Steroid-Induced Dendritic Regression Reduces Anatomical Contacts between Neurons during Synaptic Weakening and the Developmental Loss of a Behavior

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The Journal of Neuroscience, February 15, 2003, 23(4):1406

Steroid-Induced Dendritic Regression Reduces Anatomical Contacts between Neurons during Synaptic Weakening and the Developmental Loss of a Behavior
John R. Gray and Janis C. Weeks
Institute of Neuroscience, University of Oregon, Eugene, Oregon 97403-1254

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Steroid hormones alter dendritic architecture in many animals, but the exact relationship between dendritic anatomy, synapticstrength, and behavioral expression is typically unknown. In larvaeof the moth Manduca sexta, the tip of each abdominal proleg (locomotoryappendage) bears an array of mechanosensory hairs, each innervatedby a planta hair sensory neuron (PH-SN). In the CNS, PH-SN axonsmake monosynaptic, excitatory nicotinic cholinergic connectionswith accessory planta retractor (APR) motoneurons. These synapsesmediate a proleg withdrawal reflex behavior that is lost at pupation.The prepupal peak of ecdysteroids (molting hormones) triggersthe regression of APR dendrites and a >80% reduction in the amplitudeof EPSPs produced in APRs by PH-SNs that innervate posterior plantahairs. The present study tested the hypothesis that a decreasein the number of synaptic contacts from PH-SNs to APRs contributesto this synaptic weakening. Pairs of PH-SNs and APRs were fluorescentlylabeled in larvae and pupae, and the number of indistinguishablyclose anatomical contacts (putative synapses) was counted by confocallaser scanning microscopy. During APR dendritic regression, themean number of contacts from posterior PH-SNs decreased by ~80%,whereas the size of individual contacts did not change detectablyand the axonal arbors of PH-SNs did not regress. These resultssuggest that the steroid-induced regression of motoneuron dendritesphysically disconnects the motoneurons from the synaptic terminalsof sensory neurons, producing synaptic weakening and the developmentalloss of the proleg withdrawal reflex behavior atpupation.

Key words: steroid hormone; dendrite; synapse; Manduca sexta; development; confocal microscopy

  Introduction

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Steroid hormones can profoundly alter the size and complexity of dendritic arbors (for review, see García-Segura et al.,1994; Weeks and McEwen, 1997; McEwen, 2000). For example, in femalerats, the rise and fall of estradiol during the estrous cycleregulates the cyclical increase and decrease in dendritic spinedensity on hippocampal pyramidal cells (for review, see Woolley,1998). In male rats, androgen levels regulate the size of thedendritic arbors of motoneurons in the spinal nucleus of the bulbocavernosus(Kurz et al., 1986). Natural or experimentally induced changesin steroid hormone levels that alter dendritic architecture oftensimultaneously alter an animal's behavior; e.g., high estradiollevels at proestrous promote lordosis behavior in females, whereascirculating androgens support copulatory behavior in male rats.It is logical to assume that steroid-induced changes in dendriticarbors are accompanied by changes in synaptic connectivity (Matsumotoet al., 1988; Yankova et al., 2001) that contribute to changesin behavior. However, direct demonstration of this presumed chainof events in any one system islacking.

During metamorphosis of the moth Manduca sexta, steroid hormones [ecdysteroids, including 20-hydroxyecdysone (20E)] regulatedramatic changes in neurons and behavior (for review, see Levineand Weeks, 1989; Fahrbach and Weeks, 2002). A "prepupal peak"of 20E at the end of larval life triggers dendritic regressionin motoneurons (see Fig. 1A) (Weeks et al., 1992), which are subsequentlyrespecified for new functions (accompanied by dendritic regrowth)or eliminated by cell death during the pupal stage (Weeks andTruman, 1985; Weeks and Ernst-Utzschneider, 1989; Weeks et al.,1992; Kent and Levine, 1993; Duch and Levine, 2000). Pupationalso involves the loss of many larval behaviors, including theproleg withdrawal reflex (Weeks and Jacobs, 1987). This reflexis triggered by the deflection of the mechanosensory hairs locatedon the tip of each abdominal proleg (locomotory appendage) (seeFig. 1B) (Wiel and Weeks, 1996). Each hair is innervated by asingle planta hair sensory neuron (PH-SN) (Peterson and Weeks,1988), which makes monosynaptic, excitatory nicotinic cholinergicconnections with the accessory planta retractor (APR) motoneuronand related motoneurons. The proleg withdrawal reflex is mediatedby these direct sensorimotor synapses plus indirect interneuronalpathways (see Fig. 1C) (for review, see Weeks et al., 1997).

Streichert and Weeks (1995) showed that the mean amplitude of EPSPs evoked in APRs by PH-SNs decreases significantly (by ~40-80%,depending on PH-SN location) when APR dendrites regress (see Fig.1D), although APR input resistance increases. They also providedindirect evidence that the size of PH-SN arbors does not changeduring this time. These findings suggested that decreased EPSPamplitude was associated with the physical disconnection of APRdendrites from the synaptic terminals of PH-SNs. The present studysupported this hypothesis by demonstrating a developmental decreasein the number of close anatomical appositions between PH-SNs andAPRs. These findings suggest that steroid-induced dendritic regressionplays a key role in synaptic weakening and the elimination ofa behavior during postembryonic life. Some results have been publishedpreviously in abstract form (Gray and Weeks, 1999).

