Role of DE-Cadherin in Neuroblast Proliferation, Neural Morphogenesis, and Axon Tract Formation in Drosophila Larval Brain Development

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The Journal of Neuroscience, April 15, 2003, 23(8):3325

Role of DE-Cadherin in Neuroblast Proliferation, Neural Morphogenesis, and Axon Tract Formation in Drosophila Larval Brain Development
Karin Dumstrei, Fay Wang, and Volker Hartenstein
Department of Molecular Cell and Developmental Biology, University of California Los Angeles, Los Angeles, California 90095

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

In the wild-type brain, the Drosophila classic cadherin DE-cadherin is expressed globally by postembryonic neuroblasts andtheir lineages ("secondary lineages"), as well as glial cells.To address the role of DE-cadherin in the larval brain, we tookadvantage of the dominant-negative DE-cad^ex construct, the expression of which was directed to neurons, glialcells, or both. Global expression of DE-cad^ex driven by a heat pulse during the early second instar resultedin a severe phenotype that included deficits in neural proliferation.Neuroblasts appeared in approximately normal numbers but had highlyreduced mitotic activity. When the DE-cad^ex construct was driven by the glial-specific driver gcm-Gal4, theeffect of DE-cad^ex on neuroblast proliferation could be replicated, which indicatesthat DE-cadherin acts in glial cells to promote proliferationof neuroblasts. Expression of DE-cad^ex in neurons, cortex glia, or both results in abnormalities incortex layering and in trajectories of secondary axons. In thewild-type brain, neuroblasts and neurons generated at differenttime points are arranged concentrically around the neuropile,with the DE-cadherin-positive neuroblasts and young secondaryneurons at the surface, followed by older secondary neurons andprimary neurons. Axons of secondary lineages follow a straightradial course toward the neuropile. Processes of glial cells locatedin the cortex form a scaffold, called trophospongium, that enwrapsneuroblasts and neurons. Expression of DE-cad^ex in neurons, cortex glia, or both disrupted the regular placementof neuroblasts and secondary neurons and resulted in abnormaltrajectories of cell body fiber tracts. We conclude that DE-cadherinplays a pivotal role in larval brain proliferation, brain cortexmorphogenesis, and axongrowth.

Key words: DE-cadherin; larva; brain; neuroblast; morphogenesis; axon

  Introduction

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The cadherin superfamily of cell adhesion molecules plays an essential role during multiple steps of neural development. Membersof this large family include the classic cadherins, which arelinked to the actin cytoskeleton via binding to the proteins ofthe catenin family, and nonclassic cadherins that lack this link.Both classic and nonclassic cadherins preferentially homodimerize,which is important for mediation of cell-cell sorting in tissuesthat express differential patterns of cadherins (for review, seeTepass et al., 2000). In vertebrates, cadherins are widely expressedin the nervous system in distinct patterns; this finding, in conjunctionwith numerous experimental studies, corroborates the importanceof cadherins in nervous system regionalization, axon tract formation,and synaptic connectivity (for review, see Redies, 2000).

The study of the role of cadherins in Drosophila neurogenesis has been limited so far to the Drosophila classic cadherin DN-cadherin.DN-cadherin is expressed in the embryonic mesoderm and later byall neurons and their axons (Iwai et al., 1997). Loss of DN-cadherinin the embryo results in subtle defects in axon fasciculationand growth cone navigation. During larval visual system development,loss of DN-cadherin in the R7 photoreceptor leads to defects intarget specificity (Lee et al., 2001). In addition to DN-cadherin,Drosophila embryos express DE-cadherin. DE-cadherin, which isexpressed in all epithelia from the blastoderm stage onward, isdownregulated in cells that lose their epithelial characteristics,including the mesoderm, neuroblasts, and their neurons (Tepasset al., 1996; Uemura et al., 1996). Loss-of-function analysisof DE-cadherin in the embryo and during oogenesis has demonstratedits requirement for the formation and maintenance of epithelialcells and for cell-cell sorting processes (Godt and Tepass, 1998).

Recently, we have shown that during larval neurogenesis, DE-cadherin is turned on in postembryonic neuroblasts and their progeny(secondary neurons) in a dynamic pattern (Dumstrei et al., 2003).In addition, neuropile and surface glia express DE-cadherin ata high level. This global expression prompted us to speculatethat DE-cadherin-mediated adhesion between glial cells, neuroblasts,and neurons may be essential for larval brain morphogenesis. TheDrosophila brain originates in the early embryo with the delaminationand subsequent proliferation of a population of neuroblasts thatgenerate, in a stem cell-like manner, a fixed set of so-calledprimary glial and neuronal lineages. After a phase of mitotic"dormancy" that lasts from late embryogenesis to the end of thefirst larval instar, neuroblasts become active again and initiatea second wave of neural proliferation that gives rise to secondary(larval and pupal) lineages (Truman and Bate, 1988; Ito and Hotta,1992). The pattern of neuroblast proliferation and neural differentiationgenerates a concentrically organized ganglionic brain, comprisinga central neuropile formed by neuronal processes and synapses,surrounded by an outer cortex of neuronal and glial cell bodies.Neuroblasts and secondary neurons form the outer realm of thecortex. Secondary neurons are delayed in regard to morphologicaland functional differentiation (Truman, 1990). They form axonalprocesses (cell body fibers) (Strausfeld, 1976; Dumstrei et al.,2003), which penetrate the cortex and, in most cases, halt atthe cortex-neuropile border. During metamorphosis, primary andsecondary neurons become integrated into the adult neuropile (Trumanet al., 1994). Glial cells form a sheath-like covering of thelarval brain as a whole (surface glia), of individual neuronallineages or parts thereof (cortex glia), and of the neuropile(neuropile glia) (Hartenstein et al., 1998).

Given its widespread expression in neuroblasts, secondary neurons, and glial cells, it stands to reason that DE-cadherin isinvolved in multiple steps of postembryonic neurogenesis. In particular,interactions between glial cells and neurons, shown to be crucialin neural proliferation, axonogenesis, and connectivity in vertebrates(for review, see Lemke, 2001), could be controlled by DE-cadherin-mediatedadhesion. In Drosophila, surface glial cells appear to be involvedin the onset and rate of neuroblast proliferation (Ebens et al.,1993). The glia of the Drosophila optic lobe play a crucial rolein directing the connections between retinal axons and their centraltargets (Poeck et al., 2001). Other functions, including controlof placement of neurons within the cortex, trajectory of proximalaxon tracts, and ordered entry of these tracts into the neuropile,are to beexpected.

In the present study, we used a dominant-negative construct of DE-cadherin, DE-cad^ex (F. Wang, K. Dumstrei, T. Haag, and V. Hartenstein, unpublishedobservations), to investigate its function during larval neurogenesis.We show that ubiquitous expression of this construct leads toreduced neuronal proliferation that results in the absence ofmany neurons and their axon tracts. This phenotype is likely attributableto glial cell defects, because it can be phenocopied when expressingDE-cad^ex in the glial cells alone. We further confirm the hypothesis thatexpression of DE-cad^ex in the neuronal cells results in loss of normal neuronal cellbody placement in the cortex of the larval brain and irregularitiesin their axon projections through the cortex. We discuss the implicationsof DE-cadherin-dependent glia-neuronal cell interactions, as wellas the role of cell adhesion molecules in cell sorting duringneurogenesis.

