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The Journal of Neuroscience, July 2, 2003, 23(13):5684-5692
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Independent Projection Streams from Macaque Striate Cortex to the Second Visual Area and Middle Temporal Area
Lawrence C. Sincich andJonathan C. Horton Beckman Vision Center, University of California, San Francisco, San Francisco, California 94143
Abstract
Top
Abstract
Introduction
The interareal wiring of the neocortex is usually depicted as a network of single point-to-point connections, often side-stepping the possibility that some neurons may project to multiple cortical areas. The prevalence of such neurons is unknown; if they are abundant, cortical circuits are more likely to be connectionally diffuse. We used a dual-tracer approach to determine whether single neurons in the macaque primary visual cortex (V1) project to two extrastriate areas, the second visual area (V2) and the middle temporal area (MT). We found two large intermingled groups of single-labeled neurons in layer 4B of V1 projecting independently to either V2 or MT. A third, sparser group of double-labeled neurons projected to both areas; we termed these manifold neurons. We also found that MT-projecting cells were distributed indiscriminately with respect to cytochrome oxidase compartment in layer 4B, revealing a subpopulation that provides a potential source of patch input from V1 to MT. The results demonstrate that primary sensory cortices can use multiple projection strategies to distribute signals to higher areas, and suggest that feedforward projections may route signals with more specificity than feedback pathways.
Key words: visual cortex; intracortical; manifold projections; flatmount; motion; cytochrome oxidase; patch column; interpatch column
Introduction
The occipital, temporal, and parietal lobes of the cerebral cortex harbor a large number of cortical areas that respond to visual stimuli. On average, each area is connected to 15 others in the macaque brain (Felleman and Van Essen, 1991). This invites the question: do typical cortical neurons project to 15 areas, a few areas, or just one? Decades of mapping connections with single tracers have provided a basic interareal wiring diagram of the cortex. However, the use of single tracers cannot easily reveal whether a given neuron projects to multiple areas (Giolli and Towns, 1980
Surprisingly, neuroanatomists have not agreed on a term to distinguish cortical neurons that project to a single area versus multiple areas (Lockard, 1992
The existence of feedforward manifold neurons, or multiple classes of solitary neurons, requires injection of different retrograde tracers into corresponding loci within different target cortical areas. For example, in the visual system, injections must be made into recipient cortical areas at identical points in each retinotopic map. Furthermore, the cortical areas in question must be well accepted, accessible, and identifiable. The primary visual cortex (striate cortex, or V1) is ideally suited for revealing patterns of feedforward projections. It contains cells in layer 4B that project to the second visual area (V2) and middle temporal area (MT, or V5) (Lund et al., 1975
We used a dual-tracer technique to map the projections of layer 4B neurons in V1 to areas V2 and MT in the macaque (Sincich and Horton, 2002c
Materials and Methods
Experimental animals and surgical procedures. Experiments were conducted in four adult male Macaca fascicularis using procedures approved by the University of California, San Francisco Committee on Animal Research and in accordance with National Institutes of Health guidelines. Anesthesia was induced with ketamine HCl (10 mg/kg, i.m.). The animal was intubated endotrachially and anesthesia was maintained with 1.5% isoflurane in a 1:1 mixture of N2O:O2. We monitored electrocardiogram, respiratory rate, body temperature, blood oxygenation (SpO2), endtidal CO2, and inspired/expired levels of anesthetic gases throughout the experiment. A 5% dextrose in half-normal saline solution was given intravenously at 3 ml/kg per hour. After the animal was placed in a stereotaxic frame, a craniotomy was made to expose the lunate and superior temporal sulci. The dura was widely reflected to make sulci obvious.Retrograde tracers were reconstituted in filtered, sterile balanced salt solution. For MT injections along each of six to seven penetrations, four 120 nl pressure injections of 0.1% gold-conjugated cholera toxin B subunit (CTB; List Biologic, Campbell, CA) (Llewellyn-Smith et al., 1990
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Figure 2. Injection locations in V2 and MT. a, Lateral view of a macaque right hemisphere, illustrating pipette entry points. The blue sagittal plane is diagrammed in b. The dotted line is the V1–V2 border. b, Tracer deposit sites for WGA–HRP in V2 and CTB in MT, as they might appear in a sagittal section. c, Single flatmount section from the right hemisphere of Monkey 2. The blue dashed line encircles MT, as estimated from the entire series of sections. Anatomical axes: posterior–anterior, left–right; dorsal–ventral, top–bottom. d, Same section as in c, with the injection sites from an adjacent CTB/WGA–HRP-reacted section aligned and superimposed digitally. Sulci outlines are drawn in white (IOS, inferior occipital sulcus). The black box outlines the region in which a deeper section was photographed for Figure 3. e, Left hemisphere of Monkey 1, with sulcal outlines and injection sites. The black box is a region in V1 in which overlapping labeled cells appeared in a deeper layer 4B section (shown at higher magnification in Figure 4). Scale bar, 1 cm.
