Embryonic and Early Fetal Development of the Human Neocortex

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The Journal of Neuroscience, March 1, 2000, 20(5):1858-1868

Embryonic and Early Fetal Development of the Human Neocortex
Gundela Meyer¹, Jean Pierre Schaaps², Louis Moreau², and André M. Goffinet³
¹ Department of Anatomy, Faculty of Medicine, University La Laguna, 38071 La Laguna/Tenerife, Spain, ² Department of Embryology, University of Liege Medical School, B4000 Liege, Belgium, and ³ Neurobiology Unit, University Namur Medical School, B5000 Namur, Belgium

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Early corticogenesis was studied in human embryos and early fetuses from Carnegie stages 16 to 22 (5-8 gestational weeks)by using immunohistochemistry for Reelin (Reln), calretinin (CR),and glutamic acid decarboxylase (GAD). A first population of Reln-positivecells appears in the neocortical anlage at stage 16 and increasesin number at stages 17-18. At stages 19-20, a monolayer of horizontalCR- and GAD-positive, Reln-negative neurons forms in the preplate,whereas Reln-positive cells shift into a subpial position. Anothercell class, the pioneer projection neuron, is CR-positive butGAD- and Reln-negative; pioneer cells contribute early corticofugalaxons. Pioneer cells first appear below the monolayer at stage20 and form a pioneer plate at stage 21. The cortical plate (CP)proper emerges at stage 21 and inserts itself within the pioneerplate, which is thus split into a minor superficial componentand a larger deep component that presumably corresponds to thesubplate. Initial CP neurons are radially organized and mostlyCR-negative. Reln-positive cells remain consistently segregatedfrom the pioneer cells and are thus not directly involved in preplatepartition. Our data indicate that the neuronal composition ofthe human neocortical preplate is more complex than generallydescribed and that various neurons participate in a sequence ofevents that precede the emergence of theCP.

Key words: Cajal-Retzius cells; preplate; marginal zone; subplate; reelin; neuronal migration

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The correct establishment of the six-layered neocortex is critically dependent on a tightly regulated developmental programthat begins to unfold before the appearance of the cortical plate(CP). Disturbances of this complex process are increasingly recognizedas major causes of intractable epilepsies and mental disabilitiesin childhood (Faiella et al., 1997; des Portes et al., 1998; Gleesonet al., 1998, 1999; Francis et al., 1999).

Numerous experimental studies provided insight into the cellular dynamics and genetic regulation of early corticogenesis.Neurons are generated in ventricular zones (VZs) of cortical walland ganglionic eminence and reach their destination by both radialand tangential migration (Rakic, 1972; Anderson et al., 1997;Lavdas et al., 1999). The first postmitotic cells settle in theexternal field of the cortical anlage and form the so-called preplate(Rickmann and Wolff, 1981). When the CP appears, this early populationbecomes divided into two components, namely Cajal-Retzius cellsin the marginal zone (MZ) and subplate cells below the CP (Marín-Padilla,1971, 1972). Formation of the CP then proceeds by progressiveadjunction of new immigrant neurons after an "inside-out" gradient(Angevine and Sidman, 1961; Rakic, 1974). The extracellular proteinReelin (Reln), secreted by Cajal-Retzius cells, is criticallyinvolved in this process (D'Arcangelo et al., 1995, 1997; Lambertde Rouvroit and Goffinet, 1998); in the reeler mouse, in whichthe gene encoding Reln is defective, the preplate fails to splitinto MZ and subplate, and the normal migration gradient is inverted(Caviness, 1982; Goffinet, 1984; Sheppard and Pearlman, 1997).

Our previous work on rat cortical development suggested that this view may be an oversimplification in that the cellular compositionof the preplate is more complex than usually recognized (Meyeret al., 1998). A transient cell type in the MZ contributing earlyefferent projections was named "pioneer neuron" of the developingcortex. Pioneer neurons were born before most Reln-producing Cajal-Retziuscells, which are thought to represent the oldest neuron of thecortex (Marín-Padilla, 1998). Furthermore, Cajal-Retzius cellswere shown to have multiple origins. Although some were presentas early as E12, other similar neurons were added later, througha rudimentary subpial granular layer(SGL).

The events that control development of the embryonic human cortex are even less well known. In a previous paper (Meyer andGoffinet, 1998) we showed that the human SGL supplies the growingMZ with Reln-immunoreactive Cajal-Retzius-like neurons duringthe period of cortical plate migration, which complement early-bornCajal-Retzius cells. We focused on the period after the emergenceof the cortical plate and did not address the origin of humanpreplateneurons.