  Materials and Methods

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Immunohistochemistry. An antibody that recognizes bromodeoxyuridine (BrdU; Becton Dickinson, Mountain View, CA) was used ata dilution of 1:40. Anti- $beta$ -galactosidase antibody (Promega, Madison,WI) was used at a dilution of 1:100. An antibody against castorwas used at a dilution of 1:500 (Kambadur et al., 1998; kindlyprovided by Dr. W. Odenwald). A monoclonal antibody against theFasII protein was used at a dilution of 1:50 (Grenningloh et al.,1991; kindly provided by Dr. C. Goodman). An antibody againstDE-cadherin was used at a dilution of 1:200 (Dumstrei et al.,2003). Anti-syntaxin antibody that labels the neuropile was usedat a dilution of 1:10 (Fujita et al., 1982; obtained from theDevelopmental Studies Hybridoma Bank maintained by the Departmentof Pharmacology and Molecular Sciences, Johns Hopkins UniversitySchool of Medicine, Baltimore, MD). Anti-Repo antibody, whichlabels all glial cells, was used at a dilution of 1:1000 (Campbellet al., 1994; kindly provided by Dr. A. Tomlinson). Secondaryantibodies, which were Cy3-conjugated anti-rat Ig and anti-rabbitIg (Jackson ImmunoResearch, West Grove, PA) and FITC-conjugatedanti-mouse Ig (Jackson ImmunoResearch), were used at a 1:100 dilution.For antibody labeling, standard procedures were followed (Ashburner,1989).

Fly stocks. Oregon R flies were used as the wild-type stock. The following fly lines were used: UAS-DE-cad^ex, which carries two copies of the DE-cad^ex construct on the X chromosome (Wang, Dumstrei, Haag, and Hartenstein,unpublished observations); actin "cdc2"-Gal4 (Ito et al., 1997;kindly provided by Dr. J. Lengyel); hs-FLP;UAS-green fluorescentprotein (GFP) (Ito et al., 1997; kindly provided by Dr. J. Lengyel);hs-Gal4, Nrv2-Gal4;UAS-GFP (Sun et al., 1998); gcm-Gal4 (kindlyprovided by Dr. L. Zipursky); and elav-Gal4 (available from theBloomington Stock Center). Flies were grown under standard conditionsat room temperature or at 25°C. Egg collections were done on yeastedapple juice agar plates. Hatching larvae were transferred to Petridishes filled with standard fly food. Larvae were collected atdesired time points, and brains were dissected in PEMS (0.1 MPIPES, 2 mM MgSO₄, and 1 mM EGTA, pH 7.0)-buffered 4% formaldehydefor 20min.

GFP clones. The hs-FLP;UAS-GFP stock was crossed with the actin "cdc2"-Gal4 line. Progeny were raised at 25°C until the firstinstar larval stage, heat-pulsed at 37°C for 5 min, and placedback at 25°C. Wandering third instar larvae were dissected, fixed,and stained with either anti-DE-cadherin or anti-syntaxinantibodies.

BrdU incorporation. BrdU was dissolved in 40% ethanol (1 mg/100 µl) and mixed with fly medium to a final concentration of1 mg/ml. Larvae were placed in vials with BrdU-containing foodfor 5 hr, at which point the brains were either dissected andfixed immediately in 4% formaldehyde or placed in normal fly mediumuntil they reached the desired stage. After dissection and fixationfor 20 min, the brains were washed three times for 15 min eachin PBS and incubated in 2 M HCl for 45 min to denature BrdU-labeledDNA. The brains were washed three times for 15 min each and stainedwith antibody according to standard procedures (Ashburner, 1989).

To estimate the number of dividing cells in the larval brains (see histogram in Fig. 4), BrdU-positive cells were countedfrom confocal sections that were taken 10 µm apart, with the seriesstarting from the anterior section and moving posteriorly. FiveUAS-DE-cad^ex brains were counted as controls. Six gcm-Gal4;UAS-DE-cad^ex brains were counted as experimental samples. The average numberof BrdU-labeled cells per brain was calculated after the sampleswith the highest and lowest number of BrdU-labeled cells wereremoved, which left three samples for the control and four forthe experimentalsamples.

Acridine orange staining of larval brains. UAS-DE-Cad^ex16;hs-gal4 and wild-type specimens were collected as embryos for 8 hr at25°C and aged to the early second larval instar (~48 hr aftereggs were laid). After a 10 hr heat shock, larvae were transferredback to the 25°C incubator and aged until the mid third instar(~16 hr after heat shock). At that time, larval brains were dissectedin Ringer's solution and stained with acridine orange (Sigma,St. Louis, MO; 1.6 × 10⁶ M in Ringer's solution) for 5 min in the dark under gentle shaking.The brains were washed in Ringer's solution for 10 min and mountedon slides with spacers. Confocal images were taken immediatelyafter thestaining.

Confocal microscopy and three-dimensional digital models. Confocal images were taken on an MRC 1024ES microscope (Bio-Rad,Hercules, CA) with Bio-Rad Lasersharp version 3.2 software. Three-dimensionaldigital models were prepared as described by Nassif et al. (1998).

  Results

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Cellular architecture of the larval brain

The larval brain is organized into concentric layers, with a central neuropile formed by axons, the cell bodies of which formthe cortex that surrounds the neuropile (Fig. 1A). During earlylarval stages, only neurons born during the embryonic period (primaryneurons) are present. Toward the end of the first larval instar,neuroblasts located at the surface of the cortex become activeand divide with a vertically oriented spindle to produce ganglionmother cells. Ganglion mother cells undergo one more divisionto form larval (secondary) neurons and glial cells. These secondarycells form a layer surrounding the primary neurons. Within thesecondary neuronal layer, position is also correlated to timeof birth, with young neurons situated superficially and old neuronssituated deeply (Fig. 1C,D). Using the flippase/flippase recombinationtarget (FLP/FRT) system to mark cell lineages, individual clonesof secondary neurons, and their neurites were labeled (Fig. 1B).Neurites emanating from neurons belonging to one lineage forma coherent bundle, the cell body fiber tract (CBT) (Strausfeld,1976; Dumstrei et al., 2003). CBTs penetrate the cortex in a straightradial trajectory. Many tracts stop at the neuropile-cortex boundaryand do not appear to enter the neuropile during the larval period.Other CBTs enter the neuropile and navigate around the compartmentsof the neuropile without forming any arborizations that interminglewith the neuropile formed by primary neurons (Fig. 1B).

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Figure 1. Cellular architecture of the larval brain. A, Schematic cross section of a third instar larval brain. Cells shaded in red are neurons born during the larval period [secondary neurons (sn)], neuroblasts (nb), and their axon tracts (cbt). Cells shaded in gray are embryonically born neurons [primary neurons (pn)] and the central neuropile (np) formed by their axon tracts. The laterally located optic lobe (ol) is also colored in different shades of gray. Cells in green represent the glial cells. Glial cells surrounding the surface of the brain are referred to as surface glia (sg), whereas neuropile glia (ng) surround the neuropile. Cortex glia (cg) surround clusters of neuronal cells. B, Confocal cross section of third instar brain labeled with anti-syntaxin (red, neuropile). Section contains three GFP-positive clones, each consisting of a neuroblast and its progeny. Clones were induced during late first instar. The arrowhead shows the axon tract entering the neuropile, whereas the arrow points to the axon tract that stops at the neuropile-cortex boundary. co, Cortex. C, D, Confocal cross sections of early third instar brains labeled with anti-DE-cadherin (red) and anti-BrdU (green). In C, larva was fed BrdU for 5 hr and fixed immediately. In D, a 24 hr period separated the BrdU pulse and fixation. Note the superficial location of BrdU-positive neural cells in C and the deep location in D. E, Confocal cross section of third instar brain labeled with anti-Repo antibody to label nuclei of surface glia (sg), cortex glia (cg), and neuropile glia (ng). F, Confocal cross section of third instar brain in Nrv-2-Gal4;UAS-GFP labels neuropile glia (ng) and cortex glia (cg). G, GFP-positive cortex glia clone, induced during the late first instar and fixed in the late third instar. H, Schematic cross section of brain cortex (cx) at different larval stages, illustrating formation of the trophospongium. Stages are as follows: a, first instar; b, second instar; c, early third instar; d, late third instar. Cortex glial cells (cg) are in green, neuroblasts (nb) in purple, secondary neurons (sn) in shades of red, and primary neurons (pn) in gray. Numbers 1-4 indicate birth order of secondary neurons (1, early; 4, late). White arrows in F-H illustrate the larger trophospongium chambers located superficially in the cortex, whereas white arrowheads show the deeper small chambers, which appear to include individual neurons. Black arrows in H, c, point at nascent glial septum.

