Pyramidal Cells in Prefrontal Cortex of Primates: Marked Differences in Neuronal Structure Among Species

The most ubiquitous neuron in the cerebral cortex, the pyramidal cell, is characterized by markedly different dendritic structure among different cortical areas. The complex pyramidal cell phenotype in granular prefrontal cortex (gPFC) of higher primates endows specific biophysical properties and patterns of connectivity, which differ from those in other cortical regions. However, within the gPFC, data have been sampled from only a select few cortical areas. The gPFC of species such as human and macaque monkey includes more than 10 cortical areas. It remains unknown as to what degree pyramidal cell structure may vary among these cortical areas. Here we undertook a survey of pyramidal cells in the dorsolateral, medial, and orbital gPFC of cercopithecid primates. We found marked heterogeneity in pyramidal cell structure within and between these regions. Moreover, trends for gradients in neuronal complexity varied among species. As the structure of neurons determines their computational abilities, memory storage capacity and connectivity, we propose that these specializations in the pyramidal cell phenotype are an important determinant of species-specific executive cortical functions in primates.


INTRODUCTION
Pyramidal cell structure is remarkably heterogeneous in the primate cerebral cortex. Estimates of the total number of spines (putative excitatory inputs) in the dendritic trees of pyramidal cells reveal more than a 30-fold difference between populations of cells sampled in different cortical areas (Elston et al., , 2005c. Moreover, there are systematic trends for increasingly more complex phenotypes through a series of functionally related cortical areas. For example, neurons become progressively larger, more branched and more spinous with anterior progression through the dorsal and ventral visual pathways (Elston and Rosa, 1997, 1998Elston et al., 1999aElston et al., , 2005bElston, 2003b). There is a progressive systematic increase in the complexity of pyramidal cell structure through somatosensory areas 3b, 1, 2, 5, and 7 (Elston and Rockland, 2002;Elston et al., 2005g,j), which continues with anterior progression through cingulate areas 23 and 24 to granular prefrontal cortex (gPFC; Elston et al., 2001Elston et al., , 2005a. Pyramidal cells are the most common neuron in the cerebral cortex. They are the major source of intrinsic excitatory cortical synapses, and their dendritic spines are the main postsynaptic target of excitatory synapses. Moreover, they form most intra-areal projections and nearly all interareal projections (DeFelipe and Fariñas, 1992). Therefore, they are considered the principal neuronal building blocks of the cerebral cortex. Thus, specializations in their structure are likely to influence cortical function at the subcellular, cellular, and systems levels (Elston, 2002(Elston, , 2003aJacobs and Scheibel, 2002;Passingham et al., 2002;Roth and Dicke, 2005;Treves, 2005). More specifically, complexity in dendritic structure determines their biophysical properties thus influencing their functional capacity and potential for plastic changes (Koch, 1999; Pyramidal cells in prefrontal cortex of primates: marked differences in neuronal structure among species cell structure in lateral, medial, and orbital gPFC of the vervet monkey and baboon for comparison with those studied in the macaque monkey. These species were included as they represented closely related primates of similar and different brain size (Gould, 2002). We found that, in general, pyramidal cells in the gPFC were characterized by highly complex structure as compared with those in other cortical regions. In addition we found regional variation in pyramidal cell structure within the gPFC in all three species; however, the topography of the gradients differed between species. We also found marked interindividual variation in pyramidal cell structure in the gPFC in all three species of an order not observed in visual, somatosensory, motor, or cingulate cortex.