In the present work we describe the events that precede and accompany the initial formation of the human cortical plate. Byusing immunohistochemistry for Reln, calretinin (CR), and glutamicacid decarboxylase (GAD), we sought to define the origin of theearliest Reln-producing cells and to search for the possible existenceof a human homolog of the rat pioneerneurons.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Human embryonic brains were obtained after legal abortions, following national guidelines in Spain and Belgium and in accordwith the competent medical ethics committees in our institutions.In addition, fetal brains were obtained after spontaneous abortions,under the same ethicalguidelines.

We examined 10 embryonic and early fetal human brains. The embryonic material, 5-7 gestational weeks (GW) old, was classifiedon the basis of external morphology and brain features, accordingto the Carnegie stages (O'Rahilly and Müller, 1994). The ageof the fetuses was inferred from the gestational history, as indicatedby the obstetrician. One case of each of the following stageswas examined (approximate gestational age in brackets): 15 (4.5GW); 16 (5 GW); 16/17 (5.5 GW); 17 (6 GW); 17/18 (6 GW); 18 (6.5GW); 19 (6.5 GW); 20 (7 GW); 21 (7 GW); 22 (8 GW). The whole headsor, in the fetuses, the brains, were fixed in Bouin's fixative,embedded in paraffin, and cut in series of 10-µm-thick sections,in a coronal or parasagittal plane. Two cases (stages 17 and 21)were fixed in 4%paraformaldehyde.

For immunohistochemistry, sections were incubated in the primary antibodies overnight in a humid chamber. After rinsing, theywere incubated in the corresponding biotinylated secondary antibodies,rabbit anti-mouse IgG or goat anti-rabbit IgG (Dako, Glostrup,Denmark), diluted 1:200 in Tris-buffered saline (TBS), washed,and incubated in the ABC complex (Dako). Bound peroxidase wasrevealed using 0.05% 3, 3'diaminobenzidine tetrahydrochloride(DAB; Sigma, St. Louis, MO) 0.06% ammonium nickel (II) sulfate(Sigma), and 0.01% hydrogen peroxide in TBS. The sections weredehydrated, cleared, and mounted with Eukitt (O. Kindler GmbH,Freiburg, Germany). The primary antibodies were a polyclonal antibodyraised in rabbit against human CR (1:3000) (SWant, Bellinzona,Switzerland), a polyclonal antibody raised in rabbit against GAD65 and 67 (1:1000) (Chemicon, Temecula, CA), and a mouse monoclonalanti-reelin antibody 142 (de Bergeyck et al., 1998). Method specificitywas controlled by omitting the primaryantibodies.

Double-label immunocytochemistry was performed to visualize the association between Reln and CR, and Reln and GAD, in thesame section. After the first primary antiserum (anti-reelin 142diluted 1:500), sections were incubated in the corresponding anti-mousesecondary antibody and processed with DAB and ammonium nickelsulfate as described above, which yielded a black reaction product.After thorough rinses, the sections were then incubated overnightin the second primary antibody CR, 1:3000, or GAD, 1:1000. Thesecondary antibody was in this case the corresponding goat anti-rabbitIgG. After washing, the sections were immersed in 0.005% DAB with0.0001% in 0.05 M Tris buffer, pH 7.8; the reaction product appearedbrown.

Selected sections of the stage-19 case were microwaved for 1 min on full power in citrate buffer at pH 2.5 (Evers and Uylings,1994). This treatment enhanced Reln immunoreactivity without affectingthe staining pattern, although it slightly increased background(see Fig. 2, compare A-C, with microwave treatment, with D, E,withouttreatment).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Observations will be described by following the Carnegie stages as defined by O'Rahilly and Müller (1994), beginning withstage 16, corresponding to ~5 GW, up to stage 22 (~8GW).

For most authors, the term preplate implies the presence of an early external layer containing at least two cell populationsthat are subsequently split into MZ cells, usually defined asCajal-Retzius cells, and subplate neurons, by the first cohortsof the cortical plate (CP) (Rickmann and Wolff, 1981; Allendoerferand Shatz, 1994; Pearlman et al., 1998; Supèr et al., 1998 Marín-Padilla,1998). Accordingly, we use the term "marginal zone" (MZ) for thefirst stages of human corticogenesis, when the only differentiatedelements are Reln-immunoreactive (ir) neurons, and we reservethe term "preplate" for later stages when Reln-negative putativesubplate neurons haveappeared.