Three different types of glial cells (surface, cortex, and neuropile glia) can be visualized with an antibody against thehomeobox gene Repo, which is expressed in all glial lineages froman early stage onward (Campbell et al., 1994) (Fig. 1E). WhereasRepo is a nuclear antigen, glia-directed expression of GFP bydriver lines such as gcm-Gal4 (Booth et al., 2000) and Nrv2-Gal4(Sun et al., 1998), in combination with FRT/FLP-induced labeledclones, permit one to visualize the outline of individual glialcells at different stages and thereby follow the morphogenesisof the various types of glial cells. This approach reveals impressivelythe complex glial "trophospongium" (Hoyle, 1986) in the larvalbrain (Fig. 1F-H). The trophospongium is a sponge-like matrixof cortex glial processes that arise in the late embryo and growby both cell division (cortex glia clones contain six to eightcells 48 hr after clone induction) and cell size increase. Growthof the trophospongium and neuroblast proliferation appear to becoordinated in a complex manner. Thus, close to the brain surface,individual chambers of the trophospongium are large, containinga neuroblast and 15-20 neurons (Fig. 1F-H, arrow). It is possiblethat each superficial trophospongium chamber corresponds to onesecondary lineage, such that the neurons formed by one neuroblastover a certain period are "received" into one chamber, therebyisolating them from other lineages. At deeper levels, chambersbecome smaller, in many cases taking up no more than a singleneuron (Fig. 1G,H, arrowhead). This implies that there is a dynamicrearrangement of glia processes at the transition zone from largechambers to smallchambers.

DE-cadherin expression in the larval brain

The expression of DE-cadherin was monitored with a polyclonal antibody and a P lacZ insertion into the shg gene, shg^P34-1 (Tepass et al., 1996). In the embryo, DE-cadherin is expressedin all epithelial cells and is downregulated as cells undergoepithelial to mesenchymal transition. In that way, DE-cadherinis lost in neuroblasts and their progeny but is expressed in glialcells. By contrast, in the larval brain, DE-cadherin is also expressedin most neuroblasts and secondary neurons, in addition to glialcells and the cerebral tracheae that grow into the brain (Fig.2A-C). Expression in neuroblasts begins as these cells becomemitotically active and persists throughout larval life. Both DE-cadherinRNA (data not shown) and protein are still present in ganglionmother cells and postmitotic neurons located superficially aroundthe neuroblasts. Expression is downregulated after a certain interval,because deeply located secondary neurons are no longer labeledby DE-cadherin antibody or probe. This can be observed in GFP-positiveclones, induced during the early second instar and fixed duringthe mid third instar, double-labeled with DE-cadherin antibody(Fig. 2D,E). These clones contain a neuroblast and several cellsin close proximity labeled with both GFP and anti-DE-cadherin,whereas deep neurons only express GFP. The transient DE-cadherinexpression is also demonstrated by labeling dividing neuroblastswith BrdU during the second instar followed by fixing and stainingthe brains for DE-cadherin expression after 2 or 36 hr duringthe mid third instar. In the first case, BrdU-positive cells overlapwith DE-cadherin expression in newly born neurons (Fig. 2F); inthe latter case, BrdU-positive neurons born during the secondinstar have moved deep in the cortex and do not express DE-cadherin(Fig. 2G).

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Figure 2. DE-cadherin expression in the larval brain. All panels show confocal sections of third instar brains. A, Expression of FasII (green) and DE-cadherin (red). B, Expression of FasII (green) and $beta$ -galactosidase (red) driven by a DE-cadherin enhancer trap line (shg^p341). FasII is expressed in known landmark tracts in the larval brain neuropile (np). DE-cadherin (A) or $beta$ -galactosidase (B) activity is seen in the neuroblasts (nb) and those secondary neurons (sn) that are close to the neuroblasts. C, DE-cadherin expression in the surface glia (sg) and neuropile glia (ng). D, Two GFP-positive clones of neuroblasts and their progeny, induced during the late first instar, in brain labeled with anti DE-cadherin. E, High magnification of one of the clones shown in D. The neuroblast (nb) and cells in its proximity appear yellow because of expression of both GFP and DE-cadherin, whereas cells farther away from the neuroblast are labeled with GFP alone, which indicates that these cells no longer express DE-cadherin. F, G, Close-up views of parts of cross sections of early third instar brains labeled with anti-DE-cadherin (red) and anti-BrdU (green). In F, larva was fed BrdU for 5 hr and fixed immediately. In D, a 24 hr period separated the BrdU pulse and fixation. Note that BrdU label is found in DE-cadherin-positive superficial cells in F and deep in DE-cadherin expressing cells in G. co, Cortex; ol, optic lobe.

DE-cadherin is required for postembryonic neural proliferation and differentiation

The role of DE-cadherin during larval brain development was addressed with the dominant-negative construct UAS-DE-cad^ex. This construct contains the extracellular and transmembraneregions but lacks the cytoplasmic domain. The latter domain isrequired for binding to the catenins, which link the classic cadherinsto the actin cytoskeleton, and is required for the adhesive functionsof classic cadherins. Ectopic expression of this construct inthe embryo with daughterless Gal4 results in a DE-cadherin loss-of-functionphenotype. Furthermore, expression of DE-cad^ex in an shg null background does not lead to any detectable rescueof the embryonic phenotype as assayed by cuticle preparations(Wang, Dumstrei, Haag, and Hartenstein, unpublishedobservations).

Because the DE-cadherin antibody recognizes the extracellular domain of the protein, ectopic expression of the DE-cad^ex construct can be monitored with this antibody. Even though aubiquitous driver line, hs-Gal4, was used, high levels of DE-cad^ex were only observed in cells that endogenously expressed DE-cadherin,i.e., glial cells, neuroblasts, and secondary neurons (Fig. 3B,F).Less DE-cad^ex was detected in primary neurons and the neuropile (formed byprocesses of primary neurons). Like endogenous DE-cadherin, DE-cad^ex was localized at the cell membrane. This notion is supportedby the finding that DE-cad^ex expressed in cultured S2 cells is integrated in the cell membrane(Fig. 3B, inset).

