Anatomic Evidence of a Three-Dimensional Mosaic Pattern of Tonotopic Organization in the Ventral Complex of the Lateral Lemniscus in Cat

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The Journal of Neuroscience, December 15, 1998, 18(24):10603-10618

Anatomic Evidence of a Three-Dimensional Mosaic Pattern of Tonotopic Organization in the Ventral Complex of the Lateral Lemniscus in Cat
Manuel S. Malmierca¹, Trygve B. Leergaard², Victoria M. Bajo¹, Jan G. Bjaalie², and Miguel A. Merchán¹
¹ Laboratory for the Neurobiology of Hearing, Department of Cellular Biology and Pathology, University of Salamanca, and the Institute of Neuroscience of "Castilla y León" (INCyL) at Salamanca, E-37007 Salamanca, Spain, and ² Department of Anatomy, Institute of Basic Medical Sciences, University of Oslo, N-0317 Oslo, Norway

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The ventral complex of the lateral lemniscus (VCLL, i.e., the ventral and intermediate nuclei) is composed of cells embeddedin the fibers of the lateral lemniscus. These cells are involvedin the processing of monaural information and receive input fromthe collaterals of the fibers ascending to the inferior colliculus.Whereas tonotopic organization is a feature of all other nucleiof the auditory system, this functional principle is debated inthe VCLL. We have made focal injections of the tracer biotinylateddextran amine into different frequency band representations ofthe inferior colliculus in cat. Retrogradely labeled cells andterminal fibers (collaterals of efferent local axons and otherascending lemniscal fibers) were found in the ipsilateral VCLL.The spatial distribution of the labeling was analyzed using three-dimensional(3-D) reconstruction and computer graphical visualization techniques.A complex topographic organization was found. In all cases, labeledfibers and cells were distributed in multiple clusters throughoutthe dorsoventral extent of the VCLL. The shape, size, and locationof the labeled clusters suggest an interdigitation of clustersassigned to different frequency-band representations. But an overallmediolateral distribution gradient was observed, with high frequenciesrepresented medially and lower frequencies progressively morelaterally.
We conclude that the clusters may represent discontinuous frequency-band compartments as a counterpart to the continuous laminarcompartments in the remaining auditory nuclei. The 3-D orderlymosaic pattern indicates that the VCLL preserves the spectraldecomposition originated in the cochlea in a way that facilitatesacross-frequencyintegration.

Key words: auditory system; inferior colliculus; ventral complex of the lateral lemniscus; monaural system; tonotopic organization; frequency-band laminae; computer-assisted 3-D reconstruction; across-frequency integration

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

A spatial representation of tonal frequencies, termed tonotopic organization, is a fundamental organizing principle in virtuallyall central auditory nuclei (for review, see Irvine, 1992). Theorderly frequency-to-place transformation takes place in the cochlea(von Békésy, 1960). In the brain, the tonotopic organization(Irvine, 1992; Schreiner and Langner, 1997) is maintained by point-to-point(frequency-specific) connections between the auditory nuclei.The anatomic substrate for the tonotopic organization is relatedto a laminar organization of afferent fibers and recipient cells[e.g., in the cochlear nuclei (Pirsig et al., 1972; Bourk et al.,1981; Blackstad et al., 1984), inferior colliculus (Oliver andMorest, 1984; Malmierca, 1991; Malmierca et al., 1993), and medialgeniculate body (Morest, 1964)]. The present paper addresses theorganization of the nuclei of the lateral lemniscus, which inseveral respects has appeared different from that of other auditorynuclei.

Functionally, the nuclei of the lateral lemniscus constitute two separate systems of auditory processing: the dorsal nucleusof the lateral lemniscus (DNLL) belongs to the binaural system(for review, see Covey, 1993), whereas the ventral part, herecollectively referred to as the ventral complex of the laterallemniscus (VCLL; for review and definition, see Merchán et al.,1997), is part of the monaural system. The VCLL includes the ventraland intermediate nuclei and various subdivisions defined by otherson the basis of variable sets of criteria (van Noort, 1969; Adams,1979; Glendenning et al., 1981; Covey, 1993; Caicedo and Herbert,1993; Caicedo et al., 1996; Malmierca et al., 1996; Schofieldand Cant, 1997). Whereas the DNLL follows the general principleof laminar, tonotopic organization (Bajo et al., 1997; Merchánet al., 1997), such principles have not been easily demonstratedin the VCLL. In the cat VCLL, Aitkin et al. (1970) found a tendencyfor a dorsal-to-ventral gradient with low frequencies representeddorsally and high frequencies represented ventrally, whereas Guinanet al. (1972), also by electrophysiological methods, failed todemonstrate a tonotopic map. After injections of [³H]leucine into the cat VCLL, Whitley and Henkel (1984) found littleevidence of topographic projections and reported widespread labelingin the inferior colliculus (IC). In the bat, a complex tonotopicorganization may be present (Covey and Casseday, 1991; for review,see Covey, 1993; Covey and Casseday, 1995). By contrast, in recentstudies of the rat, Merchán and Berbel (1996) found a concentriclaminar pattern of retrogradely labeled cells in the VCLL aftersmall biotinylated dextran amine (BDA) injections into the centralnucleus of the IC(CNIC).

In the present study we have used the tracer BDA and extensive three-dimensional (3-D) computerized analyses to search fora tonotopic organization of the VCLL in cat. We provide anatomicevidence of a topographic projection from the VCLL to the CNIC.Our findings thereby suggest that the VCLL has a tonotopic organizationand thus follows the general principle of organization of theauditory system. The organization is, however, different fromthe characteristic laminar organization found in the remainingauditory nuclei. We discuss this organization and its possibleimplications in pitchperception.

Preliminary results have been presented elsewhere in abstract format (Merchán et al., 1996, Malmierca et al., 1997).

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Normal material. Serial sections of two formalin-fixed, paraffin-embedded adult cat brainstems were used for the identificationof the myeloarchitecture and cytoarchitecture of the lateral lemniscusand its nuclei (Figs 1, 2). The brain stems were sectioned at15 µm; one was cut transversely and the other horizontally. Sectionsof each fifth section were stained either with thionin or withthe Woelcke method for myelin (Woelcke, 1942) combined with cresylviolet cell staining. The normal material was kindly providedby Kirsten Osen (Department of Anatomy, University ofOslo).