Stages 16-18, early marginal zone

The first Reln-expressing cells were observed at stage 16 (5 GW) as a few neurons scattered below the pial surface in thelateral aspect of the cortical wall corresponding to the presumptiveneocortex (Fig. 1A). They increased in density from stages 16to 17 (6 GW), and occasionally they were also observed withinthe VZ (Fig. 1B). At stage 17, they formed a continuous row ofnearly horizontal neurons in the narrow (10-15 µm width) MZ (Fig.1C). At stage 18 (6.5 GW), the MZ was wider (30-50 µm) and containedReln-ir neurons at different stages of differentiation and locatedat variable distances from the pial surface (Fig. 1D). The moremature-looking neurons were horizontally arranged and extendedprominent processes. Smaller rounded cells, apparently less mature,lay closer to the ventricular zone. At this stage, very few neuronsoccupied an immediate subpial position. At stages 17 and 18, thepacking density of Reln-ir neurons was higher rostrally (Fig.1E) than caudally (Fig. 1F). At these early stages, a few radiallyoriented columns of Reln-ir cells were present in the VZ (Fig.1E). CR and GAD were not yet expressed by neurons in the neocorticalanlage.

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Figure 1. Reelin in early marginal zone. A, Stage 16, 5 GW. The first Reln-ir neurons appear at the outer aspect of the prospective neocortical neuroepithelium, in a narrow cell-sparse MZ. In this and the following microphotographs, the dashed line marks the border of the MZ and VZ. Scale bar, 25 µm. B, Stage 16/17, 5.5 GW. The VZ occasionally contains weakly Reln-ir cells (arrowheads), which seem to ascend to the MZ. Scale bar, 25 µm. C, Stage 17, 5.5 GW. Reln-ir neurons in the MZ increase in number. Scale bar, 50 µm. D, Stage 18, 6.5 GW. In rostral cortical areas, Reln-ir neurons lie now at different distances from the pial surface. Scale bar, 50 µm. E, Stage 17/18, 6 GW. In addition to Reln-ir neurons in the MZ, a few weakly immunostained cells (arrowheads) are present in the VZ, arranged into columns. Scale bar, 50 µm. F, Same case as in E, at a more caudal level, where Reln-ir neurons in the MZ are less numerous. Note positive cells in the deep VZ. Scale bar, 25 µm.

Stage 19, preplate

At stage 19 (6.5 GW), CR-ir cells appeared for the first time in the MZ, which from this moment might be considered the preplate,and were particularly numerous at rostral levels (Fig. 2F,G).CR-ir cells in the superficial ventricular zone were continuouswith aggregates of similar CR-ir neurons in the preplate, someof which assumed a horizontal orientation. In a few places, CR-ircells were also observed deeper in the VZ (Fig. 2G). Reln wasexpressed by numerous neurons in the rostral preplate. Columnsof Reln-ir cells spanning almost the entire width of the neuroepitheliumwere particularly prominent in the rostral cortical wall (Fig.2A-E), where they were quite regularly spaced at intervals of~75-150 µm. Whereas Reln-immunoreactivity was weak in cells inthe lower tiers of the VZ (Fig. 2D,E), it increased as the cellsapproached the preplate (Fig. 2B,C). Reln-ir and CR-ir neuronslay intermixed in the preplate, without any apparent lamination.The preplate of the presumptive caudal neocortex was narrow andcontained only a few immature Reln- and CR-expressing neurons.In the relatively more mature lateral part of the cortical wall,the first GAD-ir neurons appeared in the IZ but not yet in thepreplate.

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Figure 2. Reelin- and calretinin-ir neurons in the human preplate at stage 19, 6.5 GW. A, Low-power view of the rostral neocortex, immunostained for Reln. Arrowheads point to aggregates of Reln-positive cells in the VZ that seem to ascend to the preplate. Dashed line indicates border between VZ and preplate. Asterisks mark three radial columns of Reln-ir neurons in the VZ. Scale bar, 100 µm. B, Higher-power view of radial columns of Reln-ir neurons in the VZ. Open arrowheads indicate the pial surface, at places obscured by connective tissue. Scale bar, 50 µm. C, Higher magnification of the cell column marked by an asterisk in B and C, showing clearly the Reln immunoreactivity, which increases in intensity from the VZ to the preplate. Scale bar, 25 µm. D, Two Reln-ir cell aggregates (arrowheads) in the upper VZ, in continuity with Reln-positive neurons in the preplate. Scale bar, 80 µm. E, A single column of weakly Reln-ir cells (arrowheads) spans almost the entire width of the VZ. Scale bar, 40 µm. F, At stage 19, calretinin-ir (CR) neurons appear for the first time in the prospective neocortex, marking the beginning of the preplate period. Arrowheads point to aggregates of CR-ir neurons in the preplate. Scale bar, 100 µm. G, Occasionally, CR-ir cells are present in the VZ. Scale bar, 50 µm.