MATERIALS AND METHODS
Two adult macaque monkeys (Macaca fascicularis; 4.5 years old; MF1 ≈ 5 kg, MF2 ≈ 4.5 kg), two adult vervet monkeys (Cercopithecus pygerythrus; age unknown; VM1 = 6.1 kg, VM2 = 5.5 kg), and two adult baboons (Papio ursinus; age unknown; B1 = 23.1 kg, B2 = 23.1 kg) were used in the present study. Based on weight, musculature and appearence of the vervet monkeys and baboons we estimate that they were mature but not adolescent nor elderly. All animals were males. All tissue was sampled from the left hemisphere. Macaque tissue was taken from the anterior lateral portion of the superior frontal gyrus (corresponding to Walker's and Petrides and Pandya's area 9 or Preuss and Goldman-Rakic's area 9d) (Walker, 1940;Preuss and Goldman-Rakic, 1991a,b,c;Petrides and Pandya, 2001), the anterior medial portion of the superior frontal gyrus (area 9m of Preuss and Goldman-Rakic, corresponding to Walker's area 9), the medial frontal gyrus (corresponding to Walker's and Petrides and Pandya's area 46 or Preuss and Goldman-Rakic's area 46vr), the inferior frontal gyrus (corresponding to Walker's area 46, Petrides and Pandya's area 45A or Preuss and Goldman-Rakic's area 12vl), the medial portion of the frontal pole anterior to the rostral sulcus (corresponding to area 10 of Walker, Preuss and Goldman-Rakic and Petrides and Pandya), the end of the orbital cortex between the medial orbital sulcus and the lateral orbital sulcus, inferior to the intermediate orbital sulcus (area 12orb of Preuss and Goldman-Rakic, corresponding to Walker's area 13 and Petrides and Pandya's area 14) of the left hemisphere (Figure 2). Likewise, tissue from the vervet monkey and baboon was sampled from dorsolateral, medial, and orbital gPFC (Figure 2). Specifically, prefrontal areas 9d, 10, 46d, 12vl, and 13 were studied in the baboon and prefrontal areas 9m, 9d, 10, 13, and cingulate area 32, were studied in the vervet monkey. The homology of the specific areas included for analyses remains to be determined.
Methodology used in the present study has been outlined in detail in previous studies (Buhl and Schlote, 1987;Elston and Rosa, 1997;Elston, 2001). Briefly, the animals were deeply anesthetized by intramuscular injection of a mixture of ketamine hydrochloride (100 mg/ml) and xylazine (50 mg/ml) (2:1, 0.1 ml/kg), then an i.v. dose of sodium pentabarbitone (200 mg/kg) in accordance with protocols approved by the University of Queensland and University of the Witwatersrand Animal Ethics Committees and regulations for the care and use of animals set out by the NIH (publication No. 86-23, revised 1985). The animals were then perfused intracardially and the brain removed. The white matter was trimmed from the blocks and the remaining gray matter was "unfolded" and postfixed overnight between glass slides in a solution of 4% paraformaldehyde in 0.1 M phosphate buffer (PB). Serial thick sections (250 μm) were cut tangential to the cortical surface with the aid of a vibratome. Individual sections were incubated in a solution containing 10 −5 mol/L of the fluorescent dye 4′,6-diamidino-2-phenylindole (DAPI; Sigma D9542, St Louis,  Walker (1940), (B) Petrides and Pandya (1999) and (C) Preuss and Goldman-Rakic (1991a).  Illustrated are two cells sampled from the primary visual area (V1) and granular prefrontal cortex (gPFC) of the macaque monkey. At left are the basal dendritic trees of the two cells as seen in the tangential plane. In black is the part of the dendritic tree that would be seen in a 50-μm transverse section (of the type used in many Golgi studies). The portion of the dendrites extending beyond the section is illustrated in gray. Note the relative similarity in structure of the part of the dendritic tree revealed in the 50-μm transverse sections. At right are illustrated the dendrograms of each of the two cells, which resulted from reconstruction of the complete basal dendritic tree as seen in the tangential plane. Based on our observations, transverse sections would have to be of the order of 1 mm thick to include all dendrites (e.g., human temporal lobe; Elston et al., 2001). sections thick enough to contain the entire dendritic arborization (both apical and basal). Thus, we have focused on one dendritic "compartment" of a select group of pyramidal cells (those in layer III). It remains to be determined to what extent regional and species variation in the basal dendritic trees reflects any potential variation in their apical dendrites, and how this may differ from patterns of connectivity in other cortical areas/species (Binzegger et al., 2004).
4′,6-Diamidino-2-phenylindole(DAPI)-labeled neurons were injected under visual guidance with continuous current (up to 100 nA). Cell bodies were impaled not at the cut surface of the sections, but some tens of micrometers below the surface so that pyramidal neurons could be identified by the presence of the proximal part of their apical dendrite. Once a suitable number of neurons had been injected, the slice was processed for a lightstable reaction product (see Elston and Rosa, 1997). Briefly, the sections were processed in a solution containing 1:400,000 anti-Lucifer Yellow in stock solution [2% bovine serum albumin (Sigma A3425), 1% Triton X-100 (BDH 30632), and 5% sucrose in PB] for 5 days at room temperature, washed three times in PB, then incubated in biotinylated anti-rabbit (1:200 Amersham RPN 1004) in stock solution for 2 h, washed another three times before being processed for a further 2 h in streptavidin biotin horseradish peroxidase (1:200, Amersham RPN1051) in PB. 3,3′diamino-benzidine (DAB; Sigma D 8001; 1:200 in PB) was used as the chromogen (Figure 4). USA) in PB at room temperature for approximately 10 min and mounted between Millipore filters (AABG02500, Bedford, USA). The slice preparation was then mounted in a perspex dish on a Zeiss fixed stage microscope and the preparation visualized with UV excitation (341-343 nm).
In the present study we focused on cells at the base of layer III, enabling comparison with data obtained at the base of layer III in visual, somatosensory, motor, and cingulate cortex of these an other species. Layer III was easily identified in the DAPI-labeled sections immediately above the neuron-dense granular layer. Even in tangential sections it is easy to distinguish the transition from layer III to layer IV due to the change in density and size of somata (see Figure 3 of Elston and Rosa, 1997). Neurons were injected in tangential sections so as to be able to reconstruct the entire basal dendritic tree. Such an approach has been central to the demonstration of regional and species specializations in pyramidal cell dendritic structure as the entire tangential extent of the basal dendritic tree is revealed, unlike in most previous studies in transverse sections in which many of the basal dendrites are truncated thus selecting for uniformity (Figure 3). In addition, by injecting neurons in the tangential plane aspects of their structure can be related directly with features reported elsewhere such as intrinsic axon patches and receptive fields Kritzer and Goldman-Rakic, 1995;Pucak et al., 1996;Melchitzky et al., 1998Melchitzky et al., , 2001González-Burgos et al., 2000). However, unfortunately, it is difficult to inject large numbers of cells under visual control in were made using SPSS (SPSS Inc., IL, USA). One-way ANOVAS were used where there was a single data point for each cell, such as the size of the cell bodies of the size of the dendritic trees. When there were multiple data points for each cell, e.g., branching structure or spine density sampled radially from cell body to the distal tips of the dendrites, repeated measures ANOVAs were used.