  Materials and Methods

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Animals. M. sexta were reared individually on an artificial diet [modified from Bell and Joachim (1976)] under a 17/7 hr light/darkphotoperiod and a 27/25°C temperature cycle. Insects were stagedusing standard developmental markers (see Fig. 1A). The day ofecdysis (cuticle shedding) to the fifth (final) larval instaris designated day L0, followed by days L1, L2, and L3. The onsetof metamorphosis is marked by wandering behavior (day W0), whenlarvae cease feeding and seek a pupation site. The day of ecdysisto the pupal stage is designated day P0. All comparisons in thisstudy were made between insects on day L3 and dayP0.

Fluorescence labeling of sensory and motoneuron pairs. The PH array on each proleg tip is divisible into anterior, middle,and posterior regions. The axon of each PH-SN projects into theganglion of the same abdominal segment, where the axon terminalsform a somatotopic map based on the position of the PH in thearray (Peterson and Weeks, 1988). The terminals of posterior PH-SNsremain within the ganglion of the same body segment, whereas anteriorand middle PH-SNs send axons into neighboring ganglia and arborizethere as well (Peterson and Weeks, 1988; Streichert and Weeks,1995). We used posterior PH-SNs in the present study because therestriction of their terminals to a single ganglion facilitatedcomplete staining of the entire axonal arbor (seebelow).

To stain an individual posterior PH-SN, insects were selected on day L2, anesthetized by chilling on ice for 45 min, placedventral side up in a Petri dish, and immobilized with strips ofdental wax. The dish was filled with chilled water to a leveljust above the spiracles (respiratory openings) to maintain anesthesia.A well of petroleum jelly was formed around the tip of a prolegin abdominal segment 3 (A3) and filled with distilled water (dH₂O).A single PH from the most ventral (distal), posterior region ofthe PH array was cut at its base using iridectomy scissors. After10 min, the dH₂O in the well was replaced with a solution of ~1%tetramethylrhodamine dextran (molecular weight, 3000; MolecularProbes, Eugene, OR; henceforth termed rhodamine) in dH₂O. Thewater covering the spiracles was removed, and the immobilizedlarva was held at 4°C for 36-48 hr to reversibly arrest developmentand movement. The dye and petroleum jelly were then removed, andthe larva was returned to standard rearing conditions to continuedevelopment.

Animals with a stained posterior PH-SN were selected on either day L3 or day P0. Day L3 larvae were identified by their sizeand the presence of "frosted frass," signaling the occurrenceof the commitment pulse of 20E (Fig. 1A) (Nijhout and Williams,1974). Day P0 pupae were used for experiments within 1 hr of completingecdysis. Insects were sometimes held at 4°C for up to 24 hr toarrest development, before dissection. Animals were anesthetizedon ice and opened dorsally under saline (see below), and ganglionA3 was removed with the lateral branch of the ventral nerve (VN_L)left long on the side ipsilateral to the stained PH-SN. VN_L carriesthe axons of the two APRs that innervate the ipsilateral retractormuscle and receive monosynaptic EPSPs from ipsilateral PH-SNs(Sandstrom and Weeks, 1996). Ganglia were placed ventral sideup in a Sylgard-coated dish containing physiological saline composedof (in mM): 140 NaCl, 5 KCl, 4 CaCl₂, 28 glucose, and 5 HEPES,pH 7.4 (Trimmer and Weeks, 1989); they were then desheathed withfine forceps (Weeks and Jacobs, 1987) and observed under a WildM3C dissecting microscope (Leica Microsystems, Bannockburn, IL)using substage dark-field illumination to visualize APR cell bodies.

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Figure 1. Steroid-mediated regression of APR dendrites and dismantling of the proleg withdrawal reflex during the larval-pupal transformation of Manduca. A, top, Camera lucida drawings show individual APRs stained with cobalt chloride on day L3 (left) and day P0 (right). The outline of an abdominal ganglion is shown, with the anterior end up. The APR dendritic arbor is significantly reduced on day P0 (Streichert and Weeks, 1995; Sandstrom and Weeks, 1998). The timeline illustrates changes in relative hemolymph levels of ecdysteroids (solid line) and juvenile hormone (dashed line) from the late fourth larval instar to the early pupal stage [hormone titers redrawn from Bollenbacher et al. (1981) and Riddiford and Truman (1994)]. Developmental days relevant to this study are indicated along the horizontal axis. During the fifth (final) instar, the juvenile hormone titer drops and is followed by a small rise in ecdysteroids (20E) on day L3, termed the commitment pulse, and a larger rise in 20E spanning days W1 to P0, termed the prepupal peak. The rise of the prepupal peak of 20E triggers dendritic regression in proleg motoneurons (bold vertical arrow) (Weeks and Truman, 1985, 1986; Weeks, 1987; Weeks et al., 1992). E, Ecdysis (shedding of the cuticle from the previous stage; indicated by vertical dotted lines); L0, day of ecdysis to the fifth larval instar; L1, L2, etc., days after L0; P0, day of ecdysis to the pupal stage; W0, day of wandering (when the larva ceases feeding and burrows underground); W1, W2, etc., days after wandering. B, Lateral view of a Manduca larva (anterior to the left) with the proleg in abdominal segment 4 enlarged (inset) to illustrate the dense array of PHs (enclosed by dashed oval) near the proleg tip. C, Neural circuit for the proleg withdrawal reflex in Manduca larvae. The proleg tip (left), a proleg retractor muscle (middle), and ganglion of the same abdominal segment (right; anterior is up) are shown schematically. Neurons are indicated by filled circles. Each PH is innervated by a single sensory neuron with a cell body in the proleg epidermis and an axon that projects to the ganglion. PH-SNs excite ipsilateral proleg retractor motoneurons (MN), including the APR, via monosynaptic, nicotinic cholinergic (ACh) synapses and polysynaptic pathways through interneurons (INs) (reviewed by Weeks et al., 1997). The diagram shows the reflex circuit for the left proleg in a body segment; the circuit is duplicated for the right proleg (not shown). The ability of sensory input to evoke motor output via the circuit weakens dramatically during the larval-pupal transformation (Jacobs and Weeks, 1990; Streichert and Weeks, 1995). D, The size of EPSPs produced in APRs by PH-SNs decreases during the larval-pupal transformation. Traces show intracellular recordings from an APR on day L3 (top) and a different APR on day P0 (bottom) while stimulating action potentials in a PH-SN located in the posterior region of the PH array to evoke monosynaptic EPSPs (signal-averaged from multiple trials; APR resting membrane potential set at $-$ 60 mV). No EPSP was detectable on day P0. Data are from Streichert and Weeks (1995).