Surgical procedures, injection, and histochemistry of tracer. For the tracing experiments, nine young adult cats of eithersex (weight, 2.0-4.4 kg) were used (Table 1). The animals wereanesthetized with intramuscular injection of a mixture of ketamine(57 mg/kg) and hydrazide chlorhydrate (8.6 mg/kg). Atropine sulfatewas given to minimize the production of bronchial secretions duringthe procedure. Aqueous solutions of 10% BDA (lysine-fixable biotinylateddextran; molecular weight, 10,000; D-1956; Molecular Probes, Eugene,OR) in 0.1 M phosphate buffer, pH 7.3, was injected iontophoreticallyinto the left IC by passing pulses of positive current (7 µA;duty cycle, 7 sec) for 20-30 min. The micropipette was positionedstereotactically into the CNIC following the coordinates of acat brain atlas (Reinoso-Suárez, 1961). The electrophysiologicalmaps of Merzenich and Reid (1974) and Servière et al. (1984)were used as a guide for placing injections in different frequencyregions (Fig. 3). The micropipette was left in situ for 15 min.


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Table 1. Summary of BDA injections in the cat CNIC

After 13-25 d survival, the animals were deeply anesthetized with an overdose of pentobarbital and transcardially perfusedwith lukewarm Ringer's solution followed by a mixture of freshlydepolimerized 0.2% glutaraldehyde and 4% paraformaldehyde in 0.1M phosphate buffer, pH 7.3. The brains were stored in 30% bufferedsucrose. Complete series of sections were cut at 40 µm with afreezing microtome in one of three standard planes (Table 1).The BDA labeling was visualized with an avidin-biotinylated HRPprocedure (ABC; Vectastain, Vector Laboratories, Burlingame, CA),as outlined by Veenman et al. (1992). Sections spaced at intervalsof 160-240 µm were counterstained with cresyl violet. Sectionswere photographed through a Zeiss (Thornwood, NY) Axiophot lightmicroscope (Figs 4A, 5).

Data analysis and computer-assisted 3-D reconstruction. Detailed camera lucida drawings of labeled structures and anatomiclandmarks in the region of the lemniscal nuclei were made in everysecond section at a total magnification of 84× (Fig. 6), usinga Leitz (Wetzlar, Germany) Diaplan microscope. Four cases werereconstructed in three dimensions (animals 93007, 94070, 95041,and 96028; Table 1). The camera lucida drawings were alignedwith the aid of the surface contours, vessels, and fiducial marks(made with a fine needle inserted through the tissue blocks beforesectioning) and digitized using a modified version of the programMicroTrace (Leergaard and Bjaalie, 1995; Leergaard et al., 1995).From each drawing, the external border of the VCLL, inside thetube of lemniscal fibers, was recorded as a contour line. Labeledneurons were recorded as single points, whereas the patches oflabeled structures (plexuses of labeled terminal fibers, labeledcells, and dendrites) were recorded as contour lines surroundingthe individual patches (Fig. 4). The contour lines were used forcalculating the volume of the VCLL and the labeled subspace (Table2). For comparisons of numbers of labeled cells in differentparts of the VCLL, we used simple profile counts. Thus, labeledcells were plotted without adjustment for double counts (for reviewof unbiased counting methods, cf. Coggeshall, 1992). However,we have used these data for studying major relative differenceswithin individual animals only. In this context, the bias introducedby the counting method is negligible.

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Figure 1. Photomicrograph of a Woelcke- and cresyl violet-stained frontal section through the cat brainstem. Horizontal arrows labeled 2A-2C indicate the approximate levels of the corresponding horizontal sections shown in Figure 2. The border between the DNLL and VCLL is indicated with white arrows and a dotted line. The lemniscal fibersencapsulate and pierce the VCLL and the DNLL in a continuous system. The lemniscus is supplied medially by ascending auditory fibers from the superior olivary complex and the dorsal cochlear nucleus crossing the midline in the reticular formation (asterisk). The thinner fiber fascicles of the commissure of Probst pierce the lemniscus from the medial side at the level of the DNLL. Scale bar, 500 µm. BP, Brachium pontis; CoP, commisure of Probst; D, dorsal; LL, lateral lemniscus; M, medial; PN, pontine nuclei.

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Figure 2. Photomicrographs of pairs of adjacent horizontal sections through the lateral lemniscus at the correspondingly labeled levels in Figure 1. The sections in each pair have been stained for myelin and cells (Woelcke and cresyl violet; A-C) and cells only (thionin; A'-C'). A and A' are at the level of the DNLL; the others are through the VCLL. The cellular area, inside the tube of external fibers, is marked by a dotted line in A'-C'. Differences in cytoarchitecture between the DNLL and VCLL have been used as criteria for defining the border between the two in the present study. The DNLL (A') is seen to be populated by uniformly large cells, which occur in irregular groups between the thick, unstained fiber fascicles. The VCLL (B', C'), in contrast, appears to contain neurons of various sizes, mainly medium-sized. The cells are more evenly dispersed, particularly in the ventral part where the cell density is also larger (C'), in conformity with the less prominent internal fiber component (C). Scale bar, 1 mm. BP, Brachium pontis; L, lateral; R, rostral; SAG, sagulum.


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Table 2. Estimated volume of the VCLL, number of labeled cells, and labeled volume

For 3-D visualization and analysis of the VCLL and the distribution of labeling (Figs. 7-12), we used software solutions developedat the Department of Anatomy, University of Oslo (E.O. Andersenand J.G. Bjaalie) for the Silicon Graphics (Mountain View, CA)Indigo 2 and O2 work stations (Leergaard et al., 1995, Bjaalieet al., 1997a). The software was partly based on available modulesin Open Inventor, release 2 (a commercially available graphicstool kit). Tissue shrinkage attributable to histological processingwas estimated to be 10% (range, 8-12%). To maintain correct proportionsin the reconstructions, the z values (distances between sectionplanes) assigned to each section were reduced correspondingly.The contour lines (VCLL external border and contour lines surroundingthe plexuses of labeling) were used for resynthesizing the surfaceof the VCLL (Figs. 7, 8) and the surface of individual clustersof labeling inside the VCLL (Fig. 8). The program Nuages (Geiger,1993) was used to create a surface model of the individual clusters.The model consists of separate clusters and clusters that wereinterconnected with thin bridges. To create a maximum fit to theoriginal data, an interactive procedure was used to define whetherclusters were continuous (bridged) or segregated. In all casesthere was little variation among clusters in the density of labeledterminal fibers. To demonstrate the distribution of labeling,each cluster was subsequently filled with a random pattern ofdots with a given density. The dot representation is used in Figures9, 10 and 11A-C. In Figures 11D-F and 12, it serves as a basis fora pseudo-color-coded density map. The density maps were producedby dividing a particular projection (view along the long axisof VCLL) of the reconstruction into squares of ~5 × 5 µm usinga grid. Each square was assigned a color corresponding to thedensity of cells within a radius of 100 µm centered on the square.Linear warping of data from multiple animals was obtained by aligningthe surface contours (Fig. 10).