RESULTS
A total of 854 layer III pyramidal cells were included for analyses as they satisfied the criteria for inclusion (see Materials and Methods). Over 80,000 individual dendritic spines were drawn and tallied. Data on the size, branching complexity, and spine density of the basal dendritic trees are reported for each cortical area of both animals studied from each of the three species, as are data on cell body size and our estimates of the number of spines in the basal dendritic tree of the "average" neuron in each area.

Basal dendritic field areas
Qualitative observation revealed variation in the size of the dendritic trees of pyramidal cells among prefrontal areas 9d, 10, 12vl, 13, and 46vr in both MF1 and MF2 ( Figure 5A; Table 1). Statistical analysis (one-way ANOVAs) revealed these differences to be significant (p < 0.05) in both MF1 (F (4) = 8.92) and MF2 (F (4) = 15.33). Post hoc Scheffe tests revealed 3 of 10 possible between-area comparisons to be significantly different in MF1 and 4 of 10 in MF2 ( Table 2).

Branching patterns of the basal dendritic arbors
Plots of the branching patterns of the basal dendritic arbors of pyramidal neurons, as determined by Sholl analysis, are shown in Figure 5B. From the figure it can be seen that the branching structure of cells in prefrontal areas 9d, 10, 12vl, 13, and 46vr was not uniform. Repeated measures ANOVAs (5 × 12 design) revealed significant differences (p < 0.05) in the branching patterns in both MF1 (F (1,4) = 11.27) and MF2 (F (1,4) = 6.78). Post hoc Scheffe tests revealed 4 of 10 possible between-area comparisons to be significantly different in MF1 and 3 of 10 in MF2 ( Table 2).

Spine densities of the basal dendrites
From Figure 5C, it can be seen that plots of the average spine density, as a function of distance from the soma to the distal tips, were similar among cortical areas. Repeated measures ANOVAs revealed no significant difference in spine density for neurons in either MF1 (F (1,4) = 1.00) and MF2 (F (1,4) = 2.58). The total number of dendritic spines in the basal dendritic arbor of the "average" pyramidal neuron in each area was calculated by combining data from the Sholl analyses with that of spine densities (see Materials and Methods). These estimates revealed up to >50% difference in of the number of spines in the "average" neuron among prefrontal areas ( Figure 6; Table 3).

