Three-Dimensional Topography of Corticopontine Projections from Rat Barrel Cortex: Correlations with Corticostriatal Organization

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The Journal of Neuroscience, November 15, 2000, 20(22):8474-8484

Three-Dimensional Topography of Corticopontine Projections from Rat Barrel Cortex: Correlations with Corticostriatal Organization
Trygve B. Leergaard¹, Kevin D. Alloway², Joshua J. Mutic², and Jan G. Bjaalie¹
¹ Department of Anatomy, Institute of Basic Medical Sciences, University of Oslo, N-0317 Oslo, Norway, and ² Pennsylvania State University, Department of Neuroscience and Anatomy, Hershey, Pennsylvania 17033

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subcortical re-entrant projection systems connecting cerebral cortical areas with the basal ganglia and cerebellum are topographicallyspecific and therefore considered to be parallel circuits or "closedloops." The precision of projections within these circuits, however,has not been characterized sufficiently to indicate whether corticalsignals are integrated within or among presumed compartments.To address this issue, we studied the first link of the rat cortico-ponto-cerebellarpathway with anterograde axonal tracing from physiologically defined,individual whisker "barrels" of the primary somatosensory cortex(SI). The labeled axons in the pontine nuclei formed several,sharply delineated clusters. Dual tracer injections into differentSI whisker barrels gave rise to partly overlapping, paired clusters,indicating somatotopic specificity. Three-dimensional reconstructionsrevealed that the clusters were components of concentrically organizedlamellar subspaces. Whisker barrels in the same row projectedto different pontine lamellae (side by side), the somatotopicrepresentation of which followed an inside-out sequence. By contrast,whisker barrels from separate rows projected to clusters locatedwithin the same lamellar subspace (end to end). In the neostriatum,this lamellar topography was the opposite, with barrels in thesame row contacting different parts of the same lamellar subspace(end to end). The degree of overlap among pontine clusters variedas a function of the proximity of the cortical injections. Furthermore,corticopontine overlap was higher among projections from barrelsin the same row than among projections from different whiskerbarrel rows. This anisotropy was the same in the corticostriatalprojection. These findings have important implications for understandingconvergence and local integration in somatosensory-related subcorticalcircuits.

Key words: 3-D reconstruction; basal ganglia; cerebellum; cerebrocerebellar; double anterograde tracing; parallel circuits; pontine nuclei; somatosensory maps; somatotopy

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neurons in the cerebral cortex project to a number of subcortical targets. Many of these neurons belong to two major corticosubcorticalre-entrant circuits, one including the basal ganglia (for review,see Heimer et al., 1995; Parent and Hazrati, 1995) and anotherincluding the pontine nuclei and cerebellum (for review, see Brodaland Bjaalie, 1992, 1997; Schmahmann and Pandya, 1997). Structuraland functional specification have been studied extensively inthe first links of these circuits, i.e., in the projections fromthe cerebral cortex to the pontine nuclei (Brodal, 1968, 1978;Mihailoff et al., 1978, 1985; Wiesendanger and Wiesendanger, 1982;Bjaalie and Brodal, 1989; Leergaard et al., 2000) and the neostriatum(Webster, 1961; Malach and Graybiel, 1986; Gerfen, 1989; Allowayet al., 1999). During development, the global topography of corticopontineprojections appears to be determined by simple temporal and spatialgradients operative within source (cerebral cortex) and target(pontine nuclei) region (Leergaard et al., 1995). In agreementwith these topographic principles, we recently demonstrated thatthe adult pontine projections from primary somatosensory cortex(SI) are systematically organized in a clustered three-dimensional(3-D) map (Leergaard et al., 2000). Thus, the terminal fieldsof axons originating in different SI body part representations(perioral region, trunk, extremities) are largely segregated andpreserve the somatotopic order of the cortical map. One interpretationof this arrangement would be that there are separate channelsthrough the pontine nuclei for different major body representationsof SI. Such segregated projection systems, connecting cerebralcortical areas with the cerebellum, have previously been reportedin the monkey (Hoover and Strick, 1999) and have prompted hypothesesof parallel pathways ("closed loops") in the cerebrocerebello-thalamocorticalre-entrant circuits [for review and comparison with basal gangliacircuitry, see Middleton and Strick (2000)]. The detailed organizationof pontine projections from neighboring cortical sites withinthe same SI body part representation is not known. Projectionsat this finer level could either maintain topographic specificityand segregation or, alternatively, allow structural convergenceand functional integration, comparable with the assumed integrationin the neostriatum of functionally related signals originatingfrom separate SI cortical sites [for general considerations onparallel basal ganglia circuitry, see Alexander et al. (1986,1990), Alexander and Crutcher (1990), and Alloway et al. (1999)].

To test these hypotheses, we have analyzed the small-scale topography of corticopontine projections from the orderly representationof mystacial vibrissae in SI (Woolsey and Van der Loos, 1970;Welker, 1976). In the present study, we have mapped the 3-D patternof corticopontine projections in rats that received injectionsof two anterograde tracers in different SI whisker "barrels."We report that corticopontine projections from individual barrelsare topographically organized. Our findings also suggest thatpontine neurons can integrate functionally related signals fromneighboring cortical sites. Because most of these rats had alsobeen used to characterize the organization of corticostriatalprojections (Alloway et al., 1999), we compared the relative patternsof corticostriatal and corticopontine projections from the samecortical sites. This comparison revealed several important principlesconcerning the comparative organization of these major corticofugalpathways.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Surgical procedures and electrophysiological mapping. Thirteen adult male Sprague Dawley rats were used (see Table 1). Allanimal procedures were approved by an institutional animal welfarecommittee and were in compliance with National Institutes of Healthguidelines for the use and care of laboratoryanimals.