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Figure 3. Photomicrographs of transverse sections through the center of the BDA injection sites in the left IC of the three cats used in Figures 4-12. Stars show the location of the tip of the injection electrode. Insets, Distribution of retrogradely labeled cells in a representative section through the lateral superior olive. The injections cover the high-frequency region (A), middle-frequency region (B), and low-frequency region (C). The estimated ranges of frequency representations covered by the injections are given in Table 1. Some of the staining represents labeling of the local fiber plexus in the IC (Malmierca et al., 1995). Scale bar, 1 mm.

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Figure 4. A, Photomicrograph showing patches of labeling in the VCLL after BDA injections into the ipsilateral IC (same case as shown in Fig. 5). B, Camera lucida drawing of the same region showing the location of the labeled cell somata (points), the patch borders (thick contour lines), and blood vessels (thin contour lines, v). The user focused through the thickness of the specimen to draw the patch border at the maximum extent of labeling. This explains the small deviations between the patch borders in the photomicrograph (A) and the contour lines in the drawing (B, arrows). The points and contour lines were digitized and served as a basis for the 3-D reconstructions. Scale bar, 100 µm.

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Figure 5. Photomicrographs of a transverse section through the VCLL of cat 94070 illustrating the labeling after BDA injection into the middle-frequency region of the ipsilateral IC (compare Fig. 3B). The framed regions are shown at higher magnification in B-D. The labeled structures are distributed in 2-D patches (3-D clusters) composed of labeled cell bodies, proximal dendrites, and a terminal fiber plexus. The patches are shaped as irregular bands ~150 µm thick. Elongated, labeled cell bodies and primary dendrites appear oriented in parallel with the long axis of the bands. Labeled axons en passage course vertically throughout the tissue. Dorsally, the labeling is more diffuse. Scale bars: A, 1 mm; B-D, 200 µm. D, Dorsal; L, lateral. LL, lateral lemniscus.

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Figure 6. Series of camera lucida drawings illustrating the patches of labeling in the VCLL after injections in the high-frequency region (compare Fig. 3A) and the low-frequency region (compare Fig. 3C) of the ipsilateral CNIC. Asterisks indicate lemniscal fibers crossing in the reticular formation (compare Fig. 1). In the high-frequency case, most of the labeling is located in the lateral half of the VCLL. The low-frequency case shows a larger amount of labeling. In this case, the patches occur throughout most of the VCLL, and topographic differences are difficult to define. The central part of the VCLL, however, contains less labeling than the medial and lateral borders. Scale bar, 1 mm. D, Dorsal; M, medial; S, section number.

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Figure 7. Computer-generated surface model of the VCLL, showing how the VCLL arbitrarily has been divided into dorsal, middle, and ventral thirds. The arrow represents the long axis of the VCLL. The angle of views from caudal, lateral, and dorsal (along the long axis of the VCLL), correspond the views used in Figures 8-12. C, Caudal; D, dorsal; M, medial; R, rostral.

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Figure 8. Computer-generated stereo pairs showing the 3-D distribution of labeling within the VCLL in the high-frequency case (A, A', B, B'; case 96028; Fig. 3A) and the low-frequency case (C, C', D, D'; case 93007; Fig. 3C). The external surface of the VCLL is represented as a transparent surface. The outer boundaries of the clusters containing labeling are visualized as solid surfaces. The stereopairs A and A' and C and C' are viewed from caudal, whereas B and B' and D and D' are viewed from lateral. To see a 3-D image, the viewer must cross the eye axis to let the pair of images merge. In A and A' and B and B', the clusters, as a general rule, are located adjacent to the rostrolateral surface of the VCLL. In C and C' and D and D', the clusters show a wider distribution with a mediocaudal predominance. Scale bar, 500 µm. C, Caudal; D, dorsal; M, medial; R, rostral.

Real-time rotations on the computer screen and stereo images (Fig. 8) were used for inspection from various angles and forperceiving depth. Computer images (Figs. 7-12) were printed on TektronixPhaser 440 and Phaser 450printers.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Shape and size of the VCLL

The DNLL and VCLL are embedded in the lateral lemniscus, which stretches from the rostral border of the superior olivary complexto the base of the IC. It constitutes the direct continuationof the trapezoid body after a sharp bend in the rostral and dorsaldirections. At the level of the VCLL, the fibers form two incompletelyseparated components: external and internal (Figs. 1, 2). Theexternal fibers form a peripheral tube, which is flattened mediolaterally.They have a straight course and are more clearly fasciculateddorsally. The internal fibers intermingle with the cells and mayinclude the ascending axons of these neurons. In agreement withthis notion, these fibers are more numerous and more clearly fasciculateddorsally, where they have a rather tortuous course. At the levelof the DNLL, the internal fibers form thick fascicles that mergewith the external fiber component.

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Figure 9. Computer 3-D dot maps showing the distribution of labeled fibers and cells within the VCLL, of the high-frequency case (A, D; case 96028; Fig. 3A), the middle-frequency case (B, E; case 94070; Fig. 3B), and the low-frequency case (C, F; case 93007; Fig. 3E). In A-C, the reconstructions are viewed from caudal; in D-F they are viewed from lateral. Labeled fibers are shown as gray dots, retrogradely labeled cells as black (larger) dots, and the external surface of the VCLL as contour lines. The density of labeled cells within the clusters does not show any systematic variation between the cases and the three parts of the VCLL. Scale bar, 500 µm. C, Caudal; D, dorsal; M, medial; R, rostral.

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Figure 10. Reconstructions from the three individual cases (high-, middle-, and low-frequency cases; Fig. 9) superimposed in the same model. Yellow dots represent the distribution of labeling in the high-frequency case, red dots the middle-frequency case, and blue dots the low-frequency case. The angles of view are the same as in Figure 9. In the caudal view (B) a gradual transition from lateral (yellow) toward central (red) and medial (blue) is observed. In several places, a complementary shape of the individual clusters is seen. For example, in the dorsal third, the elongated band-like clusters of the low-frequency case (blue) fit the holes of the more continuous pattern of labeling in the middle-frequency case (red). The clusters of the low-frequency case (blue) are mostly located laterally but partly embrace and penetrate the regions occupied by labeling of the other frequencies. C, Caudal; D, dorsal; M, medial; R, rostral.

