Infusion of Brain-Derived Neurotrophic Factor into the Lateral Ventricle of the Adult Rat Leads to New Neurons in the Parenchyma of the Striatum, Septum, Thalamus, and Hypothalamus

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The Journal of Neuroscience, September 1, 2001, 21(17):6706-6717

Infusion of Brain-Derived Neurotrophic Factor into the Lateral Ventricle of the Adult Rat Leads to New Neurons in the Parenchyma of the Striatum, Septum, Thalamus, and Hypothalamus
Viorica Pencea¹, Kimberly D. Bingaman¹^,², Stanley J. Wiegand³, and Marla B. Luskin¹
Departments of ¹ Cell Biology and ² Neurosurgery, Emory University School of Medicine, Atlanta, Georgia 30322, and ³ Regeneron Pharmaceuticals Inc., Tarrytown, New York 10591

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The findings that brain-derived neurotrophic factor (BDNF) promotes in vitro the survival and/or differentiation of postnatalsubventricular zone (SVZ) progenitor cells and increases in vivothe number of the newly generated neurons in the adult rostralmigratory stream and olfactory bulb prompted us to investigatewhether the infusion of BDNF influences the proliferation and/ordifferentiation of cells in other regions of the adult forebrain.We examined the distribution and phenotype of newly generatedcells in the adult rat forebrain 16 d after intraventricular administrationof BDNF in conjunction with the cell proliferation marker bromodeoxyuridine(BrdU) for 12 d. BDNF infusion resulted in numerous BrdU⁺ cells, not only in the SVZ lining the infused lateral ventricle,but moreover, in specific parenchymal structures lining the lateraland third ventricles, including the striatum and septum, as wellas the thalamus and hypothalamus, in which neurogenesis had neverbeen demonstrated previously during adulthood. In each region,newly generated cells expressed the neuronal marker microtubule-associatedprotein-2, or neuron-specific tubulin, identified by the antibodyTuJ1. The percentage of the newly generated cells expressing TuJ1ranged from 27 to 42%, suggesting that the adult forebrain hasa more profound capacity to produce neurons than recognized previously.The extent of cell proliferation after BDNF infusion was correlatedwith the level of expression of full-length TrkB, the high-affinityreceptor for BDNF, despite the fact that the BrdU⁺ cells were not themselves TrkB⁺. Collectively, our results demonstrate that the adult brain parenchymamay recruit and/or generate new neurons, which could replace thoselost as a result of injury ordisease.

Key words: brain-derived neurotrophic factor; cell proliferation; forebrain parenchyma; intraventricular infusion; postnatal neurogenesis; subventricular zone

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The majority of the cells in the mammalian forebrain arise prenatally (Sidman and Rakic, 1973; Raedler and Raedler, 1978).However, it is now established that, in addition to the productionof sensory neurons and supporting cells in the olfactory epithelium(Graziadei and Monti Graziadei, 1976; Huard et al., 1998), bothneurons and glia continue to be generated in restricted adultmammalian forebrain structures, including the hippocampus (Altmanand Das, 1965; Schlessinger et al., 1975; Kaplan and Bell, 1984;Kuhn et al., 1996; Palmer et al., 1997) and the subventricularzone (SVZ) lining the lateral ventricles (Privat, 1975; Vaysseand Goldman, 1990; Levison and Goldman, 1993; Luskin, 1993; Loisand Alvarez-Buylla, 1994). Recent studies have raised the possibilitythat the parenchyma of the adult forebrain also harbors progenitorcells for neurons (Reynolds et al., 1992; Palmer et al., 1995;Marmur et al., 1998; Magavi et al., 2000). The source and proliferativepotential of these progenitors have not been fullydetermined.

In vitro studies have revealed that the adult striatal SVZ can be induced to generate both neurons and glia under the influenceof growth factors (Reynolds et al., 1992; Reynolds and Weiss,1992, 1996; Gritti et al., 1999). Furthermore, the in vivo exposureof the adult forebrain SVZ to neurotrophins yields an increasein the number of progenitor cells, as well as the production ofnewly generated neurons (Craig et al., 1996; Kuhn et al., 1997;Zigova et al., 1998). Administration of either epidermal growthfactor (EGF) or tumor growth factor- $alpha$ (TGF- $alpha$ ) into mouse(Craiget al., 1996) or of either EGF or fibroblast growth factor-2 (FGF-2)into rat (Kuhn et al., 1997) resulted in an expansion of the SVZsurrounding the infused lateral ventricle, as well as newborncells in the nearby striatum and septum. However, although bothEGF and FGF-2 amplified the number of striatal SVZ progenitorsin the adult brain, neither treatment resulted in a significantincrease in the production of neurons in the forebrainparenchyma.