The animals were anesthetized with intramuscular administration of ketamine (20 mg/kg) and xylazine (6 mg/kg). Each animalreceived atropine sulfate (0.05 mg/kg) to reduce bronchial secretionsand chloromycetin sodium succinate (50 mg/kg) to prevent infection.The animals were intubated with a 16 gauge plastic tube beforebeing immobilized in a stereotaxic frame. Perioperative anesthesiawas maintained by ventilation with a 2:1 mixture of nitrous oxideand oxygen containing 0.5% halothane. End tidal CO₂, cardiac rate,and body temperature were monitored throughout the procedure.The body temperature was maintained with a thermostatically controlledhomeothermic blanket. Corneal drying was prevented with ophthalmicointment. Two small holes were made in the cranium overlying theright SI whisker representations as reported previously (Allowayet al., 1999). A carbon fiber electrode (Armstrong-James and Millar,1979) was inserted through each cranial opening and lowered toa cortical depth of 800-1000 µm. Extracellular recordings of multiunitactivity were amplified and displayed by conventional means, andindividual whiskers were stimulated with a slender rod to determinethe best whisker for activating neuronaldischarges.

Tracer injections and histochemistry. The two electrophysiologically identified whisker representation sites received injectionsof either 10% biotinylated dextran amine (BDA) (Molecular Probes,Eugene, OR), or 10% rhodamine-conjugated dextran amine [FluoroRuby(FR), Molecular Probes]. FR was loaded into a glass micropipette(100 µm tip) cemented to a 1.0 µl Hamilton syringe that was placedin a microinjection unit (Kopf 5000, Kopf Instruments, Tujunga,CA). The pipette was inserted perpendicular to the cortical surface,and a volume of 25 nl of FR was injected at a depth of 1400 µmbelow the pial surface. After 5 min, the pipette was retractedto 1200 µm, and 25 nl of FR was deposited. Five minutes latera third 25 nl volume of FR was injected at a depth of 1000 µm.To avoid backflow of the tracer, the pipette was left in positionfor 10 min before retraction. BDA was injected iontophoreticallythrough a glass micropipette (35-40 µm tip). Three injectionswere placed at cortical depths of 1400, 1200, and 1000 µm, respectively,by passing a pulsed 4.0 µA current (duty cycle 7 sec) throughthe pipette for 7-8min.

After a survival period of 1 week, each rat was reanesthetized with an intraperitoneal injection of sodium pentobarbital (50mg/kg) and perfused transcardially with cold saline containing1000 U heparin and 20 mg lidocaine, followed by 500 ml cold 4%paraformaldehyde in 0.1 M phosphate buffer, pH 7.4, and finallyanother 500 ml of the same solution with 5% sucrose added. Thebrains were removed and cryoprotected in 4% paraformaldehyde with30% sucrose. Subsequently the right cerebral cortex was dissectedout as a slab and flattened between two glass slides. Tangentialsections of the cortical slab and transverse sections of the brainstemwere cut at 50 µm on a freezingmicrotome.

Alternate serial sections from the flattened cortex were processed for BDA as described previously (Kincaid and Wilson, 1996;Alloway et al., 1998, 1999). The remaining alternate sectionsthrough SI cortex were processed for cytochrome oxidase (CO) usinga previously described procedure (Wong-Riley, 1979; Land and Simons,1985; Alloway et al., 1999). The complete series of transversesections through the brainstem was processed for BDA accordingto steps 1-7 in Lanciego and Wouterlood (1994) using a streptavidin-biotinylatedhorseradish-peroxidase complex (Amersham, Buckinghamshire, UK)as a substitute for the avidin-biotin solution used in the originalprotocols. Sections were mounted on gelatin-coated glass and coverslippedwithEukit.

Digitization, 3-D reconstruction, and data analysis. The distribution of labeled axons within the pontine nuclei and severalanatomic landmarks were recorded using an image-combining computerizedmicroscope system, based on a Leica DMR microscope. Details onsoftware and technical solutions are reported in Leergaard andBjaalie (1995). Complete series of sections through the pontinenuclei were digitized using a Leitz Plan Fluotar 25× or 40× lens.The ventral surface of the pons, the outlines of the pontine gray,the contours of the corticobulbar and corticospinal fiber tracts(in the following referred to as the peduncle), the midline, andthe fourth ventricle served as referencelines.

The plexuses of BDA-labeled axons were viewed with translucent light, and the FR-labeled axons were viewed with excitationlight of 515-560 nm (Leitz N2.1 filter block). The labeled plexuseswithin the pontine gray were coded semiquantitatively as points(see also Leergaard and Bjaalie, 1995; Leergaard et al., 1995,2000). In areas with a low density of labeling, point coordinateswere placed at regular intervals along the length of single axons.In areas with dense labeling it was impossible to assign coordinatesto individual fibers. Although the distribution of labeling wasrecorded accurately, a rough correspondence was sought betweenthe density of labeling and number of digitized points, resultingin tight point clusters corresponding to dense axonal plexuses.The two categories of labeling were digitized independently, andthe correspondence of labeling and digitized image for both labeledcategories was studied carefully using alternating light microscopyand fluorescence microscopy with the 25× and 40×lenses.

