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Previous Article | Next Article
The Journal of Neuroscience, July 15, 1999, 19(14):5990-6005
Site-Specific Migration and Neuronal Differentiation of Human Neural Progenitor Cells after Transplantation in the Adult Rat Brain
Rosemary A. Fricker1, 2, Melissa K. Carpenter3, 4, Christian Winkler1, Corinne Greco3, Monte A. Gates1, 2, and Anders Björklund1 1 Wallenberg Neuroscience Center, Division of Neurobiology, Lund University, S-223 Lund, Sweden, 2 Department of Neurology, Harvard Medical School, Children's Hospital, Boston, Massachusetts 02115, 3 CytoTherapeutics, Lincoln, Rhode Island 02865, and 4 Geron Corporation, Menlo Park, California 94025
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Neural progenitor cells obtained from the embryonic human forebrain were expanded up to 107-fold in culture in the presence of epidermal growth factor, basic fibroblast growth factor, and leukemia inhibitory growth factor. When transplanted into neurogenic regions in the adult rat brain, the subventricular zone, and hippocampus, the in vitro propagated cells migrated specifically along the routes normally taken by the endogenous neuronal precursors: along the rostral migratory stream to the olfactory bulb and within the subgranular zone in the dentate gyrus, and exhibited site-specific neuronal differentiation in the granular and periglomerular layers of the bulb and in the dentate granular cell layer. The cells exhibited substantial migration also within the non-neurogenic region, the striatum, in a seemingly nondirected manner up to ~1-1.5 mm from the graft core, and showed differentiation into both neuronal and glial phenotypes. Only cells with glial-like features migrated over longer distances within the mature striatum, whereas the cells expressing neuronal phenotypes remained close to the implantation site. The ability of the human neural progenitors to respond in vivo to guidance cues and signals that can direct their differentiation along multiple phenotypic pathways suggests that they can provide a powerful and virtually unlimited source of cells for experimental and clinical transplantation.
Key words: progenitor cells; human; transplantation; neuron; subventricular zone; dentate gyrus; striatum
INTRODUCTION
The limited capacity for structural repair in the mammalian brain is in part explained by the inability of the mature CNS to generate new cellular elements in response to damage. Cell transplantation offers a possibility to circumvent this limitation. Both rodent and primate experiments show that neuroblasts and young postmitotic neurons obtained from defined parts of the neuraxis during development can survive, mature, and grow extensive functional axonal connections after transplantation to brain-damaged recipients, and both structurally and functionally replace lost neurons in the mature brain (for review, see Dunnett and Björklund, 1994
). Because of the limited migratory capacity of the differentiated cells, however, these types of implants are unable to integrate into the cellular architecture of the host.
Previous studies have shown that less differentiated precursor cells, taken at premigratory stages of neuronal development, can make use of available substrates or pathways for migration, mix with endogenous pools of precursors, and participate in ongoing neurogenesis, both during development (McConnell, 1988
Recently, neural progenitors with the capacity to give rise to all major cell types of the mature CNS have been isolated from the developing or adult CNS (Weiss et al., 1996b
Here, we have examined the question of whether progenitors isolated from the developing human CNS can exhibit in vivo neurogenic properties after implantation into the brain of adult recipients. Cells obtained from the forebrain of 6.5- to 9-week-old human fetuses were maintained as continuously dividing cultures in the presence of EGF, bFGF, and leukemia inhibitory growth factor (LIF). Cells expanded 103-107-fold in culture (over 9-21 passages) survived well after transplantation to both neurogenic and non-neurogenic sites; cells contained within these grafts showed migration, integration, and site-specific differentiation into both neurons and glia.
