Functional Specificity of Callosal Connections in Tree Shrew Striate Cortex

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The Journal of Neuroscience, March 15, 2000, 20(6):2346-2359

Functional Specificity of Callosal Connections in Tree Shrew Striate Cortex
William H. Bosking¹, Robert Kretz², Michele L. Pucak¹, and David Fitzpatrick¹
¹ Department of Neurobiology, Duke University Medical Center, Durham, North Carolina 27710, and ² Department of Anatomy, University of Fribourg, CH-1700 Fribourg, Switzerland

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Although callosal connections have been shown to link extensive regions of primary visual cortex, the distribution of theseconnections with respect to the map of visual space and the mapof orientation preference remains unclear. Here we combine opticalimaging of intrinsic signals with injection of fluorescent microspheresto assess the functional specificity of callosal connections inthe tree shrew. By imaging both hemispheres simultaneously whilepresenting a series of spatially restricted stimuli, we find thata substantial region of visual space is represented bilaterally.Each hemisphere includes a representation of the ipsilateral visualfield that is highly compressed relative to that of the contralateralvisual field and is most extensive in the lower visual field,where ~30^o of central visual space are represented bilaterally. Callosalconnections extend throughout the region of bilateral representationbut terminate in a spatially restricted manner that links visuotopicallycorresponding sites in the two hemispheres. In contrast, callosalconnections appear to terminate without regard for the map oforientation preference, showing little sign of the orientation-specificmodular and axial specificity that is characteristic of long-rangehorizontal connections. By coordinating the activity in the twohemispheres in a way that preserves nearest neighbor relationships,callosal connections may best be viewed as elements of local circuitsthat operate within a single bilateral representation of visualspace.

Key words: optical imaging; intrinsic signals; corpus callosum; horizontal connections; visual field; visual cortex; orientation selectivity; visuotopic; ipsilateral visual field

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Unlike the representation of other regions of visual space, the cortical representation of regions near the visual midlineis divided between the two hemispheres. Because of this division,callosal connections, which link together sites in primary visualcortex (V1) of the two hemispheres, are thought to play an importantrole in processing information from the central part of visualspace. Compared to other systems of cortical connections, however,there is still considerable uncertainty about how the anatomicalarrangement of callosal connections relates to the functionalarchitecture ofV1.

Based on early anatomical and physiological studies, callosal connections were thought to be largely confined to the V1/V2border and to link together neurons whose receptive fields wererestricted to regions adjacent to the vertical meridian (VM) (Choudhuryet al., 1965; Hubel and Wiesel, 1967; Berlucchi and Rizzolatti,1968). The limited extent of the connections fit the view thatcallosal connections served the role of local intrinsic circuitselsewhere in V1: in particular, these connections were thoughtto supply information from the ipsilateral visual field for cellswhose receptive fields spanned the VM (Hubel and Wiesel, 1967).However, although this restricted organization may be the rulefor higher primates, in some primates and in many nonprimate species,callosal connections are far more expansive, originating and terminatingat sites located up to 2-3 mm away from the V1/V2 border (Swadlowet al., 1978; Cusick et al., 1984, 1985; Sesma et al., 1984; Pritzelet al., 1988; Kretz and Rager, 1990; Payne, 1991; Payne and Siwek,1991; Grigonis et al., 1992). The overall extent of callosal connectivityin these species raises the possibility that callosal connectionslink sites whose receptive fields are significantly displacedfrom the VM and suggests that the callosal pathway may have morein common with the system of long-distance horizontal connectionsthat exists within a single hemisphere (Rockland and Lund, 1982;Gilbert and Wiesel, 1983). Indeed, evidence that callosal connectionsand horizontal connections share other features in common, suchas laminar distribution, a patchy termination pattern, and thetendency to link sites with similar orientation preference, hasled several authors to suggest that callosal connections and horizontalconnections might be organized according to similar principlesand have similar functions (Innocenti, 1986; Kennedy et al., 1986,1991; Houzel et al., 1994; Schmidt et al., 1997).

There are, however, reasons to question the notion of a common organizational scheme for callosal and horizontal connections.First, despite their extension away from the V1/V2 border, ithas been suggested that callosal connections may link visuotopicallycorresponding sites in the two hemispheres, rather than siteswhose receptive fields are widely displaced (Olavarria, 1996a).This hypothesis is based on physiological evidence from nonprimatespecies, indicating that the representation of visual space ineach hemisphere extends beyond the VM to include a substantialportion of the ipsilateral visual field (Hubel and Wiesel, 1967;Hughes and Vaney, 1982; Whitteridge and Clarke, 1982; Pettigrewet al., 1984; Payne, 1990; Sereno et al., 1991; White et al.,1999) and anatomical evidence for a lack of mirror-symmetry inthe topography of callosal connections (Pritzel et al., 1988;Kretz and Rager, 1990; Olavarria, 1996a). Second, evidence supportingthe orientation specificity of callosal connections is far fromdefinitive. The most direct test of this relationship, the analysisof the relation between anatomical connections and functionalmaps, has been explored in only one study (Schmidt et al., 1997).Furthermore, this analysis was performed in strabismic animals,and it is not clear to what extent lack of correlated input fromthe two eyes may have altered the normal pattern ofconnections.

In this study, we have used optical imaging techniques in tree shrews to define the maps of visual space and orientation preferencein V1 of both hemispheres. We then used anatomical tracing techniquesto evaluate both the visuotopic and orientation specificity ofcallosal connections. Our analysis reveals a substantial representationof the ipsilateral visual field within V1 such that a large partof the binocular region of visual space is represented bilaterally.Callosal connections extend throughout the region of bilateralrepresentation, but they terminate in a spatially restricted mannerthat links visuotopically corresponding sites in the two hemispheres.In addition, callosal connections appear to lack the orientationspecificity that characterizes long-range horizontal connections.Taken together, the properties of callosal connections appearto resemble those of the local component of intrinsic connectionswithin V1, rather than long-distanceconnections.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animal preparation. Thirty-one juvenile and adult tree shrews were used for these experiments. Animals were of both sexesand were between ~2 and 6 months old. No differences in the patternof intrinsic signals measured was noticed between animals of differentages or sexes, but the best signal-to-noise ratio for positionpreference experiments was obtained from animals of ~2 monthsof age. Anesthesia was induced with a mixture of ketamine hydrochloride(200 mg/kg) and xylazine (4.7 mg/kg) given by intramuscular injection.Atropine sulfate (0.08 mg) was given subcutaneously to reducesecretions. Surgical levels of anesthesia were maintained witha 2:1 mixture of N₂O:O₂ and 2% isoflurane. Body temperature wasmaintained near 38°C with a thermostatically controlled heatingblanket. Animals were placed in a stereotaxic frame, an incisionwas made in the scalp, muscle and fascia were reflected bilaterally,and the bone overlying visual cortex was thinned by scraping witha fine scalpel. All wound margins were treated with a long-lastinglocal anesthetic (bupivacaine), and pressure points were treatedwith lidocaine ointment. Animals were paralyzed by administrationof pancuronium bromide (initial dose 0.4 mg for the first 1-1.5hr, then 0.2 mg/hr). Tree shrews were artificially respired ata rate and volume sufficient to maintain expired CO₂ at 3-4%.During optical imaging, isoflurane levels were reduced to 0.5%and the N₂O:O₂ mixture to 1:1. Any signs of distress evident inthe electrocardiogram or expired CO₂ were treated by immediatelyincreasing the level ofisoflurane.