Somal areas
Individual cell bodies were drawn, in the plane tangential to the cortical layers, and plotted in Figure 5D (see also Table 4).
One-way ANOVAs revealed significant differences in cell body size between neurons in the different cortical areas in both MF1 (F (4) = 5.10) and MF2 (F (4) = 26.13). Post hoc Scheffe tests revealed 2 of 10 possible between-area comparisons to be significantly different in MF1 and 6 of 10 in MF2 ( Table 2).
Cells were only included for analysis if they had an unambiguous apical dendrite, had their complete basal dendritic tree contained within the section, and were well filled. We focused our analyses on the basal dendritic trees of supragranular pyramidal cells for several reasons. Of particular interest to us are horizontally projecting intrinsic axonal patches that arise from these cells and project to the basal dendritic trees of neighboring pyramidal cells Wiesel, 1979, 1983;Rockland andLund, 1982, 1983;Livingstone and Hubel, 1984;Martin and Whitteridge, 1984;Rockland, 1985;Kisvárday et al., 1986;McGuire et al., 1991;Fujita and Fujita, 1996). As many as 80-95% of the horizontal projection synapses of individual supragranular pyramidal cells are formed with other nearby supragranular pyramidal cells (Kisvárday et al., 1986;McGuire et al., 1991) in reciprocally connected patches (Kisvárday and Eysel, 1992). These reciprocal patches have been reported in many different cortical areas in the primate brain, and are believed to provide an anatomical basis for functional domains among the patches (Mitchison and Crick, 1982;Matsubara et al., 1985;T'so et al., 1986;T'so and Gilbert, 1988;Gilbert and Wiesel, 1989;Malach et al., 1993;Malonek et al., 1994). By focusing on the basal dendritic trees of layer III pyramidal cells we are revealing relevant information on the connectivity of these intrinsic circuits and how they may vary among cortical areas. Moreover, we have focused on these dendritic trees here so as to be able to make direct comparisons with our previous data sampled from the basal dendritic trees of layer III pyramidal cells in visual, somatosensory, auditory, motor, and cingulate cortex of thee same species.
Neurons were drawn, and their dendritic field areas determined with NIH Image by tracing a convex hull around the outermost distal dendrites (see Elston and Rosa, 1997). Sholl (1953) analyses were performed on the 2D drawings, with concentric circles of increasing radii (25 μm increments) centered on the cell body. Spine densities were calculated by drawing the entire dendrite of randomly selected cells with the aid of a Zeiss ×100 oil-immersion objective and counting the number of spines per 10 μm segment from the cell body to the distal tip (Eayrs and Goodhead, 1959;Valverde, 1967). Horizontally projecting dendrites were selected to avoid trigonometric error. All spines were drawn and no distinction was made between different spine types. In Golgi studies it is common to apply correction factors when attempting to quantify spine density as spines issuing from under the dendrite may be obscured (Feldman and Peters, 1979). No such correction factors were applied here as the DAB reaction product is more transparent than the Golgi precipitate and allows direct visualization of spines through the dendrite. Furthermore, the basal dendrites have a diameter smaller than the neck length of many spines, and any possible error that may arise because some populations of cells have thicker basal dendrites than others would only reduce the extent of differences we report for cells among cortical areas (i.e., more spinous cells have, on average, thicker parent dendrites than the less spinous cells). Estimates of the total number of spines found within the basal dendritic arbor of the "average" cell in each cortical area were made by summing the product of the average number of dendrites by the average spine density for corresponding segments along the dendrites -from the cell body to the distal tips of the dendrites (Elston, 2001). Cell bodies were drawn by tracing the outermost perimeter, excluding the proximal basal dendrites, while viewed through a Zeiss ×100 oil objective and their areas were determined with NIH Image. Statistical comparisons

Basal dendritic field areas
Qualitative observation of pyramidal cells revealed that cells in cingulate area 32 were larger than those in prefrontal areas 9d, 9m, 10 and 13 in both VM1 and VM2 ( Figure 5A; Table 5).
Statistical analysis (one-way ANOVAs) revealed a significant difference (p < 0.05) in the size of the dendritic trees of neurons in both VM1 (F (4) = 16.81) and VM2 (F (4) = 18.14). Post hoc Scheffe tests revealed that cells in cingulate area 32 had significantly larger dendritic trees than those in prefrontal areas in both VM1 and VM2, except for area 9m in VM2. None of the six possible pairwise comparisons between prefrontal areas were significantly different in VM1, two of the six pair-wise comparisons between prefrontal areas were significantly different in VM2 (Table 6).

Branching patterns of the basal dendritic arbors
Branching patterns of the basal dendritic arbors of pyramidal neurons are illustrated in Figure 5B. Repeated measures ANOVAs (5 × 13 design) revealed a significant difference (p < 0.05) in the branching patterns in both VM1 (F (1,4) = 3.05) and VM2 (F (1,4) = 10.12). Post hoc Scheffe tests revealed no significant difference in branching structure, except in VM2 where cells in area 9d differed to those in all other cortical areas ( Table 6).