MATERIALS AND METHODS
Generation and in vitro culture of human progenitor cells. Generation of the human progenitor cell lines has been described previously (Carpenter et al., 1999
The cells grew as free-floating clusters ("neurospheres"), and were prevented from attachment by gently knocking the flasks each day. Any cells that adhered to the plastic and began to extend processes were not removed by this procedure and therefore were not carried through to the next passage. The spheres were passaged by mechanical dissociation every 7-10 d and reseeded as single cells at a density of ~100,000 cells/ml. The cells used for transplantation (the 6.5FBr and 9FBr cultures) had been expanded over 9-21 passages, which corresponds to a total increase in cell numbers of ~103 at 9 passages to at least 107 at 21 passages (Carpenter et al., 1999
Labeling methods and preparation of cells for transplantation. To enable the detection of the cells in vivo, cultures were labeled with 1 µM bromodeoxyuridine (BrdU), which was added to the culture medium 48 hr before the preparation of the cells for transplantation. This resulted in ~80% labeling efficiency, with no apparent changes in growth rate of the spheres.
Cells were taken for transplantation 4-5 d after the last passage as small spheres of 5-30 cells. The spheres were collected by centrifugation at 1000 rpm for 3 min and resuspended in 1 ml DMEM/F12 medium. To check the cell viability, an aliquot of the sphere suspension was removed and mixed with trypan blue. After this was ascertained, a second cell count was performed by triturating the trypan blue aliquot to give single cells. The sphere suspension was centrifuged a second time and resuspended in a smaller volume to give the equivalent of ~100,000 cells/µl.
Transplantation. Adult female Sprague Dawley rats (B&K Universal, Stockholm, Sweden), weighing ~250 gm at the beginning of the study, were used. They were caged in groups of two and maintained on a 12 hr light/dark cycle with constant temperature and humidity, with ad libitum food and water. The animals were immunosuppressed throughout the experiment by daily injections of 10 mg/kg cyclosporin, beginning 1 d before transplantation.
Stereotaxic surgery was performed under deep equithesin anesthesia (3 ml/kg body weight, i.p.). Rats received 1 µl cell suspension bilaterally in either the SVZa, rostral migratory stream (RMS), or hippocampus, or 2 µl in the striatum, according to the following coordinates: SVZa, anterior (A) = +1.6, lateral (L) = ±1.5, ventral (V) =
4.2; RMS, A = +3.7, L = ±1.5, V =
Tissue processing. At either 2 or 6 weeks after transplantation, rats were terminally anesthetized with 5% chloral hydrate and transcardially perfused with 0.1 M PBS followed by 5 min rapid fixation with ice-cold 4% paraformaldehyde (PFA) in 0.1 M phosphate buffer. Brains were removed and placed in PFA overnight, before being transferred to 25% sucrose in PBS. Coronal or sagittal sections were cut on a freezing microtome at a thickness of 30 µm. In each case, eight series were collected for further processing.
Immunocytochemistry. For BrdU labeling, all sections were pretreated with 1 M HCl for 30 min at 65°C. Sections were incubated in primary antibodies for 36 hr at 4°C. All primary antibodies were diluted in 0.02 M potassium PBS (KPBS) containing 5% normal serum of the species in which the secondary antibody was raised and 0.25% Triton X-100, except for 32 kDa dopamine- and cAMP-regulated phosphoprotein (DARPP-32) and
-amino decarboxylase (GAD67) in which Triton X-100 was omitted. Antibodies used in this study were BrdU rat monoclonal (1:100, Chemicon, Temecula, CA), mouse monoclonal (1:25, Becton Dickinson, Franklin Lakes, NJ,),
-tubulin-III (1:400, Sigma), calbindin (1:1000, Sigma), DARPP-32 (1:20,000; Dr. P. Greengard, Rockefeller), GAD67 (1:1000, Chemicon), glial fibrillary acidic protein (GFAP, 1:500, Dakopatts), RNA binding protein (Hu, 1:1000; Dr. S. Goldman, Cornell), neuronal nuclei (NeuN, 1:100, Chemicon), tyrosine hydroxylase (TH, 1:500, PelFreeze, Rogers, AR), Vimentin (VIM, 1:25, Dakopatts), and human-specific tau (hTau, 1:100, Calbiochem, La Jolla, CA). For all immunohistochemical procedures, adjacent sections served as negative controls and were processed using identical procedures, except for incubation without the primary antibody in each case.
