The "Waiting Period" of Sensory and Motor Axons in Early Chick Hindlimb: Its Role in Axon Pathfinding and Neuronal Maturation

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The Journal of Neuroscience, July 15, 2000, 20(14):5358-5366

The "Waiting Period" of Sensory and Motor Axons in Early Chick Hindlimb: Its Role in Axon Pathfinding and Neuronal Maturation
Guoying Wang and Sheryl A. Scott
Department of Neurobiology and Anatomy, University of Utah School of Medicine, Salt Lake City, Utah 84132

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

During embryonic development motor axons in the chick hindlimb grow out slightly before sensory axons and wait in the plexusregion at the base of the limb for ~24 hr before invading thelimb itself (Tosney and Landmesser, 1985a). We have investigatedthe role of this waiting period by asking, Is the arrest of growthcones in the plexus region a general property of both sensoryand motor axons? Why do axons wait? Does eliminating the waitingperiod affect the further development of motor and sensoryneurons?
Here we show that sensory axons, like motor axons, pause in the plexus region and that neither sensory nor motor axons requirecues from the other population to wait in or exit from the plexusregion. By transplanting older or younger donor limbs to hostembryos, we show that host axons innervate donor limbs on a scheduleconsistent with the age of the grafted limbs. Thus, axons waitin the plexus region for maturational changes to occur in thelimb rather than in the neurons themselves. Both sensory and motoraxons innervate their appropriate peripheral targets when thewaiting period is eliminated by grafting older donor limbs. Therefore,axons do not require a prolonged period in the plexus region tosort out and project appropriately. Eliminating the waiting perioddoes, however, accelerate the onset of naturally occurring celldeath, but it does not enhance the development of central projectionsor the biochemical maturation of sensoryneurons.

Key words: waiting period; chick; hindlimb; axon pathfinding; neuron development; motor neuron; sensory; dorsal root ganglion; cell death; trkA; substance P; central projections

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The overall time course and sequence of events in the development of motor (Landmesser, 1988, 1994) and sensory neurons (Scott,1992a) has been described in detail, although the underlying regulatorymechanisms are far from understood. In the chick hindlimb, sensoryaxons grow out together with, but slightly later than, motor axons(Tosney and Landmesser, 1985a; Landmesser and Honig, 1986). Motoraxons grow as far as the base of the limb and then pause for 24hr in the plexus region before growing into the limb itself (Tosneyand Landmesser, 1985a). Within the plexus region the axons destinedfor particular peripheral targets come together, sort out, andmake specific pathway choices (Lance-Jones and Landmesser, 1981;Tosney and Landmesser, 1985b,c). Both motor and sensory neuronsproject accurately to their appropriate peripheral targets fromtheir earliest outgrowth (for review, see Landmesser, 1988, 1994;Scott, 1992b). Once axons reach their peripheral targets, bothmotor and sensory neurons undergo a period of programmed celldeath that serves to match the size of the neuron population withits target (Oppenheim, 1991). Peripheral targets continue to influencethe further differentiation of sensory neurons. For example, targetmuscles can determine the central projections of muscle afferents(Wenner and Frank, 1995). Moreover, cross-innervation studiesin adult rodents show that the peripheral target can influencethe biochemical phenotype of sensory neurons (McMahon and Gibson,1987).

A remaining enigma in this well documented developmental sequence is the waiting period of axons as they invade the limb.The reasons for and the functional consequences of this waitingperiod are unknown. Whether the arrest of growth cones in theplexus region is a general property of both sensory and motoraxons is unknown also. We have begun to investigate the waitingperiod in the context of the normal development of motor and sensoryneurons. In particular, we have asked, Do sensory neurons alsopause in the plexus region before invading the limb? Do neuronswait in the plexus region for maturational changes in the limbor in the neurons themselves? Do neurons require the waiting periodto project accurately to their appropriate peripheral targets?How does elimination of the waiting period affect the furtherdifferentiation of the neurons? Our results indicate that sensoryneurons, like motor neurons, pause for ~1 d in the plexus region.An analysis of axon outgrowth in embryos with transplanted olderlimbs showed that axons wait in the plexus region for maturationalchanges to occur in the limb. Neither population, however, requiresthe waiting period to project accurately to its peripheral targets.Elimination of the waiting period, which results in precociousinnervation of peripheral targets, accelerates the onset to naturallyoccurring cell death, but it does not influence the developmentof central connections or the maturation of some biochemical propertiesof sensoryneurons.

Some of this work has been presented in abstract form (Scott and Wang, 1999; Wang and Scott, 1999a).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

General
Fertile White Leghorn chick eggs from a local supplier were incubated in a humidified forced-draft incubator at 38°C. Embryoswere staged according to Hamburger and Hamilton (1951) at thetime of surgery and atdeath.

