A Role for Tectal Midline Glia in the Unilateral Containment of Retinocollicular Axons

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The Journal of Neuroscience, October 15, 1998, 18(20):8344-8355

A Role for Tectal Midline Glia in the Unilateral Containment of Retinocollicular Axons
Da-Yu Wu¹, Gerald E. Schneider¹, Jerry Silver², Michael Poston², and Sonal Jhaveri¹
¹ Department of Brain and Cognitive Sciences, Massachusetts Institute of Technology, Cambridge, Massachusetts 02139, and ² Department of Neuroscience, Case Western Reserve Medical School, Cleveland, Ohio 44106

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Retinal fibers approach close to the tectal midline but do not encroach on the other side. Just before the entry of retinalaxons into the superior colliculus (SC), a group of radial gliadifferentiates at the tectal midline; the spatiotemporal deploymentof these cells points to their involvement in the unilateral containmentof retinotectal axons.
To test for such a barrier function of the tectal midline cells, we used two lesion paradigms for disrupting their radialprocesses in the neonatal hamster: (1) a heat lesion was usedto destroy the superficial layers of the right SC, including themidline region, and (2) a horizontally oriented hooked wire wasinserted from the lateral edge of the left SC toward the midlineand was used to undercut the midline cells, leaving intact theretinorecipient layers in the right SC. In both cases, the leftSC was denervated by removing its contralateral retinal input.Animals were killed 12 hr to 2 weeks later, after intraocularinjections of anterograde tracers to label the axons from theremaining eye. Both lesions resulted in degeneration of the distalprocesses of the tectal raphe glia and in an abnormal crossingof the tectal midline by retinal axons, leading to an innervationof the opposite ("wrong") tectum. The crossover occurred onlywhere glial cell attachments were disrupted.
These results document that during normal development, the integrity of the midline septum is critical in compartmentalizingretinal axons and in retaining the laterality of the retinotectalprojection.

Key words: midline septum; GFAP; axon barrier; radial glia; axon guidance; brain compartmentalization

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Glial cells have supportive or attractive influences on axon growth (Singer et al., 1979; Whitehead and Morest, 1981; Silverand Rutishauser, 1984; Dodd and Jessell, 1988; Muller and Best,1989; Vanselow et al., 1989; Aguayo et al., 1990; Hatten, 1990;Abbott, 1991; Schachner, 1991) and play an inhibitory or repulsiverole during fiber extension (Patterson, 1988; Chiquet, 1989; Joostenand Gribnau, 1989; Steindler et al., 1989, 1990; Snow et al.,1990a; Schwab and Schnell, 1991; Schwab et al., 1993; Steindler,1993). We focus here on the latter function, particularly on thecompartmentalization of growing fiber systems by glia.

Glycoproteins expressed on oligodendrocytes inhibit axon growth. Antibodies that neutralize this inhibition allow for fiberregrowth (Schwab and Schnell, 1991; Kapfhammer et al., 1992; Schwabet al., 1993), suggesting that differentiating oligodendrogliaoutline spatial domains that contain late-developing fiber systems(Schwab, 1990; Kapfhammer and Schwab, 1994; Schwegler et al.,1995). Glial cell-associated glycoconjugates form boundaries thatdelineate compartments in the developing brain (Steindler andCooper, 1987; Steindler et al., 1989, 1990); in the barrelfieldcortex, glycoconjugate patterning reflects the organization ofwhiskers on the snout (Blue et al., 1991; Jhaveri et al., 1991b;Bennett-Clarke et al., 1994; Schlaggar and O'Leary, 1994) andmay serve to maintain the tangential coordinates of clusteredthalamocortical fibers (Steindler et al., 1990; Steindler, 1993).It is suggested that upregulation of proteoglycans within theextracellular matrix of reactive astroglia contributes to regenerativefailure of adult axons in white matter tracts (Davies et al.,1997). Glia along the spinal roof plate are implicated in blockadingdorsal column axons from invading contralaterally, most likelyvia sulfated proteoglycans (PGs) (Snow et al., 1990a,b; Pindzolaet al., 1993). Midline glia along the caudal neuraxis are absentin regions where corticospinal fibers decussate, indicating arole in retaining the laterality of corticospinal axons (Joostenand Gribnau, 1989). Differential interactions of nasal or temporalretinal axons with cells (early neurons and/or radial glia) atthe optic chiasm direct the routing of these fibers (Godementet al., 1990; Godement and Mason, 1993; Wizenmann et al., 1993;Sretavan et al., 1995).