For fluorescent double-labeling immunocytochemistry, after rinses in KPBS containing 2% of the normal sera, sections were incubated in the secondary antibodies (1:200). For rat anti-BrdU this was donkey anti-rat conjugated to FITC or Cy2 (Jackson); for mouse anti-BrdU, donkey anti-mouse conjugated to FITC or Cy2 (Jackson); for all other primary antibodies raised in mouse, rat-absorbed biotinylated horse anti-mouse (Vector); and for all primary antibodies raised in rabbit, biotinylated swine anti-rabbit (Dakopatts). All secondaries were diluted in KPBS containing 2% normal serum, and sections were reacted for 2 hr at room temperature in the dark. After three rinses in KPBS, sections were reacted with streptavidin conjugated to Cy3 (Jackson) for a further 2 hr at room temperature in the dark.
For immunohistochemistry with hTau, sections were pretreated with 3% H2O2 in 10% methanol to quench endogenous peroxidase activity. Incubation in the primary antibody was performed in KPBS containing 5% normal horse serum and 0.25% Triton X-100 for 36 hr at 4°C. After three rinses in KPBS, sections were incubated in the secondary antibody: rat-absorbed biotinylated horse anti-mouse (Vector) in KPBS containing 2% normal horse serum for 2 hr at room temperature. Further washing in KPBS was followed by incubation with avidin-biotin-peroxidase complex (Vectastain, Vector), for 1.5 hr at room temperature. 3.3-Diaminobenzidine (Sigma) in 0.03% H2O2 in KPBS was used as the chromogen.
The sections were mounted on chrome-alum-coated slides, and the fluorescent sections were coverslipped using polyvinyl alcohol-1,4-diazabicyclo[2,2,2]octane mounting medium. The hTau slides were dehydrated in ascending alcohols and coverslipped using DPX mountant.
Confocal microscopy. Colocalization of BrdU with neuronal and glial markers was conducted by confocal microscopy to enable exact definition of each of the antibodies, using a Bio-Rad MRC1024UV confocal scanning light microscope. Double-labeled cells were always verified, both by collecting serial sections of 1-2 µm throughout the specimen, and by eye, using an Olympus binocular microscope. In all figures, all double-labeled cells that are denoted were identified in this way.
RESULTS
In vitro characteristics of the transplanted cells
Two different human progenitor cell cultures obtained post mortem from the forebrain of one 6.5 week (6.5FBr) and one 9 week (9FBr) embryo were analyzed. The cells were cultured in the presence of EGF, bFGF and LIF and passaged every 7-10 d. In these cultures bFGF was necessary to maintain continuous cell proliferation over extended time periods, and this effect was further enhanced by the addition of LIF. Parallel in vitro experiments (Carpenter et al., 1999
The in vitro characteristics of the 6.5FBr and 9FBr progenitor cell cultures have been presented in detail elsewhere (Carpenter et al., 1999
Survival and differentiation after transplantation to the adult rat brain
Cells from the 6.5FBr and 9FBr cultures were transplanted, under immunosuppression, into two neurogenic sites: the dentate gyrus of the hippocampus and the SVZa and its associated RMS, as well as to a non-neurogenic site, the striatum. Transplantation was performed using cells that had been passaged 9-21 times. The cells were labeled with BrdU during the last 48 hr before transplantation. This resulted in ~80% labeling efficiency and enabled analysis of the grafts by fluorescent immunohistochemistry using a double-labeling technique for BrdU in combination with specific neuronal and glial markers. In addition, hTau was used to identify the grafted cells.
In all animals, BrdU-positive transplanted cells were identified in all graft sites, at both 2 and 6 weeks after transplantation. Similarly, staining with the human-specific tau antibody revealed cellular and axonal profiles at all transplant sites, indicating graft survival in all cases. Extensive migration of BrdU-labeled cells, as described below, were seen in all animals where the graft deposits had been correctly placed in the RMS, SVZa, or hippocampus, respectively. No evidence of tumor formation was observed.