Zero power contact lenses were used to protect the corneas, and stimulus focus was assessed by viewing the retina throughan ophthalmoscope held at screen distance from the eye. In allanimals examined, the retinal vasculature was in sharp focus withlittle or no correction used on the ophthalmoscope, and no additionalcorrective lenses were used. The location of the optic disk foreach eye was projected onto a screen in front of the animal. Underour anesthesia and paralysis conditions, the optic disk projectionswere found to lie in a very stereotyped and symmetrical positionwith respect to the animal midline. The optic disk projectionfor the left eye was located 51.4 ± 3° from the animal midlineand 6.4 ± 1.6° above eye height, and the optic disk projectionfor the right eye was located 50.5 ± 2.3° from the animal midlineand 6.7 ± 2.3° above eye height (mean ± SD; n = 12 animals). Propereye alignment was confirmed by electrophysiology (see Results).Apparent shifts in eye position during 12 hr or longer recordingsessions were small relative to the receptive field size of corticalneurons: 1.8 ± 1.7° for absolute change in azimuth for left eye,1.6 ± 1.4° for absolute change in azimuth for the right eye (mean± SD; n = 5animals).

Optical imaging. Optical imaging of intrinsic signals was accomplished using an enhanced video acquisition system (OpticalImaging, Inc.) using techniques similar to those we have describedpreviously (Bosking et al., 1997). Images of the surface of leftand right visual cortex were acquired simultaneously directlythrough the thinned bone. For all animals, red light (700 ± 10nm) was used to illuminate the cortical surface to help reducethe presence of vascular artifacts. In addition, for some animals,artifacts caused by large changes in blood flow and oxygenationin the central sinus area were reduced by using an opaque redmarker to mask out portions of this region ofbone.

Visual stimulation for optical imaging was provided by a separate stimulus computer (386 PC with SGT+ graphics board and STIMsoftware provided by Kaare Christian). The stimulus monitor wasplaced 28.6 cm in front of the animal and subtended 80° of azimuthand 60° of elevation at this distance. All stimuli were presentedat a display rate of 60 frames/sec. Stimuli for orientation preferenceexperiments consisted of high-contrast rectangular wave gratings(3° dark phase, 1° light phase, drifted at 7.5°/sec) presentedat four different orientations. Each grating was moved back andforth along an axis orthogonal to its orientation. A single trialconsisted of presentation of one orientation for 9 sec, with acquisitionof video images during the last 8 sec, an interstimulus intervalof 8 sec, and then presentation of the orthogonal orientation,again with data acquisition during the last 8 sec. Video imageswere acquired at a rate of 30 frames/sec, but all frames acquiredduring the 8 sec period were summed together before further analysis.Between 8 and 20 trials were used for each pair of orientations(0/90°, 45/135°). Difference images of orientation preferencewere obtained by subtracting data acquired during presentationof one orientation from data acquired during presentation of theorthogonalorientation.

The stimulus used for position preference experiments was a high-contrast vertical bar (0.5° in width, 60° in length), pannedback and forth within a 2° wide window for 9 sec. Video imageswere acquired at a rate of 30 frames/sec during the last 8 secof this period. All data acquired during presentation of a blankscreen were subtracted from data acquired during presentationof the vertical bar stimulus to obtain an image reflecting thecortical activity in response to the vertical bar. Each experimentconsisted of ~8-20 trials with the stimulus located in the sameposition. In separate experiments, we tested the response of theanimal with this stimulus placed in locations ranging from 16°left of center of the monitor to 16° right ofcenter.

During imaging experiments, we determined the position of the VM using one of two methods. First, the VM was operationallydefined as the screen location that gave the most symmetricalactivation of the left and right cortex. It was usually possibleto determine this position within ~1-2^o. In some animals, a separate determination of the position ofthe VM was obtained by projecting the position of the optic disksonto a screen in front of the animal and calculating the positionof a line halfway between the two disks. On average, the differencein location of the VM determined by these two methods was small(1.1 ± 1.2°; mean ± SD; n = 12), and throughout the paper we usethe VM determined by symmetrical activation as the basis for presentationsandcalculations.

Electrophysiology. In some animals, a small hole was opened in the skull over V1 after optical imaging. Tungsten electrodes,50 mm in length, 14 M $Omega$ in resistance (FHC, Bowdoinham, ME), wereinserted through the dura mater and were used to record multiunitresponses. The position of recording locations relative to thesurface vasculature was noted. Multiunit aggregate receptive fieldswere plotted using a computer-assisted minimum response technique.In most cases, we considered both the spikes of individual unitsand the general "hash" response in determining the borders ofthe receptive fields. When possible, we plotted the receptivefield for both left and right eyeresponses.

Injection of fluorescent microspheres. In eight animals in which we performed optical imaging and in one additional animalin which we did not perform optical imaging, we made pressureinjections of latex microspheres conjugated to either rhodamine(red beads) or fluorescein (green beads) using a Picospritzer(beads provided by Dr. L. Katz, Duke University). The number andtiming of pulses used to obtain a reasonable size injection wasvariable, but the general strategy was to lower the tip to a depthof 700 µm, give three to six pulses, and then repeat this procedureat depths of 600, 500, 400, 300, 200, and 100 µm. Each pulse was~5 msec in duration at a pressure of 25psi.

Histology. At the conclusion of optical imaging, or after a 3 d survival period for animals in which we made bead injections,animals were transcardially perfused with 0.9% saline followedby 4% paraformaldehyde in 0.1 M phosphate buffer and then 10%sucrose in 0.1 M phosphate buffer. Brains were removed and placedin 20% sucrose in 0.1 M phosphate buffer. Visual cortex from eachhemisphere was removed and flattened between slides overnightin 0.1 M phosphate buffer containing 20% sucrose. Tangential sections40 µm in width were cut on a freezing microtome. The first oneor two sections were often cut at 60 or 80 µm to ensure that alarge portion of the surface vasculature over V1 was capturedin one section. The distribution of bead-labeled cells in thecortex was plotted by hand using a camera lucida or with the assistanceof a computerized plotting system (Neurolucida; Microbrightfield,Colchester, VT). Hand-plotted sections were scanned into a computerfor alignment with optical imaging data. After plotting of bead-labeledsections, or in animals without bead injections, Nissl stainswere performed on the corticalsections.

Alignment of Nissl-stained tissue and bead-labeled cell distributions with optical imaging data were performed using a modifiedversion of the public domain program NIH Image (original versiondeveloped at the National Institutes of Health, available on theInternet at http:\rsb.info.nih.gov/nih-image/; see Bosking etal., 1997 for details of modification). Briefly, scanned imagesor text files containing data plotted with the Neurolucida systemwere read into memory and aligned to the reference image takenduring the optical imaging phase of the experiment. Surface andradial blood vessels were the primary landmarks used to alignsection to section and to align sections to the reference image.For the experiments presented in this report, we used alignmentroutines that allowed not only global scaling, rotation, and translationof the camera lucida or Neurolucida drawings, but also differentialx-axis and y-axis scaling and the capability to induce a definedamount of curvature to the drawing to help correct for unevenflattening or shrinkage. These additions enabled slightly moreaccurate alignments on plots that spanned large portions ofV1.