We have used cytoarchitectonic and myeloarchitectonic criteria as a basis for outlining the VCLL (Figs. 1, 2). In our drawingsand 3-D reconstructions, we intended to include only the cellulararea and not the tube of external fibers (Fig. 2, compare thecell myelin- and Nissl-stained horizontal sections). [For a documentationof the detailed cell morphology, see Adams (1979) and Glendenninget al. (1981).]

As judged from individual sections (Figs. 1, 2, 5A, 6) and 3-D reconstructions (Figs. 7-12), the VCLL is shaped like a flattenedcylinder with the long axis oriented dorsoventrally and the largerdiameter of the oval cross-section oriented rostrocaudally. Thelarger diameter is smaller ventrally, where it deviates ~30° fromthe sagittal plane (Figs. 7, 8B,D, 9D-F, 12). Measured from our3-D reconstructions, the VCLL extends ~4-5 mm dorsoventrally,0.8 mm mediolaterally, and 1-2 mm rostrocaudally. The volume showslittle variation among the reconstructed cases with a mean of4.8 mm³ (Table 2).

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Figure 11. Dot maps (A-C) and color-coded density maps (D-F) of the distribution of labeling in the VCLL. The high-frequency case is shown in A and D, the middle-frequency case in B and E, and the low-frequency case in C and F (for further details, see legend to Fig. 9). The angle of view in all images is from dorsal, skewed slightly toward rostral and lateral, following the long axis of the VCLL, as indicated in Figure 7. For descriptive purposes, we introduce a reference line from rostromedial to caudolateral tentatively through the middle of the VCLL. The color gradient in D-F shows the highest densities in red and the lowest in violet. Densities <5% of the maximum value are not shown. Scale bar, 500 µm. M, Medial; R, rostral.

Prompted by the present analyses, we have arbitrarily divided the VCLL into three parts: the dorsal, middle, and ventral thirds,respectively (Fig. 7). They basically correspond with the threedivisions introduced by Adams (1979). The dorsal third approximatelycorresponds to the intermediate nucleus of Glendenning et al.(1981). We used these subdivisions as a basis for evaluating bothdifferences in the distribution and extent of labeling withinand between cases (Table 2).

Injection sites

Our nine injections together cover the whole range of audible frequency representations in the CNIC (Table 1), as determinedby previously published tonotopic maps obtained with electrophysiologicaltechniques (Rose et al., 1963; Merzenich and Reid, 1974; Sempleand Aitkin, 1979) and [¹⁴C]2-deoxiglucose experiments (Servière et al., 1984). In thefollowing, the distribution of labeling in three representativeanimals will be illustrated and analyzed in detail: case 93007,injected in the low-frequency region; 94070, in the middle-frequencyregion; and 96028, in the high-frequency region (Table 1, Fig.3).

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Figure 12. Color-coded density maps of the distribution of labeling in the three defined parts of the VCLL, dorsal, middle, and ventral thirds, in each of the high-, middle-, and low-frequency cases. The reference lines at the top and bottom indicate the tentative orientation of the larger diameter in the cross-sections. From dorsal to ventral, the angle of the reference lines shifts ~30° (from a rostral-to-caudal orientation dorsally, to a rostromedial-to-caudolateral orientation ventrally). The maps show a tendency for a banded distribution, most prominent in the ventral and middle thirds. Several shapes are visible, e.g., U-shaped bands and finger-like extensions in the middle- and low-frequency cases. Presentation is otherwise as in Figure 7D-F. Scale bar, 500 mm. M, Medial; R, rostral.

The center of each injection site can be readily identified (Fig. 3A-C, stars). Judging by the extent of staining at the injectionsite, the three injections are segregated, although together theycover the larger part of the tonotopic axis of the CNIC. The resultinglabeling in the lower auditory nuclei, which is in agreement withprevious studies on the ascending and descending connections ofthe cat CNIC (Adams, 1979), shows that the active uptake sitesin the three illustrated cases occupy clearly segregated compartmentsalong the well known tonotopic axis of the IC. This is illustratedby the distribution of labeling in the lateral superior olive(Fig. 3, insets) which is in accordance with well establishedtonotopic map of Tsuchitani and Boudreau (1969).

General features of labeling

As expected, the VCLL is labeled only on the side ipsilateral to the injection site. The labeling includes cell somata, dendriticprocesses, thick and thin axons, and terminal plexuses, includingen passant and terminal varicosities. This is in accordance withreports by Merchán et al. (1994) and Merchán and Berbel (1996),who described retrograde transport of BDA to cell bodies and anterogradetransport into the collaterals of retrogradely labeled neuronsthat innervate the injection sites in the rat IC. In our sections,the labeled structures appear intermingled in well defined, mostlyflattened or elongated patches (Figs. 5, 6), separated by unlabeledcellular areas (as judged by comparing pairs of BDA-incubatedand cresyl violet-stained sections). The density of labeled fiberswithin the patches is approximately the same throughout the VCLL,whereas the density of labeled cells is uneven. Elongated cellsand dendrites tend to be oriented along the length of the patches.Only few labeled somata or dendrites occur outside the patches(Fig. 5D). Solitary thick and vertically oriented labeled fiberspass through the patches (Fig. 5). These axons may ascend frommore ventral parts of the VCLL or from other sources connectedwith the IC injection sites. The reconstructions show that thetwo-dimensional (2-D) patches form 3-D clusters (compare Figs.6, 8).

The extent of labeling differs among cases (Table 2). The total labeled volume (i.e., the tissue volume occupied by clustersof labeling) and the total number of labeled cells are largestin the middle-frequency case and smallest in the high-frequencycase. The extent of labeling also differs along the dorsoventralaxis of the VCLL. The differences in labeled volume and cell numbersamong the cases are most conspicuous in the dorsal third. Thehighest amount of labeling was found in the dorsal third in themiddle-frequency case. These quantitative differences could berelated both to the size and the dorsoventral location of theinjection sites. In our middle-frequency case, in which the injectionsite is relatively large and seems to involve also the ventralpart of the dorsal cortex of the IC (Fig. 3B), the labeling inthe dorsal third of the VCLL is heavier than in the othercases.

Shape and size of clusters

The clusters of labeling illustrated in Figures 5 and 6 and in dot maps (Fig. 9) are shown to advantage in the stereo pairs(Fig. 8). The individual clusters appear mostly elongated, witha highly variable thickness (down to 100 µm) and a length up to2 mm. They exhibit a systematic variation in size and shape amongthe dorsal, middle, and ventral thirds of the VCLL. There arealso differences among the threecases.