The cell body of an APR ipsilateral to the stained PH-SN was impaled with a borosilicate microelectrode filled at the tipwith 4% Lucifer yellow CH (Molecular Probes) and backfilled with0.5 M LiCl₂ (electrode resistance, ~30 M $Omega$ ). APR was identifiedby its characteristic cell-body position and time-locked extracellularaction potential recorded in the ipsilateral VN_L by means of asuction electrode led to a differential, alternating-current-coupledpreamplifier (Sandstrom and Weeks, 1996). Lucifer yellow was iontophoresedinto APR using 5-10 nA hyperpolarizing current pulses (500 msec,1 Hz) generated by a Grass 88 stimulator (Grass Instruments, WestWarwick, RI) connected to a Getting M5 intracellular amplifier(Getting Instruments, San Diego, CA). APRs were filled for atleast 20 min or until action potentials were no longer detected.The electrode was withdrawn, VN_L was crushed near the ganglion,and the preparation was left at room temperature for 30-45 minin the dark to permit dye diffusion. The ganglion was then fixedovernight in 4% paraformaldehyde at 4°C, rinsed in PBS for 10min, mounted on a poly-L-lysine-coated coverslip, dehydrated inan ascending series of ethyl alcohol, cleared in xylene, and mountedventral side up in DPX mounting medium (Electron Microscopy Sciences,Fort Washington, PA). Slides were stored in the dark at room temperatureuntil observed, usually within 2-4d.

Confocal imaging. The quality of double fills was first assessed under epifluorescence using a Leitz (Wetzlar, Germany) LaborluxD compound microscope. If staining of the PH-SN and the APR appearedto be successful, the ganglion was then examined on a Zeiss (Oberkochen,Germany) LSM 310 confocal laser scanning microscope. Rhodaminefluorescence (red) was excited with a 568 nm laser line and detectedthrough a 590 nm long-pass filter. Lucifer yellow fluorescence(green) was excited with a 488 nm laser line and detected througha 515-565 nm bandpass filter. To visualize anatomical contacts,ganglia were scanned using a 63× oil immersion objective [numericalaperture (NA), 1.25]; at this magnification, the entire x,y extentof the PH-SN arbor was contained within the field of view (seeFig. 4). Four scans of 1024 × 1024 pixels were averaged for eachoptical section, which were taken at 0.5 µm intervals. This methodproduced images with a voxel resolution of 0.2 × 0.2 × 0.9 µmin the x-, y-, and z-planes, respectively. For two-dimensionalprojections of optical sections, the total depth of tissue sampledwas computed as [(number of intervals × 0.5 µm) + 0.9 µm]. Toensure that scans in the two channels were in register, each opticalsection was scanned in the rhodamine channel and the Lucifer yellowchannel before moving to the next optical section. False colorwas used to identify the rhodamine (red) and Lucifer yellow (green)channels. The scanned volume contained the entire axonal arborof the PH-SN and the portion of APR dendritic arbor that was coextensivewith the PH-SN arbor. Accordingly, all potential sites of contactbetween a PH-SN and APR were imaged. A subset of putative synapticcontacts (see Fig. 5) was examined at higher magnification (63×oil immersion objective and 3× hard magnification in thesoftware).

The APR dendritic field spans the entire dorsoventral extent of the ganglion (Weeks and Jacobs, 1987) and extends more anteriorlythan does the PH-SN arbor (see Fig. 7A). We did not image theentire APR dendritic arbor in double fills, because only the portionof the arbor that contacts PH-SNs was relevant to this study,and photobleaching of Lucifer yellow became a factor during theprolonged scanning required to visualize the entire APR arbor.In a few cases, the entire APR arbor was scanned using a 40× waterimmersion objective (NA, 1.2), which provided a larger field ofview (see Fig. 2).