For the 3-D visualization and analysis of the distribution of labeling, we used program Micro3D for Silicon Graphics workstations(Oslo Research Park, Oslo, Norway), which was developed at theNeural Systems and Graphics Computing Laboratory, University ofOslo (http://www.nesys.uio.no/). Forerunners of this softwarewere used in several recent investigations (Leergaard et al.,1995, 2000; Malmierca et al., 1995, 1998; Bjaalie et al., 1997a,b;Berg et al., 1998; Bajo et al., 1999; Vassbø et al., 1999). Thedigitized sections were aligned interactively on the screen withthe aid of the reference lines (see above). Each section was assigneda z-value defined by its thickness and serial number. Tissue shrinkagewas estimated by comparison of drawings of sections before andafter the histochemical processing. To maintain correct in vivoproportions in the 3-D reconstructions, section thickness (whichwas originally 50 µm) was set to 47.5 µm as an adjustment fora linear shrinkage of ~5%. To facilitate the alignment, real-timerotation with inspection of the 3-D reconstructions from differentangles of view was used. The reconstructions served as a basisfor the further visualization and analyses of densities and distributionof point clusters. Surface modeling was performed with a simpletriangulation method or with the use of the software library SISL(SINTEF Spline Library) (cf. Bjaalie et al., 1997a).

To facilitate the visualization of results and comparison among cases, we used the standard pontine coordinate system andrelated diagrams for visualization presented in Leergaard et al.(2000). This coordinate system is divided into relative valuesfrom 0 to 100%. The origin of coordinates is defined by the intersectionof the midline and a line perpendicular to the midline and tangentialto the rostral border of the pontine nuclei. Only the two halfway(50%) reference lines are shown in thefigures.

The degree of overlap between the BDA- and FR-labeled terminal fields was estimated by subdividing individual sections intoan array of 35 µm² bins and counting the numbers of digitized coordinate pairs perbin. Similar solutions were used previously by others (He et al.,1993; Alloway et al., 1999). To avoid analyzing areas with verylow density of labeling, bins containing only one point were excluded.Because areas with high density of labeling were recorded by approximation,no attempt was made to differentiate the labeled zones accordingto density. Bins containing two or more red or blue points weredefined as "red" or "blue," respectively. Bins containing twoor more points of both categories were defined as "white" bins,representing overlap. The numbers of red, blue, and white binswere counted for each section, summed across sections, and usedto estimate an index of total overlap. The overlap estimate ishighly influenced by bin size and threshold criteria. If smallbins (e.g., 5 µm²) and high thresholds (e.g., >10 points per bin) were used, theamount of overlap appeared minimal, whereas by comparison, largebins and low thresholds resulted in increased overlap. We chosethe same bin size (35 µm²) as used by Alloway et al. (1999), partly to facilitate comparisonacross brain regions and partly because similar arguments forthis bin size were applicable to the pontine nuclei. Bins >35µm tended to yield overlap in situations where the labeled terminalsappeared segregated. Smaller bins were not used because clearlyoverlapping areas then tended to be defined assegregated.

We have based our analysis on an overlap index defined as the number of white bins divided by the number of red, blue, andwhite bins. Statistical ANOVA was performed using the StatisticalPackage for the Social Sciences (SPSS Inc., Chicago,IL).

Illustrations were assembled with Showcase (Silicon Graphics, Mountain View, CA), Adobe Illustrator 8.0, and Adobe Photoshop5.0. Digital photomicrographs were obtained through a CoolSnapcamera (Photometrics, Tucson, AZ). The gray-scale levels of theimages were optimized using the "curves" function for "autolevels"in AdobePhotoshop.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

For this report, results from four representative animals are illustrated and described in detail. More documentation, includingoriginal data sets with 3-D spatial coordinates, is availableat http://www.nesys.uio.no/ and http://www.cerebellum.org/.

Injection sites

In each experiment, restricted injections of BDA and FR were placed into separate regions of the SI barrel cortex (Fig. 1).Ten of the 13 experiments were selected by criterion of labelingin the neostriatum and thalamus and were used previously in astudy of corticostriatal organization (Alloway et al., 1999).All cases contained anterograde BDA and FR labeling in the pontinenuclei. All injections were restricted to the gray matter. Theoutlines and position of the injection sites were estimated withrespect to the whisker barrels by comparison of adjacent BDA-and CO-processed tangential sections through cortical layers IVand V. The position of injections in the whisker barrel fieldcorresponded to the electrophysiological recordings made beforetracer injection. The diameter of the injection sites (Table 1),defined by the maximum width of dense staining in layer V (thecortical layer containing cell bodies of corticopontine neurons),ranged from 200 to 800 µm. Each injection involved one to twobarrels (Table 1). In five cases, both tracers were confinedto the same row of barrels ("within rows"), and in eight casesthe tracers were injected into separate rows of barrels ("acrossrows"). The edge-to-edge separation between the two injectionsites was measured in layer V (Fig. 2). Injection sites neveroverlapped. Photomicrographs of representative injection sitesare shown in Figure 2.