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Figure 3. Ectopic expression of DE-cad^ex with the hs-Gal4 driver line. All panels show confocal cross sections of early third instar brains. A, C, E, G, I, Wild-type controls; B, D, F, H, J, brains of larvae containing hs-Gal4;UAS-DE-cad^ex and heat-pulsed for 10 hr during the second instar. A, B, Labeling with anti-FasII (green) and anti-DE-cadherin (red) to show reduced brain size and higher packing density of neuroblasts (nb) in experimental animal (B). Inset in B shows a cluster of S2 cells expressing the DE-cad^ex construct in their membrane (white arrowhead). C, D, Anti-BrdU (green) and anti-DE-cadherin (red) labeling. In both the control and experimental animals, BrdU was fed for 5 hr during the second instar, followed by fixation and labeling 24 hr later. BrdU-positive cells were strongly reduced in the experimental animal. co, Cortex; ol, optic lobe; np, neuropile. E, F, Labeling with anti-FasII (green) and anti-DE-cadherin (red) to show the lack of axon tracts (arrows in control shown in E) in the experimental brains (F). Both sections were taken at the anteroposterior level of the dorsal lobe of the mushroom body, demarcated by the arrowheads in E and F. G, H, Histological sections of wild-type (G) and experimental (H) brain labeled with methylene blue. Neuroblasts (nb) in wild type are embedded in clusters of small secondary neurons (sn). Secondary neurons form CBTs (cbt) that traverse the cortex. Primary neurons (pn), characterized by their larger size, are located in the deep layer of the cortex. Apoptotic cells (arrowheads; enlargement in inset) are scattered at a low frequency throughout the cortex. In experimental brain, secondary neurons and CBTs are strongly reduced. The number of apoptotic cells is not increased compared with wild type. I, J, Acridine orange labeling of apoptotic cells in central brain (cb) and optic lobe (ol) of wild-type and experimental animals. Cell death is very limited in the central brain of both wild type and mutant. co, Cortex.

Global expression of DE-cad^ex driven by a heat pulse during the early second instar followed by fixation during the mid thirdinstar resulted in severe deficits in neural proliferation andmorphogenesis. The most conspicuous phenotype was the reducedbrain size and the loss of most proximal axon tracts comparedwith control larval brains (Fig. 3A,B,G,H). As observed generallyin experiments in which transgenes are driven by Gal-4 driverlines, the expressivity of the phenotype covered a wide range.In brains most heavily affected (20-30%), neuroblasts appearedin approximately normal numbers but had highly reduced mitoticactivity, as shown by BrdU-labeling experiments. BrdU was fedfor 5 hr to second instar hs-Gal4;DE-cad^ex larvae, immediately followed by a 10 hr heat pulse and fixationafter 24 hr. In experimental brains, the number of mitotic cells(neuroblasts and ganglion mother cells) was reduced to <25% ofthat of control animals (Fig. 3D). The number of secondary neuronsproduced by dividing postembryonic neuroblasts was reduced correspondingly(Fig. 3H). Excess cell death did not appear to contribute to thereduced brain size, because labeling of DE-cad^ex and control brains heat-shocked and aged identically showed asimilar amount of acridine orange-positive cells in the brain(Fig. 3I,J). Apart from reduced brain size, the lack of properspacing between the neuroblasts is another characteristic of DE-cad^ex brains. In the control larval brains, neuroblasts were relativelyevenly spaced over the surface of the central brain (Fig. 3A),an effect caused by the growing number of secondary neurons thatpushed the neuroblasts away from each other. In the experimentallarval brains, neuroblasts were typically clustered closely together(Fig. 3B). Given the abnormal spacing of neuroblasts and theirreduced rate of mitosis, we were able to sample only a few neuroblastsin mitosis. In these cells, the orientation of the mitotic spindlewas vertical or close to vertical, just as seen in the wild-typecontrol (data notshown).

The reduced neuroblast proliferation and consecutive decrease in size of secondary lineages seen in DE-cad^ex-expressing larvae were accompanied by a global loss of CBTs.Figure 3E illustrates the centroanterior protocerebral tract (Nassifet al., 2003), which can be identified easily in wild-type brainsby its proximity to the spur of the mushroom body and which isabsent in hs-Gal4;UAS-DE-cad^ex brains (Fig. 3F). By contrast, axons formed by primary neuronsand their terminal branches that make up the neuropile appearedto be mostly undisturbed, as shown by labeling of brains withthe anti-FasII antibody (Fig. 3E,F).

The effect of DE-cadherin on neural proliferation is mediated in part by glial cells

Previous reports indicating that glial cells may produce factors controlling neuroblast proliferation (Ebens et al., 1993)prompted us to ask whether DE-cad^ex expression in glial cells alone would be able to replicate certainaspects of the phenotype that result from global heat shock-drivenexpression. In this experiment, gcm-Gal4, which is expressed inall glial cells at embryonic and early larval stages, was usedto drive ectopic DE-cad^ex expression. The DE-cad^ex expression was particularly high in the surface glia that coverneuroblasts at the surface of the brain (Fig. 4A). The gcm-Gal4;UAS-DE-cad^ex brains showed a decrease in the size of the central brain (resultsnot shown) accompanied by a reduction in neuronal proliferation.Experimental and control larvae were treated with BrdU for 5 hrat the early second instar and allowed to develop until the thirdinstar. Experimental brains had a twofold decrease in uptake ofBrdU compared with control larval brains (Fig. 4B), which suggeststhat the expression of DE-cad^ex in glia cells results in reduced mitotic activity of neuroblasts.

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Figure 4. DE-cad^ex driven in glial cells reduces neuroblast proliferation. A, Confocal section of second instar wild-type brain showing GFP expression driven by the gcm-Gal4 line and anti-FasII labeling of neuropile tracts and mushroom body. dlb, Dorsal lobe; mlb medial lobe; ped peduncle. Strong GFP expression is seen in surface glia (sg) and neuropile glia (ng); weak expression is seen in cortex glia (cg). B, Histogram showing average number of BrdU-labeled cells per brain section, obtained by feeding BrdU for 5 hr. For both control and experimental brain, BrdU-positive nuclei were counted in every fifth section for six brains (see Materials and Methods). Expression of DE-cad^ex reduces the BrdU index by ~50%.

DE-cadherin is required in secondary lineages for normal cell placement and axon tract formation

DE-cadherin is expressed at a high level in neuroblasts and recently born secondary neurons, which suggests that besides neuroblastproliferation, this adhesion molecule could be involved in neuralmorphogenesis and differentiation. To disturb DE-cadherin functionin neurons, DE-cad^ex was expressed with elav-Gal4, which is expressed in neurons butnot glial cells (Fig. 5A,B). Two phenotypes were particularlyevident: the irregular placement of secondary lineages in thecortex and the abnormal trajectory of proximal axon tracts. Incontrol brains, neuroblasts were invariably held at the brainsurface (Fig. 5C,D). By contrast, neuroblasts in DE-cad^ex-expressing brains were located at variable depths (Fig. 5E,G).This phenotype is likely the result of increased mixing betweensecondary neurons of different ages and primary neurons causedby the absence of differential DE-cadherin levels in all cells.

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Figure 5. Expression of DE-cad^ex in neuronal cells causes cortex layering defects and abnormal axonal trajectories. A, B, Elav-Gal4 drives UAS-GFP in neuroblasts and neurons in third instar brain. The arrowhead in A shows a representative lineage with neuroblast and secondary neurons. The arrow in B shows GFP-positive CBT. C, Confocal section of third instar wild-type brain labeled with anti-DE-cadherin (red) and anti-FasII (green), showing superficial location of neuroblasts (arrowhead) and straight radial trajectory of secondary axons (arrow). D, Enlargement of secondary lineage and CBT shown in C. E-G, Confocal sections of third instar brains after elav-Gal4;UAS-DE-cad^ex expression, labeled with anti-DE-cadherin (red) and anti-FasII (green) antibodies. CBTs in many instances follow a tortuous course (arrow); neuroblasts are frequently located deep in cortex (arrowhead). H, I, Three-dimensional digital models of third instar wild-type (H) and elav-Gal4;DE-cad^ex brain reconstructed from serial confocal sections of brains labeled with anti-FasII and anti-DE-cadherin. Brains are viewed laterally, with anterior to the left and dorsal to the top. The neuropile (np) is depicted in light green. The inner optic anlage (IOA) is shown in gray. CBTs are in purple. In wild type, all CBTs follow a straight, radially oriented trajectory. Numerous CBTs in elav-Gal4;DE-cad^ex brains approach the neuropile surface almost tangentially (arrows), follow a serpentine path (arrowheads), or both.