Identification of putative synaptic contacts. Only ganglia in which the arbors of both the PH-SN and the APR were completelyand brightly stained in confocal images were used to count anatomicalappositions. Staining was determined to be complete when adjacentsegments of the processes of a neuron were continuous within eachoptical section and between adjacent sections, up to the pointof termination of the process; i.e., there were no "gaps." Stainingquality was also readily assessed by comparison with images ofthe same neurons stained with cobalt chloride (Weeks and Jacobs,1987; Peterson and Weeks, 1988; Streichert and Weeks, 1995; Sandstromand Weeks, 1996). Successful staining of APRs was routine, butonly a low proportion of PH-SNs were completely and brightly stained(Melville et al., 2003). Accordingly, the number of ganglia containingan acceptably stained pair of neurons was small (n = 4 on dayL3; n = 3 on day P0; see Results). Examination of less well stainedmaterial (data not shown) supported the conclusions based on gangliaused for quantitativeanalysis.

The series of optical sections from each ganglion was imported into Scion Image (Scion Corporation, Frederick, MD). The PH-SN(red) and APR (green) channels from each optical plane were combinedinto a single frame, and all frames from a ganglion were combinedinto a stack. Individual frames from each stack were displayedon a monitor and scored by eye for sites at which (1) pixels inthe red and green channels overlapped (in which case the pixelsappeared yellow) or (2) pixels in the red and green channels abuttedwith no discernible gap between (see Fig. 5) (Lamotte d'Incampset al., 1998). We refer to sites of indistinguishably close anatomicalcontact in single frames as appositions. Three independent observers,who were kept unaware of the identity of the material, markedeach apposition in each frame of each stack, without referringto adjacent frames. An apposition was included in the final dataset when it was scored by at least two of the three observers;~90% of appositions were identified by all three observers. Asmall number of appositions (~8%) were eliminated from the finaldata set when reconstruction of the PH-SN arbor (see below) revealedthat these sites lay outside of the PH-SN arbor, resulting fromerrant pixels in the rhodamine channel. Because of the narrowoptical section thickness, appositions were often present in asimilar x,y-location in consecutive frames. Counts of appositionswere converted to counts of putative synaptic contacts (see Results)by eliminating duplicate counts of the same anatomical contactthat was imaged in multiple consecutive frames. Thus, each putativesynaptic contact was made up of one or more appositions scoredin adjacentframes.

PH-SN morphometrics. The red channel was used to generate a stack of the PH-SN axonal arbor, which was reconstructed in threedimensions using a National Institutes of Health tree-tracingmacro written by Dr. D. K. Hartline (University of Hawaii, Honolulu,HI; www.pbrc.hawaii. edu/~danh/Resources/treetracedoc.html). Totalbranch length and the number of branch points was measured foreach reconstructed PH-SN. Reconstructions were then recombinedwith the x-, y-, and z-coordinates of the scored contacts to determinethe distribution of putative synaptic contacts on the PH-SNarbor.

Statistical analysis. All statistical comparisons were performed using SigmaStat 2.0 statistical software (Jandel Scientific,San Rafael, CA). Differences were considered to be significantwhen p < 0.05.

  Results

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

APR regresses while PH-SN axonal arbors remain stable

Previous quantitative studies demonstrated that the APR dendritic arbors in segments A3-A6 regress significantly between daysL3 and P0 (Streichert and Weeks 1995; Sandstrom and Weeks, 1998);for these measurements, APRs were stained with cobalt chloride,the complete dendritic arbor was drawn as a two-dimensional projection,and the density of neuronal processes was calculated. In the presentexperiments, APRs were stained by the intracellular injectionof Lucifer yellow. For technical reasons (see Materials and Methods),in ganglia that contained both a stained APR and a stained PH-SN,only the portion of the arbor of the APR that overlapped withPH-SN axon terminals was imaged. Therefore, we did not obtainquantitative measurements of the APR dendritic extent that couldbe compared directly with previous data. However, to verify thatdendritic regression is apparent in Lucifer yellow-stained motoneurons,the complete arbor of the APR was imaged in ganglia that werenot used to count appositions with PH-SNs. Similar to observationsin cobalt-stained material (Weeks and Jacobs, 1987; Weeks andErnst-Utzschneider, 1989; Streichert and Weeks, 1995; Sandstromand Weeks, 1998), the neurites of APR were densely arrayed withfine, high-order processes that resembled dendritic spines (Fig.2A,B). In other insect neurons, these processes typically bearinput synapses (Peters et al., 1985) (see Discussion). The characteristicloss of dendrites between days L3 and P0 was readily apparentin Lucifer yellow-stained APRs (Fig. 2A,B); most major neurites(except those in posterior neuropil) were retained, whereas thedensity of smaller, higher-order branches decreased. Likewise,in ganglia used to count appositions, in which only the portionof the arbor of APR located within sensory neuropil was imaged,the dendritic extent of APR was markedly reduced on day P0 (seeFigs. 4, 7). These observations confirm that APRs undergo substantialdendritic loss between days L3 and P0 (Jacobs and Weeks, 1990;Streichert and Weeks, 1995; Sandstrom and Weeks, 1998).