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Figure 1. A, Drawing of the right cerebral hemisphere of the rat with a cartoon representation of the SI somatotopic map and the SI barrel cortex (redrawn from Welker, 1971, with permission). B, Drawing of somatotopically organized SI barrels representing the mystacial vibrissae (arranged in rows A-E, corresponding to the arrangement of vibrissae on the contralateral mystacial pad), as they appear in CO-stained sections (redrawn from Fabri and Burton, 1991, with permission). Scale bar, 1 mm. A, Anterior; M, medial; L, lateral.


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Table 1. Location, size, and relation between BDA and FR injection sites

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Figure 2. Topography of BDA and FR injections in two representative cases (A-D: D51, E-H: D53). A, B and E, F are corresponding photomicrographs of tangential sections through layer V of SI, revealing the extent of the BDA and FR injection sites in cases D51 and D53, respectively. C and G are overlays of the photomicrographs in A, B and E, F, respectively. D and H show tangential sections (corresponding to A-C and E-G, respectively) through layer IV of SI cortex labeled for CO to indicate the location of individual whisker barrels. Dashed circles indicate the boundaries of the injection sites. Arrowheads indicate corresponding sets of blood vessels in each panel. In case D51 (D), the BDA injection is located between barrels C2 and C3, whereas the FR injection is restricted to E2. In case D53 (H), the BDA injection site is located in the anterolateral barrel subfield, and the FR injection is located in E2. Scale bar, 500 µm. A, Rostral; M, medial.

General features of labeling and overall topography

The BDA and FR injections gave rise to labeling in several intracortical and subcortical targets. Topographically organizedfiber complexes were found in the ipsilateral neostriatum andin the thalamic nuclei together with retrogradely labeled cells(Alloway et al., 1999). Within the ipsilateral pontine nuclei,anterogradely labeled fibers branched extensively to form severaldense axonal plexuses that were assumed to represent terminalfields (Fig. 3). We observed beaded varicosities along the trajectoriesof all BDA and FR fibers inside the pontine nuclei. Recent ultrastructuralanalyses demonstrated that similar varicosities along corticostriatalfibers contained synaptic vesicles and thus may represent corticostriatalsynapses (Kincaid et al., 1998). Because the beaded varicositiesobserved in the pontine nuclei may represent synaptic contacts(Mihailoff et al., 1981), we have chosen to record the completetrajectory of the labeled fibers within the pontine nuclei.

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Figure 3. Photomicrographs of FR and BDA labeling in transverse sections through the pontine nuclei. A, C, Case D44; B, case D45; D, case D46. Each image is an overlay of two transparent photomicrographs, viewed by fluorescence microscopy and conventional light microscopy for visualization of FR and BDA, respectively. A shows partly overlapping clusters of FR and BDA fibers located slightly rostral to the midpontine level. B shows partly overlapping FR and BDA clusters located close to the midline at the midpontine level. C shows elongated, partially overlapping FR and BDA clusters along the ventral aspect of the peduncle. Compared with the FR labeling, the BDA labeling is slightly shifted toward dorsal and thus is considered to be located more "externally." D shows closely associated, curved FR- and BDA-labeled clusters located laterally in the pontine nuclei. The clusters are incomplete parts of a lamellar subspace. The FR labeling is shifted slightly toward dorsal and lateral and surrounds the BDA labeling externally. Further documentation of FR and BDA images is available at http://www.nesys.uio.no/and http://www.cerebellum.org/. Scale bar: A-C, 50 µm; D, 100 µm. D, Dorsal; M, medial; mid, midline; ped, peduncle; pn, pontine nuclei; tfp, transverse fibers of the pons.

The shape, size, and density of labeled plexuses produced by the two tracers were very similar. Viewed in single sections,the BDA and FR labeling were aggregated in sharply defined, roundedpatches that were 50-200 µm in diameter (Fig. 3A,B) and elongatedthin bands that were ~50-100 µm wide (Fig. 3C). The computerizedreconstructions showed that the two-dimensional (2-D) patchesare parts of 3-D clusters (Figs. 4, 5). The shape and distributionof the clusters suggest that they are incomplete components ofconcentric layers or lamellae (Fig. 6).

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Figure 4. Computer-generated 3-D reconstruction from case D46, showing the topography of corticopontine projections after injections of BDA and FR into the same whisker barrel row. Dots represent the distribution of BDA (black)- and FR (red)-labeled corticopontine fibers within the pontine nuclei. A, The computerized dot maps are shown as 3-D total projections with an angle of view from ventral, rostral, or medial. A frame of reference is superimposed onto the model, defined by planes tangential to the boundaries of the pontine nuclei. A coordinate system of relative values from 0 to 100% is introduced. The halfway (50%) reference lines are shown as dotted lines in the ventral, rostral, and medial views. The position of injection sites is indicated in outline drawing of CO-labeled barrels. B, C, Consecutive series of 200-µm-thick transverse (B) and sagittal slices (C) through the reconstruction. The numbers assigned to each slice refer to the coordinate system and indicate the rostrocaudal or mediolateral level of each slice. The clusters of red dots surround the clusters of black dots externally. Scale bars, 500 µm. A, Anterior; M, medial.

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Figure 5. Computer-generated 3-D reconstruction from case D48, showing the topography of corticopontine projections after injections of BDA and FR into different whisker barrel rows. Presentation as in Figure 4. The clusters of red and black dots are located within a single narrow lamella-shaped volume, with a dorsal (FR) to ventral (BDA) shift in the preponderance of labeling. Scale bars, 500 µm. A, Anterior; M, medial.