In this study, we analyzed the rat forebrain SVZ and parenchyma for the presence of newly generated cells after intracerebroventricularinfusion of brain-dervied neurotrophic factor (BDNF), in combinationwith the cell proliferation marker bromodeoxyuridine (BrdU), toinvestigate whether and how the adult forebrain responds to BDNFexposure. The BDNF administration resulted in numerous BrdU⁺ cells, not only in the SVZ lining the lateral ventricle, butalso in the striatal and septal parenchyma. Moreover, a high numberof BrdU-labeled cells were found in discrete regions of the thalamusand hypothalamus bordering the third ventricle. Approximately27-42% of the newly generated cells expressed a neuron-specificmarker. Furthermore, we found that the BrdU incorporation wascorrelated with the level of the high-affinity receptor for BDNF,TrkB. However, the BrdU⁺ cells and TrkB⁺ cells were in non-overlapping populations. Collectively, ourresults underscore the possibility that new neurons can be recruitedto replace those lost as a result of disease orinjury.

Parts of this work have been published previously in abstract form (Pencea et al., 1999).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Implantation of minipumps and administration of BDNF and BrdU. To determine whether the intracerebroventricular infusion ofa neurotrophic factor increases the proliferation of new neuronsin the adult forebrain, we analyzed the distribution and numberof newly generated cells in the forebrain of Sprague Dawley rats,after the administration of BDNF (n = 3) compared with that ofthe control vehicle, 0.1 M PBS, given alone (n = 3). The adultrats, weighing 220-250 gm, were anesthetized with ketamine andimplanted with an osmotic minipump (Alzet 2002; Alza ScientificProducts, Palo Alto, CA). The cannula was placed in the rightlateral ventricle 4.0 mm deep to the pial surface and +0.0 mmanteroposterior relative to bregma and 1.8 mm lateral to the midline.Each rat was infused for 12 d with 12 µl/d of either human recombinantBDNF dissolved in 0.1 M PBS (1 µg/ml) (Regeneron Pharmaceuticals,Tarrytown, NY) or PBS only. To label the newly generated cellsin the BDNF- or vehicle-infused brains, the cell proliferationmarker BrdU was delivered at the same rate (12 µg/d) and throughthe same minipump as the BDNF or PBS. After the cessation of theinfusion of BDNF and BrdU or PBS and BrdU, the cannula was leftin the lateral ventricle, and the animals were allowed to surviveanother 16 d before perfusion (Fig. 1). We also compared the distributionand phenotype of the newly generated cells after the intracerebroventricularinfusion of BDNF and BrdU or PBS and BrdU to that in animals thatreceived only daily intraperitoneal injections of BrdU (5 mg/mlin 0.0007N NaOH saline, 50 mg/kg) for 12 d.

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Figure 1. Illustration of the intraventricular infusion site, time course of delivery of BDNF or PBS in conjunction with BrdU, and structures analyzed for the distribution and phenotype of BrdU-labeled cells. A, B, In both experimental BDNF-infused (12 µg/d) and control PBS-infused animals, an osmotic minipump was used for continuous delivery of the growth factor or vehicle into the lateral ventricle, at a rate of 5 µl/hr for 12 d. The animals were concurrently infused with BrdU through the same minipump to label dividing cells. The animals were perfused 16 d after cessation of the BDNF or PBS infusate. C, A diagram of a parasagittal section of the adult rat brain demonstrating the placement in the right lateral ventricle of the cannula used to infuse the BDNF, or PBS, in conjunction with BrdU. D-H, Drawings of representative coronal sections of the adult rat brain at different anteroposterior levels, designating the structures quantitatively analyzed after the intraventricular administration of BDNF or PBS. The diagrams demonstrate that each structure analyzed (gray) for the presence of newly generated BrdU⁺ cells is adjacent to the lateral or third ventricle. The anterior part of the subventricular zone (D), striatum (E), and septum (F) surround the lateral ventricle, whereas the thalamus (G) and hypothalamus (H) are adjacent to the third ventricle. Note that, in G and H, the third ventricle is transected both ventrally and dorsally. 3V, Third ventricle; Acb, nucleus accumbens; CC, corpus callosum; CTX, cerebral cortex; DG, dentate gyrus; HYP, hypothalamus; IC, internal capsule; LV, lateral ventricle; OB, olfactory bulb; RMS, rostral migratory stream; SPT, septum; ST, striatum; SVZa, anterior part of the subventricular zone; TH, thalamus.