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Figure 3. MT-projecting cells in V1. a, Brightfield image of a CO-stained section containing CTB-labeled cells. Many layers are visible in this area because the plane of section was oblique to the cortical surface. b, Inverted dark-field image of the same section in a, showing that CTB labeling was found only in layers 4B and 6. Laminar boundaries (blue) are taken from the CO pattern. c, High magnification view of the boxed field in b, showing light, medium, and heavily labeled neurons. The two top labeled cells were also CO-rich, as evident in the proximal dendrite staining. d, Pyramidal cell from the next section. Its apical dendrite was cut off where it left the section. Stellate cells (c, top) had no apical process. Scale bars: a, b, 500 µm; c, d, 50 µm.
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Figure 4. Three different output populations in layer 4B. a, A single section cut tangentially through layer 4B of Monkey 1, processed for WGA–HRP and CTB. Individually lettered neurons are shown at higher magnification in Figure 5. b, Desaturated image of the CO pattern in layer 3, showing the distribution of labeled cells in a in patch (gray outline) and interpatch compartments. Blue dots indicate WGA–HRP-labeled cells projecting to V2, green squares indicate CTB cells projecting to MT, and red squares indicate double-labeled cells. Black arrows point to blood vessels used for alignment. Scale bar, 200 µm.
The injections were placed successfully in four hemispheres of three animals. In the remaining two hemispheres, and in both hemispheres of the fourth monkey, the injections did not produce overlapping label either because CTB was deposited in dorsal MT, leading to retrograde labeling in the wrong portion of V1, or because the WGA–HRP injections intended for V2 strayed into V1.The monkey shown in Figure 1 is from a series of experiments examining the correlation between CO stripes in V2 and the projections from V1 in macaques (Sincich and Horton, 2002b
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Figure 1. Location of V1 projection zones in V2 and MT. a, Single flatmount section cut through the superficial layers of the right occipital cortex of a macaque, showing the CO pattern in V1, V2, and MT. b, Same section as in a with areas identified and sulci outlined in white. Sulcal boundaries are tracked during the unfolding process. The blue dotted line indicates area MT as judged by the CO pattern. c, Adjacent section to a, processed for autoradiography and photographed in dark-field. The large [3H]proline injections in V1 lead to anterogradely labeled fields of axon terminals centered in V2 and MT. Scale bar, 1 cm.
Histology. After 2–3 d for transport, the animals were given a lethal dose of pentobarbital (150 mg/kg) and cardially perfused with 2 L of 0.9% saline followed by1Lof1% paraformaldehyde in 0.1 M phosphate buffer (PB), pH 7.4. The brain was removed and flatmounts were prepared containing V1 and the cortex within the lunate sulcus and STS (Olavarria and Van Sluyters, 1985
4 gm/cm 2). We cut frozen sections parallel to the pial surface, alternating between 25 µm thick for CO processing (Wong-Riley, 1979
Data analysis. In all four analyzed cases, there was heavy CTB labeling in opercular V1, including areas near the border with V2. For cell counting, labeled cells were plotted by camera lucida at 400x magnification. In flattened CTB/WGA–HRP-stained material, layer 4B cells were usually captured in a single section. Multiple (5–12) 0.25 mm 2 fields in each hemisphere were selected for cell counting in layer 4B. These fields were opposite V2 injections in all three stripe types, often straddling the stripes. We surveyed each section at low magnification to locate the portion of each section where the density of cells labeled by each tracer overlapped maximally. Selecting such regions for high magnification analysis optimized the likelihood of detecting double-labeled cells. We used the CO pattern to identify cortical layers; in all cases, layer 4A was superficial to the CTB-labeled cells. The density of labeled cells varied between animals, primarily because double-labeled regions did not necessarily contain the densest population of any one label, and because histological processing is inherently variable. Single-labeled cells in one-third of every counted field and all double-labeled cells were outlined for cell body area measurements. These outlines were transferred into Illustrator 9.0 (Adobe Systems, San Jose, CA) to calculate areas using the CADtools 2.1 extension (Hot Door, Grass Valley, CA).