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Figure 6. Computer-generated stereo pairs showing the 3-D topographic relationship of labeled FR (red) and BDA (blue) terminal fields in the pontine nuclei for two representative within row and across row cases (A-C, case D46; D-F, case D48). The position of injections is indicated in outline drawings of CO-labeled barrels. The outer boundaries of labeled clusters are demonstrated by solid surfaces. The sparse contralateral and dorsal clusters of labeling are not shown. To see a 3-D image, the viewer must cross the eye axis to let the pair of images merge. The insets in the middle column illustrate the angle of view in relation to the ventral surface of the pons, the boundaries of the pontine nuclei (transparent surfaces), and the descending peduncles (solid blue surfaces). The stereo pairs are rotated clockwise in steps of 90° around the rostrocaudal axis. In A-C, the labeled clusters arising from the same row of SI barrels are located in dual lamellae that are shifted from internal to external. In D-F, the labeled clusters arising from separate rows in SI are located within a single lamellar subspace, with a dorsal (FR) to ventral (BDA) shift in the preponderance labeling. Scale bar, 500 µm. M, Medial; R, rostral.

In general, the aggregates of BDA and FR labeling were colocalized and frequently partially overlapping (Fig. 3). Completelysegregated patches of BDA and FR labeling were often observed,whereas completely overlapping patches were not found. The widespreaddistribution and lamellar shape provides a large side-by-sideinterface between neighboring terminal fields. Furthermore, afterinjection of BDA and FR into different SI whisker barrels, weoften observed clusters of BDA- and FR-labeled fibers laterally,medially, and dorsally in the pontine nuclei (Figs. 4-6), whichindicate the presence of multiple pontine body representations.This is in agreement with previous findings from the mapping oflarger SI body representations onto the pontine nuclei (Leergaardet al., 2000).

To describe the spatial relationships between labeled clusters, we defined the internal region of the pontine nuclei as acentrally located core, relatively close to the peduncle. Regionsoutside this core, that is, medial, lateral, ventral, dorsal,caudal, or rostral to it, were referred to as external (see alsoLeergaard et al., 1995, 2000). There was little variation amongcases in the 3-D shape of labeling from different whisker barrels.In all cases, each injection produced ipsilateral labeling inseveral clusters. The largest cluster was located laterally andcaudally, relative to the central core of the pontine nuclei (Figs.4A, ventral view, B, 6A,C). A smaller cluster was located closeto the midline (Figs. 4A, 5B, ventral view, rostral view, 6A).These findings are consistent with previous work indicating thepresence of medial and lateral pontine terminal fields after tracerinjections into the SI facial and vibrissal representations (Wiesendangerand Wiesendanger, 1982; Mihailoff et al., 1985; Lee and Mihailoff,1990; Panto et al., 1995). In addition, we frequently observedloose axonal plexuses along the dorsal aspect of the ipsilateralpeduncle and in the contralateral pontine nuclei (Figs. 4A, rostralview, 5A, rostral view).

We have previously mapped the pontine projections from the major SI-body representations using a single-tracing approach (Leergaardet al., 2000). When compared with those previous results, it appearsthat the SI whisker representations surround the perioral projectionarea, which is located centrally in the pontine nuclei. The whiskerrepresentations are thus intercalated between the perioral representationsand the more externally located projections from the trunk andneck [compare Figs. 4 and 5 with Leergaard et al. (2000), theirFigs. 8 and 9). Hence, the present results are consistent withour previously published 3-D map of the corticopontine projectionsfromSI.

Corticopontine projections from SI barrels in the same row

After BDA and FR injections into the same row of barrels, the ensuing BDA and FR labeling was distributed in a pair of concentricallyarranged lamellae. Figures 4 and 6 show that the FR-labeled clustersin case D46 occupy more lateral, medial, and dorsal locationsthan the corresponding BDA clusters. Thus, the FR clusters inthis case, representing the more caudal whisker, surround theBDA clusters externally. The internal to external shift in locationof labeling is shown to advantage in the transverse and sagittalslices through the reconstruction (Fig. 4B,C, slices 50-80).

The BDA and FR clusters in case D46 were partially overlapping at practically all rostrocaudal or mediolateral levels containinglabeling (Figs. 3D, 4, 7A,B). The total amount of overlap in thiscase was 12.1%. The separation of the two injections was 930 µm.In another within row experiment (D53), the separation distancebetween the injection sites was much larger (1700 µm). Althoughthe same overall shape and lamellar distribution pattern was seenin this case, the labeled clusters were clearly more segregated(Fig. 7C,D), and the amount of total corticopontine overlap wasonly 1.7%. Five within row experiments demonstrated decreasingamount of overlap with increasing separation of the cortical sitesof origin (Table 1, Fig. 8).

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Figure 7. Dot maps and overlap analysis of selected transverse sections from four representative cases (A, B: case D46, C, D: case D53, E, F: case D48, G, H: case D51). Sections are selected from rostrocaudal levels 50% (A, C, E, G) and 80% (B, D, F, H), as indicated by arrows in the insets. The insets in the right column show the BDA (blue) and FR (red) injection sites and corresponding 3-D reconstructions in a ventral view (see also Figs. 5 and 6). A-H show blue and red dots representing the distribution of BDA and FR labeling within the pontine nuclei, whereas A'-H' show an overlap analysis of the same sections. Each digitized dot map is subdivided into 35 µm bins, and the number of BDA and FR dots is counted in each bin. Bins containing at least two BDA or FR dots are colored blue or red, respectively; those containing at least two of each type are colored white (cf. Materials and Methods). Projections from separated whisker barrels partly overlap in the pontine nuclei. The amount of overlap (Table 1) decreases when the distance separating the injection sites increases (compare A', B' with C', D', and E', F' with G', H'). Inset frames are 2 × 2 mm. Scale bars, 500 µm.