Stage 20, the monolayer

Whereas at stage 19 the neocortical preplate was characterized by a diffuse and apparently random arrangement of CR-ir andReln-ir neurons, stage 20 (7 GW) marked the beginning of its compartmentalization.A loosely organized single layer of horizontally oriented CR-ircells, referred to below as the monolayer, appeared at an approximatedistance of 20-30 µm from the pial surface all over the corticalwall (Figs. 3A, 4A). The largest neurons (long diameter 10-15µm) had a bipolar shape; one of the processes often displayedthe fine caliber of an axon, whereas the other was thicker andpresumably represented a dendrite. A rather elaborate dendriticbranching pattern indicated advanced differentiation (Fig. 3B).In addition, smaller (7-10 µm) and more rounded, apparently moreimmature neurons contributed to the monolayer. At less maturedorsal and caudal levels, the monolayer was discontinuous, andCR-ir cells had a more irregular distribution. GAD staining revealedsimilar cells with a similar distribution (Fig. 4B). Althoughdouble-labeling GAD-CR could not be performed, the morphologyof the neurons and their distance from the pia suggested at leastpartial colocalization of both antigens in the neurons of themonolayer (Fig. 4, compare A and C with B and D). However, notall neurons were CR-ir or GAD-ir, suggesting the possibility ofyet other cell populations. Double-labeling experiments of CR-Relnand GAD-Reln showed that neurons in the monolayer did not expressreelin (Fig. 4A-D).

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Figure 3. Cell populations in preplate, pioneer plate, and cortical plate. A-D, Stage 20, 7 GW. A, A loosely organized layer of mostly horizontal calretinin (CR)-ir neurons, referred to as the monolayer (ML, between the two parallel lines), appears in the preplate, superficial to the intermediate zone (IZ). Scale bar, 40 µm. B, Large neurons in the monolayer are strongly CR-ir and display a differentiated dendritic branching pattern. Arrowhead points to a dendritic ramification. Scale bar, 35 µm. A and B are from the dorsolateral cortical wall. C, In the more mature ventrolateral cortex, other CR-ir neurons begin to assemble at the inner aspect of the monolayer. Scale bar, 40 µm. D, An adjacent section, immunostained for Reln, shows that the neurons in the monolayer (between the parallel lines) do not express Reln, but that Reln-ir neurons are confined to an immediate subpial compartment (open arrowheads mark the position of the pial surface). Scale bar, 40 µm. E-H, Stage 22, 8 GW. E-G, Adjacent sections of the dorsal neocortex, a level where the pioneer plate (PP) is just segregating, immunostained for GAD (E), Reln (F), and CR (G). E, Horizontal GAD-ir neurons (solid arrowheads) lie immediately above the PP, in the deep tiers of the marginal zone (MZ), whereas the Reln-ir cell layer (F) has a subpial position. G, Neurons in the PP are strongly CR-positive. Open arrows indicate a strongly CR-ir plexus just above the PP. H, CR-stained section in the ventrolateral neocortex, where the cortical plate (CP) has split the PP into a superficial (solid arrowheads) and a deep contingent. Deep pioneer neurons, presumably representing the subplate (SP), assume a pyramidal shape but display a more differentiated dendritic branching pattern than CP neurons. CR is now strongly expressed by cells in the subpial compartment. Scale bars (E-H): 50 µm.

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Figure 4. The segregation of the subpial Reln-compartment. A-D, Stage 20, 7 GW. A and C are double-labeled with Reln (black, asterisks) and CR (light brown); B and D show Reln (black, asterisks in B) and GAD (brown). Horizontal neurons in the monolayer express CR and/or GAD but are Reln-negative. From stage 20 onward, Reln is mostly expressed by subpial neurons and only occasionally by deeper ones. The apparently Reln-negative subpial neuron in B showed traces of immunoreactivity in another focal plane. The Reln-ir neuron in C (asterisk) is immediately attached to the pial surface. Scale bars: A, B, 50 µm; C, D, 25 µm. E, F, Stage 22, 8 GW. Double-immunostaining of Reln (black) and CR (light brown) demonstrates the segregation of subpial Reln compartment and cortical plate. Occasional horizontal neurons just above the cortical plate are Reln-negative. E is from the dorsolateral neocortex; F is from a slightly more ventral area. Scale bars: E, F, 50 µm.