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Figure 2. Morphology of APRs and posterior PH-SNs in larvae and pupae. Each panel is a two-dimensional projection of a stack of 0.5 µm optical sections obtained with a confocal laser scanning microscope, showing the complete extent of the central arbor of APR (A, B) or a posterior PH-SN (C, D) on day L3 (left) or day P0 (right). APRs were stained with Lucifer yellow; PH-SNs were stained with tetramethylrhodamine dextran. Anterior is up; insets show drawings of abdominal ganglia with the typical locations of an APR (A) or a posterior PH-SN (C) illustrated. A, B, The cell body of the APR appears at the left, the dendritic arbor extends to the right, toward the ganglionic midline, and the axon projects laterally and posteriorly to exit the ganglion via a segmental nerve. The variation in cell body location and neuritic branching shown here is typical (Sandstrom and Weeks, 1996). Most APR dendrites are located in dorsal and intermediate neuropil, with a less extensive projection into ventral sensory neuropil (Weeks and Jacobs, 1987). The APR dendritic arbor is less extensive on day P0 than on day L3, especially in posterior neuropil (note the loss of processes posterior to the exit of the axon from the neuropil at the arrow). C, D, The axon (arrowhead) of each posterior PH-SN enters the neuropil from a segmental nerve and arborizes within ventral sensory neuropil. The central arbors of PH-SNs map somatotopically within the CNS based on the position of the hair on the proleg (Peterson and Weeks, 1988). Posterior PH-SNs arborize in the middle and posterior regions of ipsilateral neuropil. PH-SN arbors are similar in extent on days L3 and P0. Scale bars: (in B) A, B, 50 µm; (in D), C, D, 30 µm.

Streichert and Weeks (1995) provided evidence that the axonal arbors of PH-SNs do not regress between days L3 and P0, butthey did not quantify this observation specifically for the posteriorPH-SNs used in the present study. Therefore, from three-dimensionalreconstructions of individual rhodamine-stained, posterior PH-SNs(Fig. 2C,D), we determined the mean number of branch points andtotal branch length of the central axonal arbors on days L3 andP0. Figure 3 shows that neither measure changed significantlyduring this period of development. As described previously incobalt-stained material (Peterson and Weeks, 1988), the centralaxonal arbors of larval and pupal PH-SNs stained with rhodaminewere characterized by relatively smooth lengths of neurite punctuatedby varicosities (Fig. 2C,D, see also Figs. 4, 5, 7). In otherinsect neurons, similar varicosities are presynaptic boutons (Peterset al., 1985). The lack of axonal regression in PH-SNs is expected,given that these neurons are not respecified for new roles duringmetamorphosis (see Discussion).

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Figure 3. The central axonal arbors of posterior PH-SNs do not regress during the larval-pupal transformation. Columns indicate the mean number of branch points, and the total branch length, of the axonal arbors of posterior PH-SNs measured on day L3 (black columns; n = 5) and on day P0 (white columns; n = 4). Error bars indicate SEM. The means on days L3 and P0 did not differ significantly (Student's t test).

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Figure 4. Anatomical relationship between processes of posterior PH-SNs and APRs. Each panel shows a two-dimensional projection of five sequential frames (equal to 3.4 µm depth of neuropil) containing a Lucifer yellow-stained APR (green) and a rhodamine-stained posterior PH-SN (red). Images are oriented as in Figure 2 (anterior up). Counts of indistinguishably close anatomical juxtapositions scored as appositions in single confocal frames were converted to counts of putative synaptic contacts (arrows; see Materials and Methods). In this example, there were 15 putative synaptic contacts (represented by 21 appositions; data not shown) on day L3 and two putative synaptic contacts (represented by 4 appositions; data not shown) on day P0. An asterisk marks the putative synaptic contact shown at higher magnification in Figure 5A. The scale bar refers to both panels.

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Figure 5. Putative synaptic contacts between posterior PH-SNs and APRs viewed at higher magnification. A, Seven sequential frames that spanned the volume of neuropil containing the putative synaptic contact marked with an asterisk in Figure 4. Numbers at the bottom right of each panel indicate the depth of the section compared with the first image in the series. Overlapping appositions (arrows) between the PH-SN (red) and APR (green), indicated by yellow pixels, occurred in four consecutive frames, indicating that this putative synaptic contact spanned a depth of ~2.9 µm. B, One frame from a different preparation on day L3 in which the processes of a posterior PH-SN and an APR abutted with negligible overlap (arrow). The scale bar refers to all panels.

These findings support the hypothesis that the axonal arbors of PH-SNs remain stable between days L3 and P0 while the dendriticarbors of their postsynaptic targets, the APR motoneurons,regress.

Identification of putative synaptic contacts between APRs and PH-SNs

We tested the hypothesis that the developmental weakening of the synapses from posterior PH-SNs to APRs is associated witha decrease in the number of synaptic contacts between the presynapticand postsynaptic neurons. From each ganglion that contained apair of completely and brightly stained neurons, we acquired aseries of confocal optical sections at 0.5 µm intervals that spannedthe entire volume of the PH-SN axonal arbor. Thus, all sites ofpotential anatomical contact between the PH-SN and APR were imaged.The depth of tissue sampled to image the complete PH-SN arborwas 38 ± 4 µm (mean ± SEM) on day L3 (n = 4) and 50 ± 8 µm onday P0 (n =3).

In each optical plane, the images acquired in the red (PH-SN) and green (APR) channels were combined into a single frame.The frames were scored by multiple observers blind to the identityof the material for appositions in which pixels in the red channeloverlapped with, or directly abutted, pixels in the green channel(see Materials and Methods). Some anatomical appositions appearedin multiple adjacent frames (Figs. 4, 5), so the counts of appositionswere converted to counts of putative synaptic contacts by eliminatingduplicate counts of the same anatomical apposition that appearedin more than one frame (see Materials and Methods). We use theterm putative to refer to synaptic contacts because it is notpossible to confirm the presence of active zones or functionalsynaptic transmission based on confocal microscopy (see Discussion).Similar methods have been used to identify putative synaptic contactsin other preparations (e.g., axo-axonic contacts of Ib fibersin cat spinal cord) (Lamotte d'Incamps et al., 1998).