A group of radial cells resides along the tectal midline (Jhaveri et al., 1992; Wu et al., 1995). These are distinct fromother tectal glia in their timing of differentiation, morphology,and molecular composition. Damage to the midline surface in neonatalrodents results in a bilateral invasion (across the midline) ofthe tectum by retinal axons from a single eye (Schneider, 1973;Hsiao and Schneider, 1978; Jen and Lund, 1979); no crossing ofthe tectal midline by retinal axons is detected if the lateraltectum, but not the midline, is damaged (So and Schneider, 1978;Schneider et al., 1985). These results suggest that normally,a structure(s) along the midline compartmentalizes retinotectalaxons to one side. Here, we document an involvement of the tectalraphe glia in mediating such a barrier function. We show thatretinal axons can be induced to cross the tectal midline abnormallybut only where the pial processes of midline glia have been disrupted.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Syrian hamsters (Mesocricetus auratus) were bred in the animal facility at the Massachusetts Institute of Technology, or timed-pregnantfemales were purchased from Charles River Laboratories (Wilmington,MA). The Massachusetts Institute of Technology Committee on AnimalCare approved protocols for all surgical procedures involvinglive animals.

Surgical procedures
Unilateral tectal lesions. Postnatal day 1 (P1) hamster pups were anesthetized by hypothermia, the skin overlying the tectumwas incised, and the flat head of a pin was heated and appliedfor a few seconds to the cartilaginous skull overlying the rightsuperior colliculus (SC). The right eye was also removed. Theskin was sutured, and the pup was warmed and returned to the homenest.
Undercutting the midline glial cells. Animals were anesthetized by hypothermia on P1, and the skull covering the SC was exposedas described above. A small slit was made with a number 11 scalpelblade at the lateral edge of the skull covering the left SC; ahooked tungsten wire was inserted through the slit and pushedmedially, below the pia, all the way to the midline. The wirewas then moved in the horizontal plane to disrupt the pial processesof the raphe glia, while the retinorecipient layers of the righttectum were maintained intact. The right eye was also removedat the same time to denervate the left SC. Earlier studies hadshown that such denervation induces a larger number of retinalaxons from the remaining left eye to cross the tectal midlineand to abnormally innervate the left tectum (Schneider, 1973;So and Schneider, 1978). Animals were warmed, returned to thehome nest, and killed after varying survival times (12 hr to 3weeks). To control for effects of the eye removal, the midlineundercutting surgery was done on a group of newborn animals withoutenucleating the right eye. To control for the lesion made in theleft SC by the tungsten wire, surgery was performed on a groupof animals as described above, except that the wire was advancedjust short of the midline, and the midline (raphe) glia were notsevered; in these cases the right eye was also removed, as forthe experimental animals.

Horseradish peroxidase eye injection and retinotectal axon labeling
Hamsters with unilateral SC lesions were perfused 10-21 d after surgery. Pups (at least five at each time point) with a midlineundercut were killed at P12 or P14; two animals were perfusedon P7. Control animals were age-matched to the corresponding experimentalhamsters at the time of perfusion. One day before being killed,the animal was fully anesthetized with hypothermia (for the neonates)or with Chloropent (0.35 ml/100 gm body weight), and 1-3 µl of40-50% horseradish peroxidase (HRP) (type VI; Sigma, St. Louis,MO) made up in 2% dimethylsulfoxide was injected into the lefteye, with use of a micropipette attached to a Drummond Scientific(Broomall, PA) microdispenser or a picospritzer (World PrecisionInstruments, Sarasota, FL). Animals were killed with an overdoseof anesthesia and perfused transcardially with an initial rinseof 0.9% sodium chloride containing 0.25% of the vasodilator sodiumnitrite. This was followed by 4% paraformaldehyde made up in 0.1M phosphate buffer (PB), pH 7.4. The brains were not post-fixedbut were immediately dissected out and stored in PB for <1 week.Brains prepared for light microscopy were cryoprotected in 30%sucrose (made up in PB, pH 7.4) and cut coronally at a thicknessof 40-50 µm on a cryomicrotome. Three parallel series of sectionswere collected; one was reacted with tetramethylbenzidine (Sigma)to visualize the HRP-labeled retinal fibers as described previously(Jhaveri et al., 1988). The other two groups of adjacent sectionswere immunostained (see below). All sections were mounted ontogelatin-coated microscope slides, counterstained with neutralred, air dried, and coverslipped after brief alcohol dehydrationand xylene clearing.

Immunohistochemistry
Sections adjacent to those reacted for HRP were immunostained using monoclonal antibodies against the glial fibrillary acidicprotein (GFAP) or against vimentin (both antibodies from BoehringerMannheim, Indianapolis, IN). All steps were performed under gentleagitation. Sections were rinsed in PBS, and nonspecific bindingwas blocked by incubation in 20% normal horse serum (Life Technologies,Grand Island, NY) in PBS. They were next incubated in primaryantibody (1:30 dilution) made up in PBS containing 1% normal horseserum, 0.3% Triton X-100, and 0.2% sodium azide, for 18-24 hrat room temperature (or for 96 hr at 4°C). They were rinsed andthen transferred to biotinylated horse anti-mouse IgG (1:200 dilutionmade up in PBS, horse serum, and Triton X-100; Vector Laboratories,Burlingame, CA) for 1 hr at room temperature. Sections were rinsedagain, immersed in an avidin-biotin-HRP complex solution (ABCkit; Vector Laboratories) for 1 hr, after which the HRP was visualizedusing hydrogen peroxide, with diaminobenzidine tetrahydrochlorideas a chromagen. Control sections for immunostaining were processedusing the same solutions, except that the primary antibody wasomitted in the first incubation. Sections were mounted on gelatinizedslides, dried overnight, cleared in xylene, and coverslipped.