In addition to abnormal cortical layering, elav-Gal4;UAS-DE-cad^ex brains showed defects in the trajectory of proximal axon tracts.Proximal axon tracts in wild-type brains usually follow a straightradial course from the lineage of origin, through deeper corticallayers of older secondary neurons and primary neurons, towardthe neuropile surface, where many tracts stop (Dumstrei et al.,2003) (Fig. 5C,D). Proximal axon tracts in elav-Gal4;DE-cad^ex brains were approximately normal in number but often did notfollow a straight radial trajectory (Fig. 5E,F,I). Instead, theytraveled at various angles relative to the surface and often followeda tortuous course. This demonstrates that proximal axons are stillable to bundle together, possibly because of the expression ofadhesion systems other than DE-cadherin; however, confronted withabnormally positioned neurons, these axons often grow in the wrongdirection, are frequently "sidetracked" by obstacles in theirpath, or both. We also cannot exclude the possibility that axonoutgrowth is normal initially but tracts become warped secondarilyas a result of enhanced cell movement in the cortex because ofreduced adhesion between somata or between somata and cortexglia.

Effect of DE-cad^ex expression on glial morphology

Given that the severe abnormalities in neural proliferation and morphogenesis are caused at least in part by DE-cad^ex expression in glial cells, we asked whether this expression causesstructurally visible defects in glia. The use of anti-Repo antibodyas a marker to monitor the number and pattern of glial cells showedthat all three major types of glial cells were present (data notshown). Histological and EM sections confirmed that the surfaceglia layer was present (Fig. 6A). Structural defects were clearlyevident in the neuropile glia and cortex glia. Neuropile glialcell bodies were less flattened; the neuropile sheath was interruptedby multiple gaps and clefts, which resulted in a mixing of cellbodies and axonal processes in the boundary area (Fig. 6C). Adramatic phenotype was seen when DE-cad^ex was expressed in cortex glia by the Nrv2-Gal4 driver line (Fig.7B) and in a combination of both cortex glia and neurons by Nrv2-Gal4combined with elav-Gal4 (Fig. 7D). In both instances, cortex glialcells showed a severe reduction in processes, which left wideareas of the cortex without trophospongium. At the same time,many cortex glial cell bodies appeared to be more rounded andbulky than their wild-type counterparts (Fig. 7A,B). In corticaldomains lacking the trophospongium, neurons that express markersnormally restricted to the superficial layers, such as the castorepitope (Kambadur et al., 1998) (Fig. 7B,D), are scattered throughoutthe entire cortex. We conclude that by interfering with neuron-glialadhesion, DE-cad^ex reduces the capability of cortex glia to slide processes betweenneurons. This in turn may be responsible in part for the increasedmovement of neurons and the resulting loss of strict layeringof the cortex.

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Figure 6. Effect of DE-cad^ex on glial ultrastructure. All panels show electron micrographs of cross sections of mid third instar brains. In A and C, DE-cad^ex is activated by a heat pulse delivered during the second instar. A, DE-cad^ex does not noticeably affect the integrity of surface glia (sg), which forms a prominent sheath surrounding neuronal cell bodies (ne). Basement membrane (bm) is secreted by surface glia. B, Section of control wild-type brain showing neuronal cell bodies (ne), electron-dense septa of trophospongium formed by cortex glia (cg), and neuropile glial sheath (ng) formed around the central neuropile (np). Note tightly packed CBT (cbt) in cortex and large-diameter axons of primary neurons (ax) in neuropile. C, Expression of DE-cad^ex disrupts cortex and neuropile glia. Note interrupted neuropile glial sheath (ng) and intermixing of neuronal somata (ne) and axons (ax) at the cortex-neuropile boundary.

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Figure 7. Ectopic expression of DE-cad^ex in neurons and cortex glia affects glial morphology. All panels show confocal sections of mid third instar brains labeled with anti-castor antibody (red), a marker for recently born neurons, and Nrv2-Gal4;UAS-GFP, expressed in glia (green). A, Wild-type brain showing abundant trophospongium, formed by cortex glia (cg). Note the location of castor-positive neurons in superficial chambers of the trophospongium (arrowhead). The arrow demarcates a thick glial sheath formed by neuropile glia (ng). B, Nrv-Gal4;UAS-GFP;DE-cad^ex brain. The trophospongium is severely reduced. Castor-positive neurons are found throughout the cortex. The glial sheath surrounding the neuropile is uneven and full of gaps (arrow). C, Wild-type brain expressing GFP under the control of Nrv2-Gal4 (glia) and elav-Gal4 [neurons; faint labeling, mainly in primary neurons and neuropile (np)]. D, DE-cad^ex driven by Nrv2-Gal4 and elav-Gal4. The phenotype is similar to that shown in B, with a severely reduced trophospongium and neuropile glial sheath.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

We have previously shown that DE-cadherin is expressed in the majority of postembryonic neuroblasts and transiently in theirprogeny, as well as in all three types of glial cells. In thisreport, we demonstrate that during different phases of postembryonicneurogenesis, DE-cadherin is required for several functions thatcan be addressed experimentally. The UAS-DE-cad^ex construct containing the extracellular and transmembrane domainsof DE-cadherin was used to perturb the normal function of DE-cadherin.The nature of this perturbation is considered a dominant-negativeeffect for the following reasons (Wang, Dumstrei, Haag, and Hartenstein,unpublished observations): (1) when expressing DE-cad^ex in embryos using a ubiquitous driver line, we see a range ofdefects that phenocopy the DE-cadherin loss-of-function allelicseries; (2) expression of DE-cad^ex in a shg null background does not result in any detectable phenotypicrescue, which suggests that this construct cannot mediate adhesivecontacts; and (3) recent studies by Oda and Tsukita (1999) andLeBorgne et al. (2002) that focused on tracheal and sense organdevelopment confirmed that a DE-cad^ex construct acts in a dominant-negativemanner.

Glial cells and proliferation

We detected high levels of DE-cadherin expression in the surface glia throughout larval development. Expression of DE-cad^ex with a ubiquitous driver line, hs-Gal4, results in brains withreduced neuronal proliferation activity, which resulted in lackof secondary neurons. The proliferation deficit appeared to existin all lineages, although because of a lack of markers for specificlineages, we could not rule out that proliferation was more affectedin some lineages than others. We speculate that the effect onneuroblast proliferation is mainly attributable to DE-cad^ex expression in the surface glia, given that activation of DE-cad^ex by the glia-specific gcm-Gal4 resulted in a similar, albeit weaker,phenotype than driving with hs-Gal4. At the same time, drivingwith Nrv2-Gal4 (expressed in cortex and neuropile glia) led tono detectable defects in the size of the larvalbrains.

Despite the strong reduction in secondary neurons after global expression of DE-cad^ex, the number of surface glial cells did not appear to be affectedsignificantly. This suggests that surface glial growth is independentof neuroblast division. The mechanism of glial growth in the larvalcentral brain has not been investigated. We are currently addressingthis question by inducing labeled clones of neuronal and gliallineages. Preliminary data show that surface glia increase onlyslightly in number. Thus, occasional clones containing one ortwo isolated surface glial cells were observed (V. Hartenstein,unpublished data). Neither surface glia nor cortex glia appearto derive from mixed neural-glial clones (Hartenstein, unpublisheddata).