Analysis. Images obtained by optical imaging were 655 × 480 pixels in resolution, with ~62 pixels/mm as a result of the lenscombination used. High-frequency noise was removed from orientationdifference images by using a mean filter kernel between 5 × 5and 10 × 10 pixels in size. Low-frequency noise in the orientationdifference images was reduced by convolving the image with a 50× 50 pixel mean filter kernel and subtracting the result fromthe original image. Difference images were normalized by dividingthe deviation from the mean at each pixel by the average absolutedeviation across the entire image (Weliky et al., 1995). Finally,vector summation of the difference images was done on a pixelby pixel basis to create a color-coded orientation preferencemap (Bonhoeffer and Grinvald, 1991, 1993; Blasdel, 1992).

The only filtering applied to the imaging data for position specificity shown in Figures 6 and 7 was a mean filter 5 × 5 or7 × 7 pixels in size. To help reduce vascular artifacts in thecase presented in Figures 3 and 4, we used the reference imageto create a mask indicating the location of the major blood vesselsin the imaging field of view. This mask was used to selectivelyfilter the raw data from each image in the position series. Thegrayscale value for each pixel in the data images that was locatedin the blood vessel mask was replaced by the mean of the grayscalevalues of the surrounding pixels. To calculate the mean for eachpixel, we used the minimum area possible while requiring a minimumof 160 pixels that were not in the blood vessel mask. Grayscalevalues for those pixels that were not in the mask were not changedduring this filtering. In the region of V1 that we imaged, thisprocess altered only 17% of the pixel values. We then mean filteredeach image using a 7 × 7 kernel and replaced each frame in theoriginal position series of 17 frames with the average of thatframe and the two adjacent frames to obtain the series of 15 imagesthat are displayed in Figure 3.

The position preference map shown in Figure 4 was obtained by combining data from the 15 images shown in Figure 3. For eachpixel, a position tuning curve was constructed by obtaining thegrayscale response value for each position tested. Then a Gaussiancurve was fit to this data, and the location of the peak of theGaussian was taken as the preferred position for that site. Theequation used for this process was:

where p1, p2, p3, and p4 are parameters specifying the shape and location of the Gaussian curve and x refers to the horizontalposition of the stimulus on the screen. The initial values forthe parameters were established from the minimum and maximum pixelvalues in the raw data for that location as follows: p1 = minimumpixel value, p2 = maximum-minimum pixel value, p3 = undetermined,and p4 = 2. Using these initial values, the location of the peak(p3) was allowed to vary in steps of 0.1, and the location resultingin the smallest error was recorded. This value for p3 and thevalues listed above for the other parameters were then fed toan iterative algorithm that allowed all four parameters to vary.The algorithm implemented was a version of the downhill simplexmethod (Press, 1992). The final value of p3 after this iterativesearch was taken as the preferred position of the site in question,and the position preference map is then a simple color codingof the position preference across the sampled region of visualcortex. Limits were set for each parameter for the Gaussian fittingprocess, and any pixel in the position preference map where thelimits were exceeded was replaced by the mean of the surroundingarea. Again we used the minimum radius possible to obtain themean value, but in this case we required only 50 pixels for averaging.The final position preference map was smoothed with a 7 × 7 pixelmeanfilter.

Selectivity of labeled cell distributions. After alignment of the histological sections to the optical imaging data, we quantifiedthe orientation selectivity of the labeled cell distributionsby counting the number of cells that were found over differentregions of the orientation preference map within 10^o bins of orientation preference. For intrinsic cell distributionswe counted only the cells that were >500 µm from the injectionsite. Cells that were located in V2 were excluded from theanalysis.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Our results are grouped into four sections. In the first section, we describe the map of visual space revealed by opticalimaging and compare this map to the map of orientation preferenceand the histologically defined area 17/area 18 border. In thesecond section, we present electrophysiological experiments thatconfirm the existence of an ipsilateral visual field representationwithin V1. Finally, in the third and fourth sections, we presentthe results of experiments in which we combined optical imagingwith injection of fluorescent beads to assess visuotopic and modularspecificity of callosalconnections.

Ipsilateral visual field representation revealed by optical imaging

Optical imaging was performed directly through the thinned bone over left and right visual cortex simultaneously. We obtainedrobust patterns of differential activity related to orientationpreference from a large region of the exposed cortex of both hemispheres(Fig. 1A). We have previously described some of the prominentfeatures of the orientation preference map in the tree shrew (Boskinget al., 1997). Interestingly, bilateral imaging of orientationpreference allowed us to determine that the pattern of activityassociated with a particular orientation was not identical, ormirror symmetric, in the two hemispheres (Fig. 1A). In addition,the area of cortex that provided strong orientation differencesignals provided a convenient way to define the V1/V2 border inour optical imaging experiments. In Nissl-stained sections oftree shrew visual cortex, the area 17/18 border is clearly definedby an abrupt change in staining intensity (Fig. 1B). This bordercorresponds to the V1/V2 border defined by electrophysiology (Kaaset al., 1972) and with the limits of the area of cortex providingstrong orientation difference signal in optical imaging experiments(Fig. 1A).

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Figure 1. V1/V2 border defined by optical imaging and Nissl staining (animal TS9756). A, Bilateral pattern of orientation selectivity demonstrated by optical imaging. The midline of the animal is in the center of the image, and rostral is toward the top of the page. The dashed lines indicate the portion of the imaged area corresponding to V1 in each hemisphere. All optical imaging data for the remainder of the paper will be presented in this orientation. Dark areas of V1 were strongly activated by a grating oriented at 45°; white areas were strongly activated by a grating oriented at 135°. Strong orientation signal is visible throughout V1 on each side, but not in V2. The dashed line in right visual cortex indicating the location of the V1/V2 border was defined by the Nissl-stained section shown in B. The dashed line in left visual cortex indicating the V1/V2 border was drawn directly from the orientation difference image. B, Photomicrograph of a Nissl-stained tangential section through V1. This section was aligned to the optical imaging reference image using techniques described in Materials and Methods and corresponds to the right side of the image shown in A. The darkly stained region of the image corresponds to area 17, and the dashed line is placed at the border of the lightly stained and darkly stained regions. Scale bar applies to both figures.

To investigate the map of visual space, we compared the pattern of activity elicited by a single bar stimulus, placed in aparticular location, to the pattern of activity obtained duringpresentation of a blank screen (see Materials and Methods fordetails). This stimulus was selected because it was spatiallyrestricted in one dimension yet was still capable of driving strongcortical activation. The activity elicited by this stimulus wasrestricted to bands of cortex 1-2 mm in width that were elongatedapproximately parallel to the V1/V2 border (Fig. 2B). The strengthof the signal within these bands was not uniform, and comparisonof the activation pattern within each band with orientation differencemaps from the same animal revealed that the areas of more intenseactivation correspond to vertical iso-orientation domains (Fig.2, compare A, B; see Fig. 7A,B).

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Figure 2. Bilateral orientation difference signal and bilateral response to a stimulus at the VM (animal TS9751). A, Bilateral orientation difference signal. Dark areas of the image were preferentially activated by a vertical grating (stimulus shown in inset), and white areas were preferentially activated by a horizontal grating. B, Bilateral pattern of activity in response to a bar stimulus (0.5° wide moved in a 2° wide window placed at the VM, shown in inset). Dark areas of the image were strongly activated by the bar stimulus as compared to a blank screen. The thin black lines denote the V1/V2 border as defined by the orientation signal shown in A. Note that the cortical representation of the VM is displaced from the V1/V2 border in each hemisphere, implying the existence of a representation of the ipsilateral visual field. Scale bar applies to A and B. C, Multiunit receptive field plots for the two recording sites depicted in B. The ipsilateral (dashed lines) and contralateral eye (thick lines) receptive fields are overlapping at each location, indicating minimal misalignment of the eyes. The receptive fields are located in the right (ipsilateral) visual field, consistent with the optical imaging results.