Figure 4A,B shows representative confocal images from days L3 and P0, depicting the same volume of sensory neuropil (3.4 µmdepth) at both developmental stages. Arrows mark putative synapticcontacts between the axonal arbor of a posterior PH-SN and theAPR dendritic arbor. More putative synaptic contacts were apparenton day L3 than on day P0 (see quantitative comparisons below).Putative synaptic contacts between PH-SNs and APRs are shown athigher magnification in Figure 5. Figure 5A shows seven consecutiveframes spanning the contact marked by an asterisk in Figure 4A;appositions were scored in four consecutive frames, indicatedby overlap of the red and green channels. Figure 5B shows a singleframe from a different preparation illustrating a PH-SN varicosity(red) and an APR dendrite (green) that abutted with negligibleoverlap.

The number of putative synaptic contacts decreases during the larval-pupal transformation, but contact size does not change

Figure 6A compares the number of putative synaptic contacts between posterior PH-SNs and APRs on days L3 and P0. The meannumber of putative contacts decreased significantly from 42 to9 over this period of development, representing a 79% decrease.Concomitantly, the mean amplitude of EPSPs produced in APRs byposterior PH-SNs is ~0.30 mV on day L3 and ~0.05 mV on day P0(Fig. 1D) (Streichert and Weeks, 1995) (see Discussion).

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Figure 6. Quantification of the number and size of putative synaptic contacts between posterior PH-SNs and APRs on days L3 and P0. A, Columns indicate the mean number of putative synaptic contacts between posterior PH-SNs and APRs on day L3 (black column; n = 4) and on day P0 (white column; n = 3). Error bars indicate SEM. The number of putative synaptic contacts was significantly reduced on day P0. *p < 0.001; Student's t test. B, The putative synaptic contacts identified in all preparations on day L3 (n = 167 contacts) and on day P0 (n = 28 contacts) were divided into categories based on the number of adjacent frames (at 0.5 µm intervals) in which the contact appeared (range, 1-7 frames). The proportion of contacts in each category is expressed as a percentage of the total number of contacts counted at that stage. There were no significant differences in the proportion of contacts in each size category (i.e., contacts observed in one frame, two frames, etc.) on days L3 and P0 ( $chi$ ² analysis).

Synaptic strength can be influenced by both the number of contacts between presynaptic and postsynaptic neurons and the sizeof each synaptic contact; larger contacts may contain more activezones and release more neurotransmitter (Grantyn et al., 1984).Having demonstrated a developmental decrease in the number ofputative synaptic contacts between PH-SNs and APRs (Fig. 6A),we tested whether the size of the contacts changed. Optical sectionthickness was constant (0.5 µm), so the number of adjacent framesin which a putative synaptic contact appeared provided a roughestimate of the size of the contact. The number of adjacent framesin which individual contacts appeared ranged from 1 to 7, witha mean of 1.74 ± 0.12 (SEM) frames on day L3 (n = 167) and 1.90± 0.30 frames on day P0 (n = 28). These values did not differsignificantly (Student's t test). Conversion of these figuresto physical dimensions provides an estimate of the mean size ofputative synaptic contacts (measured along the z-axis) of 1.25-1.35µm (range, 0.5-4.4 µm). These values are similar to the sizesof contacts observed in the x,y-plane (Fig. 5) and appropriatefor insect central synapses (seeDiscussion).

We also compared the proportion of contacts that fell into different size categories at the two developmental stages. Figure6B shows that the distribution of contact size was similar ondays L3 and P0; most contacts appeared in only one or two adjacentframes, and >90% of the contacts appeared in three or fewer frames.The proportion of putative synaptic contacts in each size categorydid not differ significantly on days L3 and P0 (Fig. 6B). Thus,the number of putative synaptic contacts between PH-SNs and APRsdecreased between days L3 and P0, but the size of the contactsdid not changedetectably.

We did not image the complete APR dendritic arbor in ganglia containing a stained PH-SN (see above), so we did not reconstructthe three-dimensional structure of the motoneuron and determinethe spatial distribution of putative synaptic contacts from PH-SNs.Qualitatively, most putative synaptic contacts from posteriorPH-SNs occurred on the high-order branches of APR and not on largeneuritic trunks (Figs. 4, 5). However, because we obtained a completeimage of each PH-SN arbor, it was possible to reconstruct thesensory neuron arbors in three dimensions and to map the locationsof putative synaptic contacts with APR. Figure 7A shows representativereconstructions of posterior PH-SNs, displayed as two-dimensionalprojections, with the portion of the APR dendritic arbor thatoccupied the same volume of neuropil superimposed. The size ofthe APR dendritic arbor that was coextensive with the PH-SN axonalarbor was substantially reduced on day P0. Figure 7B shows thesame PH-SN reconstructions as in Figure 7A, with putative synapticcontacts with APR marked. As documented above (Fig. 3), the sizeof PH-SN axonal arbors appeared similar on days L3 and P0. Inthis example, there were 43 putative synaptic contacts from thePH-SN to APR on day L3 and four putative synaptic contacts fromthe PH-SN to APR on day P0. The loss of APR dendrites in posteriorneuropil (Fig. 2B) was reflected in the dearth of putative synapticcontacts in the posterior region of the PH-SN arbor on day P0.

