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Previous Article | Next Article
The Journal of Neuroscience, March 15, 2000, 20(6):2287-2294
DM-GRASP Is Necessary for Nonradial Cell Migration during Chick Diencephalic Development
Daniel S. Heffron and Jeffrey A. Golden Department of Pathology, Children's Hospital of Philadelphia and the University of Pennsylvania School of Medicine, Philadelphia, Pennsylvania
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Cell migration is fundamental to normal CNS development. Radial migration, along radial glial fibers, has been the principal pathway studied, however, nonradial or tangential cell migration has increasingly been identified at all levels of the CNS. Receptors, cell adhesion molecules, and extracellular matrix molecules have all been shown to participate in radial cell migration. In contrast, the molecular basis of nonradial cell migration has only recently begun to be elucidated. Using replication defective retroviral vectors we have determined the location and time when nonradial cell migration begins in the developing chick diencephalon. We have identified three molecules that are expressed in spatially and temporally restricted domains that are consistent with them playing a role in nonradial cell migration. One of these molecules, DM-GRASP, a transmembrane protein with five extracellular Ig domains, is expressed on the nonradially migrating cells in addition to axons. To test the hypothesis that DM-GRASP participates in guiding nonradial cell migration, we injected a replication-defective retroviral vector used for lineage tracing followed by a DM-GRASP blocking antibody. Embryos injected with the blocking antibody showed a near complete block in nonradial cell migration specifically where DM-GRASP is expressed. Furthermore, morphological analyses revealed disruption of the normal architecture of the diencephalon indicating nonradial cell migration is necessary for normal morphological development of the brain. Our data indicate that DM-GRASP is necessary for nonradial cell migration in the chick diencephalon and have provided a system to further explore the function of nonradial cell migration during CNS development.
Key words: nonradial cell migration; tangential cell migration; DM-GRASP/BEN; diencephalon; chick; CNS
INTRODUCTION
One of the remarkable features of CNS development is the extensive cell migration that occurs from the site where progenitor cells reside to where a postmitotic, terminally differentiated cell resides in the mature brain. Neurons and glia are derived predominately from progenitor cells located adjacent to the lumen of the neural tube. These regions, known as the ventricular zone (VZ) and subventricular zone (SVZ), are composed of proliferating cells. The two daughter cells resulting from a cell division may each re-enter the cell cycle, one may re-enter the cell cycle and the other may leave the cell cycle, or both may exit the cell cycle. Those cells that exit the cell cycle begin differentiation. As cells differentiate, they also migrate away from their site of birth to where they will reside in the mature nervous system.
Two major pathways of cell migration have been identified during early development; radial, from the ventricular zone out toward the surface of the neural tube, and nonradial or tangential, which is parallel to the surface of the neural tube. Radial migration was the first pathway of migration to be identified and subsequently is the best characterized. Radial cell migration is also known as glial-guided cell migration because the neuroblasts migrate along specialized glial cells known as a radial glia (Rakic, 1990
; for review, see Hatten, 1999
In contrast to radial cell migration, relatively little is known about the guidance of nonradial (also defined as tangential) cell migration. Nonradial cell migration has been observed at virtually every level of the developing nervous system including the spinal cord (Leber et al., 1990
The molecular and cellular mechanisms that direct cells to leave their radial pathway and move along nonradial pathways are beginning to be characterized. Using a library of replication-defective retroviruses we have previously determined the time during development and the location within the wall of the neural tube where nonradial migration begins in the chick diencephalon (Golden et al., 1997
DM-GRASP was identified as a candidate molecule because it was found to have the expression pattern predicted for a molecule that would participate in nonradial cell migration. DM-GRASP is a type I transmembrane protein with five Ig-like domains and many putative N-glycosylation sites on the N-terminal end (Burns et al., 1991
MATERIALS AND METHODS
Retroviral labeling. A replication-defective avian retrovirus, CHAP (a gift from Dr. C. Cepko), which encodes human placental alkaline phosphatase in place of the viral gag and pol genes, was produced according to published protocols (Ryder and Cepko, 1994
Embryos injected with LZ12 were fixed and processed as described above except that they were cut at 20 µm and they were not incubated at 65°C. After washing in PBS, the embryos were placed directly into 1 mg/ml 5-bromo-4-chloro-3-indolyl-galactoside (Sigma) made in detection buffer (35 mM ferricyanide, 35 mM ferrocyanide, and 5 mM MgCl2 in PBS). Embryos were incubated overnight and then washed three times in PBS. Embryos with infection in the diencephalon were further processed and cryosectioned for light microscopic examination as described above and immunohistochemistry as described below.