Presentation of the bar stimulus in the central regions of visual space elicited bands of activity in both hemispheres. Becausethere was very good agreement between the position of the stimulusthat elicited a symmetrical pattern of bilateral activation andthe midpoint between the two optic disk representations, we optedto use symmetrical activation to define the location of the VM(see Materials and Methods). Comparison of the location of thebands of cortical activation obtained when the stimulus was presentedat the VM with the limit of strong orientation signal in the samehemispheres (Fig. 2A) revealed that these bands were not juxtaposedto the V1/V2 border. Instead, the bands were displaced medially,the displacement being greater in more rostral portions of V1.Assuming that the eyes were properly aligned on the monitor, thisobservation implies a significant representation of the ipsilateralvisual field within V1, a departure from the results of previousphysiological mapping studies (Kaas et al., 1972; Kaas, 1980).

We checked for misalignment of the eyes in this animal by making physiological recordings from two sites in the lateral regionof V1 in the right hemisphere (Fig. 2C). At each recording site,the left and right eye receptive fields were highly overlapping.The receptive fields for these sites were located in the lowervisual field, as expected based on previous physiological mappingstudies, and were located well into the right (ipsilateral) visualfield, as predicted from the imagingresults.

Physiological recordings from additional animals (n = 6) confirmed that errors in eye alignment could not account for ourimaging results. Overlapping ipsilateral and contralateral eyereceptive fields were found in all except one animal. In the remaininganimal, the eyes were diverged by ~6^o; data from this animal are not used for any of the analysis inthis paper. To further check for systematic errors in eye alignmentthat might affect our results, we calculated the difference inthe position of receptive field centers of the ipsilateral andcontralateral eye receptive fields from all sites for which wehad binocular data. The average errors in receptive field alignmentwere calculated separately for the horizontal axis (dx) and verticalaxis (dy) for each animal. The average misalignment measured fromthe five animals was dx = $-$ 0.27° and dy = 0.73°. These misalignmentsin receptive field centers are small relative to the size of theaverage receptive fields of layer 2/3 neurons and cannot accountfor the substantial representation of the ipsilateral visual fieldthat we found inV1.

To examine the structure of the ipsilateral visual field representation, we tested cortical response to different positionsranging from up to 16° left to 16° right of the VM, spaced at2° intervals. The responses to fifteen of the stimuli tested forone case are shown in Figure 3; a bilateral pattern of activationwas elicited by all 15 of the stimuli shown. The light gray arrowsin the first and last frames of the series indicate the positionof cortical activation that is contralateral to the stimulus;the dark gray arrows indicate the position of cortical activationthat is ipsilateral to the stimulus. Note the non-mirror-symmetricpattern of cortical activation for all stimulus positions exceptthe VM. The locus of activity in the contralateral hemisphereis shifted further away from the V1/V2 border, and the locus ofactivity in the ipsilateral hemisphere is shifted closer to theV1/V2 border and occupies a much smaller extent. A similar patternof responses was seen in all animals that were tested (n = 16).

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Figure 3. Cortical response to a 0.5° wide bar stimulus placed in a series of 15 positions from 14° left of the VM ( $-$ 14°) to 14° right of the VM (+14°), spaced at 2° intervals (animal TS9762). The thin black lines in each frame outline V1 as determined by the limits of the area of strong orientation selectivity. Dark areas indicating stimulus-driven cortical activation are seen bilaterally in each image. In the first and last frames of the series, the light gray arrow indicates the location of activated cortex in the contralateral hemisphere, the dark gray arrow indicates the location of activated cortex in the ipsilateral hemisphere, and the inset indicates the location of the stimulus. Every stimulus position except the VM produced a non-mirror-symmetric pattern of cortical activation.

Animation of the series of images shown in Figure 3 provides dramatic evidence of the orderly representation of visual spaceand the smooth progression of responses seen throughout V1. Itis also possible to use these images to construct a position preferencemap that provides the same information about the structure ofthe map of visual space in a single image. For each site in cortex,the position preference was calculated by fitting a Gaussian curveto a plot of response magnitude versus position number. This curveis essentially a position tuning curve for that location in cortex,and the peak of the fitted Gaussian curve can be taken as an estimateof the position preference of that site. This procedure is repeatedfor each pixel in the image. Although this procedure is similarin principle to using vector summation to combine responses fromdifferent angle maps to create an orientation preference map,it has the advantage that it can be used to analyze noncyclicfeatures such as positionpreference.

Figure 4 shows the position preference map for the right hemisphere of the case shown in Figure 3. In this image, positionpreference is color-coded according to the key shown in the inset.Position preferences are shown only for the portion of the imagingframe that lay in V1. Three important features about the representationof visual space are apparent: (1) There is a smooth progressionof position preference across the entire extent of V1, includingthe contralateral and ipsilateral visual field representations.(2) The ipsilateral visual field representation is highly compressedrelative to the contralateral visual field representation. Withinthe contralateral visual field representation, ~12° of visualspace are represented within ~2 mm of cortex. The same amountof the ipsilateral visual field is represented within ~1 mm ofcortex. (3) The amount of the ipsilateral visual field representedvaries systematically with elevation, being largest in the representationof the lower visual field (Fig. 4, rostral portion).

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Figure 4. Position preference map for right visual cortex generated from the data shown in Figure 3 (animal TS9762). Position preference was calculated for each pixel location by fitting a Gaussian curve to a plot of the response level (grayscale value) versus position number (see Materials and Methods for details). Only regions that were within V1 (as determined by the area of strong orientation signal) are depicted. Position preference is color-coded according to the key shown in the inset. Each color represents a particular distance from the VM so that corresponding azimuths in ipsilateral and contralateral visual space are represented by the same color. The black lines indicate 2° contour intervals in the map of visual space. Note the compression of the ipsilateral visual field representation relative to the contralateral visual field representation.

Ipsilateral visual field map confirmed by electrophysiology

A comprehensive examination of the extent of the ipsilateral visual field representation and its relationship to the cytoarchitectonicallydefined area 17 was performed in one animal using electrophysiology.In Figure 5A, the locations of 10 recording sites from this animalare illustrated over a Nissl-stained section. The locations ofthe recording sites were initially plotted relative to the bloodvessel pattern in a reference image taken during an optical imagingexperiment. The tissue section was then aligned to the referenceimage to obtain the position of the recording sites relative tothe Nissl-stained section (see Materials and Methods for details).The receptive field locations from these 10 sites are shown inFigure 5B. At the first recording site, we confirmed eye alignmentby plotting both ipsilateral and contralateral eye receptive fields(thin black and dashed black boxes #1). At the remaining sites,we plotted only the contralateral eye receptive field. For sites1-6, there is a consistent movement of the receptive fields intothe ipsilateral visual field with lateral movement of the recordingsites. For sites 9 and 10, the progression of receptive fieldlocations has reversed, and there is also a large increase inreceptive field size. This implies that the V1/V2 border was betweensites 6 and 9. At site 7, we obtained receptive field plots attwo different depths. At one depth the receptive field was smalland located well into the ipsilateral visual field, suggestingthat the recording site was in V1. At another depth the receptivefield was much larger and located closer to the VM, suggestingthat the recording site was in V2. Together the evidence suggeststhat the V1/V2 border was very near sites 7 and 8, a locationthat corresponds precisely to the area 17/18 border visualizedon the Nissl-stained section that was aligned to the referenceimage. This confirms an orderly representation of the ipsilateralvisual field that extends for ~1 mm within the limits of the cytoarchitectonicallydefined area 17 and not within a separate transition zone as describedin the cat (Payne, 1990). Note that there was a large jump inreceptive field position from well into the ipsilateral visualfield to back near the VM as we crossed the border into V2. Thisresult suggests that there is a less extensive representationof the ipsilateral visual field in V2 or that it is smaller andmore difficult to detect.