Spine densities of the basal dendrites
The mean and standard deviation in spine density per 10 μm (as a function of distance from the soma to the distal tips of 10 randomly selected horizontally projecting basal dendrites of different cells in each cortical area) are plotted in Figure 5C. Repeated measures ANOVAs revealed a significant difference (p < 0.05) in the distribution of spines along the dendrites cells between    cortical areas in both VM1 (F (1,4) = 4.23) and VM2 (F (1,4) = 7.53).
Post hoc Scheffe tests revealed that spine density in area 32 was significantly different to that in areas 9d and 9m in VM1 and

Somal areas
Frequency distributions of the size of the cell bodies of pyramidal cells are plotted in Figure 5D and listed in Table 8. One-way ANOVAs revealed a significant difference in the size of the somata among neurons in VM2 (F (4) = 13.51) but not VM1 (F (4) = 1.39).
Post hoc Scheffe tests revealed that cells in cingulate area 32 in VM2 had significantly larger cell bodies than those in areas 9d and 10. Four of the six possible pair-wise comparisons between prefrontal areas in VM2 were significantly different ( Table 6).

Basal dendritic field areas
The size of the dendritic arbors was calculated and frequency distributions are plotted in Figure 5A (see also Table 9). Statistical analysis (one-way ANOVAs) revealed a significant difference in the size of the dendritic trees of neurons in both B1 (F (95) = 20.99) and B2 (F (176) = 6.50). Post hoc Scheffe tests revealed that 6 and 4 of all possible 10 pair-wise comparisons were significant in B1 and B2 (respectively ; Table 10).

Branching patterns of the basal dendritic arbors
Sholl analysis was performed and the branching profiles of the basal dendritic arbors of pyramidal neurons are illustrated in Figure 5B.
Statistical analysis (repeated measures ANOVAs) revealed a significant difference (p < 0.05) in the branching patterns of cells between cortical areas in both B1 (F (1,4) = 7.86) and B2 (F (1,4) = 3.27). Post hoc Scheffe tests revealed that 3 of all 10 pair-wise between-area comparisons were significant in B1 and 1 of all 10 comparisons was significant in B2 (Table 10).
area 10 in VM2. None of the six possible pair-wise comparisons between prefrontal areas were significantly different in VM1. Three of the six pair-wise comparisons between prefrontal areas were significantly different in VM2 (Table 6). There was a >50% difference in our estimates of the total number of dendritic spines in the basal dendritic arbor of the "average" pyramidal neuron in areas of the gPFC (Figure 7; Table 7).

a -Significant difference in the size of the basal dendritic trees. b -Significant difference in the branching structure of the basal dendritic trees. c -Significant difference in the spine density of the basal dendritic trees. d -Significant difference in the size of the cell bodies.
Significance determined as p < 0.05.

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February 2011 | Volume 5 | Article 2 | 9 Elston et al. Pyramidal cells in monkey prefrontal cortex the cell bodies between cortical areas did not always coincide with that observed for the size of their dendritic trees (Figures 5A-D).
One-way ANOVAs revealed significant differences (p < 0.05) in the size of the cell bodies of neurons between cortical areas in both B1 (F (95) = 13.87) and B2 (F (176) = 13.33). Post hoc Scheffe tests revealed that 5 of all 10 pair-wise between-area comparisons were significant in B1 and 6 of all 10 comparisons were significant in B2 (Table 10).

DISCUSSION
In the present investigation we studied pyramidal cell structure in the gPFC of the macaque monkey, the vervet monkey, and the baboon. We focused on the gPFC because of its involvement in executive functions such as conceptual thinking, prioritizing, and planning. The aim of the study was to determine whether there exists any appreciable variation in pyramidal cell structure

Spine densities of the basal dendrites
The spine density, as a function of distance from the cell body to the distal tips of the dendrites, is plotted in Figure 5C. Repeated measures ANOVAs (cortical area × distance from soma × spine density) revealed a significant difference (p < 0.001) in the distribution of spines between cortical areas in B2 (F (1,4) = 13.51), but not B1 (F (1,4) = 3.32). Post hoc Scheffe tests revealed a significance (p < 0.05) between cells in orbital and dorsolateral gPFC in B2 (Table 10). Estimates in the number of spines in the basal dendritic tree of the "average" layer III pyramidal cell revealed a >60% difference between cortical areas (Figure 6; Table 11).