The transplants from both cell cultures (6.5FBr and 9FBr), regardless of the number of passages, were indistinguishable in terms of graft survival, migrational patterns, and phenotypic differentiation of the transplanted cells. Control transplants of cells that had been killed by freeze-thawing before transplantation showed no transfer of the BrdU marker to the host cells, which is in agreement with previous reports (Gage et al., 1995
The subventricular zone and rostral migratory stream
Single deposits of 100,000 cells were deposited in or close to the SVZa, just ventral to the corpus callosum, or just above the RMS midway between the SVZa and the olfactory bulb. In the SVZa a core of BrdU-positive cells was located close to the ventricular ependyma, extending in some cases into the white matter of the overlying corpus callosum (Fig. 1A) (6 weeks survival). Cells were seen to leave the transplantation site in a stream of rostral migration (Fig. 1B) after the RMS, i.e., along the path of endogenous progenitors toward the olfactory bulb. Once they reached the bulb, BrdU-positive cells left the migratory stream, becoming dispersed throughout the subependymal, granular (Fig. 1C,D), and glomerular cell layers. The cells within the olfactory bulb were more weakly BrdU-labeled than the cells in the SVZa (which were uniformly highly labeled), suggesting that the labeled cells had undergone further cell division on their route to the bulb, similar to the endogenous progenitors from the SVZa (Menezes et al., 1995
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Figure 1. Low-power illustration of a transplant in the SVZa in a sagittal section, analyzed at 6 weeks after transplantation, shows an overview of the injection site of BrdU-labeled cells (green) and their distribution throughout the RMS. In the olfactory bulb, the cells were found dispersed through all layers. A-D, Grafted cells at different sites (indicated in the top panel), with BrdU-labeled cells shown in green and the NeuN shown in red. Double-labeled cells present in the bulb display a yellow color (C, D). A, Transplant core; B, cells migrating along the RMS; C, D, cells in the granule cell layer of the olfactory bulb. Scale bar, 250 µm. aci, Intrabulbar portion of the anterior commissure; gcl, granule cell layer.
In the RMS transplants the deposits of BrdU-labeled cells were localized just above, and occasionally within, the RMS itself (see Fig. 4A). At 2 weeks after transplantation the cells remained clustered at the graft site, and there was very little migration from the graft core. Thus only few cells were observed rostral and caudal to the graft placement at this time point. Six weeks after grafting, cells were seen to have migrated rostrally toward the olfactory bulb (see Fig. 4B) and into the granular and periglomerular layers (see Fig. 4C-F).
The immature cell marker VIM was used to delineate the SVZa and RMS along which BrdU-positive cells were seen in their migratory stream (Fig. 2A). BrdU-positive cells were not VIM positive. The vast majority of the BrdU-labeled nuclei did not diverge from the RMS; however, in the region adjacent to the transplant core, occasional cells could be seen migrating dorsally toward the overlying cortex (data not shown). Some of the cells migrating within the RMS were double-labeled with the early neuronal markers Hu (Fig. 2B) and
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Figure 2. Confocal images of BrdU-labeled (green) and double-labeled cells (yellow) transplanted in the SVZa at 6 weeks after transplantation. A, Vimentin (VIM) staining delineates the RMS. BrdU-positive cells (arrows) were observed along the RMS but were not VIM positive. B, Many host cells present within the RMS were positively stained with an antibody to Hu, a neuronal phenotypic marker, and some transplanted cells were also Hu positive (arrowhead, enlarged in the inset). C, Many Hu-positive transplanted cells (arrowheads) were located within the granule cell layer of the olfactory bulb. The inset shows two Hu-positive, BrdU-labeled cells (one strongly and one weakly BrdU labeled). D, Approximately half of the transplanted cells (arrowheads) were double-labeled with NeuN in both the granule cell layer (D) and the periglomerular layer (E). G, Glomerulus. Insets in D and E show double-labeled cells in higher magnification. F, G, A small proportion of the BrdU-positive cells found in the periglomerular layer were also TH positive (arrowheads). Scale bar (shown in A): A-F, 100 µm; G, 50 µm.