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Figure 5. Physiological confirmation of the ipsilateral visual field representation (animal TS9756). A, Location of 10 recording sites relative to a Nissl-stained section cut tangentially through layer 4; the darkly stained region of the tissue corresponds to V1. B, Multiunit receptive field plots for the recording locations shown in A. For site 1 the contralateral (thick black line) and ipsilateral eye (dashed line) receptive fields were determined separately to confirm proper eye alignment. Receptive fields for all other sites were plotted using the contralateral eye only. Receptive fields for sites that appeared to be in V1 are shown in black, and receptive fields for sites that appeared to be in V2 are shown in gray. At site 7, recordings were made at two different depths, and receptive fields from both depths are shown. Based on these recordings, the V1/V2 border appeared to be near sites 7 and 8, which corresponds to the position of the border on the Nissl-stained section.

Visuotopic specificity of callosal connections

The non-mirror-symmetric activation patterns observed in response to individual stimuli bear a striking resemblance to thenon-mirror-symmetric pattern of callosal connections that havebeen previously described in the tree shrew and other species(Pritzel et al., 1988; Kretz and Rager, 1990; Olavarria, 1996a).This observation suggests that callosal connections may link locationsin the two hemispheres that respond to the same part of visualspace. We tested this idea by combing optical imaging with injectionof fluorescently labeled microspheres(beads).

The relation between the pattern of bead labeling and cortical activity patterns was assessed by using the pattern of surfaceand radial blood vessels to align the anatomical data from tangentialsections to the optical imaging data. As shown in Figure 6A, linedrawings of the blood vessels in the first section (yellow lines)were aligned to the reference image taken during the optical imagingphase of the experiment. Figure 6B provides a higher magnificationview of the alignment of the blood vessels in the first section(yellow) as well as the alignment of the radial vessels (blue)from a deeper section that contained bead labeled cells. Errorsin alignment between sections were small, usually less than thediameter of the radial blood vessels.

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Figure 6. Visuotopic specificity of callosal connections. A-D, Results from an experiment in which optical imaging of intrinsic signals was combined with injections of fluorescent microspheres (animal TS9803). A, Alignment of the drawing of the first histological section (yellow overlay) to the reference image taken during optical imaging. The filled red and green ellipses indicate the location and approximate size of bead injections made in right visual cortex. Scale bar in A applies to A and C-F. For details of alignment procedure, see Materials and Methods. B, Higher magnification view of the alignment of the first tissue section (yellow overlay) and a deeper tissue section (blue overlay) that contained bead-labeled cells. C, Location of bead injections (filled red and green ellipses) and bead-labeled cells (red and green squares) shown over the cortical response to a stimulus placed 8° right of the VM, as shown in the inset. The blue lines indicate the position of the V1/V2 border in each hemisphere. The red injections were made in a region of cortex that responded to this stimulus, and many of the red bead-labeled cells are found in an area of left visual cortex that also responded to this stimulus. D, The same bead injections and labeled cells as shown in C shown over the response to a stimulus placed at the VM. The green bead injections were made in an area that responded to this stimulus, and green bead-labeled cells in the opposite hemisphere are found in a region that also responded to this stimulus. E, F, Visuotopic specificity of callosal connections originating in the ipsilateral visual field representation (animal TS9768). E, Bead injections and labeled cell distributions shown over the cortical response to a stimulus placed 4° right of the VM, as shown in inset. F, Bead injections and labeled cells shown over the cortical response evoked by a stimulus located at the VM.

At the conclusion of the alignment process, we created overlays by replacing the reference image with the optical imagingdata and the radial vessel plot with the plots of injection sitesand bead-labeled cells. In Figure 6, C and D, two overlays areshown for the same case that is illustrated in Figure 6, A andB. The red bead injections were made into a region of cortex thatwas activated by a stimulus centered 8° to the right of the VM(Fig. 6C). Most of the red bead-labeled cells in the left hemispherewere found in an area that was activated by the same stimulus.The green bead injection sites were made into a region that wasactivated by a stimulus centered on the VM (Fig. 6D). The greenbead-labeled cells in the left hemisphere were found in a morelateral position than those labeled with red beads; this regionwas activated by the stimulus that was centered on the VM andnot by the stimulus that was centered 8° to the right of the VM.This experiment confirms that callosal connections tend to linksites in the two hemispheres that represent the same region ofvisualspace.

Two overlays from an experiment in which we performed optical imaging and then made bead injections into an area of cortexrepresenting part of the contralateral visual field are shownin Figure 6, E and F. Three injections of both red and green beadswere made in two lines that extended roughly along isoazimuthlines, as determined by optical imaging. Both sets of bead injectionswere made within an area of cortex that responded strongly toa stimulus placed 4° right of the VM (Fig. 6E). Again, the majorityof the bead-labeled cells lie over regions of right visual cortexthat were also activated by this stimulus, indicating that thereis at least a rough visuotopic correspondence between the siteslinked by callosal connections. The precision of the correspondencecan be appreciated in several ways. First, note that althoughthe red and green bead-labeled cell distributions are overlapping,the green bead-labeled cells, which were labeled by a more medialset of injections in left cortex, occupy a more lateral positionin right visual cortex. The direction and magnitude of this shiftare precisely what we would expect if callosal connections linkvisuotopically corresponding points. Second, the red bead injectionswere made in an area of cortex that also responded when a stimuluswas placed at the VM, whereas the green bead injections were madein an area that did not respond to this stimulus (Fig. 6F). Correspondingly,most of the red bead-labeled cells are found in the activatedregion of the right cortex, whereas most of the green bead-labeledcells lie lateral to this region (Fig. 6F). Finally, the distributionsof labeled cells observed after injection of beads into the contralateralvisual field representation (Fig. 6E,F) occupy a much less extensiveregion of cortex than those obtained from injection of beads intothe ipsilateral visual field representation (Fig. 6C,D, red injections).This pattern correlates with the difference in magnification factorfor the ipsilateral and contralateral visual fieldrepresentations.

Another example of the visuotopic specificity of callosal connections comes from an experiment in which we made single injectionsof red and green beads that were separated by only 500 µm (Fig.7). The bead injections made in this case were slightly largerthan those made in the two cases shown so far, and they were locatedwithin the ipsilateral visual field representation of left visualcortex. These factors explain the larger size of the labeled celldistributions seen in this case (Fig. 7A). The injections weremade at a location that had a preferred position of ~2° left ofthe VM and, as expected, the distribution of labeled cells inthe right hemisphere is centered on a region of cortex that respondedstrongly to the same stimulus (Fig. 7A). In addition, althoughthe red and green distributions are highly overlapping, they areslightly shifted in the correct direction to maintain visuotopiccorrespondence.