Somal areas
Frequency distributions of the size of the cell bodies of layer III pyramidal cells, in the plane tangential to the cortical surface, are plotted in Figure 5D (see also  Sampling from the same cortical regions in the two animals (stylized at top right) resulted in remarkably similar trends in these estimates in visual, somatosensory, motor, and limbic cortex of both animals (top right). In granular prefrontal cortex (gPFC), however, we found unprecedented differences in our estimates of the total number of dendritic spines in the basal dendritic tree of the "average" layer III pyramidal cell among cortical areas (bottom left), despite standardizing the regions sampled between cases (bottom right). V1 = primary visual, V2 = second visual, V4 = fourth visual, 3b = primary somatosensory, 1/2/5/7 = somatosensory association, 4 = primary motor, 6 = premotor, 23 = posterior cingulate, 24 = anterior cingulate, 9/10/12/13/46 = prefrontal areas, 32 = cingulate.
Frontiers in Neuroanatomy www.frontiersin.org species specializations or interindividual variation. In either event, the extent of variation observed in the gPFC is unparalleled in any other cortical regions studied (visual, somatosensory, motor, and cingulate cortex) in all cases examined. Evolutionary, developmental, and functional implications of these findings are discussed below.
within the gPFC, and compare any such variation across species. The results reveal significant differences in pyramidal cell structure among cortical areas within the gPFC in all animals studied. Moreover, the extent and topology of these trends differed between animals. However, it remains unclear whether regional variation in pyramidal cell structure reported here represent     difference in our estimates of the total number of dendritic spines in the basal dendritic tree of the average neuron observed in the primary visual cortex was 16%, 25% in primary motor cortex and less than 9% in cingulate cortex (Elston and Rosa, 1997;Elston et al., 2005g,h,i). Moreover, trends for increasing complexity in the dendritic trees of pyramidal cells in visual somatosensory, motor, and cingulate cortex have always been consistent between individuals of any given species, where as this is not the case in the gPFC (Figure 7). The large number of pyramidal neurons included in these studies (Table 13) makes it unlikely that this observation is attributable to different numbers of cells included for analyses in each region. However, differences in sulcal patterns and sampling of different locations within a given cortical area (e.g., dorsal vs. ventral) are likely to have contributed to these apparent interindividual differences. For example, differences in pyramidal cell structure have been reported in layer III within V1 according to visuotopy and within inferotemporal cortex according to gross location (cf. Elston and Rosa, 1997;Elston et al., 1999a,b). A better understanding of these apparent interindividual differences will require that more individuals are included for analyses. It should be noted that these differences in our estimates of the total number of dendritic spines in the basal dendritic trees of layer III pyramidal cells in the gPFC equate to four times those reported in the entire basal dendritic trees in V1.

PHENOTyPIC SPECIALIzATION Of THE PyRAMIDAL CELL wITHIN THE gPfC
Here we found differences in the relative trends in morphological complexity among cortical areas in the gPFC between individuals. For example, cells in the dorsolateral gPFC were the most spinous in both the macaque monkey and baboon, but those in the orbital and medial gPFC were the most spinous in the vervet monkeys. These differences may be attributable to the selection of cortical areas included for analyses in each of the different species, but it is worthwhile noting that no such interspecies differences have been observed in visual, somatosensory, motor, or limbic cortex of these same species. Instead, trends reported in the visual, somatosensory, motor, and limbic cortex of the macaque monkey are the same as those reported in the vervet monkey and baboon ( Figure 6). Moreover, trends reported in these cortical areas in the macaque monkey, vervet monkey, and baboon are similar to those reported in all other primate species studied to date (Elston et al., 2005a,b,c,g,h,i,j).

NEURONAL HETEROgENEITy IN gRANULAR PREfRONTAL CORTEx
The gPFC has been divided into several cortical areas, the number, and location of which varies between studies (Vogt and Vogt, 1919;Walker, 1940;Petrides and Pandya, 1988Barbas and Pandya, 1989;Preuss and Goldman-Rakic, 1991a,b,c;Carmichael and Price, 1996;Petrides, 1998;Barbas et al., 1999;Barbas, 2000;Pandya and Yeterian, 2000). While these studies have been instrumental in characterizing regional and species differences in the gPFC, they provide limited quantitative data on cortical microcircuitry. Examination of the present results ( Figure 5) reveals new findings on the cortical microstructure not predictable from these cytological and connectional data. Namely, cortical pyramidal cells of similar size cell bodies may be characterized by dendritic trees of different size, branching structure, and spine density. Vice versa, pyramidal cells of different cell body size may have dendritic trees of similar size, branching structure or spine density. This lack of correspondence between cell body size and the structure of the dendritic tree has been reported in other cortical regions in primates, including the sensorimotor and cingulate cortex (Elston and Rockland, 2002;Elston et al., 2005a,f,g,i,j). Thus, while cytoarchitecture is an excellent means of detecting differences in areal and laminar structure in the cerebral cortex, it provides little insight into regional differences in patterns of connectivity and the integrative capabilities of the component neurons.
Previously we published a report in which pyramidal cell structure was compared in areas 10, 11, and 12 of the macaque monkey, and revealed quantifiable differences in cell morphology among these regions (Elston, 2000). The present data confirm and extend this original observation. In particular, previously we reported up to a 20% difference in our estimates of the numbers of spines in the dendritic tree of the average cell in areas 10 and 12 of the macaque monkey. Here we found up to a 22% difference in these estimates between areas within the gPFC of the macaque monkey (12vl and 46vr in case MF1). We found up to a 27% difference in these estimates in the vervet monkey (areas 9d and 9m in case VM1) and a 70% difference in the baboon (areas 9d and 12vl of case B2). Furthermore, as discussed above, we found different trends in the gradients of neuronal complexity among cortical areas within the gPFC within and between species. In future studies it will be worthwhile to study age, hemisphere, and sex effects to better understand the extent of heterogeneity in pyramidal cell structure in the gPFC.