Antibody injections. DM-1 and DM-2 hybridomas were a gift from Dr. Susannah Chang. Blocking (DM-2) or control (DM-1) hybridoma supernatant was centrifuged and filtered through a 0.2 µm membrane. Fast green dye was added to the supernatant at a final concentration of 0.0125%. The antibody was injected into a vitelline vein on the surface of the yolk at a rate of 3-5 µl/min through a heat-pulled micropipette attached to a 100 µl Hamilton syringe. Approximately 12 µl was injected on E4 and 16 µl on E5, followed by harvesting on E6. DM-1 and DM-2 were also concentrated with a protein-A column and dialyzed against PBS to an estimated concentration of 500 µg/ml. Four microliters of the concentrated antibody were injected on E4 and 6 µl on E5. The injection of smaller volumes of concentrated antibody appeared to improve embryo survival. For those embryos harvested on E10 and E14, in addition to the injection of antibody on E4 and E5, 20 µl was injected on E6.
Immunohistochemistry. Cryosections prepared as described above for viral histochemistry were rinsed in PBS, and sections were blocked in 10% goat serum, 0.1% Tween-20 in PBS, and incubated in primary antibody for 1 hr at room temperature to overnight at 4°C. Primary antibodies included Tuj1 (neuron-specific class III tubulin; Geisert and Frankfurter, 1989
Antibodies injected in vivo were detected by fixing and processing the embryos as described above. Sections were rinsed in PBS and blocked as described above. After blocking, the embryos were incubated directly in the appropriate secondary followed by washing in PBS and then coverslipped with Vectashield. Sections were again examined with a Zeiss Axioplan microscope equipped with epifluorescence.
Histology. Antibody injected or control E10 and E14 brains were quickly dissected out in PBS and fixed overnight in 4% paraformaldehyde in PBS at 4°C. Brains were then rinsed in PBS, dehydrated, and infiltrated with paraffin without vacuum. The brains were then oriented in paraffin blocks and cut coronally at 7 µm on a Zeiss microtome. Sections were collected and baked on Superfrost/Plus slides (Fisher Scientific) at 37°C overnight. Sections were then deparaffinized, rehydrated, stained with hematoxylin and eosin according to standard protocols, coverslipped with Permount (Fisher Scientific), and examined with a Nikon E400 microscope.
BrdU incorporation studies and TUNEL assays. Embryos injected with DM-1 or DM-2 antibody as described above were injected with BrdU solution on E7, E8, or E10. A 30 gauge needle was used to inject 100 µl of a 10 µg/ml solution of BrdU in sterile PBS into the amniotic sack. Embryos were harvested into 4% paraformaldehyde 30 min after injection. Cryosections were prepared as above. BrdU was detected by incubating cryosections in 2N HCl for 1 hr at 37°C. Slides were rinsed five times in PBS and incubated for 1 hr in primary antibody (G3G4; Developmental Studies Hybridoma Bank) diluted 1:50 in 1% bovine serum albumin, 1% DMSO, 0.1% Triton X-100, and 10% goat serum in PBS. Primary antibody was detected as described above. Cell death was assayed by injecting embryos with DM1 or DM2 antibody then harvesting on E7, E8, and E10 as described above. TUNEL assays were performed on cryosections of these embryos as previously reported (Golden et al., 1999
RESULTS
Candidate molecules for guidance of nonradial cell migration in the developing CNS were defined as those expressed in a pattern coincident with the onset of nonradial cell migration (Golden et al., 1997
2-laminin (data not shown). Although DM-GRASP is located on subsets of axons before and on E4 (Chédotal et al., 1995
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Figure 1. Immunofluorescence with an antibody to DM-GRASP/BEN. On E4, no staining is seen in the wall of the diencephalon (A, DAPI staining to show location of diencephalic wall; B, secondary antibody conjugated to Texas Red), although occasionally small axons were seen coursing dorsal to ventral. By E5 DM-GRASP/BEN is expressed at high levels outside the VZ (C, red fluorescence). At higher magnification (D) individual cells are decorated with the DM-1 antibody (arrows). V, Ventricle.