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Table 1. The proportion of BrdU-labeled cells, which also express other markers of mature CNS phenotypes, at 6 weeks after transplantation to different regions of the adult rat brain Using a human-specific antibody to the cytoskeletal protein tau, positive staining was observed at the injection site in both cellular and axonal profiles (Fig. 3A). Typically, cells that remained at the graft core or migrated only a short distance from the implantation site had developed axons that projected laterally into either the corpus callosum or striatum adjacent to the transplant (Fig. 3A,B). Tau-positive cells were distributed along the RMS, several millimeters from the graft site (Fig. 3C,D). These cells often showed a short leading process, oriented in the direction of the RMS (Fig. 4). Small tau-positive profiles were observed in the deeper layers of the olfactory bulb, and occasionally mature cells with extensive processes were found in this region (Fig. 3E,F). High background from the immunohistochemical procedure precluded the identification of tau-positive profiles in the periglomerular layer.
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Figure 3. Grafts to the SVZa stained with a human-specific antibody to tau, at 6 weeks after transplantation. A, Sagittal section showing neuronal cell bodies and axons located within the SVZa, between the striatum (ST) and the overlying corpus callosum (CC). B-D, Higher magnification of individual neuronal profiles at the periphery of the transplant (B) and migrating in the RMS (C, D). E, F, Individual cells located deep within the olfactory bulb, showing morphological features of mature neurons. Scale bars: A, 100 µm; (shown in F) B-F, 10 µm.
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Figure 4. Confocal images of BrdU-labeled (green) and double-labeled cells (yellow) transplanted in the RMS. A, A typical graft at 2 weeks after transplantation, situated in the RMS with only moderate migration of grafted cells in either rostral and caudal direction from the graft core. B, At 6 weeks after transplantation cells were seen migrating along the RMS. A small proportion of the transplanted cells were labeled with the early neuronal marker
The hippocampus
Transplants of 100,000 cells were placed within the hilar region of the dentate gyrus. At both 2 and 6 weeks after grafting, many of the injected BrdU-positive cells remained as a cluster just below the granule cell layer (Fig. 5A). This position of the cell deposit is characteristic for cells that are implanted by passive injection into the dentate gyrus, because of the presence of a cleavage plane underneath the granule cell layer (Wells et al., 1988
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Figure 5. Confocal images of BrdU-labeled (green) and double-labeled cells (yellow) transplanted in the hippocampus. A, The core of transplanted cells was located within either the dorsal or ventral blades of the granule cell layer (GCL) in the dentate gyrus. B, C, By 2 weeks after transplantation, Hu- and NeuN-positive BrdU-labeled cells were observed at some distance from the graft core, mainly in the subgranular layer and also within the granule cell layer (arrowheads). D, BrdU-labeled transplanted cells positive for the neuronal marker
The BrdU-labeled cells that had integrated into the granular and subgranular layers had the same size and shape as the intrinsic host granule cells, and a large number of them expressed the neuronal markers Hu (Fig. 5B), NeuN (Fig. 5C), and
Staining with the hTau antibody revealed scattered axonal and cellular profiles, both within the graft core and in individual cells that had migrated away from the initial transplant site within the granular and subgranular cell layers (Fig. 6A). At 2 weeks the cells appeared fairly immature, with a few short Tau-positive processes. At 6 weeks, cells with morphological features of neurons with processes were observed (Fig. 6B,C). Tau-positive cells were also seen in the hilus and molecular layer and along the needle tract.
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Figure 6. Hippocampal transplants stained with the hTau antibody. A, A transplant in the dentate gyrus at 6 weeks after transplantation. B, A tau-positive cell with a typically immature neuronal profile with one primary process. C, A more differentiated tau-positive neuron with more complex processes, situated within the subgranular layer (arrowhead in A). Scale bar (shown in A): A, 150 µm; B, C, 30 µm. ML, Molecular layer; GCL, granule cell layer; H, hilus.