Quantitation
The tectal midline was reconstructed in dorsal view from coronal sections through the brains of six animals in which the midlineglial processes were undercut. Alternate sections from these brainswere stained with GFAP or reacted for visualizing the HRP-labeledretinal axons. Hatched lines (see Fig. 11) represent the distance(arbitrary scale) along the rostrocaudal axis where pial processesof the raphe glia were intact (i.e., not cut by the sweep of thehooked wire). The distance along the rostrocaudal axis over whichHRP-labeled retinal fibers could be seen crossing the midlinewas represented by Xs (see Fig. 11). The region of the midlinealong which the pial processes of glial cells were disrupted,but no HRP-labeled axons were seen crossing to the opposite side,was represented as a thick line (see Fig. 11).

1,1'-Dioctadecyl-3,3,3',3'-tetramethylindocarbocyanine perchlorate labeling of retinal axons and 4-(4-dihexadecylaminostyryl)-N-methylpyridinium iodide labeling of midline radial glia
Midline undercutting surgery was performed on P1 pups, as above. On P2 (24 hr after surgery), the pups were reanesthetizedby hypothermia, and a solution of 1,1'-dioctadecyl-3,3,3',3'-tetramethylindocarbocyanineperchlorate (DiI) (Molecular Probes, Eugene, OR) dissolved indimethyl formamide was injected into the left eye. Animals wereallowed to survive for another 1-2 d, were overdosed with pentobarbital,and perfused with 4% paraformaldehyde, and 4-(4-dihexadecylaminostyryl)-N-methylpyridiniumiodide (DiA) (Molecular Probes) was placed in the dorsal wallof the ventricle at the level of the cerebral aqueduct of Sylvius.The labeled brain was returned to 4% paraformaldehyde for 4-15d at room temperature. Brains were then cut on a vibratome into100-µm-thick transverse sections, and tissue was collected in0.1 M PB, mounted onto microscope slides, and coverslipped wetin PBS. The edges of the coverslips were sealed with nail polish.DiI labeling of retinal axons in the tectum was analyzed and photographedwith a Nikon epifluorescence microscope using a rhodamine filter.DiA-labeled radial processes on the same section were photographedwith use of a fluorescein filter.

Electron microscopy
Normal hamsters and hamsters that had received a unilateral heat lesion of the SC on P0 or P1 survived until P6, at whichpoint they were perfused with 4% paraformaldehyde and 3% glutaraldehydein PBS. The brains were removed and post-fixed in the same solution.Coronal sections through the midbrain were cut on a vibratome,rinsed in PBS, osmicated (1% osmium tetroxide in PB) for 1-3 hrat room temperature, and rinsed again in buffer. They were sequentiallydehydrated in a series of ethyl alcohols and then in a mixtureof ethyl alcohol and Spurr's resin and were finally polymerizedin fresh Spurr's resin. Semithin sections, stained with toluidineblue, provided orientation to trim the block around the tectalmidline. Ultrathin sections were cut on a DuPont (Billerica, MA)MT-5000 ultramicrotome; they were mounted on formvar-coated coppermesh grids, stained with lead citrate and uranyl acetate, andviewed on a Zeiss 109 electron microscope.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Midline radial glia and retinotectal projections in P0 hamsters

In normal animals, the tectal midline is comprised of tightly bundled radial cells whose perikarya are positioned around thelumen of the ventricle and whose radial processes span the thicknessof the colliculus and are embedded in the pial surface. We referto these radial extensions as the pial processes of the midlineglia. Details of the development of these cells have been providedby Wu et al. (1995). Here, we briefly review salient light microscopeobservations that are relevant to the present study.

On P0-P1, vimentin immunoreactivity revealed radial cells in the lateral tectum, as well as along the midline (Fig. 1A-C);the latter were particularly striking because of their densityand the bundling of their processes. These midline cells retainedtheir vimentin expression at least until P12 (Fig. 2A). No lateralradial cells stained positively with the GFAP antibody that weused in this study. On the other hand, the midline cells wereintensely reactive for this intermediate filament protein, bothin neonates and at least through the second week of postnatallife (Figs. 1D, 2B) but not in embryonic animals. As has beenshown before for all normal rodents, HRP-labeled retinal axonsthat projected to the superficial gray layer (SGS) of the contralateraltectum were retained within the SC on one side, with no encroachmentof the visual axons across the tectal midline (Fig. 2C,D). (Retinotectalaxons that are deflected ipsilaterally at the chiasm normallyapproach the tectum from the rostral end, as do the ones fromthe contralateral eye; they do not cross the tectal midline.)The following experiments describe the relationship between thedamage inflicted on the midline glia and the altered projectionpatterns of retinotectal afferents (Jhaveri, 1993a,b; Jhaveriand Hoffman-Kim, 1996).