Embryonic surgery
Several types of surgical manipulations were performed on embryos between stage (St.) 15 and St. 22 [embryonic days 2.5-3.5(E2.5-E3.5)]. A window was cut in the shell over the embryo. Thevitelline and amniotic membranes over the posterior part of theembryo were torn open, and the area was stained lightly with 0.5%sterile neutral red in Ringer's solution (Scott, 1984). The desiredportion of the tissue was excised with sharpened tungsten needles,as described below. The embryo was moistened with several dropsof Ringer's solution. Eggs were sealed with paraffin and a coverslipand returned to the incubator until the desiredstage.
Motor and sensory neuron removal. To test whether sensory neurons require motor neurons to wait in or exit from the plexusregion, we eliminated motor neurons at St. 17-18 by aspiratingthe ventral two-thirds of the neural tube, leaving the dorsalone-third of the neural tube (including neural crest) intact,as described previously (Landmesser and Honig, 1986; Scott, 1988;Wang and Scott, 1999b). To test whether motor axon outgrowth isinfluenced by sensory axons, we eliminated sensory neurons byremoving the neural crest at St. 15-16 (Scott, 1984), leavingthe ventral neural tubeintact.
Heterochronic limb transplantation. Older donor limb buds were prepared from St. 21-22 embryos by severing the limb bud adjacentto the lateral boundary of the somites. Then donor limb buds weretransferred to younger (St. 17) host embryos from which one limbbud similarly had been removed. Conversely, younger limb budswere transplanted from St. 17-18 donors to older St. 21-22 hosts.In each case the undisturbed contralateral host limb bud servedas a control for the grafted limb. As a further control, severalSt. 17 or St. 21 embryos received sham operations in which onelimb bud was simply removed and replaced. Moreover, in a few donorembryos we removed the whole neural tube opposite somites 22-31at St. 15-16 before axon outgrowth. Denervated donor embryos wereallowed to develop to St. 21-22, when their aneural limbs weretransplanted to normal St. 17hosts.
To determine the extent of limb tissue that was transplanted, in particular whether or not the plexus region was derived fromtransplanted or host tissue, in a few cases we transplanted anolder quail limb bud onto a younger chick host. Embryos with obviousabnormalities or that did not fit the criteria described in Resultswerediscarded.

Retrograde labeling
To analyze the peripheral and central innervation patterns in transplanted limbs, we retrogradely labeled sensory and/or motorneurons with DiI [2.5 mg/ml in dimethylformamide (DMF); MolecularProbes; Eugene, OR] in operated embryos at St. 29-34. Embryoswere removed from the eggs and placed in a bath of oxygenatedRinger's solution at room temperature. The embryos were decapitatedand eviscerated, and a ventral laminectomy was performed. Dorsalroot ganglia (DRGs) from the last thoracic (T7) to the fourthlumbosacral (LS4) segment or selected hindlimb muscles (sartorius,femorotibialis, or adductor) were exposed and injected with DiI.After injection the embryos were maintained in oxygenated Ringer'ssolution at 28°C for 6 hr, when they were fixed in 4% paraformaldehyde.Then the embryos were stored in paraformaldehyde at 37°C for another2-3 weeks to allow for thorough retrogradelabeling.
Injected embryos were observed first as whole mounts with fluorescence optics to assess the overall pattern of transporteddyes. Subsequently, a region of the embryo containing the spinalcord and DRGs from T6 through the lumbosacral enlargement wascut out and embedded in gelatin-albumin. Blocks were hardenedovernight with 1% glutaraldehyde and serially sectioned at 80µm with a vibratome. To observe the mediolateral distributionof motor neurons and the central projections of sensory neuronsin the spinal cord, we cut the blocks transversely; to observethe segmental distribution of motor and sensory neurons, we cutother blocks longitudinally. Sections were mounted in 90% glycerol/10%PBS containing 0.1% p-phenylenediamine (Johnson and Nogueira Araujo,1981) to retard fading. Labeling was viewed with a Zeiss Axioskopmicroscope or an Olympus Fluoview confocal scanning lasermicroscope.

Immunohistochemistry
To distinguish between sensory and motor axons in single sections, we double-labeled sections, using one antibody that stainsall axons [3A10, 1:100; Developmental Studies Hybridoma Bank (DSHB),University of Iowa, Iowa City, IA] and a second antibody thatlabels only sensory axons (anti-trkC; kindly provided by Dr. F.B. Lefcort, Department of Biology, Montana State University, Bozeman,MT). Axons that stained with 3A10, but not with anti-trkC, wereconsidered to be motor neuron axons. Quail cells were identifiedwith QCPN (1:50; DSHB). To examine the biochemical maturationof sensory neurons, we stained sections with anti-substance P(1:200; PharMingen, San Diego, CA) or anti-trkA (1 µg/7 ml; providedby Dr.Lefcort).
Normal and operated embryos from St. 20-26 were fixed in 4% paraformaldehyde for several hours to overnight (depending onthe stage), cryoprotected in 20% sucrose in PBS, and sectionedwith a cryostat. For staining with all antibodies except anti-trk,the sections were incubated for 1 hr at room temperature in PBScontaining 5% normal goat serum (NGS) and 0.1% Triton X-100. Thenthe sections were incubated at 4°C overnight in primary antibodydiluted in the same buffer. Immunoreactivity was detected by usingFITC, rhodamine, and/or Texas Red-conjugated secondary antibody.Anti-trkC and anti-trkA staining was amplified with Tyramide SignalAmplification (TSA, New England Nuclear, Boston,MA).