In the high- and low-frequency cases, the clusters in the ventral and middle thirds appear like mostly vertically orientedirregular plates interconnected by thin bridges. In the dorsalthird, they are smaller, elongated (band-like), narrow, and tortuousand tend to be oriented rostrocaudally. In the middle-frequencycase (Fig. 9B,E), the clusters form a more continuous system,which appears like a winding central core with peripheral extensions,whereas in the dorsal third, on the contrary, it consists of small,rounded clusters that merge into a spongeous pattern (also seeFig. 5A). This dorsoventral difference is also present in a reconstructionfrom another, sagittally sectioned middle-frequency case (95041;Table 1, reconstruction not shown). A possible interpretationwould be that the more continuous system of labeling in the middlefrequency case is a "negative image" of the clusters of the otherfrequencies. The shape, size, and location of the labeled clustersthereby suggest an interdigitation of clusters assigned to differentfrequency band representations. This interpretation is supportedby the model shown in Figure 10, where the three reconstructionsaresuperimposed.

Topographic organization

In all cases, the labeled clusters are found at all dorsoventral and rostrocaudal levels (Figs. 6, 8-10). In the horizontal domain,however, the distribution of labeling (Figs. 6, 8-12) varies as afunction of the location of the injection sites along the tonotopicaxis of the IC. The distribution pattern is complicated, and differencesbetween cases are difficult to see in individual sections (Fig.6). The 3-D reconstructions, however, reveal a mediolateral distributiongradient with high frequencies represented mainly laterally andmiddle and lower frequencies progressively more medially (Figs.8-12). In the following, we will describe the three cases indetail.

In the high-frequency case, an angle of view from caudal shows that the labeling is concentrated in the lateral half of theVCLL (Figs. 8A, 9A, 10B). In the middle-frequency case, the labelingappears evenly distributed in the rostrocaudal dimensions buttends to avoid the medial and lateral borders of the complex (Fig.9B,E). In the low-frequency case, the clusters occur throughoutmost of the VCLL. However, in the ventral and middle thirds, thelabeling is skewed toward the medial and caudal surfaces, withfour to six finger-like extensions along the lateral surface andinto the central parts of the nucleus (Figs. 8C, stereo view required,9C). In the dorsal third, the labeling is more evenlydistributed.

An angle of view from dorsal (Fig. 11), along the "dorsoventral" long axis of the VCLL (as shown in Fig. 7, arrows), is helpfulfor further understanding the topographic differences. For descriptivepurposes, we introduce a horizontal reference line from rostromedialto caudolateral through the middle of the VCLL. The labeling inthe high-frequency case is largely confined to the lateral half(Fig. 11A). In the middle- and low-frequency cases, the distributionof labeling is more widespread (Fig. 11B,C, respectively). However,in the middle-frequency case, there is a zone of higher densityof labeling centered on the reference line (Fig. 11B). In the low-frequencycase, by contrast, there is a high-density zone on each side ofthe reference line, with the higher density of labeling medially(Fig. 11C). The same distribution gradients are shown in the color-codeddensity maps for the VCLL as a whole (Fig. 11D-F) and in more detailin each third from dorsal to ventral (Fig. 12).

Some further topographical details are revealed in Figure 12. In the high-frequency case (Fig. 12A-C), the labeling is confinedto a laminar subspace, visible as rostrocaudally oriented bandsin the lateral half of each image. In the middle-frequency case(Fig. 12D-F), the highest densities of labeling are located inthe center with gradually decreasing densities toward the externalborder. The high densities (red and yellow) have a banded distribution,particularly in the ventral two-thirds (Fig. 12E,F). In the low-frequencycase (Fig. 12G-I), the highest densities are located in the medialhalf, with extensions toward lateral. The high densities (fromred to blue) form a band-like pattern also in the ventral two-thirds(Fig. 12H,I).

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

By combined tract-tracing methods and computer-assisted 3-D reconstructions, we have provided anatomic evidence in cat fortopographic connections between the VCLL and the IC. The labelingpattern has three main characteristics: (1) labeled cell bodies,dendrites, and terminal fibers of similar frequencies colocalizein distinct clusters; (2) the shape and size of clusters differfrom ventral to dorsal; and (3) there is a topographic organization,with low-frequency clusters predominating medially and high-frequencyclusters predominating laterally. The present data therefore indicatethat a tonotopic organization is present in the VCLL and in itsconnections. However, this topography is different and uniquecompared with other auditory structures and may serve functionsother than mere frequencycoding.

Clustering

The clustered pattern of projection from the VCLL to frequency-specific domains in the IC conforms with previous observationsin cat (van Noort, 1969; Roth et al., 1978; Adams, 1979; Glendenninget al., 1981; Henkel and Spangler, 1983; Whitley and Henkel, 1984;Oliver, 1987; Glendenning and Hutson, 1998). The present studycomplements these studies by demonstrating the 3-D organizationof the clusters (previously depicted as 2-D patches) and the colocalizationof labeled somata, dendritic processes, and terminal fields ofaxonal collaterals (originating in the lower auditory centersprojecting to the IC and locally in the VCLL; cf. Whitley andHenkel, 1984). Our material, as well as corresponding BDA experimentsin rat, shows that the space between the labeled clusters containsunlabeled cells (Merchán and Berbel, 1996, their Fig. 3). Thisdemonstrates that the clustering is a primary feature not merelycaused by molding factors such as fascicles of unlabeled fibers(internal fibers; see Figs. 1, 2). Such fibers could originatefrom sources not connected with the IC [i.e., principal cellsof the medial nucleus of the trapezoid body (Glendenning et al.,1981; Spangler et al., 1985), octopus cells of the posteroventralcochlear nucleus (Cant, 1997; Schofield and Adams, 1997), andspherical and globular cells of the anteroventral cochlear nucleus(Friauf and Ostwald, 1988; Smith et al., 1991, 1993)]. The clusterpattern contrasts the laminar tonotopic organization of otherbrainstem auditory nuclei, e.g., the inferior colliculus (Malmiercaet al., 1995), but it is a well known feature from other brainregions such as the striatum (Gaybriel and Ragsdale, 1978; Gerfen,1992) and the nearby pontine nuclei (Brodal and Bjaalie, 1997).

Tonotopy

The interdigitating, clustered pattern has hampered previous attempts to reveal a tonotopic organization of the VCLL. In thepresent study, however, using sophisticated 3-D computerized analyses,we have demonstrated a topographic distribution pattern, whichmost probably represents the substrate for a tonotopicorganization.