Tissue processing and immunohistochemistry. Sixteen days after the cessation of the intracerebroventricular BDNF and BrdU,PBS and BrdU, or intraperitoneal BrdU, the animals were anesthetizedwith pentobarbital (50 mg/kg) and perfused transcardially withheparanized saline (5 U of heparin per milliliter of 0.9% NaCl),followed by 4% paraformaldehyde in 0.1 M phosphate buffer, pH7.4. Brains were cryoprotected with 30% sucrose in 0.1 M phosphatebuffer, pH 7.2, embedded in Tissue-Tek OCT compound (Sakura Finetek,Torrance, CA), and sectioned on a cryostat in the coronal planeat 20 µm.

To reveal newly generated BrdU-positive cells, the sections were incubated for 30 min in 1N HCl at 60°C to denature the DNA.Subsequently, the sections were incubated first in blocking serum(10% normal goat serum in 0.1 M phosphate buffer containing 0.02%Triton X-100, pH 7.4), abbreviated NGS for 1 hr, and then for48 hr with a 1:200 dilution of a mouse IgG anti-BrdU (AccurateChemicals, Westbury, NY) in NGS. For fluorescent visualizationof BrdU-labeled cells, the sections were incubated for 1 hr atroom temperature in a rhodamine-conjugated goat anti-rat secondaryantibody (1:200dilution).

Some sections were processed to visualize only BrdU-labeled cells, whereas others were double-labeled with anti-BrdU, as wellas an antibody to a cell type-specific marker to determine thephenotype of the newly generated cells. To identify neurons, weused the antibody TuJ1 (1:400) (Covance, Richmond, CA), a mousepolyclonal IgG that recognizes neuron-specific $beta$ III-tubulin (Leeet al., 1990) usually expressed by immature neurons, or a monoclonalantibody to microtubule-associated protein-2 (MAP-2) (1:200; RocheProducts, Indianapolis, IN), which recognizes more differentiatedneurons (Bernhardt et al., 1985; Johnson and Jope, 1992). We alsoused a polyclonal antibody to glial fibrillary acidic protein(GFAP) (1:500 dilution; Dako, Glostrup, Denmark) (Bignami et al.,1972) to identify astrocytes and either a mouse monoclonal antibodyto galactocerebrosidase (GalC) (gift from Dr. Rao, Universityof Utah, Salt Lake City, UT) at a 1:200 dilution (Ranscht et al.,1982, 1987) or mouse monoclonal anti-myelin proteolipid protein(PLP) (Chemicon, Temecula, CA) at a 1:200 dilution (Cheng et al.,1998) to identify oligodendrocytes. As a marker for undifferentiatedcells, a mouse monoclonal antibody to the intermediate filamentprotein nestin (Hockfield and McKay, 1985; Frederiksen and McKay,1988; Lendahl and McKay, 1990) was used as an undiluted supernatant(Developmental Studies Hybridoma Bank, Iowa City, IA). In addition,to analyze the expression pattern of TrkB, the high-affinity tyrosinekinase receptor for BDNF, some sections were also incubated withanti-TrkB_606-619, a polyclonal antibody that recognizesthe intracellular domain of the full-length rat TrkB (amino acids606-619) (gift from Dr. S. Feinstein, University of California,Santa Barbara, CA) at a 1:25 dilution. For fluorescent visualizationof all cell type-specific antibodies and anti-TrkB, fluorescein-conjugatedsecondary antibodies were used at a 1:200 dilution. All secondaryantibodies were from Jackson ImmunoResearch (West Grove, PA).The slides were coverslipped with VectaShield (Vector Laboratories,Burlingame, CA) and viewed using a Zeiss (Oberkochen, Germany)Axiophot fluorescent microscope equipped with rhodamine and fluoresceinfilters, as well as a dual filter for visualizing rhodamine andfluorescein fluorescence simultaneously. For confirmation of thephenotype of individual BrdU⁺ cells, sections were also viewed using a confocal scanning lasermicroscope (Zeiss Axioplan equipped with LSM 510). To reveal thecytoarchitecture of the structures analyzed, some sections weredehydrated in ethanol, counterstained with cresyl violet, rehydrated,and coverslipped with DPX (BDH Laboratory Supplies, Poole, UK).All microscopic images were processed using Adobe Photoshop (AdobeSystems, Mountainview,CA).