Cell death
To analyze cell death of motor and sensory neurons in embryos with heterochronic limb transplants, we fixed embryos from St.28-36 in Bouin's solution for at least 24 hr, dehydrated themin graded ethyl alcohol, and embedded them in paraffin. Transverse8-10 µm sections were stained with cresyl violet or thionine.In one-half of the operated embryos motor neurons were countedin every tenth section of both sides of the embryo from segmentLS1 through LS8, as described by Clarke and Oppenheim (1995).In the other half the motor neurons were counted only in segmentLS3. To estimate the size of DRGs, which was taken as an indicationof sensory neuron number, we measured the diameter of the largestprofile of the LS3 DRG on both the experimental and control sides,using Image-1 software (Universal Imaging, West Chester,PA).
In addition, apoptotic motor and sensory neurons were identified with TUNEL staining in paraffin sections by using an In SituCell Death Detection kit (catalog #1684795, Roche Molecular Biochemicals,Indianapolis, IN). Labeled motor and sensory neurons were countedin every third section throughout segment LS3 on both sides oftheembryo.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Sensory and motor axon outgrowth through the plexus region

Normal axon outgrowth
During normal development the motor axons grow as far as the base of the hindlimb and then pause for 24 hr in the plexus regionbefore invading the limb itself (Tosney and Landmesser, 1985a).To determine whether sensory axons, which grow out slightly laterthan motor axons (Tosney and Landmesser, 1985a; Landmesser andHonig, 1986) (Fig. 1), also wait in the plexus region, we comparedthe time course of sensory axon growth into the limb with thatof all axons and of motor neurons in embryos from St. 20-25. Sensoryaxons were identified with anti-trkC, as described in Materialsand Methods.

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Figure 1. Sensory axons grow out slightly later than motor axons. Shown is a transverse section through the spinal cord and plexus region of a St. 22 embryo stained with 3A10 to label all neurons and stained with anti-trkC to label sensory neurons. Motor axons are labeled only with 3A10 and appear green; sensory axons are double-labeled and appear yellow. Note that sensory axons lag only slightly behind motor axons.

The pattern of early sensory axon growth closely parallels that of all axons. Outgrowth of sensory axons from rostral lumbosacraldorsal root ganglia (DRGs LS1-3) is obvious by St. 21, and manyaxons have arrived at the plexus region by St. 22 (Fig. 2D). Theydid not emerge from the plexus region and enter the limb properuntil late St. 24 (Fig. 2E,F). Thus, sensory axons like motoraxons wait in the plexus region for ~24 hr before advancing intothe limb.

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Figure 2. Transverse sections through embryos of different stages show the timing of sensory and motor axon outgrowth. A-C, Sections stained with 3A10 to show normal outgrowth of all axons (both sensory and motor). D-F, Sections stained with trkC to show normal outgrowth of sensory axons. G-I, Sensory axon outgrowth in the absence of motor neurons. After early removal of the ventral neural tube the lateral motor column is missing, but DRGs (arrows) still develop. J-L, Outgrowth of motor axons in the absence of sensory neurons. After neural crest removal, DRGs are missing, but the lateral motor column develops normally. Note that axon outgrowth in each condition is similar to that of the normal control axons shown in the top row.

Sensory axon outgrowth in the absence of motor neurons
Both anatomical evidence (Tosney and Landmesser, 1985b) and experimental evidence (Landmesser and Honig, 1986; Scott, 1988)suggest that motor axons may direct sensory axon outgrowth. Thus,sensory axon growth may be arrested in the plexus region simplybecause motor axons pause there for 1 d. To test this possibility,we removed motor neurons at St. 17, before axon outgrowth, andcharted the timing of sensory axon outgrowth in the absence ofmotor neurons. Fifteen of the 70 operated embryos survived andwere missing motor neurons from at least segments LS1-3. No ventralhorn formed in the operated region, but DRGs developed normally(arrows, Fig. 2G-I).
Sensory axon outgrowth in the absence of motor neurons was indistinguishable from normal. Sensory axons reached the plexusregion at approximately St. 21 (data not shown) and accumulatedin this region during St. 22 (Fig. 2G) and St. 23 (Fig. 2H). Theybegan to exit the plexus region late in St. 24 (data not shown)and clearly had begun to grow into the limb by St. 25 (Fig. 2I).Moreover, in the absence of motor neurons the sensory axons divergedinto dorsal and ventral branches like normal. Thus, sensory axonscan grow to the plexus region, pause there, and exit appropriatelyfrom this region on schedule without cues from neighboring motorneurons.