The striatum
The transplants were placed centrally within the head of the caudate-putamen. At both 2 and 6 weeks after grafting, the grafted cells were found as a BrdU-labeled cell cluster at the site of implantation. Many of the BrdU-labeled cells, however, were observed to have migrated into the surrounding host striatum, without any preferential direction, to a distance of ~1-1.5 mm from the graft core (Fig. 7A). The size of individual BrdU nuclei varied considerably, both within the graft core and in cells that were located in the adjacent host striatum (<0.4 mm from the graft core). All of the cells that had migrated over longer distances were of small size and more faintly labeled, suggesting a dilution of the BrdU label caused by cell division. In sagittal sections the BrdU-positive cells could be seen to be aligned with the gray matter, interspersed with the fibers of the internal capsule.
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Figure 7. Confocal images of BrdU-labeled (green) and double-labeled cells (yellow) transplanted in the striatum. A, Coronal section through the graft core at 6 weeks after transplantation, showing a dense cluster of cells at the injection site and migration of BrdU-labeled cells away from the graft core, in both gray and white matter. Inset shows region in box at higher magnification, also illustrated in F. B, Many of the transplanted cells were positively stained with Hu (red), even within the graft core (arrowheads, enlarged in the inset). C, No BrdU/NeuN double-labeled cells were found in the graft core or among those cells that had migrated into the host striatum. Arrows indicate transplanted cells that were found in close association with NeuN-positive host neurons (red). D, A number of transplanted cells were positive for the enzyme GAD67 in the periphery of the graft core (arrowheads). One of the double-labeled cells is shown at higher magnification in the inset. E, BrdU/DARPP-32 double-labeled cells were occasionally observed (arrowhead and inset at higher magnification). These were generally faintly labeled and found only in the immediate vicinity of the transplant core. F, Similarly, BrdU/Calbindin double-labeled cells were found both in the periphery of the graft and in adjacent regions of the host striatum. Scale bar (shown in A): A, 300 µm; B, 150 µm; D-F, 25 µm.
Double-staining revealed that the majority of the BrdU-positive cells in the graft core and in the adjacent host striatum were double-labeled for the early neuronal marker Hu (Fig. 7B) but negative for NeuN (Fig. 7C). Many BrdU/Hu double-labeled cells occurred also at the graft-host border and within the adjacent host striatum, up to a distance of ~0.3-0.4 mm from the graft core. Although the majority of the Hu-positive cells within the graft core were small in size and round or oval in shape, similar to the Hu-positive cells within the SVZ of the host brain, a substantial proportion of the BrdU/Hu-positive cells at the graft-host border and in the host striatum were larger in size (10-15 µm), i.e., in the range of the Hu-positive neurons within the host striatum. None of the cells expressed NeuN, which is also the case, however, for most of the host striatal neurons. All BrdU-labeled cells located farther away from the graft core were Hu negative. These cells were all of small size and often found in satellite positions, closely apposed to host striatal neurons (Fig. 7C, arrows) or close to blood vessels. The location and staining properties of these small-sized cells suggest that they had differentiated, at least in part, into glia. Colocalization of BrdU and the astrocyte marker GFAP was unequivocally demonstrated at the graft-host border, i.e., within the area of GFAP-positive reactive astrocytes surrounding the graft core (see Fig. 9D, inset).
The neuronal phenotype of the transplanted cells was further investigated using antibodies against the GABA-synthesizing enzyme GAD67, which is present in the vast majority (>90%) of the neurons within the striatum; DARPP-32, which is a marker for the medium-sized spiny striatal projection neurons; and calbindin, which is normally present in the medium spiny projection neurons in the matrix component of the striatum (for review, see Gerfen, 1992
Staining with the hTau antibody revealed a graft core of clustered tau-positive cells and fibers (Fig. 8A). In sagittal sections, loose bundles of tau-positive fibers were seen to leave the graft core in both the rostral and caudal direction, along the white matter bundles of the internal capsule. In cross section, these fibers were found primarily within the white matter bundles (Fig. 8B, arrows). Individual cells were also observed at some distance from the graft core (Fig. 8A,B, arrowheads). In these cases, the cell bodies were often located within the gray matter, with their processes projecting into the white matter tracts. At 6 weeks, tau-positive axons could be traced caudally from the graft core within the internal capsule bundles for a distance of ~1-2 mm; some of these fibers were seen to enter the globus pallidus, and in some cases scattered tau-positive fibers could be traced as far as the entopeduncular nucleus.