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Figure 1. Coronal sections through the SC of a hamster on the day after birth (P1). The tissue was stained with an antibody against vimentin (A-C) or against the GFAP (D). Vimentin-positive radial processes extend between the ventricular surface and the pial surface (A, B). The midline cells (C) are densely bundled and intensely vimentin-reactive, and their pial processes are embedded in the pial surface. Only the midline cells are GFAP-positive in the P1 tectum (D). Scale bar (in C): A, D, 200 µm; B, C, 50 µm.

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Figure 2. Coronal sections through the SC of a P12 hamster immunostained to visualize vimentin (A) and GFAP expression (B). Note that at this age, the lateral radial cells exhibit little expression of either protein, whereas both vimentin and GFAP can still be detected in the midline cells. Filled arrows point to pia, and open arrows point to pial ends of midline glial cells. C, D, Dark-field (polarized light) and light-field images, respectively, of the distribution of the normal retinotectal projection as seen in a coronal section through the midbrain of a P12 animal whose left eye was injected with HRP. The sections were reacted with tetramethylbenzidine and counterstained with neutral red. Arrows in D point to the midline. Radial processes are not specifically stained in this preparation. Scale bar (in D): A-D, 200 µm.

Disruption of the midline after heat lesions of the tectum

As a consequence of heat damage at the tectal surface, the underlying tissue became necrotic, and a cyst formed in this region(Fig. 3). Eight days after lesion, HRP-labeled retinal axons couldbe followed into the region of damage and across the tectal midlineinto the contralateral SC. These axons took two paths to the oppositeside. The first was a membranous bridge, which provided a substratefor the axons to travel over the cyst and into the contralateralSC (Fig. 3A,B). Immunostaining of sections immediately adjacentto the ones in which HRP-labeled retinal axons had been visualizedin this bridge revealed that GFAP-positive processes (of unknownorigin) lined this upper membranous route (Fig. 3D). In addition,retinal axons were also seen coursing along the surface of theremnant SC, subjacent to the necrotic tissue (Fig. 3A,B) (So,1979; Harvey et al., 1986). This second route occurred in theregion where the pial processes of the midline raphe cells hadbeen disrupted (Figs. 3, compare A,B and C,D; 4): most of thepial attachments of the raphe glia had pulled back from the surfaceor were degenerating. The neatly bundled GFAP-positive processes,normally attached at the pial surface of the midline, were nolonger visible (Fig. 4). However, the glial cell somata, alongwith their more proximal radial processes, were still tetheredat the ventricular surface (Figs. 4A,B, 5C). Higher magnificationviews (Fig. 5) showed that the disruption of the radial processescreated a "gap" just below the pial surface (Fig. 5A,C) and thatretinal axons were confined to travelling through this gap. Nevertheless,surface view reconstructions of the tectal midline illustratedthat the gap in the midline glia was not coextensive with theregion over which the axons crossed but that it spanned a largerrostrocaudal extent of the SC than the region within which retinalaxon crossover occurred (see Fig. 11, quantitation for the midlineundercut cases presented below).

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Figure 3. Two sets of adjacent sections through the tectum of two P8 animals (A and C from one animal, B and D from the other) that had suffered unilateral (right side) tectal lesions on P1; their right eyes were removed at the same time. On P7, the left eyes were injected with HRP, and a day later the animals were killed. In each brain, one set of sections were reacted for visualizing the HRP and photographed with dark-field optics (A, B), whereas immediately adjacent sections (C, D) were immunostained with an antibody against GFAP, which permits visualization of glia. Note the HRP-labeled axons crossing the tectal midline along the membranous bridge that forms above the necrotic tissue cyst in the right SC (the necrotic tissue within the cyst falls out during histological processing) and also along a lower route that passes below the cyst over the remnant right tectal tissue. The complementary relationship between where retinal axons are able to travel and where the glial process are disrupted is especially obvious in C. Higher magnification views of the disrupted regions in C and D are depicted in Figure 5. Scale bar (in D): A-D, 200 µm.

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Figure 4. Coronal sections through the SC of two hamsters (A and C from one animal, B and D from the other) that survived 18 hr after suffering heat damage to one SC. Boxed areas in A and B are shown at higher magnification in C and D, respectively. The damaged tissue has become necrotic (the cyst is especially noticeable over the right SC in B), and the disruption of distal process of midline glial cells is evident with immunostaining for vimentin (A, C), as well as for GFAP (B, D). Arrows in D point to the ends of some distal processes. Note end feet of lateral radial glia in upper left of C. Scale bars: (in B) A, B, 200 µm; (in D) C, D, 50 µm.

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Figure 5. A, C, Higher magnification views of Figure 3C,D to show the disruption of the distal processes of the midline glia. Comparable levels from the tectal midline of normal animals are shown in B and D. Coronal sections immunostained with an antibody against GFAP. Scale bar (in D): A-D, 100 µm.