A horizontal frequency gradient axis has been demonstrated previously in the VCLL of the rat (Merchán and Berbel, 1996).A concentric organization was proposed, with low frequencies representedperipherally and high frequencies in the center. In the ventralhalf of the VCLL, however, the high-frequency zone came to thelateral border of the complex (Merchán and Berbel, 1996, theirFig. 8), in accordance with the situation in thecat.

Our findings are compatible with the data shown in two electrophysiological studies of cat (Aitkin et al., 1970) and rabbit(Batra and Fitzpatrick, 1997). Aitkin et al. (1970) inserted electrodesvertically and recorded best frequency responses to pure tonestimulation. Their Figure 1 illustrates a case in which the electrodepassed medial to the junction between the DNLL and VCLL and thenpenetrated the VCLL obliquely from dorsomedial to ventrolateral.As the electrode passed through the VCLL, a full sequence of bestfrequencies from low to high was recorded. This was interpretedas a dorsoventral tonotopic organization. However, given the angleof the electrode penetration, the findings of Aitkin et al. (1970)are consistent with the mediolateral tonotopic gradient demonstratedin the present study. More recently, Batra and Fitzpatrick (1997)have recorded single units in the medial region of the rabbitVCLL with best frequencies <2kHz.

The present observations are also compatible with previous anatomic studies. After injections of horseradish peroxidase infrequency-specific regions of the IC, Adams (1979) showed retrogradelylabeled cells throughout the dorsoventral extent of the VCLL.With the use of anterograde labeling after injections of [³H]leucine in the VCLL, Whitley and Henkel (1984) likewise concludedthat the VCLL has a widespread and diffuse projection to the CNIC.However, in agreement with our findings, an injection centeredon the lateral part of the VCLL (Whitley and Henkel, 1984, theirFig. 4C) produced heavier labeling in the high-frequency regionof the CNIC (their Fig. 3). After an injection in the medial partof the VCLL (Whitley and Henkel, 1984, their Fig. 4E), a higheramount of labeling occurred in the low-frequency part of the CNIC.Indeed, Whitley and Henkel (1984) discussed that their smallestinjection located in the medial edge of the VCLL could be interpretedas an evidence of a mediolateral tonotopicorganization.

Dorsoventral differences

Although the overall topographic gradient is the same throughout the dorsoventral aspect of the VCLL, the dorsal third differsfrom the middle and ventral thirds in other ways: (1) the clusterpattern is different (Fig. 8); (2) the extent of labeling suggeststhat it has a different projection to the IC, also including thedorsal cortex (Whitley and Henkel, 1984); (3) it is made of presumablyexcitatory cells, in contrast to the glycinergic and GABAergiccells of the ventral two-thirds (Winer et al., 1995; Saint Marieet al., 1997; Vater et al., 1997; Riquelme et al., 1998); and(4) it receives a glycinergic input from the medial nucleus ofthe trapezoid body (Glendenning et al., 1981; Spangler et al.,1985).

Functional significance

In most auditory nuclei, tonal frequencies are represented in continuous laminar compartments (for review, see Irvine, 1992).In this context, the clustered, interdigitating tonotopic patternfound in the VCLL represents an exception. Other neural systems,however, contain organizational principles resembling those reportedhere for the VCLL. The pontine nuclei, intercalated in the mainpathway from the cerebral cortex to the cerebellum, have beenshown to contain a loose laminar organization of both corticopontinefiber and pontocerebellar neurons (Nikundiwe et al., 1994; Bjaalieet al., 1997b). At a small scale, both fibers and cells, topographicallyrelated to specific cerebral and cerebellar areas, are locatedin clusters. At a large scale, the clusters tend to occupy laminarsubspaces, which are usually thick and probably overlapping. Theinterdigitating, frequency-specific clusters seen in the VCLL(Fig. 10) resemble this pattern. This organization may create alarge interface between compartments connected to different partsof the CNIC, comparable to the situation in the pontine nuclei,in which there seem to be extensive interfaces between differentterminal fields originating in different parts of the cerebralcortex. Also in the cerebral cortex, axonal clusters are viewedas devices for maximizing neuronal diversity rather than devicesfor segregation of information in separate processing streams(Malach, 1994). In the VCLL, the pattern of widespread, interdigitatingclusters, confined within distinct compartments, could likewiseserve to create diversity of neuronal properties.

The functional implication of this pattern would depend on the spatial relationship of the dendritic arbors to the clusterborders. In our study, the labeled dendritic processes are regularlyconfined to a cluster. Reservations, however, have to be madefor unlabeled dendrites. Vater et al. (1997) demonstrated thatcalyx-like terminals on VCLL cells form collaterals contactingdendritic processes of nearby cells. They therefore suggestedthat VCLL dendrites could extend into multiple tonotopic areas.The few Golgi studies of dendritic arbors (Willard and Martin,1983; Willard and Ryugo, 1983) and electrophysiological studiesof tuning curves (Guinan et al., 1972; Covey and Casseday, 1991,1995) in the lateral lemniscal nuclei are, however, inconclusivein thisregard.

Then what is the role in audition of the clustered, interdigitating tonotopic pattern of the VCLL? Currently, there is goodpsychophysical evidence to suggest that pitch perception needsnot only spectral (Goldstein, 1973; Yost, 1982) but also temporal(Moore and Rosen, 1979) information. There is a wealth of dataindicating that the VCLL neurons are well suited to analyze thetemporal properties of the auditory signals (Covey and Casseday,1991; for extensive review, see Covey and Casseday, 1995). Licklider(1951), and later Meddis and Hewitt (1991), have launched a modelto explain human pitch perception. This model proposes the summationof the autocorrelated cell responses across frequency-selectivechannels as a mechanism for extracting a combination of both temporaland spectral information. The model has been tested successfullyfor various types of pitch stimuli (Meddis and O'Mard, 1997).It requires a neuronal circuitry that can generate (1) delayedversions of the input signal, (2) convergence of the delayed signalsonto single cells, and (3) convergence between different frequencychannels. The VCLL could meet these requirements by (1) the multipleladder-like collaterals of the long lemniscal afferents, (2) thelocal collaterals with ventral neurons supplying successivelymore dorsal neurons (Whitley and Henkel, 1984), and (3) the spatiallyspecific, but still interdigitating, frequency representations.The detailed circuitry of the VCLL, however, remains to be verified,and it is uncertain how the inhibitory nature of the neurons inthe ventral two-thirds of the VCLL would suit the model. The presentfindings, nevertheless, open new avenues to further investigationof this hitherto poorly understood link in the ascending auditorypathway.