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Figure 8. Striatal transplants stained with the hTau antibody. Six weeks after transplantation, coronal sections revealed tau-positive neuronal profiles densely packed within the graft core (A). Individual cells with neuronal profiles were observed also in the host striatum adjacent to the graft (arrowheads in A and B). Axonal processes were seen to extend caudally within the white matter bundles of the internal capsule (arrows in A and B). Scale bars: A, 500 µm; B, 100 µm.
DISCUSSION
These present results show that the long-term propagated human neurosphere cultures contained progenitors that can respond in vivo to cues present in both neurogenic and non-neurogenic regions of the adult rat brain. The expression of phenotypic markers provided evidence for site-specific neural differentiation within each of the three grafted regions. In the olfactory bulb the cells that integrated into the granular and periglomerular layers expressed NeuN, TH, and GAD67, similar to the dopaminergic and GABAergic cells normally present in these regions. In the dentate gyrus some of the cells assumed a position, morphology, and phenotype similar to the NeuN/calbindin-positive granule cells within the granule cell layer. And in the striatum, cells located in the periphery of the transplants expressed GAD67 and calbindin as well as low levels of the striatum-specific marker DARPP-32.
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Figure 9. GFAP was used to label astrocytes within the graft areas (red) to assess the extent of colocalization with BrdU-labeled transplanted cells (green). A, Cells within the RMS at 6 weeks after transplantation were often closely associated with GFAP profiles, although no double-labeled cells were observed (arrows). B, Within the granule cell layer of the olfactory bulb, BrdU-positive cells were interspersed with, but not colocalized with, GFAP (arrows). C, In the dentate gyrus, cells within the transplant core were occasionally closely associated with GFAP-positive cytoplasmic staining, possibly indicating a double-labeled cell. D, Staining within the striatum revealed a dense network of GFAP-positive processes (red) intermingled with the BrdU-positive cells (green). Many clear examples of double-labeled cells were observed (arrowheads), although examples of BrdU single-labeled cells were also frequently observed (arrows). Insets show BrdU/GFAP double-labeled cells at higher magnification. Scale bar (shown in A): A, C, 50 µm; B, 25 µm; D, 150 µm.
A combination of EGF, bFGF, and LIF was used to expand the human progenitors. It has been shown previously that EGF and bFGF act cooperatively in promoting the proliferation of rat and human neural progenitors (Vescovi et al., 1993
Site-specific differentiation of the grafted cells
In the SVZa, which is one of the two sites where neurogenesis continues into adulthood in the mammalian CNS, the endogenous neuronal progenitors have been shown to migrate along the RMS and reach the bulb within 2-15 d after their generation in the SVZa (Lois and Alvarez-Buylla, 1994
The transplanted human neural progenitor cells expressed the early neuronal markers Hu and
In hippocampus the transplanted cells distributed along the subgranular and granular layers of the dentate gyrus. Although cells were observed also in other layers of the dentate and the CA3 region, cells expressing neuronal markers occurred only within the subgranular or granular layers, suggesting that the human progenitors, similar to rat hippocampal and cerebellar progenitors (Gage et al., 1995
Cells grafted to the striatum generate both neurons and glia
Expression of neuronal markers in the striatal transplants indicate that a substantial fraction of the grafted human progenitors had developed toward a neuronal phenotype. Many of the Hu-positive cells within the transplant core were small and round or oval in shape, similar to the neuronal precursors normally present in the proliferative subependyma in the adult brain. These cells did not express any of the more mature neuronal markers and therefore may be classified as poorly differentiated neuronal precursors. The GAD67-, calbindin-, and DARPP-32-positive cells were exclusively located at the graft-host border and within the adjacent host striatum, up to a distance of ~0.3-0.4 mm. The size and shape of these cells were similar to the medium-sized neurons of the host striatum. Many of these are GABAergic and stain positively for GAD67; one subclass, the striatal projection neurons, is further characterized by the expression of calbindin and/or DARPP-32.