Surface glia-derived signals controlling the onset of mitotic activity of neuroblasts have been reported previously (Ebenset al., 1993; Park et al., 1997). According to these studies,the Anachronism (Ana) protein is expressed on membranes of surfaceglial cells surrounding the brain, peripheral nerves, and sensorycomplexes. Loss of Ana results in premature neuroblast proliferationin the larval brain. Thus, after a normal course of proliferationand mitotic quiescence, neuroblasts and optic anlagen in ana larvaestart proliferating during the early first instar, resulting inmorphogenetic abnormalities of both central brain and optic lobe(Ebens et al., 1993). We speculate that DE-cadherin forms partof another molecular pathway that mediates glia-neuroblast interactionsthat affect neuroblast division. Findings in the embryo, as wellas recent results by Akong et al. (2002) on the role of the $alpha$ -catenin-bindingprotein APC2, support thisnotion.

In the embryo, two lines of evidence implicate DE-cadherin in cell division. First, recent findings by Lu et al. (2001) indicatethat the zonula adherens, formed by high concentrations of thecadherin-catenin complex (CCC) near the apical pole of epithelialcells, acts as a spindle-anchoring center that pulls the mitoticspindle into a horizontal position. Loss of the zonula adherens,induced by removal of the apical membrane protein Crumbs, resultsin ectodermal cells with vertical mitotic spindles. The same phenotypeis observed after elimination of the function of DE-cadherin byexpression of DE-cad^ex (Wang, Dumstrei, Haag, and Hartenstein, unpublished observations).In DE-cad^ex-expressing embryos, mitotic spindles in the surface layer areoriented randomly, with vertical spindles occurring as frequentlyas horizontal spindles. The control of mitotic spindle orientationby the CCC has also been reported for the sense organ precursorcells that divide and give rise to the mechanosensory bristlesof the notum (Le Borgne et al., 2002). According to the presentfindings, as well as a recent study by Akong et al. (2002), mitoticspindles are little or not affected in larval brain neuroblasts,although the onset of frequency of mitosis of these cells is abnormal.This difference between embryonic and larval neural precursorsmay be related to the fact that in the embryo, neuroblasts delaminatefrom an epithelial layer (the neurectoderm), whereas such a layeris absent in the larval brain. Here, only glial cells cap theneuroblasts, and it is possible that the role of glial cells inneuroblast spindle orientation is different from that played bythe embryonicneurectoderm.

At an even earlier stage, at the onset of gastrulation, DE-cadherin is involved in coordinating invagination and mitosis ofmesoderm cells. In wild-type embryos, the mesoderm invaginatesas an epithelial layer. Subsequently, mesoderm cells undergo asynchronous round of mitosis, accompanied by an epithelial-mesenchymaltransition (Campos-Ortega and Hartenstein, 1985). If DE-cad^ex is expressed by a maternally activated driver line, mesodermcells divide and become mesenchymal prematurely (Wang, Dumstrei,Haag, and Hartenstein, unpublished observations). An almost identicalphenotype was described recently for the mutation tribbles (trb;Grosshans and Wieschaus, 2000; Mata et al., 2000; Seher and Leptin,2000). Trb encodes a cytoplasmic kinase that inhibits the cdc25homolog String (Stg), thereby delaying mitosis of the mesoderm.It is possible that, similar to many other cytoplasmic enzymes,Trb is linked to the cytoskeleton, or even directly to the CCC.In this case, it would be plausible that Trb activity requiresan intact CCC, explaining why disruption of DE-cadherin resultsin loss of Trb activity and premature mesodermmitosis.

APC2, a Drosophila homolog of the adenomatosis coli (APC) protein, also plays a role in anchoring mitotic spindles in embryosand controlling proliferation of larval neuroblasts. The proteincolocalizes with the other components of the CCC in embryos (McCartneyet al., 2001), as well as larval neuroblasts and neurons (McCartneyet al., 1999). Loss of APC2 negatively affects the number of neuroblaststhat are reactivated in the larval period (Akong et al., 2002).No effect on the (vertical) orientation of mitotic spindles ofthose neuroblasts that do divide was reported, similar to ourfindings on larval brain in which DE-cad^ex is expressed ubiquitously or in surface glialcells.

It is not yet clear how the different phenotypes that resulted from disturbance of DE-cadherin can be integrated into onecoherent picture. In epithelial cells [or modified epithelialcells such as sensory organ precursors investigated by LeBorgneet al. (2002)], it is plausible that DE-cadherin, as part of theCCC, which links the cytoskeleton to the membrane, should be involvedin mitotic spindle orientation. To date, there is no informationas to how spindle orientation and the timing, or frequency, ofmitosis are related, if at all. Ectodermal cells that divide verticallyafter deleting the zonula adherens appear to enter mitosis atapproximately the same time at which they would divide normally(Lu et al., 2001). In the larva, where DE-cadherin and other CCCcomponents are positively required for proliferation, no significanteffect on spindle orientation can be seen (Akong et al., 2002;this study). It is possible that the effect of DE-cadherin onspindle orientation in epithelial cells and proliferation in neuroblastsare unrelated. The positive involvement in neuroblast proliferationcould be a reflection of the surface glia-derived mitogenic signalthat activates neuroblasts. Thus, in the brain, DE-cadherin mightbe involved primarily in mediating glia-neuroblast interactions.If these interactions fail, the mitogenic signal, which is separatefrom DE-cadherin, is unable to exert its effect on neuroblasts.This view would also explain why embryonic neuroblasts, whichdo not depend on glial cells for proliferation, show no requirementfor DE-cadherin (Tepass et al., 1996).

DE-cadherin and brain cortex morphogenesis: effect of cell sorting

The defect in cortex layering and cell body fiber trajectory that we saw in larval brains in which DE-cad^ex was expressed is likely the result of two interrelated effectsof DE-cadherin. First, given that DE-cadherin is expressed inneurons and cortex glia and that DE-cad^ex causes structural changes in the trophospongium, this in itselfwould have an effect on the layering of neuroblasts and neurons.Second, cell sorting based on differential DE-cadherin expressionmay be involved. Thus, DE-cadherin is expressed at high levelsin neuroblasts, ganglion mother cells, and newly born neuronsbut is turned off in older neurons and is never expressed in primaryneurons. This expression gradient could be instrumental for maintainingthe layered arrangement of neuroblasts, ganglion mother cells,and neurons of different ages. Removal or lowering of DE-cadherinlevels by DE-cad^ex would disturb this gradient, which could cause cell mixing andthereby a breakdown of the layered organization of the cortex.Classic experiments by Townes and Holtfreter (1955) had shownthat dissociated cells expressing different adhesion moleculeswill sort out according to the type of molecule they express.The same effect can be achieved if cells express the same adhesionsystem at different concentrations (Steinberg and Takeichi, 1994).In vivo studies strongly suggest that cell sorting based on differentDE-cadherin concentrations is involved in normal ovary morphogenesis(Godt and Tepass, 1998). During vertebrate neurogenesis, cellsorting mediated by expression of different members of the cadherinsuperfamily is an important process in establishing compartmentsor subregions of the brain. For example, in the Xenopus neuraltube, F-cadherin functions to position the neuroepithelial cellsat the sulcus limitans (Espeseth et al., 1998). Similarly, inthe embryonic mouse brain, cadherin 6 and R-cadherin maintainthe boundary between the lateral ganglionic eminence and the presumptivecerebral cortex, respectively (Inoue et al., 2001).