With the appearance of the monolayer, Reln-ir cells shifted into a subpial position and became clearly segregated from thedeeper horizontal neurons (Figs. 3D, 4A-D). Only in the dorsaland caudal regions were reelin-ir neurons also located at deeperlevels of the preplate, although the more differentiated neuronsoccupied more superficial positions than smaller, more immaturecells that lay near the VZ. In the most mature part of the prospectiveneocortex, i.e., the lateral field facing the lateral ganglioniceminence, a new type of more rounded neurons, the pioneer cells,began to aggregate below the monolayer neurons (Figs. 3C, 4A).Pioneer neurons will be described in more detail below; at stage20, their descending axons were not easily identified .

Stages 21 and 22, pioneer plate and cortical plate

The most significant change at stages 21 and 22 (7-8 GW) was the emergence of the CP. This key event was accompanied by theappearance of new neuronal types and preceded by the formationof a transient cell condensation, the pioneer plate. The mostprominent cell type of the pioneer plate was a strongly CR-positivebut GAD- and Reln-negative neuron, the axon of which coursed intothe IZ and gave rise to early efferent connections of the cortex(Fig. 5G). Accordingly, we considered this cell type the pioneerprojection neuron of the human cortex. Although, as mentionedabove, the first pioneer cells were already observed in the mostdifferentiated ventrolateral cortex at stage 20, at that momenttheir axons were only short processes that did not exceed 20 µm.

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Figure 5. Partition of the pioneer plate and establishment of the cortical plate. A-F, Stage 21, 7 GW. A-C, Sections from the more immature dorsal cortex at stage 21, stained for CR (A), GAD (B), and Reln (C). A, The pioneer plate, populated with intensely CR-ir neurons, is thin and contains many superficial horizontal cells, which resemble those of the monolayer at stage 20. B, GAD-ir neurons are less abundant than CR-ir cells and concentrated at the level of the superficial pioneer plate. C, Reln-ir neurons are located immediately below the pia. D-F are from the relatively more mature lateral cortex, stained for CR (D), GAD (E), and Reln (F). D, The lateral pioneer plate consists of several rows of densely aggregated, intensely CR-positive neurons that lack a radial orientation. E, GAD-ir neurons are less numerous than those expressing CR and more abundant in the external aspect of the pioneer plate. F, Reln is expressed specifically by cells in the subpial compartment. G-J, Stage 22, 8 GW, immunostained for CR. There is a gradual splitting of the pioneer plate from the most dorsal (G) to intermediate (H, I) and more lateral (J) levels. G, A pioneer plate stage similar to that shown in D, with the difference that an incipient radial cell orientation is now evident, as well as the presence of a fiber tract (small arrows point to axons). H-J, At progressively more lateral levels, the intensely CR-positive pioneer neurons become more and more separated into a superficial population (arrowheads) and a deep, radially oriented population that presumably represents the subplate (SP). The cortical plate (CP) consists of initially moderately CR-positive and later CR-negative neurons that become inserted within the pioneer plate. All microphotographs were taken at the same magnification. Scale bar (shown in C): 25 µm. Case 21, showing less perfect tissue preservation, could have undergone more retraction during histological procedures.

The pioneer plate was prominent at stage 21, when large numbers of pioneer neurons settled at the inner aspect of the monolayer,which thus became less distinct. In the relatively more immaturedorsal and caudal regions of the cortical wall (Fig. 5A), thepioneer plate was formed by two or three cell rows that were continuouswith the horizontal cells of the monolayer, still present in themedial cortical wall. Horizontal cells were also observed in thesuperficial tier of the pioneer plate (Fig. 5A), whereas the pioneerneurons were more rounded. The pioneer plate gradually increasedin thickness in more lateral regions, where it comprised fourto seven cell rows (Fig. 5D). In the developmentally more advancedventrolateral cortex, the pioneer plate became invaded by anotherpopulation of GAD-negative, CR-negative, or weakly positive neurons.This step, the partition of the pioneer plate by the first cohortsof the cortical plate, was initiated at stage 21 and continuedinto stage22.

At stage 22 (8 GW), the pioneer plate was recognizable in the dorsal cortex as a compact aggregate of intensely CR-positiveneurons (Figs. 3G, 5G), which resembled the lateral pioneer plateof stage 21 but in addition displayed signs of a more advancedcytological differentiation, such as a slightly more verticalorientation in the deeper tiers and a more triangular soma shapeand emission of oblique dendrites in the upper tier (Fig. 5G,H,arrowheads). The descending axons were now clearly visible inthe IZ as a CR-ir fiber tract (Fig. 5G, small arrows). The radialdisposition of the deep pioneer plate component was progressivelymore accentuated in intermediate and lateral cortical areas, wherethey assumed a pyramidal shape with a prominent apical dendrite(Fig. 5H-J). Concurrently, the deep and superficial contingentsof the pioneer plate became more and more separated through theinterposition of another population of initially moderately CR-positive(Fig. 5H,I) and later CR-negative neurons (Fig. 5J), which weinterpreted as the first cohorts of the CP. The superficial pioneercells appeared increasingly spaced from medial to lateral (compareFig. 5H-J with Fig. 4H, from the most differentiated ventrolaterallevel of the same case), indicating that no further members wereadded to this early cellpopulation.