Midline ultrastructure in the normal SC and in the tectal lesion cases

In normal animals, ultrastructural examination of the pial processes of tectal midline glia revealed electron-lucent, radiallyoriented profiles that were rich in glycogen granules and mitochondria(see spared radial fibers in Fig. 6, which shows a micrographfrom a lesioned animal). The distal tips of these processes wereenlarged, forming end feet that attached at the basal lamina.On P6, small unmyelinated axons, many of which were likely collateralarbors of normal retinotectal fibers, could be identified, clusteredin the upper layers of the developing SC; near the midline, thesefibers were abutted against the radial processes. In experimentalanimals that had been subjected to heat-induced unilateral tectallesions, ultrastructural examination documented a close interactionbetween axons and non-neuronal cells. This was especially evidentin the tissue bridge that formed above the necrotic colliculartissue; immature glial processes that invaded this region hadthe ability to actively extend long ramified processes. The axonsand their growth cones were closely apposed to these processes(Fig. 7).

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Figure 6. Electron micrograph of the midline roof plate in a hamster <1 d after a tectal lesion. Note the beginnings of the lesion cavity (open arrow) in one region, whereas a normal-looking raphe glial cell (arrowheads), comprised of an electron-lucent process, is still intact nearby. The end foot (EF) is attached at the basal lamina (BL); the basal processes of these cells extend (bottom right) toward the central canal. Scale bar, 1 µm.

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Figure 7. Electron micrographs of the tissue bridge that formed over the superficial SC in P6 animals that had been subjected to an heat lesion of the tectum on P0 or P1. a, Note the bundle of fasciculated axons (large open arrow) located between the glial cells (white arrow) that reconstitute the glial limiting membrane (filled arrows). MAC, Macrophage; BV, blood vessel; LC, lesion cavity. b, Higher magnification of putative growth cone (GC) that has wrapped itself around an axon; in the upper left of the photomicrograph, the basal lamina (BL) on the surface of the tectal tissue is visible. c, Glial process (arrowhead), which may serve as a scaffolding for the growth of axons, that are regenerating across the tissue bridge. d, Close apposition of glial cells within the tissue bridge (curved open arrow), which are connected by adherens junctions, shown at higher magnification in e. Scale bar (in a): a, 10 µm; b-d, 1 µm; e, 0.4 µm.

Undercutting the midline cells

A second approach to damaging the pial processes of the midline glia, one that retained the integrity of the retinorecipienttectal zones, was to undercut the radial cells. This techniqueinvolved the insertion of a tungsten wire at the lateral edgeof the left SC and pushing it medially toward the midbrain septumto sever the distal portions of the raphe glia from the cell bodyand more proximal processes (see Materials and Methods). In mostcases, the wire track encroached slightly into the medial portionof the right SC (Fig. 8A). The right eye was also removed at thetime of surgery. This increased the number of retinal axons thatcrossed over into the denervated (left) SC.

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Figure 8. A horizontally oriented wire was used in this animal to undercut the pial processes of midline glia. The lateral to medial extent of the tract, including the overreach into the right SC (A, B, white arrows), is visible in this section. Note that the track remains below the retinorecipient layers and that within a short time after surgery, the distal processes of midline glia are already beginning to degenerate (d). Scale bars, 100 µm.

Eighteen hours after surgery, the horizontal cut made by the passage of the tungsten wire could be visualized in histologicalmaterial (Fig. 8). Degradation of the severed distal processeswas evident in tissue immunostained with the anti-vimentin antibody(Fig. 8B); however, the lower portions of the radial glial processes(below the wire cut) and the glial perikarya (located near theventricular surface) appeared to remain viable. Over the nextcouple of weeks, the edges of the tissue along the wire trackcame together and could be identified by immunostaining for GFAP(Fig. 9A, arrowheads). The left SC was shrunken because of theremoval of its contralateral retinal input at the time of neonatalsurgery. Labeled retinal axons from the left eye could be followedto their normal zone of termination in the SGS of the right SCand were also seen streaming across the tectal midline into theSGS of the left SC (Fig. 9B,D). Adjacent sections were stainedfor visualizing HRP-labeled retinal axons or GFAP-reactivity.These documented a correlation at the midline between the zonein which severed pial processes of the raphe glia had been disrupted(Fig. 9A,C, double arrows) and the region over which retinal axonswere able to navigate across the midline (Fig. 9B,D). It shouldalso be noted in Figure 9 that at the midline the ventral-mostextent of retinal axons reached no further than the region beyondwhich the basal processes of the glia were intact. Sections fromcontrol animals (data not shown) documented that no recrossingof the midline was seen when the wire stopped short of the rapheglia or when the eye was removed but the midline was not undercut.

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Figure 9. Pairs of immediately adjacent sections through the SC of two P14 brains (A and B from one animal, C and D from the other) in which the midline processes were undercut on P1 and the left SC was denervated by removing the right eye. Coronal sections through the SC were immunostained with an anti-GFAP antibody (A, C) or were reacted with tetramethylbenzidine to visualize HRP-labeled retinal axons originating in the remaining left eye (B, D). The point at which the wire entered the left SC is delineated by gliosis (A, arrowheads), as seen with GFAP immunostaining. Double thin arrows in A and C indicate the point above which the midline processes were severed. In B and D, the distribution of HRP-labeled retinal axons is shown. Note that in both cases, the retinotectal projection to the right SC is targeted to normally retinorecipient layers, and a significant contingent of labeled retinal axons can be traced across the tectal midline into the SGS of the left SC. Open arrows in B and D indicate the position of the tectal roof plate. Scale bar (in D), 200 µm.