Motor axon outgrowth in the absence of sensory neurons
Because sensory axons grow out slightly later than motor axons (Tosney and Landmesser, 1985a; Landmesser and Honig, 1986)(see Fig. 1), we asked whether motor axons pause to allow sensoryaxons to catch up before invading the limb. To approach this question,we eliminated sensory neurons by removing the dorsal half of theneural tube including the neural crest opposite somites 22-31at St. 15-16, leaving the ventral neural tube intact, and chartedthe time course of motor axon outgrowth. Seven of the 15 operatedembryos survived and were missing DRGs LS1-3 (or more). As illustratedin Figure 2J-L, in the absence of sensory neurons the motor axonsgrew out, paused, and invaded the limbnormally.

Sensory and motor axon outgrowth after heterochronic limb transplantation

Together, these results show that sensory and motor axons can grow to, wait in, and exit from the plexus region independentlyof each other. We next asked why these axons wait in the plexusregion and what allows them to leave. Are outgrowing axons tooimmature to respond to permissive cues in the limb, or is thelimb itself not yet favorable for axon growth? To distinguishbetween these possibilities, we analyzed axon growth and the waitingperiod in embryos in which we grafted an older St. 21-22 limbbud onto a younger St. 17 host. If axons from younger embryosgrow directly into the older limb without stopping in the plexusregion, this would suggest that axons pause to allow maturationalchanges to occur in the limb. Conversely, failure of axons toinvade the older limb until the host reaches St. 24-25 would suggestthat younger axons are incapable of responding to cues from thelimb, and the waiting period enables maturational changes to occurin theaxons.

Eighty-five of the 260 operated embryos survived and had normal-appearing transplanted limbs. Embryos in which the transplantedlimb was deformed or developed a hemorrhagic clot were discarded.In addition, five chick hosts successfully received quail limbbud transplants. Further, 14 St. 17-18 embryos, all of which survived,received sham operations in which the limb bud simply was removedandreplaced.

As described previously (Swanson and Lewis, 1982), the grafted hindlimbs developed according to their own autonomous timetable.Thus, at the time of analysis the grafted limb was larger andone to three stages more mature than the host limb, as illustratedin Figure 3, A and B. However, because early developmental stagesare shorter than later stages, as the embryos matured the absolutedifference in the number of stages between the host and graftedlimbs became smaller. Anti-quail antibody staining showed thatthe entire limb, including part of the plexus region, was derivedfrom transplanted tissue (Fig. 3C). Thus, axons from the hostembryo encountered older, more mature tissue as they exited fromthe plexus region and entered the transplanted donor limb.

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Figure 3. After transplantation of older donor limbs, grafted limbs (left in each panel) develop normally and are more mature than host limbs. A, An embryo immediately after transplantation of a St. 22 limb bud to a St. 17 host embryo. B, The embryo shown in A has developed to St. 23, whereas the transplanted limb is now St. 25. C, The plexus region is partly included in the transplanted tissue. Shown is a transverse section through an embryo in which a quail limb bud was transplanted to a younger chick host. Quail tissue is identified with antibody QCPN.

The initial outgrowth of axons toward the plexus region was nearly identical on both the operated and control sides of theembryo. For example, in the embryo shown in Figure 4A (St. 22host: St. 23.5 graft), axons have reached the plexus region buthave not entered either limb. Similar results were obtained infour additional embryos in which the donor limb was St. 24 oryounger. Analysis of slightly older embryos showed that axonsinnervated grafted limbs on a schedule dictated by age of thelimb rather than the age of the host, as illustrated in Figure4B. In this embryo the axons have grown into the grafted St. 25limb but still are waiting like normal in the plexus region ofthe St. 23 host limb. Innervation of the grafted and host limbsis indistinguishable from innervation of normal St. 25 and St.23 limbs, respectively. Similar results were obtained in threeother St. 23 host: St. 25 transplant embryos. This pattern wasmaintained at later stages; innervation of donor limbs (St. 27-28)was more extensive than that of the younger hosts (St. 25-26)(n = 5; Fig. 4C), as previously reported (Swanson and Lewis, 1982).

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Figure 4. Axons from the host embryo grow into donor limbs (left in each panel) on a schedule appropriate for the age of the transplanted limb. A, Axons have not yet grown into the St. 23.5 transplanted limb or St. 22 host limb. B, Axons have begun to grow into the St. 25 grafted limb but are still waiting in the plexus region of the host St. 23 limb. C, Axons have grown more extensively into the St. 27.5 grafted limb than into the St. 25 host limb. D, Axons have grown into the St. 24.5 aneural transplanted limb and have distributed normally, whereas they have not yet left the plexus region in the host St. 23 limb. E, Axons from a St. 25 host embryo have accumulated in the plexus region of the St. 22 donor limb, but only a few axons (arrow) have entered the immature limb.