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Figure 8. Scatter plot of the variation in overlap of pontine terminal fields as a function of the distance separating injection sites in cortical layer V. The total amount of overlap in the pontine nuclei decreases with increasing separation of the injection sites and is significantly higher among projections originating from barrel columns in the same row of SI cortex (see also Table 1).

Corticopontine projections from SI barrels in different rows

When BDA and FR injections were placed in different rows, the ensuing labeled terminal fields had a lamellar shape as describedabove. Instead of producing a dual lamellar pattern, however,the labeled clusters for both tracers appeared to be localizedwithin a single lamellar volume. Case D48 illustrates this findingin both sagittal and transverse slices (Fig. 5B, slices 50-80;5C, slices 60-80). The BDA labeling arising from a barrel in rowD tended to extend more ventrally in the pontine nuclei than theFR labeling arising in an adjacent barrel in row C (Figs. 5B,slices 60-80, 6D-F). These topographic differences however, wereless conspicuous than the marked inside-out pattern observed inthe within row cases. In case D48, the injection sites were separatedby only 120 µm in cortical layer V, and total corticopontine overlapwas 14.5% (Fig. 7E,F). In another across row case (D51), the twoinjection sites were separated by 630 µm (Fig. 7G,H). The labeledclusters in D51 were also confined within a lamellar subspace.The clusters appeared to be more segregated than in case D48,as indicated by a reduction in the total amount of corticopontineoverlap (9.6%). As Table 1 indicates, we observed decreasingamounts of corticopontine overlap with increasing separation ofthe tracer injection sites (Table 1, Fig. 8).

Quantitative estimate of overlap

The degree of overlap between the BDA- and FR-labeled terminal fields was calculated by subdividing individual sections intoan array of 35 µm² bins and counting the numbers of digitized coordinate pairs perbin (for details, see Materials and Methods). The total overlapindex ranged from 0.5 to 20%, with a mean index of overlap of7.1 ± 1.8% (SEM). Generally, the index of overlap appeared higherin the within row than in the across row group (Table 1, Fig.8). The highest overlap (20%) was observed after nearby injectionsin the same row of whiskers (Table 1, case D45). The lowest overlap(0.5%) was found in a case with injections in separate rows (Table1, case D49). Furthermore, the amount of overlap varied relativeto the separation of injection sites (Table 1, Fig. 8). To comparethe effect of these two parameters, the within row and acrossrow groups were sorted into groups with <1000 µm separation ("closerseparation") and groups with injection sites separated by 1000µm or more ("farther separation"). For these four groups, we wantedto describe the variation of overlap as a function of two categoricalparameters: the relative position and the separation of injections.A two-way ANOVA showed that there was no interaction between thetwo parameters (p = 0.898). Thus, the difference between the groups,with respect to one parameter, is the same, regardless of thelevel of the other factor. Furthermore, a two-way ANOVA (withoutinteraction) showed that there was a significant reduction inoverlap from the within rows to the across rows group (p = 0.049)and a significant reduction from the closer separation to thefarther separation groups (p = 0.031). Based on the ANOVA model,the reduction in average overlap was 43.5% from the within rowsto the across rows group and 47.4% from the closer separationto the farther separation group. In summary, our analyses showthat the degree of partial overlap between pontine terminal fieldsdecreases with increasing separation of the cortical sites oforigin and that there is a significantly higher degree of overlapbetween within row cases as compared with across row cases (seealso Fig. 8).

Comparison of corticopontine and corticostriatal projections

Ten animals used in the present study were previously used in a comparable study of the neostriatum (Alloway et al., 1999).Four of these animals were within row cases (D43, D44, D45, D46)and six were across row (D41, D42, D48, D49, D51, D52). Comparisonsof these two brain regions revealed that the corticopontine projectionshave several principles of organization in common with corticostriatalprojections. Thus, in both target regions, terminal fields weresomatotopically organized in distinct, partially overlapping clustersthat reside in curved lamellar zones (Fig. 9). As shown in thepresent study, corticopontine projections from the same row ofbarrels were distributed side by side in adjacent lamellae, whereasprojections originating in different rows occupied largely separateregions within a single lamellar volume (Fig. 9G-I). In the corticostriatalprojection, however, projections originating in different whiskerbarrel rows terminated in different lamellae (Fig. 9E) (Brownet al., 1998; Alloway et al., 1999; Wright et al., 1999). In furthercontrast to the corticopontine projections, corticostriatal projectionsoriginating from cortical sites in the same SI barrel row terminatedin lamellae with ends that merged into each other to occupy asingle, more elongated lamellar volume (Fig. 9) [see also Allowayet al. (1999), their Fig. 10]. Despite differences in the anatomicorganization of the corticopontine and corticostriatal projections,both pathways displayed a significantly higher degree of overlapfor projections arising from the same row of barrels (Allowayet al., 1999; present study).