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Figure 7. Spatial distribution of putative synaptic contacts from posterior PH-SNs to APRs on days L3 and P0. A, Each panel shows a two-dimensional projection of the reconstructed axonal arbor of a posterior PH-SN (red) on days L3 (left) and P0 (right), with the portion of the APR dendritic arbor (green) that occupied the same volume of neuropil as the PH-SN superimposed. Images are oriented as in Figure 2 (anterior is up). The arbor of APR within sensory neuropil was less extensive on day P0 than on day L3, providing fewer opportunities for synaptic contact (also see Fig. 4). B, Each panel shows a two-dimensional projection of the same reconstructed PH-SNs (red) that appear in A. The locations of putative output synapses onto APR are marked in yellow (the yellow dots indicate the location, not the size, of the putative synaptic contacts). Arrowheads indicate the site at which the PH-SN axons entered the neuropil. In this example, there were 43 putative synaptic contacts between the posterior PH-SN and APR on day L3 and four putative synaptic contacts on day P0.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Previous studies demonstrated that the steroid-induced regression of the dendritic arbor of motoneuron APR is associated witha decrease in the amplitude of monosynaptic EPSPs from PH-SNsand the developmental loss of a proleg withdrawal reflex (Jacobsand Weeks, 1990; Streichert and Weeks, 1995). The present studyused double fluorescence confocal microscopy to test the hypothesisthat physical disconnection of APR dendrites from the synapticterminals of PH-SNs contributes to the synaptic weakening andbehavioral loss. The dendritic morphology of APRs stained withLucifer yellow on days L3 and P0 (Figs. 2, 4) was indistinguishablefrom that of APRs stained with cobalt at these stages (Fig. 1A)(Streichert and Weeks, 1995; Sandstrom and Weeks, 1998). In particular,the region of APR dendritic arbor that overlaps with PH-SN axonterminals was regressed (Fig. 7A) (Jacobs and Weeks, 1990). Thepresent study (Fig. 3; also see Figs. 2C,D, 7B) improved on previousindirect evidence that PH-SN axonal arbors do not regress at pupation(Streichert and Weeks, 1995). Thus, fluorescently stained materialviewed by confocal microscopy corroborated previous observationsthat PH-SN arbors are structurally stable while the dendritesof proleg motoneurons regress atpupation.

Staining APRs with Lucifer yellow was routine, whereas staining PH-SNs with rhodamine via the hair shaft had a low successrate that limited the number of double fills in which contactscould be counted. Only brightly and completely stained neuronswere used for quantitative analysis (see Materials and Methods).The mean number of putative synaptic contacts between a posteriorPH-SN and an APR decreased from 43 on day L3 to nine on day P0(Fig. 6A), whereas the size of individual contacts did not changedetectably (Fig. 6B). The 79% decrease in the number of putativesynaptic contacts parallels an 83% decrease in the mean amplitudeof the EPSPs at these synapses (Streichert and Weeks, 1995). Becausethe input resistance of APR increases by 40% during this period(Streichert and Weeks, 1995), the actual decrease in synapticcurrent may exceed 83%. Furthermore, the loss of posterior dendritesin APR (Figs. 1A, 2B, 7A) should preferentially eliminate PH-SNinputs that are electrotonically the most distant from the cellbody of the APR (Fig. 7) and that make a lesser contribution toEPSP amplitude. Nevertheless, EPSP amplitude is severely reducedon day P0. The correspondence between the developmental decreasein the number of putative synaptic contacts and EPSP amplitudesupports the idea that these two features arerelated.

For technical reasons (see Materials and Methods) we used only posterior PH-SNs. However, because EPSP amplitude decreasessignificantly for PH-SNs located in all regions of the array (Streichertand Weeks, 1995), we expect that the contact number likewise decreasesfor all PH-SNs.

Validity of the analysis

These results raise two major issues of interpretation. The first concerns the identification of indistinguishably close contactsobserved at the light microscopic level as synapses, and the secondconcerns synaptic strength. Several lines of evidence supportthe designation of appositions between PH-SNs and APRs as putativesynapses. First, the size and shape of the contacts resemble centralsynapses in other systems. Putative synapses were identified asindistinguishably close or overlapping profiles in images witha pixel resolution of 0.2 µm, with the mean contact length inthe z-axis estimated to be 1.25-1.35 µm (see Results). This sizeis consistent with other insect sensorimotor synapses (e.g., outputsynapses from locust wing hinge stretch receptor neurons to wingmotoneurons) (Peters et al., 1985) and central synapses in general(for review, see Edwards, 1995). Most contacts occurred en passantfrom PH-SN varicosities onto high-order dendrites of an APR (Fig.5). Axonal varicosities (boutons) typically contain output synapsesin insects [cockroach (Blagburn et al., 1985), locust (Watsonand Burrows, 1985), Manduca (Sun et al., 1997)] and other species(DeRiemer and Macagno, 1981; Glanzman et al., 1989; Tse et al.,1991; Magoski and Bulloch, 1997). Output synapses may also bemade by fine, smooth processes (Watson and Burrows, 1982; Granzowet al., 1985; Walmsley et al., 1987; Lamotte d'Incamps et al.,1998). Close appositions observed at the light microscopic levelhave been confirmed to be synapses by electron microscopy in anumber of cases (Muller and McMahan, 1976; Pilowsky et al., 1990;Sorra and Harris, 1993; Buhl et al., 1994; Gonchar et al., 2002).In summary, the morphology of appositions between PH-SNs and APRsis entirely consistent with synaptic contacts, an assumption thatcan be tested in futureexperiments.