Cell sorting might also be the mechanism by which the complementary expression of DE-cadherin and the only other Drosophilaclassic cadherin, DN-cadherin, exerts an effect on larval brainmorphogenesis. DN-cadherin is expressed globally by embryonicprimary neurons and their neurites (Iwai et al., 1997). This expressionis carried over from the embryonic into the larval period. Asa result, the entire larval neuropile is labeled (Hartenstein,unpublished data). None of the classes of glial cells expressDN-cadherin. Furthermore, with the notable exception of mushroombody cells, which are DE-cadherin-negative, secondary neuronsdo not express DN-cadherin. This expression pattern representsthe exact opposite of the pattern exhibited by DE-cadherin, whichis globally expressed in neuroblasts, secondary neurons, and glialcells but not in primary neurons and the mushroom body. It ispossible that the complementary expression of the two classiccadherins in the larval brain is involved in the separation ofdifferentiated primary lineages and immature secondary lineages.So far, no functional study of DN-cadherin in the central larvalbrain has been performed. In the pupal optic lobe, DN-cadherinplays a role in targeting afferent retinal axons to their propertermination site in the optic lobe (Lee et al., 2001). Additionalstudies, including ectopic expression of DN-cadherin in secondarylineages or removal of both cadherins from brain neurons, arerequired to address the role of these molecules in brainmorphogenesis.

DE-cadherin and brain cortex morphogenesis: role of cortex glia

Cortex glial cells form a scaffold of processes, adequately termed trophospongium by Hoyle (1986), around neuronal somatalocated in the cortex. In Drosophila, the trophospongium has notbeen described in much detail, and its origin during embryonicdevelopment or remodeling during metamorphosis is entirely unknown.Buchanan and Benzer (1993) demonstrated that loss of the drop-deadgene causes lethality in early adulthood and is accompanied bystructural defects, primarily of the cortex glia. Electron micrographspresented in that report documented the morphology of cortex gliain adult brains of wild-type and drop-dead flies. Similar to resultspresented here, adult cortex glia formed 20- to 50-nm-thick electron-densesheaths around individual neurons or, in some cases, small packetsof neurons. This trophospongium is fully established in the earlylarva around primary neurons (Younossi-Hartenstein et al., 2003)(Fig. 1H, a). As neuroblasts become active and produce secondarylineages, the trophospongium expands to form additional chambersthat take up the newly generated neurons. These superficial chambersare larger than the deep ones, typically containing an entirelineage formed by a neuroblast and 20-30 ganglion mother cellsor neurons (Fig. 1H, b). As lineages grow, the oldest neuronsbecome separated from their younger siblings by newly formed cortexglia processes (Fig. 1H, c, d). The ordered formation of cortexglial processes may well represent a mechanism that establishesand maintains the position of a neuron within the cortex. Changesin cortex glial morphology, such as reported here to result fromDE-cad^ex expression, may well be responsible for the neural layeringdefects.

The role we ascribe here to cortex glia in the Drosophila larval brain is highly reminiscent of the role of radial glial cellsin vertebrates. Radial glial cells in the neural tube form processesthat extend from the ventricular zone through the entire thicknessof the ventral tube. These processes form a scaffold on whichthe neurons migrate from the ventricular layer, where they areborn, into the mantle layer (Rakic, 1972). Experimental studiesconfirm that clonally related neurons migrate preferentially alonga common radial glial process and thereby form a vertical columnof neurons (Walsh and Cepko, 1988).

Radial glia represent a peculiar cell type restricted to embryos in mammals but persisting into adulthood in all other vertebrategroups. According to recent findings, radial glial cells are asubclass of neuroepithelial cells that start to express molecularmarkers of astrocytes without being firmly committed to a glialfate. Thus, it could be shown that in mouse, radial glial cellsof the early embryo continue dividing and producing neurons andastroglia (for review, see Parnavelas and Nadarajah, 2001). Inview of the similar role cortex glia in insects and radial gliain vertebrates appear to play, it is tempting to speculate thatfuture studies will uncover fundamental similarities in the molecularmechanisms underlying the interaction between neurons and glialcells. Currently, it is difficult to compare glial cells in differentphyla. Thus, given that glial cells, as defined morphologically,appear to be absent from many simple invertebrate animals (includingflatworms and nematodes; Radojcic and Pentreath, 1979), it isunlikely that the bilaterian ancestor possessed these cells. Consequently,glial cells in vertebrates and insects (as well as other "higher"protostome phyla, including annelids and molluscs) represent convergenttraits, having evolved independently from neurons or epidermalcells in animal phyla that developed a complex nervous system.Comparative molecular studies investigating the pathways thatcontrol glial fate in different animals will shed more light onthe question of how to evaluate the phylogenetic and functionalrelationship between glial cells of differentphyla.

  FOOTNOTES

Received June 27, 2002; revised Jan. 22, 2003; accepted Jan. 30, 2003.

This work was supported by University of California, Los Angeles, United States Public Health Service National Research ServiceAward GM07185 to F.W. and National Institutes of Health GrantNS 29367 to V.H. We thank Drs. C. Goodman, W. Odenwald, J. Lengyel,A. Tomlinson, and L. Zipursky and the Bloomington and Umea StockCenter for sending fly stocks and antibodies. The following antibodieswere obtained from the Developmental Studies Hybridoma Bank, developedunder the auspices of the National Institute of Child Health andHuman Development and maintained by the University of Iowa, Departmentof Biological Sciences (Iowa City, IA): armadillo antibody, developedby Dr. E. Wieschaus; and crumbs antibody, developed by Dr. E.Knust.

Correspondence should be addressed to Dr. Volker Hartenstein at the aboveaddress.