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Figure 9. Diagrams of the comparative topography of corticostriatal (Alloway et al., 1999) and corticopontine (present study) projections from within row and across row sites in the SI whisker barrel cortex. The gray or hatched regions illustrate the areas that would be occupied by labeled fibers after tracer injections into barrel columns. The 2-D principles of topographic distribution of terminal fields in neostriatum and pontine nuclei are summarized in the right column (C, F, I). When subcortical projections are traced from two cortical locations within the same row of SI whisker barrels (A), typical representations are located end to end within a single curved volume laterally in the neostriatum (D), and in characteristic clusters, located in dual lamellar zones that are shifted inside-out in the pontine nuclei (G). When one site of cortical origin (hatched) is shifted to a different row, representations are observed in separate side-by-side terminal fields in the neostriatum (E) and in end-to-end terminal fields confined to a single lamellar subspace in the pontine nuclei (H). There is a relationship between the neurogenetic gradient (6 = early generated parts, 1 = later generated parts) (Altman and Bayer, 1987; Bayer and Altman, 1987, 1991) and the anatomic connections between cortex and neostriatum and pontine nuclei. Thus, projections from early generated locations in SI (anterolaterally located barrels) innervate early established parts of the target structures. A, Anterior; D, dorsal; M, medial; R, rostral.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study demonstrates that corticopontine projections from the rodent SI barrel fields are topographically organized. Bycombining double anterograde tracing with computerized 3-D reconstructiontechniques, we found that the projections from individual SI barrelsterminate in concentrically arranged lamella-likesubspaces.

Clustered projections from barrels in the same row terminate in different lamellae, whereas projections from different barrelrows terminate in regions within the same lamellar subspace. Comparisonsof corticopontine and corticostriatal projection patterns in thesame animals revealed similarities as well as differences. Althoughboth corticopontine and corticostriatal projections terminatein lamella-shaped regions, barrels within a whisker row projectto lamellae organized side by side in the pontine nuclei, butend to end in the neostriatum (Fig. 9). Nevertheless, for bothcorticofugal systems, terminal overlap was greater for projectionsarising from SI whisker barrels in the same row than for projectionsarising from barrels in different rows. This organizational schememay shed new light on corticopontine topographic organization,pontine integration of information originating in nearby corticalsites, and putative roles of the pontine nuclei in cerebrocerebellarcommunication.

Establishment of corticopontine and corticostriatal topography

Developmentally, there is a striking resemblance between corticopontine and corticostriatal projections. Thus, the topographyof these projections seems to correlate with neurogenetic gradientsin cortex (source) and target regions. In the cerebral cortex,the neurogenetic gradient extends from anterolateral toward posteriorand medial, in parallel with the rows of barrels in SI (Hicksand D'Amato, 1968; Smart, 1984; Bayer and Altman, 1991; Erzurumluand Jhaveri, 1992; Bishop et al., 2000). A similar gradient wasreported for the development of electrophysiological specificity(McCandlish et al., 1993). Thus, anterolaterally located barrels(high numbers) are developed before the more medially and posteriorlylocated barrels (low numbers). In the pontine nuclei, the earlyestablished region is located in the central core (Altman andBayer, 1978, 1987), and this region receives projections fromthe early, established anterolateral cortex (Leergaard et al.,1995; see also Leergaard and Bjaalie, 1998; Leergard et al., 2000).The present findings are in agreement with this distribution principle.Thus, SI barrels with high numbers (early) project to a regionclose to the central core (early), and projections from barrelswith lower numbers (later) wrap around this core. In the neostriatum,SI barrels with high numbers project to the ventrolateral part,and barrels with lower numbers project to successively more dorsomedialregions (Alloway et al., 1999; Wright et al., 1999). Again, thistopographic distribution follows the neurogenetic gradient ofthe neostriatum (Bayer and Altman, 1987). The further shapingof the terminal fields in these pathways is presumably accomplishedthrough a multitude of developmentalmechanisms.

Representation of cortical barrels in the pontine nuclei

In virtually all species, corticopontine projections terminate in several, sharply defined clusters (for review, see Brodaland Bjaalie, 1992, 1997). The present study demonstrates thatneighboring cortical injections give rise to paired clusters atseveral locations in the pontine nuclei. This finding indicatesthe presence of multiple, somatotopically organized representationsof the SI map in the pontine nuclei. This intricate corticopontinetopography has been interpreted as a basis for the fractured mapsof tactile representations found in the cerebellar hemispheres(Schwarz and Thier, 1995). Indeed, the transformation from a cortical2-D map to a pontine 3-D map gives opportunities for some newneighboring relationships (Leergaard et al., 2000; see also Leergaardand Bjaalie, 1998; Schwarz and Thier, 1999). However, a more characteristicfeature of corticopontine mapping is the preservation of somatotopicorder. By means of 3-D reconstruction and single tracing techniquesin rat, we demonstrated that neighboring relationships of majorbody representations are largely preserved in the SI-pontine projections(Leergaard et al., 2000). In the present study, we have shownsimilar preserved spatial relationships among terminal fieldsoriginating in different SI whisker barrels. The tendency forcontinuous topographic representations is further emphasized bythe finding of decreasing overlap of terminal fields with increasingseparation of cortical site of origin. We therefore hypothesizethat there are gradual shifts in the location of terminal fields,i.e., smooth shifts in the cortical influence on neurons in thepontine nuclei. Thus, a linear shift of neural activity withinor across rows of barrels in the cerebral cortex would evoke gradualshifts (inside-out or within lamellae, respectively) of activityin multiple pontine neuronalgroups.