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Figure 7. Visuotopic specificity and lack of modular specificity of callosal connections (animal TS9821). In this animal, one injection of red beads, indicated by the red circle, was placed in an area of cortex that had a vertical orientation preference and a position preference of 2° left. One injection of green beads, indicated by the green circle, was made at a slightly more lateral position that had a horizontal orientation preference and a position preference of 4° left. As in Figure 6, red bead-labeled cells are indicated by red squares, green bead-labeled cells are indicated by green squares, and blue lines indicate the position of the V1/V2 border. A, Bead injections and labeled cell distributions are shown over the cortical response to a stimulus placed 2° left of the VM. B, Bead injections and labeled cell distributions shown over a difference image in which dark areas of the image indicate areas of cortex that responded preferentially to a vertical grating. Although the red injection was made in a vertical domain, and the green injection was made in a horizontal domain, the labeled cell distributions show no orientation specificity in the opposite hemisphere. Scale bar in B applies to A and B. C, Distribution of red bead-labeled cells, now shown as white squares, over an orientation preference image for part of the right hemisphere. D, Distribution of green bead-labeled cells over an orientation preference image for part of the right hemisphere. The scale bar and color key in D each apply to both C and D.

Modular and axial specificity of callosal connections

Although the two injections in the case shown in Figure 7 were separated by a fairly small distance in cortex, they were centeredin regions that had orthogonal orientation preferences, allowingus to assess the orientation specificity of the callosal labelin the opposite hemisphere. Figure 7B shows the location of thetwo injection sites and the labeled cell distributions over adifference image in which dark areas responded preferentiallyto a vertical stimulus. The red injection was located at a sitethat preferred vertical, and the green injection was located ata site that preferred horizontal. As illustrated in Figure 7A,the red and green cell distributions occupy highly overlappingregions of the opposite hemisphere. If callosal connections selectivelylink sites in the two hemispheres that have similar orientationpreferences, we would expect each distribution to be arrangedin a patchy or modular fashion. In addition, we would expect thered- and green-labeled cells to be largely segregated, with redcells found over regions with a vertical orientation preference,and green cells found over regions with a horizontal orientationpreference. None of these expectations were met. As seen in Figure7B, neither distribution is found selectively over the light ordark regions of the difference image. Furthermore, the red andgreen bead-labeled cells show little sign of a complementary distribution.The fine scale organization and orientation specificity of thedistributions can be better examined by displaying each separatelyover an orientation preference map for the right hemisphere (Fig.7C,D). Both populations of labeled cells appear rather evenlydistributed, and each covers regions of cortex that include awide range of orientationpreferences.

The case shown in Figure 7 suggests that callosal connections lack specificity with respect to the map of orientation preference.However, it could be argued that the size of the injections mayhave been too great to reveal an underlying modular specificity.To verify that our methods are suitable for detecting the orientationspecificity of cortical connections, we directly compared thespecificity of intrinsic connections and callosal connectionsresulting from the same injection of beads in three animals. Oneof these experiments is shown in Figure 8. A single injectionof red beads was made in the left hemisphere in an area of cortexthat had a preferred orientation of ~60^o. In Figure 8A, the resulting distribution of labeled cells isshown over a difference image in which dark areas responded preferentiallyto a 45^o stimulus. The labeled cells in left cortex extend for severalmillimeters rostral and caudal of the injection site, and arefound mostly over dark areas of the difference image, indicatingmodular specificity related to orientation preference. The labeledcells in the right hemisphere, on the other hand, are confinedto a smaller area of cortex and show no obvious modularity. Thesame distributions are shown over the orientation preference mapfor this case in Figure 8, B and C. The intrinsic connectionsexhibit some variability near the injection site, but are foundpreferentially over blue-green areas of the map at longer distances(Fig. 8B). Few cells are found over the red and purple regionsof the map, representing sites with an orientation preferencenear horizontal. Cells in the opposite hemisphere, on the otherhand, appear evenly distributed with respect to the orientationpreference map (Fig. 8C).

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Figure 8. Comparison of modular specificity of intrinsic and callosal connections in a single animal (animal TS9824). A single injection of red beads was made in this animal in an area of the left cortex that had an orientation preference of near 60°, and the labeled cells in both hemispheres were plotted. A, Injection and labeled cells shown over an orientation difference image in which dark areas indicate regions of cortex that responded preferentially to a 45° grating. The red circle indicates the limits of the injection site, and red squares indicate red bead-labeled cells. Labeled cells are found in a distribution that is elongated along roughly the rostrocaudal axis, corresponding to the preferred orientation of the injection site, and are found preferentially over dark areas of the difference image in left cortex. Labeled cells in the opposite hemisphere are found in a more restricted and symmetrically shaped distribution and show no preference for dark or light domains. B, Distribution of labeled cells found in the left cortex shown over an orientation preference map for that hemisphere. Labeled cells tend to lie over blue and green regions of the orientation preference map, indicating a preference for sites with orientation preferences between 45 and 90^o. C, Distribution of labeled cells found in the right hemisphere displayed over an orientation preference map for that hemisphere. Labeled cells show no preference for a particular orientation. Orientation preference is color-coded according to key shown in Figure 7. Scale bar in C applies to B and C.

To quantify the specificity of the labeled intrinsic connections (n = 3) and of labeled callosal connections (n = 6), we createdcell tuning curves by calculating the percentage of the totalnumber of cells found in different orientation preference binsrelative to the preferred orientation of the injection site. Figure9A shows that each of the three intrinsic cases showed a strongbias toward connecting sites with similar orientation preferenceto the injection site, and the group average shows the same bias.Although two of the tuning curves for individual callosal distributionsshown in Figure 9B do seem to show a peak near the preferred orientationof the injection site, the overall tuning of the callosal distributionswas much more erratic, and the group average is close to whatwould be expected for flat, or random, tuning.

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Figure 9. Quantification of orientation specificity of labeled cell distributions. A, Tuning curves for intrinsic cell distributions. Each curve shows the percentage of total cells found in different orientation preference bins relative to the preferred orientation of the injection site. Cells shown in the 0° bin had the same orientation preference as the injection site, those shown in the 90° bin had an orientation preference orthogonal to the injection site. Only cells located further than 500 µm from the injection site were considered for this analysis. The three gray curves show the tuning for the three individual cases we examined; the thick black line shows the group average. The dotted line indicates the percentage of the total labeled cells that would be expected in each bin for an even distribution (5.56%). B, Tuning curves for callosal cell distributions. The six gray curves show the tuning for the six individual cases we examined; the thick black line shows the group average. C, Comparison of specificity of callosal and intrinsic connections. Each bar indicates the percentage of the total number of cells or boutons that are found in areas that have similar (± 35°) orientation preference to the injection site (mean ± SD). The percentages reported for specificity of intrinsic and callosal connections measured by retrograde labeling with beads are from the present results, the percentage reported for specificity of intrinsic connections measured by anterograde labeling with biocytin comes from a previous report (Bosking et al., 1997). The dashed line indicates the percentage of cells or boutons that would be expected for an even distribution (38.9%).