A second key issue in interpreting our results is the strength of individual synaptic contacts between PH-SNs and APRs. Theamplitude of an EPSP reflects the number of release sites andthe size of the synaptic current produced at each release site,which is in turn determined by the amount of neurotransmitterreleased, the number of receptors, and other factors (for review,see Edwards, 1995). The size of contacts between PH-SNs and APRsdid not change detectably between days L3 and P0 (Fig. 6B), butmore subtle alterations in synapse structure that could affecttransmission (e.g., a decrease in the number of active zones orin the size of the postsynaptic density) are undetectable at thelight microscopic level. It is well established that synapticstrength and synaptic morphology can be regulated independently(Tsujimoto et al., 1990; Stewart et al., 1996; for review, seeDavis and Goodman, 1998), so the developmental weakening of synapsesfrom PH-SNs to APRs could be accomplished entirely by electrophysiologicalchanges rather than by altering the number of contacts. However,analysis of EPSP time-to-peak and the intrinsic electrical propertiesof APRs suggest that the developmental decrease in EPSP amplituderesults from a decrease in binomial n (i.e., the number of contactsor release sites) rather than from other factors (Streichert andWeeks, 1995). Evidence against the possibility that a change insynaptic release properties from PH-SNs is involved in synapticweakening comes from heterochronic mosaic animals, in which PH-SNsare maintained in the larval state by treating their somata withjuvenile hormone, whereas APRs undergo normal dendritic regression(Streichert and Weeks, 1995). The EPSP amplitude decreases betweendays L3 and P0 at these heterochronic mosaic synapses, suggestingthat genomic actions of 20E on PH-SNs are not required for synapticweakening. On the postsynaptic side, the possibility that 20Eaffects the electrophysiological properties of APR, such as thenumber or density of ACh receptors, can be investigated in cellculture (Melville et al., 2003; and our unpublishedobservations).

Although such factors could contribute to synaptic weakening, the existing anatomical and electrophysiological data supportthe hypothesis that the massive reduction in the number of physicalcontacts between PH-SNs and APRs (Fig. 6A) plays a predominantrole in the developmental reduction in EPSP amplitude. Fewer contactsshould produce less total synaptic current, and hence a smallerEPSP. Relationships between the number of synaptic contacts andsynaptic strength at monosynaptic connections have been amplydemonstrated in other systems [crayfish (Nakagawa and Mulloney,2001), mollusc (Glanzman et al., 1989), frog (Kuno et al., 1971;Grantyn et al., 1984), goldfish (Korn et al., 1981), and cat (Malenkaand Nicoll, 1997)]. By this scenario, the predominant locus forthe weakening of synapses from PH-SNs to APRs is postsynaptic,because of the steroid-induced regression of APRdendrites.

Relationship to neural circuits for behavior

The excitatory synapses from PH-SNs to APRs constitute the direct pathway in the neural circuit for the larval proleg withdrawalreflex (Fig. 1C) and are the major source of synaptic drive toproleg retractor motoneurons during the reflex (Jacobs and Weeks,1990; Streichert and Weeks, 1995). Hence, the steroid-inducedweakening of these synapses has direct behavioral relevance incontributing to the weakening and loss of the proleg withdrawalreflex at the end of larval life. After pupation, some APRs areeliminated by programmed cell death, whereas the others undergosteroid-induced dendritic regrowth, receive new synaptic inputs,and are respecified for new functional roles (Weeks and Ernst-Utzschneider,1989; Sandstrom and Weeks, 1998; Lubischer et al., 1999). Dendriticregression and synaptic loss extricates APRs from outmoded larvalcircuits and prepares the motoneurons to be incorporated intonew circuits for the next life stages. The PH-SNs are believedto die after pupation (Streichert and Weeks, 1995) and so arenot expected to undergoregression.

Our findings represent the first demonstration in a single system that a steroid-induced change in dendritic architectureis associated with a change in the strength of monosynaptic connectionsand a change in behavior. Steroid hormones have pervasive effectson dendritic architecture and behavior (see Introduction), butthe demonstration of specific links between hormones, synapses,and behavior is difficult. Many fundamental issues regarding steroideffects on neurons and behavior can be readily addressed in theexperimentally accessible insect nervous system (for review, seeFahrbach and Weeks, 2002). Application of this level of analysisto the vertebrate nervous system should reveal intriguing insightsinto the regulation of sexually differentiated and other behaviorsby steroidhormones.

  FOOTNOTES

Received July 24, 2002; revised Nov. 22, 2002; accepted Dec. 4, 2002.

This work was supported by National Institutes of Health Grant R01 NS23208 (J.C.W.). We thank Dr. Daniel Hartline for adviceon three-dimensional reconstruction, Dr. David Lenzi for serviceas a blinded observer, and Dr. William M. Roberts, Dr. JohnathanMelville, M. Jade Zee, and Ari Winbush for helpful suggestionson thismanuscript.

Correspondence should be addressed to Janis C. Weeks, 1254 Institute of Neuroscience, University of Oregon, Eugene, OR 97403-1254.E-mail: weeks{at}uoneuro.uoregon.edu.

J. R. Gray's present address: Department of Biology, University of Saskatchewan, 112 Science Place, Saskatoon, SK S7N 5E2Canada.

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