The nonradial condensation of pioneer cells into a pioneer plate might be interpreted as a preliminary step before the formationof the CP. The radially arranged CR-negative neurons would thencorrespond to the first representatives of the cortical plateproper, which divide the pioneer plate into a superficial anda deep part. The deep pioneer plate component would representthe subplate (Fig. 5I,J, SP), or presubplate following the terminologyof Kostovic and Rakic (1990).

During the process of pioneer plate formation, we consistently observed horizontally elongate or rounded GAD-positive neuronsconcentrated mostly at the external border of the pioneer plate(Fig. 5B,E); they resembled the neurons of the former monolayer.In the more differentiated stage 22, GAD-ir neurons extended longhorizontal processes along the upper border of the pioneer plate(Fig. 3E). Comparison with adjacent sections stained for Reln(Fig. 3F) and CR (Fig. 3G) showed that the GAD-expressing neuronslay below the Reln-positive subpial compartment, at a level immediatelyabove the pioneer plate, filled with a dense CR-ir plexus (Fig.3G, open arrows).

At stages 21 and 22, Reln-ir neurons remained arrayed into a single subpial row, separated from pioneer and cortical platesby a cell-sparse marginal zone ~15 µm wide (Figs. 3F, 4E,F, 5C,F,).Only occasionally did we observe a small Reln-ir neuron deeperin the MZ, most commonly in the less mature corticalregions.

With increasing differentiation of the CP, CR expression became more prominent in subpial Reln-ir neurons (Fig. 3H). The furtherdevelopment of Cajal-Retzius cells/Reln-expressing neurons ofthe human MZ has been described previously (Meyer and Gonzalez-Hernandez,1993; Meyer and Goffinet, 1998) and will thus not be consideredhere.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The mechanisms that control early cortical development remain poorly understood. A general consensus holds that an early cellularcompartment, the preplate, is split into the MZ containing Cajal-Retziuscells and subplate (Marín-Padilla, 1971, 1972). Numerous birthdatingexperiments confirmed the partition of early-born preplate neurons(Raedler and Raedler, 1978; Kostovic and Rakic, 1980; Luskin andShatz, 1985; Chun and Shatz, 1989; Wood et al., 1992). Thus far,however, the cellular identity of the preplate components hasnot been fully defined in humancortex.

Our data show that the initial formation of the human cortex is a complex process that involves several neuronal populations.Some of these cell classes have not been described previously,possibly because the rodent and carnivore cortices on which thecurrently prevailing concepts are founded do not provide the necessarytemporospatial resolution. We suggest the following sequence ofevents (Fig. 6). The first step is the appearance of Reln-expressingneurons along the outer aspect of the neuroepithelium and theestablishment of a cell-sparse MZ (stages 16-18). This is followedby the formation of a monolayer of horizontal, CR- and/or GAD-positiveneurons, concurrent with the segregation of a Reln-positive subpialcell compartment (stage 20). A third event is the condensationof a "pioneer plate" populated by CR-positive, GAD-negative pioneercells (stage 21). The fourth stage corresponds to the appearanceof the CP proper within the framework of the pioneer plate (stages21-22). Early cortical development is thus characterized by continuouschanges involving neuronal populations that cannot be simply definedin terms of Cajal-Retzius cells and subplate.

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Figure 6. Diagrammatic representation of the developmental events proposed in this study, from stage 16 to stage 22. All figures were drawn at the same magnification with the aid of a camera lucida. Blue, Reln; light green, early CR-ir neurons in the monolayer; red, GAD; dark green, pioneer cells; yellow, cortical-plate neurons. The first Reln-ir neurons appear at stage 16, in a narrow MZ, and increase in number from stages 17 to 19. The first CR-ir neurons appear at stage 19 in what could now be called the preplate. Together with GAD-ir neurons, which appear at stage 20, they form the monolayer within the preplate. Concurrently, Reln-ir neurons settle in the subpial compartment. At stage 21, the pioneer plate aggregates below the monolayer and sends the first corticofugal fibers. The pioneer plate is split apart into a minor superficial component and a large deep component (the subplate) through the first cohorts of the cortical plate, at stages 21 and 22. In this scheme, possible colocalizations have not been taken into account. IZ, Intermediate zone; MZ, marginal zone; PP, preplate; VZ, ventricular zone.