We compared the specificity of callosal connections and intrinsic connections by quantifying the percentage of labeled cellsfound in areas with similar (±35°) orientation preference to theinjection site (Fig. 9C). Also included in this comparison isthe specificity of intrinsic connections as measured in our previousstudy using biocytin as an anterograde tracer and counting thenumber of labeled boutons (Bosking et al., 1997). The two measuresof the specificity of intrinsic connections are in good agreementand exhibit a large difference from the percentage of iso-orientationcontacts expected for an even distribution. Callosal connections,on the other hand, show a much smaller, if any, bias toward linkingsites with the same orientationpreference.

Although we did not attempt to quantify the axial specificity of our labeled cell distributions, callosal connections do notexhibit the orientation-specific elongation that is characteristicof long-range intrinsic connections. Neurons in layer 2/3 giverise to horizontal connections that extend for greater distances,and make more contacts, along an axis in the map of visual spacethat corresponds to their preferred orientation (Bosking et al.,1997; Fig. 9). This type of axial specificity is apparent in thecase shown in Figure 8, in which a single injection of beads ledto an elongated distribution of cells within the same hemisphere.The distribution is elongated along an axis that is slightly shiftedfrom the vertical axis in the map of visual space, correspondingto the 60° orientation preference of the injection site. A muchsmaller, and more symmetrically shaped, distribution of cellsis observed in the opposite hemisphere. In general, the callosalcell distributions we observed occupied a much smaller extentof cortex, and when injections were made near the representationof the VM, the labeled cell distributions were roughly symmetricin shape in the opposite hemisphere (Figs. 6C,D, green-labeleddistributions, 8). When asymmetric distributions of labeled cellswere seen in the opposite hemisphere, the asymmetry was eitherelongation or compression along an axis roughly orthogonal tothe V1/V2 border. This anisotropy in connections is likely tobe explained by the compression of the ipsilateral visual fieldrepresentation along the horizontal axis. Injections made in theipsilateral visual field representation led to labeled cell distributionsin the contralateral visual field representation of the oppositehemisphere that were expanded along this axis; i.e., orthogonalto the V1/V2 border (Figs. 6C,D, red-labeled cell distributions,7). Injections in the contralateral visual field representation,on the other hand, led to labeled cell distributions in the ipsilateralvisual field representation of the opposite hemisphere that werecompressed along this axis (Fig. 6E,F, green-labeleddistributions).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The results presented here provide several new insights into the functional organization of callosal connections. First, theseconnections are organized in a highly topographic manner, linkingtogether sites in the two hemispheres that respond to the sameregion of visual space. Second, callosal connections are not limitedto regions of V1 that represent the VM: because of the presenceof a substantial ipsilateral visual field representation, callosalconnections may exert an influence over almost the entire binocularvisual field representation of tree shrew V1. Finally, unlikeother systems of cortical connections, callosal connections terminatewithout respect for the modular arrangement of orientation-selectiveneurons. Combined, these results provide a more complete pictureof the functional architecture that forms the substrate for processingof information from central visual space and suggest ways in whichthe role of callosal connections may be distinguished from thatof other corticalconnections.

Bilateral representation of central visual space

The presence of an ipsilateral visual field representation is not unique to the tree shrew. Although it is most frequentlyassociated with albino or pigment-deficient animals (Hubel andWiesel, 1971; Shatz, 1977a; Shatz and LeVay, 1979; Ault et al.,1995), an ipsilateral visual field representation has been demonstratedin normally pigmented individuals from a variety of nonprimatespecies including cat, ferret, ground squirrel, rabbit, opossum,hamster, and sheep (Clarke and Whitteridge, 1976; Tiao and Blakemore,1976; Hughes and Vaney, 1982; Whitteridge and Clarke, 1982; Pettigrewet al., 1984; Volchan et al., 1988; Payne, 1990; Sereno et al.,1991; White et al., 1999). The presence of an ipsilateral visualfield representation appears to be linked to the decussation patternof ganglion cells in the retina, specifically the fact that thecrossed projection is not limited to the nasal retina, but extendswith reduced density across the representation of the VM and intothe temporal retina (Illing and Wassle, 1981; Pettigrew et al.,1984; Morgan et al., 1987; Baker and Reese, 1993; Ault et al.,1995; Jeffery et al., 1998). Indeed, the characteristics of thecrossed temporal projection help to explain some of the uniquefeatures of the ipsilateral visual field representation. For example,the compression (low magnification) of the ipsilateral visualfield representation relative to that of the contralateral visualfield representation is consistent with the difference in thedensity of ganglion cells that supplies the two representations.Likewise, the variation in the extent of the ipsilateral visualfield representation with eccentricity is consistent with thevariation in the extent of the crossed temporal projection. Inthe tree shrew, for example, the ipsilateral visual field representationis smallest near the representation of the horizontal meridianand expanded in the lower visual field. Correspondingly, the densityof the crossed temporal projection is lowest near the area centralisand highest in regions of the retina that support the upper andlower visual field (Jeffery et al., 1998). We were unable to determinewhether the ipsilateral visual field representation is also expandedfor the upper visual field in the tree shrew, because this regionof cortex is not accessible for imaging. In the cat, however,the ipsilateral visual field representation is expanded in boththe upper and lower visual field (Payne, 1990).

Visuotopic arrangement of callosal connections

Our results show that callosal connections are arranged in a highly specific manner with respect to the bilateral representationof visual space within V1. Callosal connections extend for upto 15° into the contralateral visual field representation in V1,a figure that matches the extent of the ipsilateral visual fieldrepresentation. Moreover, these connections are arranged in atopographic fashion that links visuotopically corresponding sitesin the twohemispheres.

The best evidence for visuotopic correspondence comes from experiments in which we combined imaging for position with injectionsof retrograde tracers. Injections into an active zone in one hemispherealways labeled cells in the other hemisphere that were in zonesactivated by the same visual stimulus. The alignment was not perfectin every experiment, inasmuch as the labeled cells were not alwayscentered on the area of activation, but it seems likely that theseslight misalignments are attributable to the small (1-2°) errorsin eye alignment that we detected with multiunit physiologicalrecordings. Further support for visuotopic precision in callosalconnections comes from experiments in which we injected two differenttracers at nearby locations in cortex. Labeled cells were alwaysfound in overlapping, but precisely shifted, distributions inthe opposite hemisphere, and the magnitude and direction of theshift was consistent with the demonstrated visuotopy. In addition,injections of tracers into the ipsilateral visual field representationalways labeled a large patch of cells in the other hemisphere,whereas injections into the contralateral visual field representationlabeled a comparatively small patch (compare Fig. 6C,D and Fig.7 to Fig. 6E,F). These differences are consistent with the differencein magnification factor of the ipsilateral and contralateral visualfield representations. Overall, these results provide strong supportfor the view that callosal connections are centered around visuotopiccorrespondence. It is also clear, however, that these connectionsprovide input from a moderate-sized region surrounding exact correspondence.Thus, a particular site in one hemisphere would receive inputvia callosal connections primarily from sites in the other hemispherethat had overlapping receptive fields, but also from sites whosereceptive fields could be displaced by as much as the receptivefield diameter of a layer 2/3 neuron (5°).