Quantitative analyses. The density of BrdU-labeled cells, expressed as cells per cubic millimeter, was determined in the striatum,septum, thalamus, and hypothalamus, in both the BDNF-infused andPBS-infused brains. We selected for comparisons correspondingcoronal sections exhibiting the same cytoarchitectonic features,determined using the rat atlas of Paxinos and Watson (1982), inall of the BDNF- and PBS-infused brains. This allowed cells tobe counted in coronal sections at comparable rostrocaudal positions.The counts were made, using a 40× objective, by placing an opticalgrid (field size, 250 × 250 µm) starting from the wall of thelateral or third ventricle and proceeding into the parenchymauntil BrdU⁺ cells were no longer detectable. The density of BrdU-labeledcells was calculated for each structure analyzed in every animal,and statistical analyses were performed using the Student's ttest (IBM Statistica; StatSoft Inc., Tulsa,OK).

The number of double-labeled BrdU⁺-TuJ1⁺ and BrdU⁺-GFAP⁺ cells in the striatum, septum, hypothalamus, and subventricular zonesurrounding the lateral ventricle was counted when viewed witha conventional or confocal microscope in at least three sectionsper brain. In each animal, the phenotype of 330-850 striatal cells,200-900 septal cells, 200-1200 hypothalamic cells, and 600-2500subventricular cells was analyzed. The counts of double-labeledcells were analyzed statistically using two-way and one-wayANOVA.

To compare the nuclear diameter of the newly generated cells in the striatum, septum, hypothalamus, and thalamus, in BDNF-and PBS-infused animals, 25-40 cells per structure were analyzedin each animal. The maximum nuclear diameter was measured usingIP Lab Scientific Processing (Scanalytics Inc., Fairfax, VA),and an average nuclear diameter was calculated for each structurein each animal. These means were then combined to determine theaverage diameter of newly generated cells in the parenchyma ofthe BDNF- and PBS-infused brains. In the same sections, ~250 BrdU⁺ cells per animal were analyzed with IP Lab Scientific Processingto determine the percentage of newly generated cells present inpairs. The cells were considered to form a pair if their BrdU⁺ nuclei were adjacent (<3 µm apart) to oneanother.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We examined the effect of intracerebroventricular administration of BDNF on the distribution and phenotype of newly generatedcells in the adult forebrain. BDNF or PBS (control) was infusedcontinuously for 12 d into the right lateral ventricle of adultrats (Fig. 1A,B). A steady-state level of BDNF is achieved byintracerebroventricular infusion within 3 d (Anderson et al.,1995). To label the newly generated cells, the cell proliferationmarker BrdU was delivered by intracerebroventricular infusionconcurrently with the BDNF (BDNF-BrdU) or PBS (PBS-BrdU) (Fig.1A,B). The animals were perfused 16 d after BDNF or PBS withdrawal(day 28) (Fig. 1A,B) to permit newly generated cells to integratein the host brain. The distribution and phenotype of the newlygenerated BrdU⁺ cells were analyzed along the rostrocaudal extent of the lateraland third ventricles (Fig. 1D-H). A third group of animals receiveddaily BrdU intraperitoneal injections for 12 d, without any intracerebroventricularinfusion. These animals were also perfused 16 d after the lastBrdUinjection.