A functional blocking antibody (DM-2) and a nonblocking antibody (DM-1) to DM-GRASP were previously characterized (Burns et al., 1991
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Figure 2. An embryo intravascularly injected at E6 with DM-2 and harvested 12 hr later shows localization of DM-GRASP/BEN on cells (arrow) outside the VZ (compare with Fig. 1c). Sections were treated with secondary antibody conjugated to FITC after fixation and cryosectioning. V, Ventricle.
DM-2 blocks axons from growing out along other axons (Burns et al., 1991
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Figure 3. Axons were immunolabeled with Tuj1, indicating that DM-2 treatment did not disrupt early axon growth through the diencephalon (arrow points to labeled axons). Embryos were treated on E4 and E5 with DM-2 and evaluated on E7. V, Ventricle.
We next investigated whether DM-2 blocked nonradial cell migration. Stage 10-13 embryos were injected with a replication-defective retroviral vector (Golden et al., 1995
The injection of DM-2 specifically blocked nonradial cell migration in the diencephalon (Fig. 4, Table 1). Nonradial dispersion of cells was seen in approximately one-third of all clones after PBS injections (Table 1). Embryos injected with DM-1 showed nearly a third of clones with both radial and nonradial cell dispersion, similar to the distribution of clones in control embryos (Table 1). In contrast, embryos injected with DM-2 showed only two clones with nonradially dispersed cells. Furthermore, the two clones with nonradial cell migration were found in the most ventral aspect of the diencephalon where DM-GRASP is not expressed. The three groups (no antibody, DM-1, and DM-2) were compared by
2 analysis, and the difference between these groups was found to be statistically significant (
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Figure 4. Embryos injected with DM-1 or no antibody (A, B) showed clones (identified with the LZ12 retrovirus) with both radial and nonradial cell dispersion. The ventricle is at the bottom (defined by the bottom series of black dots), and the pial surface is at the top (defined by the top series of black dots) in each image. Radial clones span from the VZ at the bottom of each image toward the top. Nonradial cell dispersion (arrows) was identified in approximately one-third of all clones (A, B). Only radial clones were found in embryos treated with DM-2 (C, D; with two exceptions, see Results).
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Table 1. Number (and percentage) of clones showing radial (Radial) migration alone or radial and nonradial (Nonradial) cell dispersion after embryos were injected with control media (No Antibody), DM-1, or DM-2 The disruption in nonradial cell migration did not affect radial cell migration. Greater than 90% of clones, despite the presence or absence of nonradial cell dispersion, showed radial dispersion from the ventricular zone independent of whether the embryo was exposed to DM-1, DM-2, or no antibody. Occasional clones (~8%) showed cells restricted to the ventricular zone indicating no radial migration had occurred. Given that clones restricted to the ventricular zone were found in approximately equal proportions in treated and untreated embryos, radial cell migration appears unaffected. Embryos injected with DM-1 showed similar numbers of both radially and nonradially distributed clones when compared to control embryos. In contrast, nonradial cell dispersion was not observed in the dorsal diencephalon in any embryo injected with DM-2.