Together, these results suggest that axons wait in the plexus region for maturational changes to occur in the limb. However,the plexus region in donor limbs already had been invaded by axonswhen the limb bud was excised. This early innervation could alterthe plexus region, thereby allowing host axons to exit prematurelyafter heterochronic transplantation. To eliminate this possibility,we transplanted aneural St. 21 limb buds (see Materials and Methods)to normal St. 17 hosts. In all six embryos that were examined,axons innervated the donor limb on a schedule appropriate forthe transplanted limb (Fig. 4D). Moreover, axons diverged intodorsal and ventral bundles, as in normal embryos. Thus, the acceleratedinnervation of grafted older limbs does not result from theirpreviousinnervation.

To test further whether the waiting period is attributable to maturational changes in the neurons or in the limb, in a fewcases we grafted younger limb buds onto older donor embryos (n= 7). From the results described above, we expected that hostaxons would wait in the plexus region until the transplanted limbreached St. 24-25, regardless of the age of the host. Indeed,most host axons grew out and accumulated in the plexus regionof the younger transplanted limb. However, a few axons escapedthis region and projected into the grafted limb despite its relativelyimmature age, as shown in Figure 4E. Nevertheless, innervationof these young limbs always lagged behind that of the older hostlimb. Further examination of control embryos receiving sham operationsat St. 21 (see below) indicated that this operation resulted inthe death of some host neurons, most likely neurons whose axonswere severed during surgery. Thus, embryos in which younger limbbuds were transplanted onto older hosts were not studiedfurther.

Specificity of sensory and motor neuron projections after heterochronic limb transplantation

During normal development the axons from different segmental levels come together within the plexus region and sort out beforeprojecting selectively to their respective peripheral targets(Tosney and Landmesser, 1985b). As described above, we have shownthat the waiting period of axons in the plexus region essentiallycan be eliminated by transplanting an older limb bud onto a youngerhost embryo. In these embryos the axons grow into the transplantedlimb with little or no delay. Thus, we have used this preparationto ask whether the waiting period is essential for motor and sensoryneurons to establish their appropriate peripheralprojections.

To investigate this, we injected DiI into the sartorius, femorotibialis, or adductor muscle of eight embryos with graftedlimbs that were one to two stages older than their St. 30-32 hosts.The rostrocaudal distributions of labeled sensory and motor neuronsinnervating host and donor muscles were identical, as shown inthe longitudinal section in Figure 5A. Similar results were obtainedin one additional embryo sectioned longitudinally and in six embryossectioned transversely. Moreover, the transverse sections of operatedembryos showed that the mediolateral distribution of motor neuronsinnervating transplanted limbs was also normal. For example, adductormotor neurons innervating host and donor limbs were located medially(Fig. 5B), whereas sartorius motor neurons were located laterally(Fig. 5C). Thus, the peripheral projections of motor and sensoryneurons are established appropriately when axons grow into thelimb without first pausing within the plexus region. The possibilityexists, however, that there are subtle changes in innervationpatterns [for example, changes in spatial relationships amongsensory and motor axons in peripheral nerves (Honig et al., 1998)]when the waiting period is eliminated. Such changes would nothave been detected with the techniques used here.

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Figure 5. Sensory and motor axons project to the appropriate peripheral targets when the waiting period is eliminated by transplantation of an older donor limb. A, Longitudinal sections through the spinal cord and DRGs show that sensory and motor neurons innervating femorotibialis muscle in host (left) and donor (right) limbs are located in the same segments. Photographs are from adjacent sections of the same embryo. B, C, Transverse sections show that motor neurons innervating the adductor muscle in host and donor limbs are located medially (B), whereas sartorius motor neurons are located laterally (C).

Maturation of motor and sensory neurons after premature innervation of peripheral targets

Sensory and motor axons grow into grafted limbs several stages earlier than into host limbs after heterochronic transplantationof older donor limbs. To determine whether this premature innervationof peripheral targets accelerates neuronal maturation, we analyzedthree aspects of neuronal development in operated embryos $---$ programmedcell death, the development of central projections of sensoryneurons, and the biochemical maturation of sensoryneurons.