In two animals, midline cells were undercut on P1, the right eye was removed, and a solution of DiI was injected in the lefteye via a trans-scleral approach. The animals were perfused onP3, and crystals of DiA were placed along the upper surface ofthe aqueduct of Sylvius to visualize the radial glia in the postnatalSC. Two days later, the DiA labeling revealed the full extentof the radial fibers that had survived the wire cut; in the leftSC, they stretched dorsally from the ventricle, stopping abruptlyjust below the optic fiber layer, at the point where their distalprocesses had been severed by the wire (Fig. 10A,B). At least upto 2 d after surgery, there was no indication of regenerationof the severed pial processes. In the same brains, DiI-labeledretinal axons could be followed from the left eye to the rightSC. It was clear that even within 2 d of undercutting the midlinecells, a few retinal processes had begun to cross the tectal midlineand to enter the wrong (left) SC (Fig. 10C, curved arrows).

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Figure 10. In this animal, the midline was undercut with a wire inserted into the left SC on P1; the wire was extended medially just past the midline (asterisk in A depicts the farthest reach of the wire into the right SC), and the right eye was removed at the time of the undercutting. DiI was injected into the left eye at the same time, and the animal was perfused 2 d later. DiA was placed in the dorsal wall of the ventricle. Coronal sections through the SC of this animal are photographed with a fluorescein filter, which reveals the DiA labeling. In A, the sections are additionally dimly transilluminated to show the tectal surface. The radial glia in the lateral portion of the right SC, lateral to the asterisk, are intact and can are dimly visible as they enter the superficial layers (A). B and C show the same higher magnification view of the section shown in A. B is viewed with a fluorescein filter and shows cut radial glia and midline glia (arrows). C is a double exposure obtained first with use of a fluorescein and then with a rhodamine filter. Thus, in C, the distribution of DiI-labeled retinal axons is seen relative to the cut midline processes. White arrowheads in C point to a retinal axon that has already grown several hundred micrometers into the wrong SC. Curved arrows point to retinal axons where they stream over the midline. Scale bars (in A and C), 100 µm.

Double exposure photography using fluorescein and rhodamine filters documented a complementary relationship between the regionin which the abnormal crossover of retinal axons occurred andthe area over which the cut processes of the midline glia werewithdrawn (Fig. 10). Note that these first few retinal axons thatventured across the midline were not fasciculated but seemed totravel individually; nor did they necessarily show a preferencefor growing along the pial surface, as do the earliest retinalfibers that enter the SC in the normal embryo (Jhaveri et al.,1991a). Recrossing retinal afferents were, instead, distributedthroughout the gap created by the undercutting (Fig. 10C). We wereable to trace a few crossing axons retrogradely from their terminalsin the left SC and found that they also had small collateral branchesin the "correct" SC (data not shown). Thus, it appears that atleast at this early stage, retinal ganglion cell axons fated toterminate in the right SC might expand their target area by branchinginto the left SC but without relinquishing their normal territory.

The recrossing of the tectal midline by retinal axons was robust several days after the midline glia were damaged. By P14,retinal axons from the left eye were found to occupy one-halfto two-thirds of the mediolateral extent of the left SC (Fig.9B,D); moreover, there was no obvious indication at this stagethat they achieved this massive extra projection by a compensatorydecrease in the density of projections to their appropriate terminationzone in the right SC. If both eyes were left intact but the midlineglia were cut, HRP-labeled retinal axons from the left eye terminatedin the right SC and also crossed the midline, but the latter wererestricted to the medial-most portion of the "wrong side" of theSC, indicating that there may be a competition between the twoeyes for tectal terminal space (data not shown) (cf. So and Schneider,1978).

Dorsal view reconstructions of the tectal midline in six animals that had the raphe glia undercut documented that there wasa mismatch between the total extent over which the glial processeswere cut and the total extent over which retinal axons were detectedcrossing to the wrong SC. As illustrated in Figure 11, for allsix cases the extent of the gap created by disruption of the gliawas larger than the region of crossover of retinal fibers. Gapsvaried in length from 300 to 960 µm, whereas the distance overwhich retinal fibers traversed ranged from 240 to 800 µm. Thisresult was qualitatively verified in additional cases for whichthe midline was not reconstructed.