These data indicate that the human neural progenitors can undergo neurogenesis also in the the normally non-neurogenic environment of the adult striatum and assume neuronal phenotype(s) similar to those normally present here but that in the absence of suitable substrates for migration they remain close to the implantation site. Interestingly, in sections stained with the hTau antibody some of these newly formed neurons were seen to extend long axon-like processes that could be traced along the fascicles of the internal capsule to the globus pallidus and in some cases also the entopeduncular nucleus, a distance of ~2 mm.
The cells that migrated over longer distances within the adult striatum were all Hu negative and of small size. Many of them were found in satellite position to the medium-sized host striatal neurons or close to blood vessels, suggesting that they had assumed a glial-like phenotype (Fig. 9). A migratory capacity of immature glia (or glial precursors) within the adult CNS has been reported for both astrocytes and oligodendrocytes by several investigators (Blakemore and Franklin, 1991
Implications for brain repair
The human neurosphere cultures are particularly suitable for transplantation in that they can be harvested and implanted without dissociation and detachment from a culture substrate. The cultures used here had been expanded up to 10 million-fold, which means that each transplant of 100,000-200,000 cells in theory could be derived from a single cell in the original cell preparation. Because the in vivo properties of the cells were indistinguishable over a wide range of passages (from 9 to 21), the present culture system could provide an almost unlimited source of human neural progenitor cells for transplantation.
The present results show that subpopulations of cells contained within the human neurosphere cultures can respond appropriately to specific extracellular cues present in each of the four target regions in the adult rat brain. Because the human neurosphere cultures are likely to contain a mixture of multipotent and lineage-restricted progenitors, the specific migratory patterns seen in the different locations may be explained either by the ability of an undifferentiated stem cell-like cell to differentiate along alternative neuronal or glial pathways in response to diverse local cues, or alternatively, by the presence of different subpopulations of lineage-restricted neuronal or glial precursors that were already committed to specific neuronal or glial fates. The present data seem compatible with both alternatives.
In conclusion, the long-term propagated human neural progenitors described here demonstrate a remarkable capacity for migration, integration, and site-specific differentiation in the adult brain. The growth factor combination used here acted to maintain the progenitors as a constitutively proliferating cell population without losing their capacity to respond to those extracellular cues normally present in the adult CNS. With further refinement of the procedure, e.g., by application of cell enrichment and cell sorting techniques, this culture system may provide an almost unlimited source of human neural progenitors at different stages of differentiation and lineage restriction. Such cells will be of great interest both as an experimental tool and as an alternative to primary embryonic brain tissue for intracerebral transplantation.
FOOTNOTES Received Dec. 7, 1998; revised April 15, 1999; accepted April 27, 1999.
This study was supported by the Wellcome Trust, the Swedish Medical Research Council, the Wenner Gren Foundation, and CytoTherapeutics Inc. We thank Åke Seiger and Lars Wahlberg for the supply of human embryonic tissue; Tomas Björklund, Cristina Ciornei, Alicja Flasch, Birgit Haraldsson, Jennifer Jackson, Ulla Jarl, Anna Karin Olden, Sandy Sherman, and Gertrude Stridsberg for excellent technical assistance; and Joe Hammang for useful discussion and comments on this manuscript. The Hu antibody was a generous gift from Dr. Steven A. Goldman, and the DARPP-32 antibody was a generous gift from Dr. Paul Greengard.
Correspondence should be addressed to Dr. Rosemary Fricker, Department of Neurology, Division of Neuroscience, Harvard Medical School, 350 Enders Building, Children's Hospital, 330 Longwood Avenue, Boston, MA 02115.
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