Nonradial cell migration was specifically blocked in the diencephalon of chick embryos. Examination of the mesencephalon (tectum), where nonradial cell dispersion has also been observed in chick embryos (Gray and Sanes, 1991
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Figure 5. Nonradial dispersion of cells (arrows) is observed in the tectum of DM-2-treated embryos where DM-GRASP is not expressed at this developmental time (clones identified by alkaline phosphatase histochemistry after CHAPOL retroviral infection).
Because the injection of DM-2 inhibited nonradial cell migration, the morphological consequences of blocking this pathway of migration were examined in E10 and E14 embryos. After injection of antibody on E4, E5, and E6, embryonic brains were fixed, sectioned, and stained with hemotoxylin and eosin. Embryos injected with DM-1 showed no morphological abnormalities (Fig. 6) when compared to control embryos. In contrast, embryos injected with DM-2 showed a disruption in the normal anatomy and size of the diencephalon (Fig. 6). Despite the severe cytoarchitectural abnormalities, the disruption appeared specific. For example, the ventral lateral geniculate nucleus appeared to be preserved in embryos injected with DM-2, whereas the nucleus rotundum and other dorsal nuclei were absent or markedly distorted. The dorsal diencephalon was specifically affected, whereas the tectum and cerebellum appeared normal. Occasional brains showed anomalies of the telencephalon, however, we have focused on the diencephalon where we could correlate the morphological studies with our studies of lineage and clonal dispersion (Golden and Cepko, 1996
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Figure 6. Histological sections of the diencephalon of E10 embryos treated with DM-1 (right) or DM-2 (left). Both sections are taken at approximately the same anatomic level. Embryos injected with DM-1 showed normal diencephalic morphology, whereas those injected with DM-2 had a small diencephalon, loss of neuropil, and poorly organized nuclear groups. This is particularly true for the dorsal nuclei. The ventral nuclei (e.g., ventral lateral geniculate body; vLG) were somewhat better preserved although small, whereas the dorsal nuclei (e.g., nucleus rotundum, R; dorsal lateral, DL; and dorsal medial, DM) nuclei could not be delineated. Furthermore, the sulcus limitans (arrowhead) was extremely deep in DM-2-treated embryos compared to controls or embryos treated with DM-1.
The diencephalon was found to be both small and the morphology was disrupted. The small size of the diencephalon raised the possibility that the injection of DM-2 antibodies specifically interrupted cell proliferation and/or led to increased cell death. To determine if cell death was increased by injection of the DM-2 antibody, TUNEL assays were performed to assess the amount of cell death after injection of no-antibody, DM-1, or DM-2. No qualitative difference was observed between embryos injected with PBS, DM-1, or DM-2 (Fig. 7). A higher percentage of cells were labeled with the TUNEL technique on E8, when compared to E7, however, this was in embryos from all experimental groups, indicating a normal increase in cell death in the diencephalon during development (Fig. 7). The number of TUNEL-positive cells was again low on E10 (Fig. 7).
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Figure 7. TUNEL assay on sections through the diencephalon of E7, E8, and E10 embryos after injection of either DM-1 or DM-2. No difference was observed in the pattern or number of TUNEL+ cells between these two experimental groups or those injected with PBS alone. A slight increase in the number of TUNEL-positive cells was observed at E8 in all of the experimental groups. These data likely reflect the normal programmed cell death that occurs in the diencephalon during development.
To determine if cell proliferation was inhibited by the antibody injections, BrdU incorporation studies were performed. Immunofluorescent staining for BrdU again showed no qualitative difference in the number of labeled cells after injection of no antibody, DM-1, or DM-2 (data not shown). A review of the E10 and E14 hematoxylin- and eosin-stained sections indicates a greater density of cell nuclei in the diencephalon. These data suggest that the DM-2 antibody may have pleotropic affects that include blocking nonradial cell migration and other developmental processes that result in the abnormal morphology of the diencephalon.