Newly generated cells appear in distinct regions surrounding the lateral and third ventricles after combined intracerebroventricular administration of BDNF and BrdU

To determine which regions surrounding the lateral and third ventricles have the capacity to produce new cells in responseto BDNF infusion into the adult lateral ventricle, we systematicallyanalyzed the distribution of BrdU⁺ cells in the subventricular zone and parenchyma along the rostrocaudalextent of the forebrain. Our analysis revealed that newly generatedcells were present surrounding the lateral ventricle on the infusedside but not on the contralateral side, indicating that the BDNF-BrdUdid not diffuse contralaterally. An unexpected finding was that,in addition to newly generated cells along the rostrocaudal extentof the rostral migratory stream (RMS) as reported previously (Zigovaet al., 1998), we also detected newly generated cells: (1) inother regions of the SVZ immediately surrounding the lateral ventricle,(2) in the parenchyma adjacent to the lateral ventricle (Fig.2A), and (3) in the parenchyma of specific structures surroundingthe third ventricle, in which cell proliferation has not beendescribed previously (Fig. 2B). In particular, newly generatedcells were visualized in the striatum, septum, corpus callosum,and cerebral cortex, as well as in the thalamus and hypothalamus(Figs. 2, 3). The presence of newly generated cells in specificparts of the thalamus and hypothalamus surrounding the third ventriclesuggests that BDNF-BrdU may have flowed caudally from the infusedlateral ventricle into the third ventricle.

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Figure 2. The distribution of newly generated cells in the parenchyma surrounding the lateral and third ventricles after the coinfusion of BDNF and BrdU into the lateral ventricle of an adult rat brain. The newly generated cells (bright orange) are identified in 20 µm coronal sections with an antibody to BrdU and visualized with a rhodamine-conjugated secondary antibody. A, A representative fluorescent photomicrograph demonstrating BrdU⁺ cells in the parenchyma surrounding the infused lateral ventricle 16 d after a 12 d infusion of BDNF-BrdU. The striatal SVZ (arrows) has numerous BrdU⁺ cells, whereas the rest of the SVZ, including that lining the septum, is almost devoid of newly generated cells. Moreover, the dorsal half of the striatal SVZ appears thicker than the ventral part. The distribution of the BrdU⁺ cells in the striatal parenchyma exhibits a medial to lateral gradient, with the number of BrdU⁺ cells decreasing as a function of distance from the lateral ventricle. The distribution of BrdU⁺ cells in the septal parenchyma is more homogenous, although there is a relatively sharp decrease in the number of BrdU⁺ cells at the border between septum and fornix (dashed line). Note that, on both sides of the lateral ventricle, the BrdU⁺ cells extend more than a few hundred micrometers into the parenchyma. A small number of the newly generated cells can also be observed in the corpus callosum overlying the lateral ventricle. The midline of the section is approximately at the left edge of the photomicrograph. B, A representative fluorescent photomicrograph showing BrdU⁺ cells in the parenchyma surrounding the third ventricle of a BDNF-infused brain. In the hypothalamus, the newly generated cells extend bilaterally at least a few hundred micrometers into the parenchyma, and their distribution is relatively homogenous. Similar to the septal SVZ (shown in A), the hypothalamic ventricular lining is devoid of BrdU⁺ cells. 3V, Third ventricle; CC, corpus callosum; HYP, hypothalamus; LV, lateral ventricle; SPT, septum; ST, striatum. Scale bar, 100 µm.