INTERINDIVIDUAL VARIATION IN THE PyRAMIDAL CELL PHENOTyPE
While we would expect to find some degree of interindividual variation in cell structure, that observed in the gPFC is unprecedented. We found, for example, a 56% difference in our estimates of the total number of dendritic spines in the basal dendritic tree of the average neuron in area 12vl between the two macaque monkeys. Likewise we found a 43% difference in our estimates of the total number of dendritic spines in the basal dendritic tree of the average neuron in area 9m between the two vervet monkeys and a 48% difference in area 10 between the two baboons. These percentages are considerably higher than those reported in visual somatosensory, motor, and cingulate cortex of these same animals, or, indeed all other species studied. For example, the maximum interindividual Another possibility is that the different trends reflect species differences. The lineage leading to modern day vervet monkeys diverged from that leading to modern day baboons and macaque monkeys approximately 10 million years ago. The lineage leading to modern day baboons diverged from that leading to macaque monkeys about 7 million years ago (Gould, 2002). Thus, it is tempting to conclude that highly complex pyramidal cells in the dorsolateral gPFC is a characteristic of the latter species, which may differ from that in other primates that diverged earlier, such as New World monkeys and the great apes. Alternatively, the apparent species differences may reflect regional variation in neuronal maturation rates (Jacobs and Scheibel, 1993;Jacobs et al., 1995Jacobs et al., , 1997Page et al., 2002;Duan et al., 2003;Elston et al., 2009Elston et al., , 2010a or arise through sampling different subsets of projection neurons in the different cortical areas, which have been shown to differ in both their morphology (Schofield et al., 1987;Hallman et al., 1988;Hübener and Bolz, 1988;de Lima et al., 1990;Hübener et al., 1990;Einstein, 1996;Matsubara et al., 1996;Duan et al., 2002;Soloway et al., 2002;Elston and Rosa, 2006) and density (Jones and Powell, 1970;Barbas, 1992;Young, 1992;Pandya and Yeterian, 2000;Petrides, 2000;Collins et al., 2005) in different cortical areas. In either case, the result is consistent with our main conclusion that pyramidal cells develop differently among cortical areas and mature into specialized circuits. Clearly, more comparative and developmental data on pyramidal cell structure are required to reveal a more complete picture.
Not withstanding these limitations on the interpretation of the trends for regional variation in pyramidal cell structure within the gPFC, the present results confirm previous findings that pyramidal cells in the gPFC are characterized by a highly complex structure Elston, 2000;Elston et al., 2001;Jacobs et al., 2001). However, previously it was reported that pyramidal cells in the gPFC have a more complex phenotype than those in the visual, somatosensory, and motor and cingulate cortex (Elston and Rosa, 1997, 1998Elston and Rockland, 2002). The present data reveal that, in the macaque monkey, cells in inferotemporal and anterior cingulate cortex were more spinous than those area 12vl (case MF2; Elston et al., 1999aElston et al., , 2005apresent results). Likewise, cells in the anterior cingulate gyrus in both the vervet monkey and baboon have larger, more branched and more spinous dendritic trees than those in some cortical areas within the gPFC (Elston et al., 2005f,i). Therefore, the present data reveal that some but not all pyramidal cells in the gPFC have a more complex structure than those in other cortical regions. More specifically, those in the gPFC have the most complex branching structure and the highest spine density while those in the anterior cingulate gyrus and inferotemporal cortex may have the largest dendritic trees. As discussed below, these different morphological parameters are likely to influence different aspects of cellular and systems function.