DISCUSSION
Two patterns of cell migration are recognized during early development of the CNS, radial and nonradial. These two patterns of cell migration have been observed at all levels of the neural axis, suggesting they are both essential components of development (Baehr et al., 1988
DM-GRASP is a type I transmembrane protein and a member of the Ig superfamily (Burns et al., 1991
Other molecules have also been shown to bind to DM-GRASP (Bowen et al., 1995
Our data suggest that cell migration along nonradial pathways is required for normal morphological development of the diencephalon. Given the marked differences in size between the DM-1- and DM-2-treated embryos, we first addressed whether the morphological disruption resulted from increased cell death or a decrease in cell proliferation. Our data indicate that a marked increase in cell death did not result from injection of the DM-2 supernatant. A qualitative difference in cell proliferation was also not observed; however, we did not test whether our treatment altered the length of the cell cycle. An increased density of cells was noted in the diencephalon of embryos exposed to DM-2 (D. Heffron and J. Golden, unpublished observations). These data suggest that the disruption of the diencephalon is primarily a result of blocking nonradial cell migration, however, DM-2 may have additional effects on diencephalic development that are also reflected in the morphological phenotype.
The disruption of nonradial cell migration resulted in abnormal nuclear organization. The diencephalon, like the midbrain and hindbrain, is organized into discrete collections of neurons known as nuclei. Each nucleus has a specific function, set of functions, or defined neurochemical transmitter. Our data indicate that nonradial cell migration is required in at least the diencephalon for the organization of these functional neuronal groups. The dorsal diencephalon was particularly affected while some nuclei of the ventral diencephalon could be defined. Given that DM-GRASP is expressed preferentially in the dorsal diencephalon, the data on nuclear disorganization appears to correlate with this expression. Furthermore, the two clones that showed nonradial cell migration were located ventrally where nuclear organization was better preserved and DM-GRASP is not expressed.
Our data imply other molecules are likely to participate in the guidance of nonradial cell migration in other regions of the CNS. As noted above, nonradial cell migration has been identified at virtually every level of the developing nervous system. We have observed nonradial cell migration in the tectum and in two clones in the ventral diencephalon in embryos injected with the DM-GRASP blocking antibody. Given that DM-GRASP is not expressed in these areas at the time of development we have studied, it was not surprising for nonradial migration to appear normal in these regions of the neural tube. However, this does imply that distinct molecules will control nonradial cell migration in various regions of the neural tube.
The role of nonradial cell migration during CNS development has been an open subject. In the mouse telencephalon at least some cortical GABAergic interneurons are derived from the ganglionic eminence and must migrate tangentially into the cortex (Anderson et al., 1997
The rostral migratory stream is a specialized route of cell migration (Lois et al., 1996
Our data provide insight into both the role of nonradial cell migration in the chick diencephalon and a first step toward elucidating the molecular and cellular guidance mechanisms for this pathway of cell movement. The role and mechanisms of nonradial cell migration in other regions of the nervous system remains to be determined. Identifying the molecules involved in guiding nonradial cell migration will allow additional studies that will begin to answer some of these provocative questions. Additional genetic studies, disrupting these genes in mice or zebrafish, are also likely to provide valuable information into the role of nonradial cell migration during development. Finally, the identification of DM-GRASP as a necessary molecule for nonradial cell migration will allow us to begin identifying other components of this cellular pathway. Knowing that DM-GRASP can interact with Ng-CAM (DeBernardo and Chang, 1996
FOOTNOTES Received Aug. 18, 1999; revised Dec. 8, 1999; accepted Jan. 5, 2000.
This work was supported by the Klingenstein foundation and the National Institutes of Health. We would like to thank Dr. S. Chang for providing us with the DM-1 and DM-2 antibodies. Dr. J. Sanes kindly provided the LZ-12 producing cell line. The 5E1 and 8D9 antibodies were provided by the Developmental Studies Hybridoma Bank, University of Iowa. We thank the members of the Golden laboratory and Dr. D. Pleasure for their constructive criticism.
Correspondence should be addressed to Jeffrey Golden, Department of Pathology, Abramson Research Center, Room 516c, Children's Hospital of Philadelphia, 3400 Civic Center Boulevard, Philadelphia, PA 19104. E-mail: goldenj{at}mail.med.upenn.edu.
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