Cell morphology is not readily determined in tangential sections. In many cases, we could not decide whether a cell was one of two known morphologies, stellate or pyramidal. However, in particularly well labeled cells, apical dendrites could be observed by focusing through the section. Pyramidal cells often had three basal dendrites, giving them a triangular appearance in the top-down view (see Fig. 5b,d). In contrast, stellates had more compact cells bodies, with less tapering at the start of their lateral dendrites. Because weak labeling would lead to the underestimation of pyramidal cells, we did not quantify the proportion of pyramidal versus stellate cells.
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Figure 5. Distinct cell types project to V2 and MT. a, b, WGA–HRP-labeled cells were most often small stellate (a, asterisk) or pyramidal neurons and less frequently medium-sized pyramids (b). CTB-labeled neurons included the large Meynert cells characteristic of layer 4B (c) and pyramids ranging in size (d). e, f, Double-labeled cells were always medium-sized cells. g, h, Single-labeled neurons could often be found situated within the same cortical column. i, Distribution of cell body areas for each type of labeling across all animals, showing that double-labeled cells (red) formed a subpopulation among the smaller V2-projecting cells (gray) and MT-projecting cells (white). Only one of every three fields were measured for the single-labeled cells. Scale bar: a–h, 20 µm.
To quantify the relationship between MT-projecting neurons and CO patches, we analyzed only areas in which CTB-labeled cell density was high. We aligned digital images of sections from layer 3 and 4B with Photoshop 6.0 (Adobe Systems) using blood vessels as guides. Minor scaling and no warping were needed for alignment. Vessel profiles in the layer 3 CO image were filled in with the mean image luminance. A low-pass Fourier-filtered version of this image (cutoff frequency, 1.1 cycles/mm) was subtracted from the original to produce a gray-level flattened version of the CO pattern. This image was blurred with a Gaussian filter (
= 70 µm). To produce a spatial average of the CO values surrounding MT-projecting cells similar to that of Boyd and Casagrande (1999
2 test was used to determine whether the distribution of cells among these three gray levels differed significantly from chance. Analysis routines were written in MatLab 5.0 (MathWorks, Natick, MA).
Results
To guide the placement of tracers into retinotopically corresponding locations in V2 and MT, we first mapped the terminal fields of V1 neurons projecting to these extrastriate areas. We subsequently verified the location of the cortical areas postmortem by staining the tissue for CO. V1, V2, and MT are all recognizable in CO sections if the cortex is unfolded and flattened before histological processing (Fig. 1a). V1 contains the characteristic rows of CO patches (Horton and Hubel, 1981We used these maps along with sulcal landmarks to guide the retrograde tracer injections into retinotopically similar areas in V2 and MT (Fig. 2a). WGA–HRP was injected along a narrow strip of exposed V2, representing parafoveal visual space near the lower vertical meridian (Gattass et al., 1981
In four hemispheres from three animals, the two tracers were injected successfully in similar retinotopic locations in V2 and MT (Fig. 2c–e). In these cases, the WGA–HRP injections were confined to V2. The CTB injections landed in the ventral MT, in which the central visual field is represented. MT has a vague boundary in CO-stained tissue, making it difficult to be sure the CTB injections were strictly limited to this cortical area. In fact, in several cases, we suspect some CTB landed just outside MT (Fig. 2d,e). However, two lines of evidence indicate that these extraneous tracer deposits did not contaminate our results. First, CTB-labeled cells in V1 were found exclusively in the lower two-thirds of layer 4B and in upper layer 6 (Fig. 3). These are the same two layers found to project to MT in all previous studies (Lund et al., 1975
Injection of these two tracers gave rise to overlapping fields of labeled neurons in V1, near the dorsal V1–V2 border. High densities of cells filled with WGA–HRP or CTB were intermingled in layer 4B, which is
A survey of a representative field (Fig. 4a) from Monkey 1 revealed 897 cells containing WGA–HRP and 78 cells containing CTB. Only six neurons were double labeled (Fig. 4b). The density of WGA–HRP cells (598 cells per square millimeter) was extremely high, suggesting that we labeled a high proportion of the cells in the field that projected to V2. The density of the MT-projecting cells (52 per square millimeter) was lower but similar to that reported in a previous study (Shipp and Zeki, 1989
Double-labeled cells were also scarce in the other three hemispheres (Table 1). The abundance of single-labeled cells in layer 4B showed that neurons representing identical points in visual space project to different visual areas. This raises the possibility that V2 and MT receive input from different cell types. Both pyramidal and stellate cells are known to project from layer 4B to V2 and MT (Tigges et al., 1981
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Table 1. Cells labeled by tracer injections in V2 and MT
We have shown previously that V1 cells in layer 4B projecting to the thick CO stripes of V2 are clustered into interpatch compartments (Sincich and Horton, 2002a