  References

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Akong K, Grevengoed EE, Price MH, McCartney BM, Hayden MA, Peifer M (2002) Drosophila APC2 and APC1: distinct intracellular localization and complex overlapping roles in the embryos, larval brain, and imaginal discs. Dev Biol 250:71-90[Web of Science][Medline].
Ashburner M (1989) In: Drosophila: a laboratory manual. Cold Spring Harbor, NY: Cold Spring Harbor Laboratory.
Booth GE, Kinrade EF, Hidalgo A (2000) Glia maintain follower neuron survival during Drosophila CNS development. Development 127:237-244[Abstract].
Buchanan RL, Benzer S (1993) Defective glia in the Drosophila brain degeneration mutant drop-dead. Neuron 10:839-850[Web of Science][Medline].
Campbell G, Goring H, Lin T, Spana E, Andersson S, Doe CQ, Tomlinson A (1994) RK2, a glial-specific homeodomain protein required for embryonic nerve cord condensation and viability in Drosophila. Development 120:2957-2966[Abstract].
Campos-Ortega JA, Hartenstein V (1985) In: The embryonic development of Drosophila melanogaster. Berlin: Springer.
Dumstrei K, Wang F, Nassif C, Hartenstein V (2003) Early development of the Drosophila brain. V. Pattern of postembryonic neuronal lineages expressing Shg/DE-cadherin. J Comp Neurol 455:451-462[Web of Science][Medline].
Ebens AJ, Garren H, Cheyette BN, Zipursky SL (1993) The Drosophila anachronism locus: a glycoprotein secreted by glia inhibits neuroblast proliferation. Cell 74:5-27[Web of Science][Medline].
Espeseth A, Marnellos G, Kintner C (1998) The role of F-cadherin in localizing cells during neural tube formation in Xenopus embryos. Development 125:301-312[Abstract].
Fujita SC, Zipursky SL, Benzer S, Ferrus A, Shotwell SL (1982) Monoclonal antibodies against the Drosophila nervous system. Proc Natl Acad Sci USA 79:7929-7933[Abstract/Free Full Text].
Godt D, Tepass U (1998) Drosophila oocyte localization is mediated by differential cadherin-based adhesion. Nature 395:387-391[Medline].
Grenningloh G, Rehm EJ, Goodman CS (1991) Genetic analysis of growth cone guidance in Drosophila: fasciclin II functions as a neuronal recognition molecule. Cell 67:45-57[Web of Science][Medline].
Grosshans J, Wieschaus E (2000) A genetic link between morphogenesis and cell division during formation of the ventral furrow in Drosophila. Cell 101:523-531[Web of Science][Medline].
Hartenstein V, Nassif C, Lekven A (1998) Embryonic development of the Drosophila brain. II. The glia cells of the brain. J Comp Neurol 402:32-48[Medline].
Hoyle G (1986) Glial cells of an insect ganglion. J Comp Neurol 246:85-103[Web of Science][Medline].
Inoue T, Tanaka T, Takeichi M, Chisaka O, Nakamura S, Osumi N (2001) Role of cadherins in maintaining the compartment boundary between the cortex and striatum during development. Development 128:561-569[Abstract].
Ito K, Hotta Y (1992) Proliferation pattern of postembryonic neuroblasts in the brain of Drosophila melanogaster. Dev Biol 149:134-148[Web of Science][Medline].
Ito K, Sass H, Urban J, Hofbauer A, Schneuwly S (1997) GAL4-responsive UAS-tau as a tool for studying the anatomy and development of the Drosophila central nervous system. Cell Tissue Res 290:1-10[Web of Science][Medline].
Iwai Y, Usui T, Hirano S, Steward R, Takeichi M, Uemura T (1997) Axon patterning requires DN-cadherin, a novel neuronal adhesion receptor, in the Drosophila embryonic CNS. Neuron 19:77-89[Web of Science][Medline].
Kambadur R, Koizumi K, Stivers C, Nagle J, Poole SJ, Odenwald WF (1998) Regulation of POU genes by castor and hunchback establishes layered compartments in the Drosophila CNS. Genes Dev 12:246-260[Abstract/Free Full Text].
Le Borgne R, Bellaiche Y, Schweisguth F (2002) Drosophila E-cadherin regulates the orientation of asymmetric cell division in the sensory organ lineage. Curr Biol 12:95-104[Web of Science][Medline].
Lee CH, Herman T, Clandinin TR, Lee R, Zipursky SL (2001) N-cadherin regulates target specificity in the Drosophila visual system. Neuron 30:437-450[Web of Science][Medline].
Lemke G (2001) Glial control of neuronal development. Annu Rev Neurosci 24:87-105[Web of Science][Medline].
Lu B, Roegiers F, Jan LY, Jan YN (2001) Adherens junctions inhibit asymmetric division in the Drosophila epithelium. Nature 409:522-525[Medline].
Mata J, Curado S, Ephrussi A, Rorth P (2000) Tribbles coordinates mitosis and morphogenesis in Drosophila by regulating string/CDC25 proteolysis. Cell 101:511-522[Web of Science][Medline].
McCartney BM, Dierick HA, Kirkpatrick C, Moline MM, Baas A, Peifer M, Bejsovec A (1999) Drosophila APC2 is a cytoskeletally-associated protein that regulates wingless signaling in the embryonic epidermis. J Cell Biol 146:1303-1318[Abstract/Free Full Text].
McCartney BM, McEwen DG, Grevengoed E, Maddox P, Bejsovec A, Peifer M (2001) Drosophila APC2 and Armadillo participate in tethering mitotic spindles to cortical actin. Nat Cell Biol 10:933-938.
Nassif C, Noveen A, Hartenstein V (1998) Embryonic development of the Drosophila brain. I. The pattern of pioneer tracts. J Comp Neurol 402:10-31[Web of Science][Medline].
Nassif C, Noveen A, Hartenstein V (2003) Early development of the Drosophila brain. III. The pattern of neuropile founder tracts during the larval period. J Comp Neurol 455:417-434[Web of Science][Medline].
Oda H, Tsukita S (1999) Nonchordate classic cadherins have a structurally and functionally unique domain that is absent from chordate classic cadherins. Dev Biol 216:406-422[Web of Science][Medline].
Park Y, Caldwell MC, Datta S (1997) Mutation of the central nervous system neuroblast proliferation repressor ana leads to defects in larval olfactory behavior. J Neurobiol 33:199-211[Web of Science][Medline].
Parnavelas JG, Nadarajah B (2001) Radial glial cells. Are they really glia? Neuron 31:881-884[Web of Science][Medline].
Poeck B, Fischer S, Gunning D, Zipursky SL, Salecker I (2001) Glial cells mediate target layer selection of retinal axons in the developing visual system of Drosophila. Neuron 29:99-113[Medline].
Radojcic T, Pentreath VW (1979) Invertebrate glia. Prog Neurobiol 12:115-179[Web of Science][Medline].
Rakic P (1972) Mode of cell migration to the superficial layers of fetal monkey neocortex. J Comp Neurol 145:61-84[Web of Science][Medline].
Redies C (2000) Cadherins in the central nervous system. Prog Neurobiol 61:611-648[Web of Science][Medline].
Seher TC, Leptin M (2000) Tribbles, a cell-cycle brake that coordinates proliferation and morphogenesis during Drosophila gastrulation. Curr Biol 10:623-629[Web of Science][Medline].
Steinberg MS, Takeichi M (1994) Experimental specification of cell sorting, tissue spreading, and specific spatial patterning by quantitative differences in cadherin expression. Proc Natl Acad Sci USA 91:206-209[Abstract/Free Full Text].
Strausfeld N (1976) In: Atlas of an insect brain. Berlin: Springer.
Sun B, Wang W, Salvaterra PM (1998) Functional analysis and tissue-specific expression of Drosophila Na⁺, K⁺-ATPase subunits. J Neurochem 71:142-151[Web of Science][Medline].
Tepass U, Gruszynski-DeFeo E, Haag TA, Omatyar L, Torok T, Hartenstein V (1996) shotgun encodes Drosophila E-cadherin and is preferentially required during cell rearrangement in the neurectoderm and other morphogenetically active epithelia. Genes Dev 10:672-685[Abstract/Free Full Text].
Tepass U, Truong K, Godt D, Ikura M, Peifer M (2000) Cadherins in embryonic and neural morphogenesis. Nat Rev Mol Cell Biol 1:91-100[Web of Science][Medline].
Townes PL, Holtfreter J (1955) Directed movement and selective adhesion of embryonic amphibian cells. J Exp Zool 128:53-120[Web of Science].
Truman JW (1990) Metamorphosis of the central nervous system of Drosophila. J Neurobiol 21:1072-1084[Web of Science][Medline].
Truman JW, Bate M (1988) Spatial and temporal patterns of neurogenesis in the central nervous system of Drosophila melanogaster. Dev Biol 125:145-157[Web of Science][Medline].
Truman JW, Talbot WS, Fahrbach SE, Hogness DS (1994) Ecdysone receptor expression in the CNS correlates with stage-specific responses to ecdysteroids during Drosophila and Manduca development. Development 120:219-234[Abstract].
Uemura T, Oda H, Kraut R, Hayashi S, Kotaoka Y, Takeichi M (1996) Zygotic Drosophila E-cadherin expression is required for processes of dynamic epithelial cell rearrangement in the Drosophila embryo. Genes Dev 10:659-671[Abstract/Free Full Text].
Walsh C, Cepko CL (1988) Clonally related cortical cells show several migration patterns. Science 241:1342-1345[Abstract/Free Full Text].
Younossi-Hartenstein A, Salvaterra P, Hartenstein V (2003) Early development of the Drosophila brain. IV. Larval neuropile compartments defined by glial septa. J Comp Neurol 455:434-450.

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