fORM SERVES fUNCTION
As reviewed in detail elsewhere (Elston, 2002(Elston, , 2003aJacobs and Scheibel, 2002) differences in the size, branching complexity, spine density in the dendritic trees may influence various aspects of function at the subcellular, cellular, and systems levels. For example, differences in the size of the dendritic trees may influence the sampling geometry of neurons, the topographic relationship between the pattern of inputs and the size of the dendritic tree influenc-ing receptive field properties Malach, 1994). Differences in the diameter and total length of the dendrites determines their electrotonic properties (Rall, 1959(Rall, , 1989Mainen and Sejnowski, 1986;Rothnie et al., 2005). Differences in the number of branches in the dendritic tree may influence the potential to compartmentalize the processing of inputs within the arbor and, thus, the functional capacity of the neurons, as well as the decay of the backpropagating potentials believed to be important in Hebbian type reinforcement of inputs (Rall et al., 1992;Stuart et al., 1997;Segev and Rall, 1998;Mel, 1999;Spruston et al., 1999;Vetter et al., 2001;Elston, 2007). Differences in the number and density of spines along the dendrites may influence the potential for local summation and/or the inhibitory vetoing of inputs (White, 1989;Koch, 1999). In addition, as each dendritic spine in mature cortex receives at least one asymmetrical synapse (Arellano et al., 2007), which have been demonstrated to contain the excitatory transmitter glutamate (DeFelipe et al., 1988;Petralia et al., 1994a,b,c), differences in the total number of spines in the dendritic tree likely reflect differences in the number of excitatory inputs to the neuron: highly spinous cells receiving more excitatory inputs than less spinous cells (Elston, 2002(Elston, , 2003a. These differences in the density and distribution of inputs throughout the dendritic trees, and the spatial distribution of the dendritic tree, have been shown to influence both the functional capacity of neurons and the memory storage capacity of cortical circuits they comprise (Poirazi and Mel, 2001;Stepanyants et al., 2002;Losonczy et al., 2008;Spruston, 2008). The dramatic differences in the branching structure of, and number of spines in, the dendritic trees of neurons in the gPFC of primates  makes it implausible that function in this region of the brain is the same across species. Indeed, modeling studies have demonstrated a difference of up to two orders of magnitude in the memory capacity of cortical circuitry attributable to differences in the branching structure and number/distribution of inputs throughout the dendritic trees of the component pyramidal cells (Mel, 2002;Chklovskii et al., 2004).
Perhaps not surprisingly, differences in discharge properties of cortical neurons have also been reported among cortical regions. For example, neurons in the gPFC are characterized by tonic discharge properties that are sustained despite interruption from distractors, those in association cortex are characterized by tonic discharge properties that may be interrupted by distractors and those in and primary sensory cortex are characterized by phasic activity (Fuster and Alexander, 1971;Fuster, 1973;Fuster et al., 1982;Fuster and Jervey, 1983;Ashford and Fuster, 1985;Funahashi et al., 1989Funahashi et al., , 1993Miller et al., 1993Miller et al., , 1996Constantinidis and Steinmetz, 1996;Sakai et al., 2002;Shinomoto et al., 2005).
Finally, from the intrinsic point of view of cortical organization, there are also significant differences in the distribution of GABAergic interneurons in different cortical areas of primates (Lewis and Lund, 1990;Gabbott et al., 1997;DeFelipe et al., 1999;Elston and González-Albo, 2003;Ballesteros-Yánez et al., 2005;Benavides-Piccione and DeFelipe, 2007;Inda et al., 2007;Blazquez-Llorca et al., 2010). Since GABAergic neurons are involved in the shaping the activity of pyramidal neurons, it is likely that the different intrinsic functional attributes of the cortical regions examined depends on all these features or in a combination of them. Further connectivity determine the computational abilities cortical circuits, the present data suggest regional and species differences in computations performed in the gPFC of macaque monkeys, vervet monkeys, and baboons. Functions often ascribed to the gPFC, such as planning, prioritizing, and conceptualization, are likely then to be influenced by specialization in the pyramidal cell phenotype.
correlative physiological and microanatomical/neurochemical studies would be necessary to perform to find out the role of each cortical component on the processing of information characteristic of the different cortical areas.

CONCLUSION
Here we found significant differences in pyramidal cell structure among cortical areas within the gPFC of the macaque monkeys, vervet monkeys, and baboons. Moreover we found species differences when comparing pyramidal cell structure between homologous/corresponding cortical areas. The data suggest regional as well as interindividual and species differences in the functional capabilities of pyramidal cells in different cortical areas of the gPFC of cercopithecid primates. Because pyramidal cells comprise >70% of neurons within the gPFC, differences in the number of dendritic spines (putative excitatory inputs) found within their dendritic trees suggest that cortical areas within the gPFC are characterized by different patterns of connectivity. As patterns of