Quantitative analysis of the distribution of CTB-labeled cells in each animal confirmed the lack of any tendency for MT-projecting cells to favor patches or interpatches. Figure 6a shows a 3 x 4.25 mm field of V1, neighboring the field shown in Figure 4a and photographed in dark-field illumination to reveal CTB labeling in layer 4B. The layer 3 CO section aligned with this field (Fig. 6b) was gray-level coded and superimposed on a plot of the cells (Fig. 6c). Generating a spatial average of the CO density in the tissue surrounding each cell showed that MT-projecting cells did not preferentially reside in patches or interpatches (Fig. 6d). This analysis was repeated in three additional hemispheres representing eccentricities from 1 to 15° for a total of 1688 cells. No correlation with CO patches was found at any eccentricity (Fig. 6d–g) (Shipp and Zeki, 1989
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Figure 6. MT-projecting cells are independent of the CO patch system. a, Inverted dark-field image of CTB-labeled cells in layer 4B. The top left corner of the section passed out of layer 4B. Black arrows point to blood vessels used for alignment. b, CO section from layer 3 aligned with the section in a. c, Gray-level rendered image of CO density, divided into three zones of equal area for
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Table 2. Distribution of MT-projecting neurons among CO columns in V1
Our data indicate that the direct V1
MT pathway is rooted diffusely in both patches and interpatches, whereas the indirect V1
Discussion
Using a dual-tracer method, we found that V2 and MT receive substantially independent input from V1. Manifold cells were uncommon, despite our efforts to maximize their labeling by choosing populations that cohabit a single layer and injecting retinotopically overlapping locations in V2 and MT. Cell-size differences supported the idea that separate populations project to each extrastriate area.Our data show that layer 4B neurons play a more diverse role in visual processing than previously thought. In overviews of the visual system, layer 4B has been treated as a single entity, transmitting a magnocellular-dominated motion signal to the extrastriate cortex (Livingstone and Hubel, 1988
) (Yabuta et al., 2001
The pyramidal cells of layer 4B receive both magnocellular and parvocellular inputs (Sawatari and Callaway, 1996
The projection from V1 to V2 thick stripes originates from interpatches (Sincich and Horton, 2002a
Although we found no relationship between MT-projecting cells and CO patches, which is in agreement with a previous study (Shipp and Zeki, 1989
Our findings modify the overall picture of interareal connections in the visual system. Connections have always been depicted as being formed unitarily by areas or layers; however, neurons are the basic projection units. We do not know how prevalent manifold projections are, in part because a functional relationship between injected sites (e.g., homotopy in sensory areas) is required to produce double labeling. Injections with dual tracers are seldom made into related portions of different cortical areas (Kennedy and Bullier, 1985
If the brain distributes signals using many segregated classes of solitary neurons and manifold neurons, conventional wiring schemes must be revised to incorporate an exponential increase in the number of potential information channels. Because every cortical area projects to many other areas, our results also emphasize that each "link" between the areas is composed of at least one solitary and one manifold connection. For example, a network of five areas fully connected with solitary axons would have n(n – 1) = 20 links. This number jumps to n2(n – 1)/2 = 50 links, if one assumes that neurons in each area send a solitary axon or a manifold axon to two other areas. Because some neurons may target three or more areas, this equation does not account for the number of conceivable projections. Of course, not all of these projections need to exist. In a cortical scheme based on an n(n – 1) model, only 31% of the possible connections have been demonstrated (Felleman and Van Essen, 1991
The small percentage of double-labeled cells that we found indicates that feedforward cortical projections, at least from V1, are predominately solitary. Solitary neurons also dominate feedback projections, but manifold neurons appear to be relatively more common (Salin and Bullier, 1995
The finding of three potential output channels from layer 4B of V1, in which, until recently, only a single channel was assumed (Livingstone and Hubel, 1988
Footnotes
Received Jan. 2, 2003; revised Apr. 9, 2003; accepted Apr. 11, 2003.This work was supported by National Eye Institute Grants EY10217 (J.C.H.), EY13676 (L.C.S.), and EY02162 (Beckman Vision Center). Support was also received from That Man May See, The Bunter Fund, and Research to Prevent Blindness (J.C.H.). The California Regional Primate Research Center is supported by National Institutes of Health Base Grant RR00169. We thank D. L. Adams, J. A. Movshon, and H. L. Read for their comments on this manuscript.
Correspondence should be addressed to Dr. Lawrence C. Sincich, Beckman Vision Center, University of California, San Francisco, 10 Koret Way, San Francisco, CA 94143-0730. E-mail: sincich{at}itsa.ucsf.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/235684-09$15.00/0
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