  FOOTNOTES

Received June 29, 1998; revised Oct. 2, 1998; accepted Oct. 6, 1998.

Financial support was provided by Spanish Direccíon General de Enseñanza Superior Grants PB95-1129 and PB97-1326 (to M.A.M)and by grants from the Research Council of Norway, The Nansenfoundation, and The Jahre foundation (to J.G.B.). M.S.M. was supportedby the Spanish Ministerio de Educación y Ciencia and the Commissionof the European Union. V.M.B. was supported by the Spanish Ministeriode Educación y Ciencia. We thank Enrique López-Poveda, DouglasL. Oliver, Kirsten K. Osen, and Enrique Saldaña for valuablecomments and I. Plaza, F. R. Nodal, G. F. Lothe, C. Knudsen, andE. O. Andersen for expert technicalassistance.
Correspondence should be addressed to Dr. Manuel S. Malmierca, Laboratorio de Neurobiología de la Audición, Departamentode Biología Celular y Patología, Facultad de Medicina. Universidadde Salamanca. C/Alfonso X el Sabio, s/n Campus "Miguel de Unamuno,"37007 Salamanca,Spain.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Adams JC (1979) Ascending projections to the inferior colliculus. J Comp Neurol 183:519-538[ISI][Medline].
Adams JC (1997) Projections from octopus cells of the posteroventral cochlear nucleus to the ventral nucleus of the lateral lemniscus in cat and human. Auditory Neurosci 3:335-350.
Aitkin LM, Anderson DJ, Brugge JF (1970) Tonotopic organization and discharge characteristics of single neurons in the nuclei of the lateral lemniscus of the cat. J Neurophysiol 33:421-440[Free Full Text].
Batra R, Fitzpatrick DC (1997) Neurons sensitive to interaural temporal disparities in the medial part of the ventral nucleus of the lateral lemniscus. J Neurophysiol 78:511-515[Abstract/Free Full Text].
Bajo VM, Merchán MA, Malmierca MS, Bjaalie JG, Nodal FR (1997) The topographical organization from the dorsal nucleus of the lateral lemniscus to the central nucleus of the inferior colliculus in the cat. Assoc Res Otolaryngol Abstr 20:165.
Bjaalie JG, Daehlen M, Stensby TV (1997a) Surface modelling of biomedical data. In: Numerical methods and software tools in industrial mathematics (Tveito A, Daehlen M, eds), pp 9-26. Boston: Birkhauser.
Bjaalie JG, Sudbø J, Brodal P (1997b) Corticopontine terminal fibres form small scale clusters and large scale lamellae in the cat. NeuroReport 8:1651-1655[ISI][Medline].
Blackstad TW, Osen KK, Mugnaini E (1984) Pyramidal neurones of the dorsal cochlear nucleus: a Golgi and computer reconstruction study in cat. Neuroscience 13:827-854[ISI][Medline].
Brodal P, Bjaalie JG (1997) Salient anatomic features of the cortico-ponto-cerebellar pathway. Prog Brain Res 114:227-249[ISI][Medline].
Bourk TR, Mielcarz JP, Norris BE (1981) Tonotopic organization of the anteroventral cochlear nucleus of the cat. Hear Res 4:215-241[ISI][Medline].
Caicedo A, Herbert H (1993) Topography of descending projections from the inferior colliculus to auditory brainstem nuclei in the rat. J Comp Neurol 328:377-392[ISI][Medline].
Caicedo A, d'Aldin C, Puel J-L, Eybalin M (1996) Distribution of calcium-binding protein immunoreactivities in the guinea pig auditory brainstem. Anat Embryol 194:465-487[Medline].
Coggeshall RE (1992) A consideration of neural counting methods. Trends Neurosci 15:9-13[ISI][Medline].
Covey E (1993) The monaural nuclei of the lateral lemniscus: parallel pathways from cochlear nucleus to midbrain. In: The mammalian cochlear nuclei: organization and function (Merchán MA, Juiz JM, Godfrey DA, Mugnaini E, eds), pp 321-334. New York: Plenum.
Covey E, Casseday JH (1991) The monaural nuclei of the lateral lemniscus in an echolocating bat: parallel pathways for analyzing temporal features of sound. J Neurosci 11:3456-3470[Abstract].
Covey E, Casseday JH (1995) The lower brainstem auditory pathways. In: Hearing in bats (Popper AN, Fay RR, eds), pp 235-295. New York: Springer.
Friauf E, Ostwald J (1988) Divergent projections of physiologically characterized rat ventral cochlear nucleus neurons as shown by intra-axonal injection of horseradish peroxidase. Exp Brain Res 73:263-284[ISI][Medline].
Gaybriel AM, Ragsdale CW (1978) Histochemically distinct compartments in the striatum of human, monkey and cat demonstrated by acetylchlolinesterase staining. Proc Natl Acad Sci USA 75:5723-5726[Abstract/Free Full Text].
Geiger B (1993) In: Three-dimensional modelling of human organs and its application to diagnosis and surgical planning. Report 2105. Sophia-Antipolis, France: Institut National de Recherche en Informatique et en Automatique.
Gerfen CR (1992) The neostriatal mosaic: multiple levels of compartmental organization in the basal ganglia. Annu Rev Neurosci 15:285-320[ISI][Medline].
Glendenning KK, Hutson KA (1998) Lack of topography in the ventral nucleus of the lateral lemniscus. Microsc Res Tech 41:298-312[ISI][Medline].
Glendenning KK, Brunso-Bechtold JK, Thompson GC, Masterton RB (1981) Ascending auditory afferents to the nuclei of the lateral lemniscus. J Comp Neurol 197:673-704[ISI][Medline].
Goldstein JL (1973) An optimum processor theory for the central formation of the pitch of complex tones. J Am Soc Audiol 54:1496-1515.
Guinan Jr JJ, Norris BE, Guinan SS (1972) Single auditory units in the superior olivary complex: II. Locations of unit categories and tonotopic organization. Int J Neurosci 4:147-166.
Henkel CK, Spangler KM (1983) Organization of the efferent projections of the medial superior olivary nucleus in the cat as revealed by HRP and autoradiographic tracing methods. J Comp Neurol 221:416-428[ISI][Medline].
Irvine DRF (1992) Physiology of the auditory brainstem. In: The mammalian auditory pathway: neurophysiology (Popper A, Fay RR, eds), pp 153-231. New York: Springer.
Leergaard TB, Bjaalie JG (1995) Semi-automatic data acquisition for quantitative neuroanatomy. MicroTrace $---$ computer programme for recording of the spatial distribution of neuronal populations. Neurosci Res 22:231-243[ISI][Medline].