Programmed cell death
A cursory examination of transverse sections of operated embryos suggested that premature innervation of grafted limbs affectedprogrammed cell death. The lateral motor column (LMC) and DRGsthat innervated older, donor limbs appeared smaller than the respectivecontrol neuron populations (Fig. 6A-D). In contrast, the sizeof the LMC and DRGs was similar on the two sides of sham-operatedembryos (data not shown), indicating that the apparent reductionin the size of the LMC and DRGs after heterochronic limb transplantsresulted from the early innervation of targets in older donorlimbs rather than from the surgery itself. To quantify these apparentdifferences, we counted surviving motor neurons in the LMC throughoutthe entire lumbosacral region in six embryos and in segment LS3in five additional embryos (Table 1). Cell counts confirmed thatat most stages that were examined fewer motor neurons innervatedthe older transplanted limb. The difference in the number of motorneurons innervating the two limbs was not distributed across theentire LS region but instead was concentrated within one to twospinal segments in each embryo, again suggesting that this differencewas not simply an artifact of surgery. There was a tendency forthe biggest differences between control and experimental LMC tooccur at more rostral segmental levels in younger embryos andat progressively more caudal levels in progressively older embryos,mirroring the normal rostrocaudal progression of cell death (Gouldet al., 1999). For example, in embryo WP110 (St. 28: St. 29) thegreatest difference occurred in segment LS1 (host/graft = 1.23),whereas in embryo WP174 (St. 36: St. 36+) the greatest differenceoccurred in segment LS7 (host/graft = 1.68). Moreover, examinationof the LMC in a single segment, such as LS3, suggested that celldeath occurred independently in control and experimental LMC butthat programmed cell death had a head start on the experimentalside. The difference in the number of LS3 motor neurons innervatinghost and donor limbs in very young or relatively old embryos wasnegligible, but it was significant at St. 30-32 (p = 0.003; pairedStudent's t test). These results are explained most easily ifcell death had not yet begun at LS3 in the youngest embryos, waswell underway among motor neurons innervating St. 31-32 donorlimbs, and was complete on both sides of the oldest embryos.

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Figure 6. Innervation of older donor limbs accelerates the onset of naturally occurring cell death among motor (A, B) and sensory (C, D) neurons. Both the lateral motor column (A) and DRGs (C) that innervate older donor limbs (A, St. 32; C, St. 33) are smaller than those innervating the respective control host limbs (B, St. 30; D, St. 31). A and B are from a single representative section of segment LS3. C and D show the largest profile of DRG LS3 on each side of one operated embryo. There were no differences in the size of the lateral motor column or DRGs after sham operations (data not shown). E, TUNEL staining of a transverse section through a St. 29 embryo with an older donor St. 32 limb (left). Apoptotic motor and sensory neurons are more abundant among neurons innervating the older donor limb.


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Table 1. Relative number of motor and sensory neurons innervating older donor and host limbs

Sensory neuron survival was assayed by measuring the diameter of the largest profile of DRG LS3 on both sides of all operatedembryos. On average, DRG LS3 was ~10% larger on the control side(Table 1), suggesting that cell death also began earlier amongsensory neurons innervating older donorlimbs.
To verify that programmed cell death indeed did occur earlier in neurons innervating older limbs, we performed TUNEL stainingon sections of four embryos with grafted older limbs. Apoptoticcells were observed in the LMC and DRGs on the operated side beforethe onset of cell death on the control side, and apoptotic cellswere more abundant in the LMC and DRGs on the operated side atall stages that were examined (St. 28-St. 32) (Fig. 6E, Table2).


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Table 2. Relative number of apoptotic motor and sensory neurons in embryos with older donor limbs

Together, these results show that early target innervation accelerates the onset of programmed cell death. Possible mechanismsresponsible for triggering cell death prematurely are discussedbelow. Similar analyses were not performed in embryos with transplantedyounger limbs, because motor neurons were depleted after shamoperations performed at St. 21-22.

Central projections and biochemical maturation of sensory neurons
It is well established that peripheral targets can influence the development and specificity of central connections of muscleafferents (Wenner and Frank, 1995). Thus, we asked whether prematureinnervation of peripheral targets also accelerates the establishmentof central projections of sensory neurons. To test this possibility,we injected DiI into individual muscles (n = 8) or DRGs (n = 8)in embryos with grafted older limbs and examined the central projectionsof sensory neurons in transverse sections. During normal developmentsensory afferents at lumbosacral levels begin to arrive at theedge of the spinal cord (the dorsal root entry zone, or DREZ)by St. 25 but do not grow appreciably into the future gray matteruntil after St. 30 (Lee et al., 1988; Davis et al., 1989; Sharmaet al., 1994). The development of central projections followedthis time schedule on both control and operated sides, despitethe fact that sensory neurons reached their peripheral targetsseveral stages earlier on the operated side. For example, as shownin Figure 7A, sensory axons have not left the DREZ on either sideof this St. 29 embryo, although they innervate a St. 31 transplantedlimb. At later stages, once axons begin to invade the gray matter,the central projections are nearly identical on both sides, asillustrated in Figure 7B (St. 32 host: St. 34 graft). Similarresults also were observed in the eight other embryos that wereexamined for selectivity of peripheral projections (see above).

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Figure 7. Neither the development of central projections nor the biochemical maturation of sensory neurons is accelerated by premature innervation of peripheral targets. A, Sensory neurons that innervate an older donor limb (St. 31) do not invade the dorsal horn in advance of neurons innervating the host (St. 29) limb. B, The central projection of sensory neurons (arrows) that innervate a St. 34 transplanted limb are indistinguishable from those of neurons innervating the St. 32 host limb. C, D, There is no obvious difference in expression of either substance P (C) or trkA (D) in DRGs innervating transplanted and host limbs, although the donor limbs are approximately two stages older.