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Figure 11. Schematic dorsal view reconstructions of the tectal midlines from animals (ages P12 and P14 at time of perfusion) that had the raphe glia undercut on P1. The number of sections through the rostral (R) to caudal (C) extent of each SC was counted; the extent of the midline is depicted along a line (arbitrary units). The region of each midline along which the distal processes of the raphe glia were observed as being intact is marked with hatching; the extent of each midline where the pial processes were disrupted is depicted with a thick straight line; the region of each midline over which retinal axons were seen crossing abnormally to the opposite side is marked with Xs. Numbers (in arbitrary units) representing the length of the rostrocaudal extent of the undamaged region for the gap (Gap) created by disrupting the midline glia and for the length of the midline over which retinal axons are seen crossing (Xng) are indicated. The length (in micrometers) for the disrupted region (Gap) and for the distance over which retinal crossover is observed (Cross) are provided at the bottom of each reconstruction.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The spatiotemporal deployment of a group of glial cells at the tectal midline would permit them to subserve the unilateralconfinement of retinotectal axons in normal animals (Fig. 12A)(Raedler et al., 1982; Barradas et al., 1989; Harvey et al., 1993;Wu et al., 1995). Lesion of one SC leads to an abnormal crossingof retinal afferents but only if the tectal midline is disrupted(Mustari and Lund, 1976; Hsiao and Schneider, 1978; Jen and Lund,1979; Schneider et al., 1985). Here, we use two early lesion paradigmsto document the direct involvement of the tectal raphe glia inthe containment of retinal axons. With both perturbations, glialprocesses degenerate and retinal axons cross the collicular midline(Fig. 12B).

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Figure 12. Cartoon summary of conclusions from this study. Left, The course of retinal axons as they leave the eye, pass through the lateral geniculate body, and approach the tectal midline is shown. Retinal axons stop at the midline glia, and the laterality of the retinotectal projection is maintained in normal animals. Right, The midline cells have been undercut in the neonatal animal, and one eye is removed. This releases the midline blockade, and a crossover of retinal axons to the opposite SC is seen in the region in which pial processes of the midline glia have been damaged.

Cells that colonize the midline of the neuraxis

There is considerable speculation about the role of specialized cells in forming barriers against migrating neurons or againstgrowing axons (Joosten and Gribnau, 1989; Silver et al., 1993;Heyman et al., 1995; Brunso-Bechtold and Henkel, 1996). In thespinal cord, interactions between gene products of the bone morphogeneticprotein 4, sonic hedgehog, and related genes (Liem et al., 1995;Jordan et al., 1997) may determine the formation of the roof plateand floor plate and affect growth patterns of sensory and motorprojections (Ruiz i Altaba and Jessell, 1993; Dosch et al., 1997;Knecht and Harland, 1997; Mehler et al., 1997). Floor plate cellsexpress a chemotropic factor that attracts axons of commissuralneurons toward the midline (Tessier-Lavigne et al., 1988; Kennedyet al., 1994; Colamarino and Tessier-Lavigne, 1995a). Roof plateglia are implicated in blockading dorsal column fibers from contralateralencroachment (Snow et al., 1990a,b). Cells in the optic chiasmare involved in the guidance of temporal and nasal retinal axons(Silver, 1984; Godement and Mason, 1993; Wizenmann et al., 1993).Specialized glia also form boundaries in regions that lie offthe midline (Steindler et al., 1990; Silver et al., 1993; Steindler,1993; Heyman et al., 1995). However, apart from the work on thecrossing of ventral commissural axons through the floor plate,the relationship between midline cells and the guidance of axonsthat encounter them has been correlative. Here, we show a causalrelationship between disruption of the tectal midline glia anda rerouting of retinotectal afferents.

Permissive versus inductive mechanisms for retinal axon crossing

After heat damage to the developing SC, a membranous bridge forms over the necrotic tissue (So and Schneider, 1978; So, 1979;Harvey et al., 1986). This structure is rich in GFAP-positiveglial processes, many of which have a close spatial relationshipwith growing tectal afferents (Figs. 3D, 6, 7). Glia that invadethe bridge likely provide the substrate on which retinal axonsnavigate across the tectal midline. Because we never see a bridgewithout retinal axons coursing along it, its substrate is likelyboth permissive and instructive for the growth of retinotectalafferents. However, such an influence is not easy to quantifybecause of technical difficulties in retaining bridge tissue duringhistological processing. Retinal axons also cross via a secondroute, under the necrotic tissue, through the area in which themidline glia have been undercut. Midline reconstructions revealthat the region of damage and the region over which retinal axonscross are not coextensive. The axons occupy only a fraction ofthe gap in the roof plate and do not grow across any part of thetectal midline where the raphe glia are not disrupted. Collectively,these observations indicate that disruption of glial processesleads to the formation of a permissive, but not instructive, substratefor the growth of immature retinal axons (So and Schneider, 1978;Kapfhammer et al., 1992). Thus, additional signals must be involvedin determining exactly where retinal axons travel within the disruptedzone (see below).

