuscular junction. Science 282:1508-1511[Abstract/Free Full Text].
Gates HJ, Ridge RM (1992) The importance of competition between motoneurones in developing rat muscle; effects of partial denervation at birth. J Physiol (Lond) 445:457-472[Abstract/Free Full Text].
Gordon T, Yang JF, Ayer K, Stein RB, Tyreman N (1993) Recovery potential of muscle after partial denervation: a comparison between rats and humans. Brain Res Bull 30:477-482[Web of Science][Medline].
Guth L, Samaha FJ (1970) Procedure for the histochemical demonstration of actomyosin ATPase. Exp Neurol 28:365-367[Web of Science][Medline].
Hoffman H (1950) Local re-innervation in partially denervated muscle: a histo-physiological study. Aust J Exp Biol Med Sci 28:383-397.
Jacob JM, Robbins N (1990) Differential effects of age on neuromuscular transmission in partially denervated mouse muscle. J Neurosci 10:1522-1529[Abstract].
Jansen JKS, Fladby T (1990) The perinatal reorganization of the innervation of skeletal muscle in mammals. Prog Neurobiol 34:39-90[Web of Science][Medline].
Johnson GD, Nogueira Araujo GMdeC (1981) A simple method of reducing the fading of immunofluorescence during microscopy. J Immunol Methods 43:349-350[Web of Science][Medline].
Jordan CL, Pawson P, Arnold AP, Grinnell AD (1992) Hormonal regulation of motor unit size and synaptic strength during synapse elimination in the rat levator ani muscle. J Neurosci 12:4447-4459[Abstract].
Krnjevic K, Miledi R (1957) Adrenaline and failure of neuromuscular transmission. Nature 180:814-815[Web of Science][Medline].
Kugelberg E (1976) Adaptive transformation of rat soleus motor units during growth. J Neurol Sci 27:269-289[Web of Science][Medline].
Liley AW (1956) An investigation of spontaneous activity at the neuromuscular junction of the rat. J Physiol (Lond) 132:650-666.
Lingle CJ, Steinbach JH (1988) Neuromuscular blocking agents. Int Anesthesiol Clin 26:288-301[Web of Science][Medline].
Love FM, Thompson WJ (1998) Schwann cells proliferate at rat neuromuscular junctions during development and regeneration. J Neurosci 18:9376-9385[Abstract/Free Full Text].
Lubischer JL, Thompson WJ (1997) Partial denervation of soleus muscle results in an age-dependent decrease in the efficacy of the remaining neuromuscular junctions. Soc Neurosci Abstr 23:1720.
Redfern PA (1970) Neuromuscular transmission in new-born rats. J Physiol (Lond) 344:89-111[Abstract/Free Full Text].
Rich MM, Lichtman JW (1989) In vivo visualization of pre- and postsynaptic changes during synapse elimination in reinnervated mouse muscle. J Neurosci 9:1781-1805[Abstract].
Ridge RMAP, Rowlerson A (1990) Sprouting motoneurons break as well as make contacts in partially denervated rat muscle. J Physiol (Lond) 425:15P.
Rochel S, Robbins N (1988) Effect of partial denervation and terminal field expansion on neuromuscular transmitter release and nerve terminal structure. J Neurosci 8:332-338[Abstract].
Slack JR, Hopkins WG (1982) Neuromuscular transmission at terminals of sprouted mammalian motor neurones. Brain Res 237:121-135[Web of Science][Medline].
Steinbach JH, Chen Q (1995) Antagonist and partial agonist actions of d-tubocurarine at mammalian muscle acetylcholine receptors. J Neurosci 15:230-240[Abstract].
Son Y-J, Thompson WJ (1995a) Schwann cell processes guide regeneration of peripheral axons. Neuron 14:125-132[Web of Science][Medline].
Son Y-J, Thompson WJ (1995b) Nerve sprouting in muscle is induced and guided by processes extended by Schwann cells. Neuron 14:133-141[Web of Science][Medline].
Thompson WJ (1978) Reinnervation of partially denervated rat soleus muscle. Acta Physiol Scand 103:81-91[Web of Science][Medline].
Thompson WJ, Jansen JKS (1977) The extent of sprouting of remaining motor units in partly denervated immature and adult rat soleus muscle. Neuroscience 2:523-535[Web of Science][Medline].
Trachtenberg JT, Thompson WJ (1996) Schwann cell apoptosis at developing neuromuscular junctions is regulated by glial growth factor. Nature 379:174-177[Medline].
Trachtenberg JT, Thompson WJ (1997) Nerve terminal withdrawal from rat neuromuscular junctions induced by neuregulin and Schwann cells. J Neurosci 17:6243-6255[Abstract/Free Full Text].
Ziskind L, Dennis MJ (1978) Depolarising effect of curare on embryonic rat muscles. Nature 276:622-623[Web of Science][Medline].

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