Leergaard TB, Lakke EAJF, Bjaalie JG (1995) Topographical organization in the early postnatal corticopontine projection: a carbocyanine dye and 3-D computer reconstruction study in the rat. J Comp Neurol 361:77-94[ISI][Medline].
Licklider JCR (1951) A duplex theory of pitch perception. Experimentia 7:128-133[ISI][Medline].
Malach R (1994) Cortical columns as devices for maximizing neuronal diversity. Trends Neurosci 17:101-104[ISI][Medline].
Malmierca MS (1991) In: Computer-assisted three-dimensional reconstructions of Golgi impregnated cells in the rat inferior colliculus Doctoral thesis Universities of Oslo and Salamanca.
Malmierca MS, Blackstad TW, Osen KK, Karagülle T, Molowni RL (1993) The central nucleus of the inferior colliculus in rat: a Golgi and computer reconstruction study of neuronal and laminar structure. J Comp Neurol 333:1-27[ISI][Medline].
Malmierca MS, Rees A, Le Beau FEN, Bjaalie JG (1995) Laminar organization of frequency-specific local axons within and between the inferior colliculi of the guinea pig. J Comp Neurol 357:124-144[ISI][Medline].
Malmierca MS, Le Beau FEN, Rees A (1996) The topographical organization of descending projections from the central nucleus of the inferior colliculus in guinea pig. Hear Res 93:167-180[ISI][Medline].
Malmierca MS, Merchán M, Bajo VM, Bjaalie JG (1997) The ventral nucleus of the lateral lemniscus in cat is tonotopically organized. Assoc Res Otolaryngol Abstr 20:164.
Meddis R, Hewitt MJ (1991) Virtual pitch and phase sensitivity of a computer model of the auditory periphery I: pitch identification. J Am Soc Audiol 89:2866-2882.
Meddis R, O'Mard LP (1997) A unitary model of pitch perception. J Am Soc Audiol 102:1811-1820.
Merchán MA, Berbel P (1996) Anatomy of the ventral nucleus of the lateral lemniscus in rats: a nucleus with a concentric laminar organization. J Comp Neurol 372:245-263[ISI][Medline].
Merchán MA, Saldaña E, Plaza I (1994) Dorsal nucleus of the lateral lemniscus in the rat: concentric organization and tonotopic projection to the inferior colliculus. J Comp Neurol 342:259-278[ISI][Medline].
Merchán MA, Bajo VM, Malmierca MS, Bjaalie JG (1996) The laminar organization of the nuclei of the lateral lemniscus (NLL): a tracer and computer reconstruction study in cat. Paper presented at the 2nd International Symposium on Acoustical Signal Processing in the Central Auditory System, Prague, September.
Merchán MA, Malmierca MS, Bajo VM, Bjaalie JG (1997) The nuclei of the lateral lemniscus: old views and new perspectives. In: Acoustical signal processing in the central auditory system (Syka J, ed), pp 211-226. New York: Plenum.
Merzenich MM, Reid MD (1974) Representation of the cochlea within the inferior colliculus of the cat. Brain Res 77:397-415[ISI][Medline].
Moore BCJ, Rosen SM (1979) Tune recognition with reduced pitch and interval information. J Exp Psychol 31:229-240.
Morest DK (1964) The laminar structure of the inferior colliculus of the cat. Anat Rec 148:314.
Nikundiwe AM, Bjaalie JG, Brodal P (1994) Lamellar organization of pontocerebellar neuronal populations. A multi-tracer and 3-D computer reconstruction study in the cat. Eur J Neurosci 6:173-186[ISI][Medline].
Oliver DL (1987) Projections to the inferior colliculus from the anteroventral cochlear nucleus in the cat: possible substrate for binaural interaction. J Comp Neurol 264:24-46[ISI][Medline].
Oliver DL, Morest DK (1984) The central nucleus of the inferior colliculus in the cat. J Comp Neurol 222:237-264[ISI][Medline].
Pirsig W, Noda Y, Lehmann I (1972) Tonotope Abbildung der Cochlea im Nucleus cochlearis ventralis des Meerschweinchens. Arch Klin Exp Ohren Nasen Kehlkopfheilk 202:494-500.
Reinoso-Suárez F (1961) In: Topographischer Hirnatlas der Katze für experimental-physiologische Untersuchungen. Darmstadt: Merck.
Riquelme R, Merchán MA, Ottersen OP (1998) GABA and glycine in the ventral nucleus of the lateral lemniscus: an inmunocytochemical and in situ hybridization study in rat. Assoc Res Otolaryngol Abstr 21:93.
Rose JE, Greenwood DD, Goldberg JM, Hind JE (1963) Some discharge characteristics of single neurons in the inferior colliculus of the cat: I. Tonotopical organization, relation of spike-counts to tone intensity, and firing patterns of single elements. J Neurophysiol 26:314-319.
Roth GL, Aitkin LM, Andersen RA, Merzrnich MM (1978) Some features of the spatial organization of the central nucleus of the inferior colliculus of the cat. J Comp Neurol 182:661-680[ISI][Medline].
Saint Marie RL, Shneiderman A, Stanforth DA (1997) Patterns of $gamma$ -aminobutyric acid and glycine immunoreactivities reflect structural and functional differences of the cat lateral lemniscal nuclei. J Comp Neurol 389:264-276[ISI][Medline].
Schofield BR, Cant NM (1997) Ventral nucleus of the lateral lemniscus in guinea pigs: cytoarchitecture and inputs from the cochlear nucleus. J Comp Neurol 379:363-385[ISI][Medline].
Schreiner CE, Langner G (1997) Laminar fine structure of frequency organization in the auditory midbrain. Nature 388:383-386[Medline].
Semple MN, Aitkin LM (1979) Representation of sound frequency and laterality by units in central nucleus of cat inferior colliculus. J Neurophysiol 42:1626-1639[Abstract/Free Full Text].
Servière J, Webster WR, Calford MC (1984) Isofrequency labelling revealed by a combined [¹⁴C]-2-deoxyglucose, electrophysiological, and horseradish peroxidase study of the inferior colliculus of the cat. J Comp Neurol 228:463-477[ISI][Medline].
Smith PH, Joris PX, Carney LH, Yin TCT (1991) Projections of physiologically characterized globular bushy cell axons from the cochlear nucleus of the cat. J Comp Neurol 304:387-407[ISI][Medline].
Smith PH, Joris PX, Yin TCT (1993) Projections of physiological characterized spherical bushy cell axons from the cochlear nucleus of the cat: evid