The present findings were foreshadowed by earlier anatomical studies in the tree shrew showing that callosal projections extendseveral millimeters away from the V1/V2 border and that they areorganized in a non-mirror-symmetric manner such that sites nearthe V1/V2 border are connected with sites displaced from the V1/V2border in the opposite hemisphere (Sesma et al., 1984; Cusicket al., 1985; Pritzel et al., 1988; Kretz and Rager, 1990; Lyonet al., 1998). However, without the knowledge of the ipsilateralvisual field representation within V1, the full significance ofthis pattern was not appreciated. A similar anatomical study inthe cat, where an ipsilateral visual field representation hadbeen identified (Whitteridge and Clarke, 1982; Payne, 1990, 1991;Payne and Siwek, 1991), proposed at least a rough visuotopic correspondencefor callosal connections (Olavarria, 1996a). However, these experimentsdid not combine anatomy and physiology in the same animal and,as a result, the exact relationship between the visual field locationsof the injection sites and the distribution of labeled cells couldnot beassessed.

The visuotopic organization demonstrated here challenges the classical view that callosal connections are concerned exclusivelywith the visual midline and are the sole source of ipsilateralvisual field input for cells whose receptive fields straddle thevisual midline (Hubel and Wiesel, 1967; Berlucchi and Rizzolatti,1968). Instead, callosal connections appear to provide visuotopicallycorresponding inputs for neurons whose receptive fields are wellremoved from the VM as well as for neurons whose receptive fieldsspan the visual midline. As noted by others, there is no needfor callosal connections to extend cortical receptive fields acrossthe midline because information from the ipsilateral visual fieldis already present in the pattern of ganglion cell projectionsto the lateral geniculate nucleus (Blakemore et al., 1983). Thus,callosal connections are arranged in register with lateral geniculateterminations, i.e., they link sites in the two hemispheres thatreceive lateral geniculate inputs representing the same regionof visual space. How the inputs from these two sources contributeto the responses of individual cortical neurons, however, remainsunclear. Although the density of projection suggests that geniculate-derivedinputs are likely to dominate the responses of layer 2/3 neurons,under certain circumstances callosal connections appear to becapable of supporting the selective responses of neurons in lieuof LGN inputs (Choudhury et al., 1965; Berlucchi and Rizzolatti,1968; Lepore and Guillemot, 1982; Blakemore et al., 1983).

The demonstration that callosal connections provide topographically precise connections for regions of visual space that arerepresented bilaterally also offers a simple explanation for differencesamong species in the cortical extent of the callosal connections:species differences in the amount of visual space that is representedbilaterally. The relatively restricted extent of callosal connectionsin many primates and the widespread distribution of callosal connectionsin most nonprimates and in abnormally pigmented animals parallelsthe extent of the crossed inputs from the temporal retina (Shatz,1977b,c; Swadlow et al., 1978; Cusick et al., 1984, 1985; Sesmaet al., 1984; Kennedy et al., 1986; Pritzel et al., 1988; Kretzand Rager, 1990; Payne, 1991; Payne and Siwek, 1991; Grigoniset al., 1992; Ault et al., 1995). It follows, then, that the visuotopicprecision demonstrated here is a feature of callosal connectionsin most mammals, regardless of the extent of the bilateralrepresentation.

Lack of orientation specificity to the callosal projections

Our results demonstrate that there is little orientation specificity to the distribution of callosal connections. Restrictedinjections of tracers into sites that produced a prominent patchydistribution of labeled cells in iso-orientation domains of theipsilateral hemisphere resulted in a single patch of labeled cellsin the contralateral hemisphere that displayed little sign ofselectivity for the orientation preference of the cells at theinjection site. This result is perhaps surprising based on theresults of anatomical and physiological experiments performedin thecat.

In general, callosal connections in the cat have been regarded as terminating in an orientation-specific manner, and it ispossible that there are differences between the organization ofcallosal connections in these two species. However, the evidenceon this point is far from definitive. For example, the demonstrationthat callosal connections terminate in a patchy manner has ledsome investigators to suggest linkage between sites with similarorientation preference (Houzel et al., 1994). However, other studiesdemonstrate that the patchy distribution of callosal connectionsis related to other types of functional units such as ocular dominancedomains or cytochrome oxidase blobs (Boyd and Matsubara, 1994;Olavarria, 1996b). Only one study has addressed the relation betweencallosal connections and orientation domains defined by uptakeof 2-deoxyglucose, and the authors concluded that callosal connectionswere biased for sites with the same preferred orientation (Schmidtet al., 1997). However, this study was based on the analysis ofconnections in strabismic animals, and it is not clear whetherdecorrelating the activity in the two eyes alters the normal relationshipbetween callosal connections and maps of orientation preference.Interpretation of this result is also made difficult by the factthat the analysis was based on experiments that combined 2-DGlabeling for both ocular dominance and orientation, and it isnot clear how much of the specificity can be attributed to orientationalone. Clearly, this issue warrants further study in normalanimals.

Functional architecture of callosal interactions

Our results demonstrate that callosal connections are organized according to principles that differ significantly from long-rangehorizontal connections (Fig. 10). Both the modular and axial specificitythat are such striking features of long-range horizontal connectionsare largely absent from callosal connections. Indeed, the primaryfactor constraining the distribution of callosal connections appearsto be visuotopic correspondence. In this respect, callosal connectionsseem similar to local intrinsic connections-connections that extendin a symmetrical fashion for a radius of ~500 µm and contact neuronsthat have largely overlapping receptive fields and may exhibita wide range of preferred orientations. By coordinating the activityin the two hemispheres in a way that preserves nearest neighborrelationships, callosal connections may best be viewed as elementsof local circuits that operate within a single bilateral representationof visual space.

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Figure 10. Summary of the bilateral representation of visual space and the specificity of horizontal and callosal connections in the tree shrew. A, Map of visual space modified from one first presented by Kaas et al. (1972) to reflect the ipsilateral visual field representation revealed by optical imaging. The dorsal portion of V1 is shown for both left and right visual cortex. Rostral is toward the top of the page. The thick black lines form the border of V1, and the thin black lines in each hemisphere indicate isoelevation and isoazimuth lines within the map of visual space. The dark gray and light gray regions beneath the map of visual space simulate vertical and horizontal orientation preference domains, respectively. The small dark gray circles in each hemisphere indicate the location of cells that would be likely to provide input to the site in left cortex indicated by the larger gray circle. The intrinsic inputs, in left cortex, are nonspecific at short distances, but at longer distances they originate mainly from sites along the vertical axis in the map of visual space and whose orientation preference is near vertical. The callosal input originates from a much smaller region of the opposite hemisphere and comes from regions that have both vertical and horizontal orientation preference. B, Visual field depiction of input received via horizontal connections. The dark gray rectangle in the background indicates the receptive field of a cell located where the large gray circle is found in the left cortex. The open rectangles indicate the receptive field locations of the cells that would provide input to this cell via horizontal connections. These inputs have receptive fields that span a total distance of ~30^o of visual space. The cell receives input from many other cells with overlapping receptive fields that can be of any orientation and from other cells that have nonoverlapping receptive fields and whose receptive fields are displaced along a vertical line in visual space and have an orientation preference near 90^o. C, Visual field depiction of input received via callosal connections. The inputs received from callosal connections have receptive fields confined to a much smaller region of visual space, and they include a wide range of orientation preferences.

  FOOTNOTES

Received Oct. 7, 1999; revised Jan. 10, 2000; accepted Jan. 10, 2000.

This work was supported by National Eye Institute Grant EY06821, Swiss National Science Foundation Grant 31-49772.96, anda McKnight Investigator Award (D.F.).
Correspondence should be addressed to David Fitzpatrick, Box 3209, Duke University Medical Center, Durham, NC 27710. E-mail:fitzpat{at}neuro.duke.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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