Specificity of glial barriers and putative molecular bases for the barrier

A critical question concerns the specificity of glial barriers in relation to different axon systems. Barriers that blockgrowth of only certain fiber populations and ones that universallyblock all growing fibers may function in the brain. For instance,retinotectal axons do not cross the tectal midline, but contralaterallyprojecting fibers in the tectal commissure are able to successfullynavigate across this region. This may be either because each systemis differentially responsive to the midline glia, or because intertectalaxons cross the midline before glial differentiation (Jhaveri,1993a,b) and before the expression of putative inhibitory moleculesalong the tectal roof plate. Similarly, dorsal spinal commissuralaxons cross the roof plate after the ingrowth and unilateral compartmentalizationof sensory axons in dorsal columns when putative axon-inhibitorymolecules are no longer detected along the roof plate. These observationssuggest that the barrier function of midline cells might be universaland that if axon systems were to bypass the blockade, they wouldbe compelled to grow through before its functional maturationor after its ephemeral expression of inhibitory molecules hasdiminished. One could argue that selective decussation of nasal(but not temporal) retinal axons at the optic chiasm belies thisnotion: axons from nasal and temporal retina approach the ventralmidline at approximately the same time, but each interacts differentiallywith chiasm cells (Godement and Mason, 1993; Sretavan et al.,1994). However, ipsilateral deflection of temporal axons occursearly during chiasm formation (Drager, 1985; Reese and Colello,1992; Baker and Reese, 1993); later, both temporal and nasal retinalaxons project contralaterally, again invoking temporally variablefactors in the decision to cross or not. Also, ipsilaterally directedcorticotectal axons cross the tectal midline after deafferentationof the contralateral colliculus but in the absence of any damageto the midline glia (Mustari and Lund, 1976; Jen et al., 1978;Rhoades and Chalupa, 1978; Land et al., 1984); however, the expandedcorticotectal projection crosses the midline at deeper levelsof the SC (Jen et al., 1978; Harvey and Worthington, 1990), whereretinal fibers do not normally reach.

The molecular bases for tectal midline barrier functions are unknown, but PGs have been incriminated. In vivo, some PGs arepresent in regions in which axons do not grow (Snow et al., 1990a,b;Cole and McCabe, 1991; McKeon et al., 1991; McCabe and Cole, 1992;Gonzalez et al., 1993; Pindzola et al., 1993; Silver et al., 1993;Heyman et al., 1995; Brunso-Bechtold and Henkel, 1996; Jhaveriand Hoffman-Kim, 1996; Reese et al., 1997). In the developingSC, sulfated PGs are detected in tissue harvested from the midline(where retinal axons do not grow) and also from the lateral tectum(where retinal axons do extend). Biochemical characterizationshows that PG core proteins are similar at the tectal midlineand laterally but that those along the midline are more heavilyglycosylated (Hoffman-Kim et al., 1996, 1998). This suggests thatthe glycosaminoglycans, and not the protein cores, are likelyparticipants in the barrier function. In vitro observations ofretinal explants growing on glial carpets also confirm that theglia harvested from the midline region are less supportive ofretinal axon extension (Young et al., 1997). Thus, it is likelythat PGs on glial cells or in the extracellular matrix surroundingglial cells subserve the avoidance of the tectal midline by retinalaxons. Garcia-Abreu et al. (1995, 1996) document a differentialPG content in glia harvested from the middle versus lateral thirdsof the midbrain and show that tectal neurons exhibit differencesin neurite outgrowth patterns on the two types of glia.

Diffusible molecules such as netrins, secreted by floor plate cells, can act as chemoattractants and chemorepellants to guidethe growth of specific afferent systems (Colamarino and Tessier-Lavigne,1995b). Mice deficient in netrin (Serafini et al., 1996; Guthrie,1997) or its receptor (Fazeli et al., 1997) show disrupted decussationof some axons but not of others, indicating a specificity of responsesby different afferents to this class of molecules. A diffusiblefactor that repels commissural axons has been reported for thespinal cord roof plate (Augsburger et al., 1996), which must actin concert with chemoattractants released by the floor plate toguide the growth of the ventrally crossing fibers. For the hamsterSC, evidence points to an inhibitory role for PGs (membrane boundor secreted into the extraneuronal matrix) in relation to retinalaxon growth (see above). However, the observation that retinalaxons do not completely fill the gap created by disruption ofthe midline glia (Fig. 11) suggests that, at least in animals witha damaged midline, a second diffusible chemorepellant substancereleased by these glia is also at work. If such a diffusible factordoes emanate from the roof plate, perhaps it is not a very potentplayer during the normal development of the retinotectal fibersgiven the fact that many of these fibers encroach so close tothe tectal midline. Finally, the recent discovery of genes suchas robo (Kidd et al., 1998a,b) and sax3 (Zallen et al., 1998)demonstrates that the genetic make-up of afferent neurons, andnot just the molecular composition of the extraneuronal environment,is an additional factor in determining whether or not successfuldecussation of axons can take place.

  FOOTNOTES

Received Dec. 31, 1997; revised July 23, 1998; accepted July 30, 1998.

This work was supported by National Institutes of Health Grants EY00126 (G.E.S.), EY05504 (S.J.), and EY02621 (Vision CoreGrant). We thank Chrysty Remillard for help with the photographyand Dr. Alan Harvey for discussions on interactions of nonretinalafferents with the tectal midline.
Correspondence should be addressed to Dr. Sonal Jhaveri, Department of Brain and Cognitive Sciences, E25-642, MassachusettsInstitute of Technology, Cambridge, MA 02139.

Dr. Wu's present address: University of Southern California School of Medicine, Department of Cell and Neurobiology, Los Angeles,CA 90033

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