Several biochemical markers of sensory neurons begin to appear at approximately the time that axons reach their peripheraltargets, suggesting that the acquisition of these markers maybe triggered by target innervation. For example, substance P (Newand Mudge, 1986) and trkA (this study) are first detectable inlumbosacral DRGs at approximately St. 24-25, and staining becomesmore robust at later stages. To investigate whether the appearanceof these biochemical markers can be accelerated by early innervationof peripheral targets, we stained frozen sections of embryos withheterochronic limb transplants with anti-substance P and anti-trkAat selected embryonic stages. There was no obvious differencein expression of either substance P (Fig. 7C) or trkA (Fig. 7D)in DRGs on the host and experimental sides, although these DRGsinnervated St. 25-26 and St. 27-28 limbs,respectively.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Although "waiting periods" have been well documented in several systems (Tosney and Landmesser, 1985a; Shatz et al., 1990;Sharma and Frank, 1994), neither their underlying mechanisms northeir functional significance is well understood. The experimentsdescribed here address these issues for sensory and motor axonsthat wait in the plexus region of the hindlimb during embryonicdevelopment. By transplanting older or younger donor limbs tohost embryos, we have shown that axons wait in the plexus regionfor maturational changes to occur in the limb rather than in theneurons themselves. Neither sensory nor motor axons require aprolonged delay in the plexus region to project to their appropriateperipheral targets. Furthermore, our results suggest that prematuretarget contact can accelerate the onset of programmed cell deathbut does not enhance the development of central connections orbiochemical maturation of sensoryneurons.

Functional significance of the waiting period

Timing of sensory and motor outgrowth
Tosney and Landmesser (1985a) first described the waiting period of motor axons in the plexus region in the chick hindlimb.Their observation that outgrowth of sensory axons lags behindthat of motor axons (see Fig. 1) suggested, however, that sensoryaxons might enter the limb without pausing in the plexus region.We have shown that this is not the case. Sensory axons reach theplexus region only slightly later than motor axons, wait for ~1d, and then advance into the limb with the motor axons. Moreover,by eliminating either motor or sensory neuron precursors, we haveshown that the timing of outgrowth of each population is unaffectedby the presence or absence of the other. These observations areconsistent with our previous findings that sensory and motor innervationpatterns can develop independently in embryonic chick hindlimbs(Wang and Scott, 1999b).

What cues are responsible for the waiting period?
Why do axons wait in the plexus region and what allows them to leave? One possibility is that outgrowing axons are too immatureto respond to permissive cues in the limb. Alternatively, thelimb may not yet be favorable for axon growth. Our data from heterochroniclimb transplants support the latter hypothesis. Axons from hostembryos innervated donor limbs on a schedule dictated by the ageof the limb. This finding is consistent with previous work bySwanson and Lewis (1982), who mapped innervation patterns in embryosafter heterochronic wing transplants. Our studies, however, focusedon the initial ingrowth of axons into the limb, whereas the earlierstudies examined embryos at stages when innervation patterns werewell established. Thus, we have shown that the accelerated developmentobserved in earlier studies is attributable to axons growing intoolder donor limbs without first pausing in the plexusregion.
Our findings are also consistent with the observation that in vitro motor neurons will not grow on slices of limb taken fromSt. 22 embryos, but they will grow readily on slices from olderembryos (Landmesser, 1988), as if the younger limb tissue eitherlacks attractive factors or expresses inhibitoryfactors.
The molecular nature of the signals that permit axons to leave the plexus region and invade the limb is unknown. Candidatesinclude inhibitory and permissive molecules for which the expressionpattern changes at approximately the time that axons grow intothe limb [e.g., chondroitin-6-sulfate (Oakley and Tosney, 1991),ephA7 (Araujo et al., 1998), semaphorin III (Wright et al., 1995),various isoforms of laminin (Lentz et al., 1997)]. Clearly, discoveringthe signals that control axon growth into the limb and the mechanismsthat regulate their expression is a challengingtask.

Functional consequences of eliminating the waiting period

Specificity of target innervation
The plexus is an important region in which axons destined for individual targets come together, sort out, and make specificpathway choices (Lance-Jones and Landmesser, 1981; Tosney andLandmesser, 1985b,c). During normal development axons spend ~1d in the plexus region before projecting to their respective targets.Here we have shown that this prolonged delay is not required foraxons to project accurately to their appropriate peripheral targets.The distributions of motor and sensory neurons retrogradely labeledfrom individual muscles in host and older transplanted limbs wereindistinguishable, despite the fact that axons grew into the donorlimbs with little or no delay. Whether the waiting period canbe eliminated in other systems without affecting the accuracyof target innervation isunknown.

Neuronal maturation

After transplantation of older donor limbs, host neurons project to limbs that are one to three stages more mature than hostlimbs. Because peripheral targets clearly can influence some aspectsof neuronal phenotype [e.g., neuronal survival (Calderó et al.,1998), peptide expression (McMahon and Gibson, 1987), centralconnectivity (Wenner and Frank, 1995)], we asked whether innervationof older, more mature targets that occurs after heterochroniclimb transplantation would accelerate neuronalmaturation.