Local integration or parallel pathways?

Organized topography is a prerequisite for parallel processing of information originating in different cortical domains. Thepresent study has demonstrated a clustered and lamellar topographyfor pontine projections from individual cortical barrels thatcould serve parallel processing functions. Two findings, however,suggest convergence of afferent signals from several barrels ontosingle pontine neurons. First, there is partial overlap (up to20%) (Table 1) between terminal fields after injections intonearby barrels. Second, the pontine terminal fields originatingin individual cortical barrels are generally more narrow thanthe dendritic trees of pontine neurons, as judged from comparisonsof our data with available illustrations of Golgi-stained (Mihailoffet al., 1981) or Lucifer Yellow-injected pontine cells (Schwarzand Thier, 1995). A comparison of Golgi-stained pontine neurons(Mihailoff et al., 1981, their Fig. 46) with the tracer-stainedterminal fields in our Figure 3D shows the potential for localintegration in the pontine nuclei. Thus, in line with the viewpresented by Malach (1994) for corticocortical connections, wesuggest that sharply defined, clustered terminal fields may facilitateintegration of signals and increase diversity of inputs to singleneurons [see also discussion by Brodal and Bjaalie (1997), Malmiercaet al. (1998); for a discussion of contrasting views, see Schwarzand Thier (1999), Bjaalie and Leergaard (2000), Schwarz and Thier(2000)]. The modular organization of the neostriatum has alsobeen viewed as suitable for specific integrative purposes (Graybiel,1990; Brown, 1992; Brown et al., 1998; Alloway et al., 1999).

In the context of putative parallel and re-entrant circuits (cerebro-ponto-cerebello-thalamo-cerebral loops) (Middleton andStrick, 2000), our data indicate that there is convergence alreadyat the level of the pontine nuclei of pathways originating inindividual adjacent cortical barrels ("open loop"). With increasingdistance between cortical barrels, we found that the degree ofoverlap in the pontine nuclei gradually decreases (resemblingmore "closed loops"). In the basal ganglia circuitry, Alexanderand coworkers (Alexander et al., 1986, 1990; Alexander and Crutcher,1990) proposed that functional integration would take place withinrather than among functionally related parallel circuits. In theneostriatum, such local integration is also indicated by the partiallyoverlapping projections from individual SI whisker barrels (Allowayet al., 1999). It is less clear whether pontine projections fromthe SI whisker barrel cortex overlap with projections from corticalregions representing other modalities (Ruigrok and Cella, 1995;Brodal and Bjaalie, 1997; Schwarz and Thier, 1999), or to whatdegree terminal fields from subcortical sources of pontine afferents(Kosinski et al., 1986, 1988; Aas, 1989; Aas and Brodal, 1989;Lee and Mihailoff, 1990; Mihailoff, 1995) (for review, see Ruigrokand Cella, 1995; Allen and Hopkins, 1998; Liu and Mihailoff, 1999)overlap with projections fromSI.

Implications for cerebellar functions

The organized SI-pontine topographic pattern reported in this study seems suitable for both specific integration (primarilyof signals from neighboring whisker barrels, possibly also ofother inputs, as discussed above) and segregation (of signalsfrom widely separated whisker barrels). The pattern predicts thatsequential activation of a column of whiskers (i.e., whiskersin the same location of different rows) leads to sequential activationof different neurons within the same lamellar subspace. Sequentialactivation of whiskers in the orthogonal direction (i.e., whiskerswithin the same row) would result in sequential activation ofdifferent lamellae in the pontine nuclei. Both spatial and temporalfeatures of whisker activation would be preserved in the pontinenuclei and would thus presumably reach thecerebellum.

It is not obvious how this anatomic arrangement would directly relate to cerebellar function. Ivry (1997) has suggested thatthe cerebellum is specifically involved in the processing of timinginformation. It would appear that the SI-pontine projection patternreported here is organized to preserve timing information in themovements of whiskers. A second theory of cerebellar functionthat would seem consistent with our findings is the sensory dataacquisition hypothesis of Bower (1997a,b). This theory, whichemerged from an analysis of the cerebellar perioral representationsof tactile surfaces in the rat, proposes that the cerebellum isspecifically involved in the control of sensory data acquisition.Furthermore, this theory proposes that the cerebro-ponto-cerebellarpathway is responsible for transferring information on the timingand context of cerebral cortically directed sensory acquisitionmovements and behaviors as well as information about the ongoingprocessing of sensory tactile data within the cerebral cortex.The organized pontine topography combined with local integrationcapabilities discussed above could represent a substrate for suchinformationtransfer.

  FOOTNOTES

Received May 12, 2000; revised Aug. 17, 2000; accepted Aug. 29, 2000.

Financial support was provided by European Community Grant Bio4 CT98-0182 to J.G.B., The Research Council of Norway, The NorwegianAcademy of Sciences, and National Institutes of Health Grant NS37532to K.D.A. We thank Annabjørg Bore and Christian Pettersen forexpert technical assistance, Petter Laake for helpful assistancewith the statistical analysis, and James M. Bower and Per Brodalfor valuable comments on thismanuscript.
Correspondence should be addressed to Dr. Jan G. Bjaalie, Department of Anatomy, Institute of Basic Medical Sciences, Universityof Oslo, P.O. Box 1105 Blindern, N-0317 Oslo, Norway. E-mail:j.g.bjaalie{at}basalmed.uio.no.

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