Reelin-expressing cells

Reln-expressing neurons are the only postmitotic cell population in the neocortical anlage during stages 16-18; they increasein number while the cortical wall grows. The presence of radialcolumns of Reln-ir neurons traversing the ventricular zone suggestsa local origin, as described for Reln-producing cells in the mouse(Alcántara et al., 1998). However, local origin and radial migrationdo not exclude the possibility that Reln-ir neurons move tangentiallyin MZ and preplate. Indeed, their monopolar morphology, horizontalorientation, and prominent leading processes are strongly reminiscentof tangentially migrating neurons (Austin and Cepko, 1990; O'Rourkeet al., 1992, 1995). In addition, we cannot rule out that someReln-ir neurons invade the preplate tangentially from noncorticalsources such as the medial ganglionic eminence, which is knownto produce Reln-ir Cajal-Retzius cells in the rodent (Lavdas etal., 1999). At later stages, after the emergence of the CP, furtherpopulations of Reln-ir neurons are added to the MZ by longer distancetangential migration from the periolfactory basal forebrain throughthe SGL (Meyer and Goffinet, 1998; Meyer and Wahle, 1999). Duringa protracted period, from 5 GW to midgestation, Reln-ir neuronswith different morphological and neurochemical profiles are thuscontinuously delivered into preplate and MZ through both radialand tangential migration. As a corollary, the definition of Reln-producingCajal-Retzius cells as the earliest-born cell class of the cerebralcortex ismisleading.

Horizontal monolayer cells

At stages 19/20, around 7 GW, a new cell type appears as a CR- and/or GAD-positive, but Reln-negative neuron disposed horizontallyin a single layer. Although this layer is sometimes discontinuousor the cells may be aligned in two rows, the overall impressionis clearly that of a single, loosely organized layer in whichthe dominant cell type is the horizontal neuron. The colocalizationof CR and GAD in these neurons needs to be explored further, althoughsimilar morphology and location suggest substantial overlap. Inparallel to the formation of the monolayer, Reln-ir elements shiftinto a subpial position and are no longer seen in intermediatezone and lowerpreplate.

The horizontal CR/GAD-ir neurons may define a new step in cortical development. They appear before the pioneer cells and maybe important for the unfolding of subsequent events. Preliminaryevidence (G. Meyer, unpublished observations) shows that theyalso express the disabled-1 (Dab1) protein and are thus presumablyresponsive to the Reln signal (Cooper and Howell, 1999). Thisdifferential expression of Reln and Dab1 may explain why Reln-irneurons are segregated from the monolayer. The GAD-ir neuronsin the monolayer are possibly identical with the GABA-positivecells described by Zecevic and Milosevic (1997). We show herethat they are Reln-negative, although their morphology stronglyresembles that of Cajal-Retzius cells of classical Golgi studies.However, some GAD-ir neurons in the rodent preplate may also expressReln (Meyer et al., 1998; Lavdas et al., 1999) and can thus beconsidered a subpopulation of the Cajal-Retzius cell family. Wecarried out double labeling to substantiate the segregation ofmonolayer and Reln-positive subpial compartment; however, ourtechnique did not allow us to reliably assess colocalization ofGAD and Reln, or CR and Reln in the same cell, and further studiesare needed to sort out the neurochemical profiles of preplateneurons. Similarly, the question of the origin of these GAD-irneurons cannot be addressed in our material. They may have a localorigin, or they may migrate from ganglionic eminences, as do GABAergicinterneurons and some Cajal-Retzius cells in rodents (Andersonet al., 1997; Tamamaki et al., 1997; Lavdas et al., 1999).

Our results suggest that the GAD-ir monolayer neurons remain in a superficial position relative to pioneer plate and corticalplate. They may form a barrier between MZ and CP, and they mayplay a role at the end of the migratory pathway, when CP neuronsdetach from their radial glia guide on reaching the upper borderof the CP. Certainly this cell type deserves furthercharacterization.