Programmed cell death
For example, programmed cell death of motor and sensory neurons normally is regulated by their peripheral targets (Hollydayand Hamburger, 1976; Carr and Simpson, 1978; Calderó et al.,1998). We found that fewer healthy motor and sensory neurons andmore apoptotic neurons innervated older donor limbs than innervatedthe control limb in the same embryo. Several lines of evidenceindicate that these differences reflect the precocious onset ofcell death. First, decreased production of neurons is unlikelyto contribute to the observed differences because the peripherydoes not appear to influence neuron proliferation (Hollyday andHamburger, 1976; Calderó et al., 1998). Second, neuron numberwas not altered in sham-operated embryos. Third, the numbers ofsurviving motor neurons on each side of operated embryos weresimilar to values previously reported for embryos of the sameage as the respective limbs (Calderó et al., 1998). Finally,the overall pattern of neuronal survival, as described in Results,mirrored the general rostrocaudal progression of cell death (Gouldet al., 1999). Such consistencies would not be expected if thereduction in neuron number were an artifact ofsurgery.
Why does innervation of older donor limbs trigger the early onset of neuronal cell death? The most parsimonious explanationis that axons that innervate older donor limbs contact peripheraltargets earlier than usual. During normal development the neuronsrequire target-derived neurotrophic factors for survival (Oppenheim,1991). Production of neurotrophic factors and neuronal dependenceon these factors first appear at approximately the time that axonscontact peripheral targets (Davies et al., 1987; Vogel and Davies,1991). In vitro, premature exposure to neurotrophic factors triggerspremature dependence on these factors (Vogel and Davies, 1991).Thus, in our experiments the precocious innervation of transplantedlimbs most likely caused the precocious dependence of host neuronson limb-derived trophic factors, thereby accelerating the onsetof naturally occurring celldeath.

Central projections and biochemical maturation of sensory neurons
During normal development sensory neurons also observe a waiting period before projecting to targets in the spinal cord (Leeet al., 1988; Davis et al., 1989; Sharma et al., 1994). This waitingperiod was still observed by sensory neurons in operated embryos.Central projections developed on schedule and were not acceleratedby premature innervation of older donor limbs. This perhaps isnot surprising, because cells in the dorsal horn express inhibitorymolecules such as collapsin (Shepherd et al., 1996, 1997) whensensory axons first arrive there. Growth-promoting molecules suchas slit2 protein (Wang et al., 1999) begin to appear and collapsindisappears (Shepherd et al., 1996, 1997) at approximately thetime that axons invade the gray matter. Whereas it is clear thatperipheral targets can determine the central connections of sensoryneurons (Wenner and Frank, 1995), our results show that precociousinnervation of these targets does not promote sufficient maturationof either sensory neurons or the spinal cord to accelerate theestablishment of centralconnections.
Similarly, expression of substance P and trkA in DRG neurons was not obviously enhanced by innervating the older donor limbs.This finding is surprising in light of the observation that theperipheral target can regulate expression of substance P in matureanimals (McMahon and Gibson, 1987). What normally triggers expressionof substance P is unknown. Our results with trkA, however, areconsistent with the observation that expression of trkA in developingsensory neurons is not modulated by NGF (Davies et al., 1995),which normally is produced by targets of NGF-dependent neurons.Further experiments will be necessary to elucidate the mechanismsand signals that regulate the appearance of these biochemicalmarkers in sensory neurons. Clearly, simple contact with a peripheraltarget is notsufficient.
Much is still unknown about target influences on neuronal differentiation. Here we have shown that our ability to manipulatethe relative timing of target innervation can be exploited todiscriminate between direct target-related and intrinsic eventsin neuronal development. The molecular signals responsible fortarget influences remain to beelucidated.

  FOOTNOTES

Received March 8, 2000; revised April 24, 2000; accepted May 1, 2000.

This work was supported by National Institutes of Health Grant NS16107 to S.A.S. We thank Drs. S. M. Cahoon-Metzger, M. L.Condic, and M. S. Rao for helpful comments on this manuscript.We also thank Dr. F. B. Lefcort for her generous gift of trk antibodies.Antibodies 3A10 (developed by Drs. T. M. Jessell and J. Dodd)and QCPN (developed by Drs. B. and J. Carlson) were obtained fromthe Developmental Studies Hybridoma Bank developed under the auspicesof the National Institute of Child Health and Human Developmentand maintained by The University of Iowa, Department of BiologicalSciences, Iowa City, IA52242.
Correspondence should be addressed to Dr. Sheryl A. Scott, Department of Neurobiology and Anatomy, University of Utah Schoolof Medicine, 50 North Medical Drive, Salt Lake City, UT 84132.E-mail: sheryl.scott{at}hsc.utah.edu.

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RESULTS
DISCUSSION
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