Pioneer cells

Stage 21 is characterized by the aggregation of rounded neurons that are CR-ir but GAD- and Reln-negative and thus differentfrom the horizontal monolayer neurons. We name these cells "pioneercells" because they emit descending axons that course into theintermediate zone. The initial condensation of pioneer neuronshas no recognizable radial organization, which sets it apart fromthe radially organized cortical plate. The superficial pioneerneurons may be homologous to the transient pioneer neurons describedin the rat MZ (Meyer et al., 1998), whereas the deep componentwould correspond to the rodent subplate (Bayer and Altman, 1990;de Carlos and O'Leary, 1992) or human presubplate (Kostovic andRakic, 1990). Rat pioneer neurons both in MZ and subplate contributethe first efferent fibers to the internal capsule (de Carlos andO'Leary, 1992; Meyer et al., 1998; Molnár et al., 1998). Thereare important differences, however, between rat and human pioneerneurons. First, in rat, MZ-pioneer neurons are born before mostReln-ir Cajal-Retzius cells (Meyer et al., 1998), whereas in manthey appear relatively late, almost concurrently with corticalplate neurons. As described above, the first stages of human preplateare dominated by Reln-ir neurons, not by Reln-negative pioneerneurons. We cannot rule out the possibility that we failed todetect early human pioneer neurons; however, in cresyl violet-stainedsections, we did not observe any large rounded cell body beforestages 20/21. A second difference becomes evident after the insertionof the first cortical plate contingent into the pioneer plate:the proportion of pioneer cells remaining at the upper borderof the CP, relative to those that settle in the subplate, is lowerin man than in rat. In man, the pioneer plate is thus dividedinto a minor superficial cell population, and a larger subplatecomponent, by the first migratory cohort of the CP proper. Itis worth pointing out, however, that the development of the humansubplate is a protracted process that extends over several months(Kostovic and Rakic, 1990). The subplate, or presubplate describedhere, may be the earliest representative of a larger neuronalnetwork.

Pioneer plate partition and CP formation

During the initial appearance of the CP, Reln-positive cells remain in a strictly subpial location and are thus not physicallyimplicated in preplate partition. It is the insertion of the CPwithin the framework of the pioneer neurons that results in thepartition of the pioneer plate. Whereas CP neurons are characterizedby their radial arrangement, with the appearance of the CP thesubplate neurons also assume a pyramidal shape and radial orientation.However, the differentiated processes of subplate neurons, usuallyseveral basal dendrites and a single apical dendrite, indicatea high degree of maturity, in contrast with the immature morphologyand tight compaction of CP neurons. This is in keeping with theconcept of the subplate as an early compartment involved in pathfindingof pioneer efferent and afferent fibers (Allendoerfer and Shatz,1994). The pioneer neurons in the deep MZ become increasinglyspaced as development proceeds, which may be caused by dilutionor cell death, as in the rat where they disappear before birth(Meyer et al., 1998).

The developmental sequence outlined here implies that complex cellular events take place during early corticogenesis. Theongoing characterization of mouse mutations that perturb earlycorticogenesis in specific and diverse ways shows that a wholeintegrated molecular network remains to be sorted out. The reeler-likephenotype is generated by mutations not only of the reeler genebut also of the disabled 1-gene (Howell et al., 1997; Sheldonet al., 1997; Ware et al., 1997; Rice et al., 1998) and in micethat are doubly deficient for the lipoprotein receptors VLDLRand ApoER2 (Trommsdorff et al., 1999), suggesting that these genesform part of a "reelin-signaling pathway" (Bar and Goffinet, 1999;Cooper and Howell, 1999). The cellular counterpart of this molecularpathway is presumably more intricate than the conventional preplatescheme of Cajal-Retzius and subplate neurons. Our study providesevidence that the Reln-expressing neurons in the MZ, usually identifiedas Cajal-Retzius cells, are not directly involved in preplatepartition. Similarly, the role of the monolayer neurons, perhapsthe first cellular target in the Reln-signaling pathway, shouldbe examined further in animal models. Presumably, the situationin man is even more complex, and some malformations may resultfrom mutations in genes that control specific events in corticogenesis.The present work should be considered a first attempt to dealwith thiscomplexity.

  FOOTNOTES

Received Aug. 9, 1999; revised Nov. 30, 1999; accepted Dec. 2, 1999.

G.M. is supported by Grant PB 97-0582-CO2-02, Ministerio de Educación y Cultura, Spain. Work in the laboratory of A.M.G.is supported by Grants Action de Recherches Concertées 186, Fondsde la Recherche Scientifique Médicale 3. 4544.95, and FondationMédicale Reine Elisabeth, all from Belgium. We thank VictoriaBello for technical assistance and José Antonio Ayala for excellentphotographic work. We are grateful to Paula Plaza for help withFigure 6.
Correspondence should be addressed to Gundela Meyer, Department of Anatomy, Faculty of Medicine, University La Laguna, 38071La Laguna/Tenerife, Spain. E-mail: gmeyer{at}ull.es.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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