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Figure 3. A comparison of the number and distribution of the newly generated cells in forebrain structures surrounding the lateral and third ventricles after the intraventricular coinfusion of BDNF and BrdU or PBS and BrdU. The newly generated BrdU-positive cells (bright orange) were identified in 20 µm coronal sections with an antibody to BrdU and visualized with a secondary antibody conjugated to rhodamine. A, B, Representative fluorescent photomicrographs of infused hemispheres showing BrdU⁺ cells in the anterior part of the subventricular zone and the adjacent frontal cortex after infusion of PBS-BrdU (A) or BDNF-BrdU (B) into the ipsilateral lateral ventricle. After BDNF infusion, the SVZa (B) is expanded in diameter relative to the SVZa of the PBS-infused brain (A). Moreover, after BDNF infusion (B), the number of newly generated cells (e.g., arrowheads) present in the frontal cortex surrounding the SVZa is much higher than that observed in the PBS-infused brain (A). C, D, Representative fluorescent photomicrographs of infused hemispheres demonstrating the number of BrdU⁺ cells in the striatum in brains infused with PBS (C) or with BDNF (D). After BDNF or PBS infusion, BrdU⁺ cells are dispersed throughout the striatal parenchyma, although there are substantially fewer new cells in the PBS-infused brain (C). Moreover, in the BDNF-infused brain (D) compared with the PBS-infused brain (C), the number of newly generated cells in the striatal SVZ is higher, and more of these cells tend to occur in clusters. E, F, Representative fluorescent photomicrographs of infused hemispheres demonstrating the newly generated cells in the septum adjacent to the infused lateral ventricle. The number of BrdU⁺ cells (e.g., arrowheads) in the septal parenchyma of the BDNF-infused brain (F) is much higher than the number of labeled cells in the PBS-infused brain (E). In both cases, however, the septal SVZ is almost devoid of BrdU⁺ cells. G, H, Representative fluorescent photomicrographs showing BrdU-positive cells in the thalamus, adjacent to the dorsal lumen of the third ventricle, after the infusion of PBS-BrdU (G) or BDNF-BrdU (H). The number of BrdU⁺ cells (e.g., arrowheads) present in the thalamic parenchyma of the BDNF-infused brain (H) is higher than the number observed in the PBS-infused brain (G). In both sections, there are a few BrdU⁺ cells lining the wall of the third ventricle. I, J, Representative fluorescent photomicrographs demonstrating the relative number of BrdU⁺ cells in the hypothalamus of the PBS-infused (I) compared with BDNF-infused (J) brain. After BDNF infusion (J), numerous BrdU⁺ cells (e.g., arrowheads) are dispersed throughout the hypothalamic parenchyma, whereas after the PBS infusion (I), fewer BrdU⁺ cells (e.g., arrowheads) are present. Note that very few BrdU⁺ cells line the third ventricle in the sections from both the BDNF-infused and PBS-infused brains. 3V, Third ventricle; CTX, frontal cortex; LV, lateral ventricle; HYP, hypothalamus; SPT, septum; ST, striatum; TH, thalamus. Scale bars, 100 µm.

To determine whether there was a relationship between the parenchymal structures in which the BrdU⁺ cells were found and the morphology of the newly generated cells,in addition to double-labeling with BrdU and cell type-specificmarkers (as described below), we used the nuclear shape and diameterof the labeled cells as a way to compare the diversity of labeledcells in different regions of the forebrain. In the BDNF-infusedbrains, the nuclear diameter and morphology of the newly generatedcells varied according to the regions in which they were located,and the largest mean nuclear diameter (range of 9.22-9.53 µm)was found in the striatum. The nuclei of the BrdU⁺ cells in the striatum and septum tended to be round, whereasthe nuclei in the hypothalamus and thalamus were usually elongated.These results indicate that a diversity of cell types was generatedas a function of the location of the cells. However, despite thisdiversity, in all of the structures analyzed, the BrdU⁺ cells were present frequently in close apposition to each other,such that they were aggregated in pairs (Fig. 4). In the parenchymalstructures containing BrdU⁺ cells, the percentage of paired cells was relatively uniformwithin a given structure, varying from an average of 22% in thehypothalamus to 37% in the striatum. The presence of pairs ofBrdU⁺ cells may indicate that cell division occurs in situ in the parenchyma.

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Figure 4. Pairs of newly generated cells in the parenchyma of the striatum after intraventricular infusion of BDNF. A, A representative fluorescent photomicrograph of a 20 µm coronal section demonstrating that, 16 d after withdrawal of a 12 d infusion of BDNF-BrdU, a high proportion of the newly generated cells within the striatal parenchyma occur in pairs. The cleavage plane between pairs of cells (e.g., arrows) appears random, with no preferential orientation relative to the ventricular surface. Midline is to the right, and dorsal is up. B, A representative photomicrograph of the septal parenchyma, viewed with confocal microscopy, showing a pair of newly generated BrdU⁺ cells. The short distance (<2 µm) between the pairs of BrdU⁺ nuclei combined with the high frequency of pairs (shown in A) suggests that, after BDNF administration, cell division may occur in situ. Scale bars: A, 50 µm; B, 10 µm.

Our analysis showed that the number of newly generated cells in the brains of rats infused with PBS-BrdU was substantiallylower than in the brains infused with BDNF-BrdU, although thedistribution of the newly generated cells was similar in bothsets of animals (Figs. 3, 5). However, the distribution of BrdU⁺ cells after intracerebroventricular infusion of BrdU combinedwith either BDNF or PBS differs from that observed after onlyintraperitoneal administration of BrdU. In the animals that receivedintraperitoneal injections, the BrdU-labeling was present mainlyin the subventricular zone adjacent to the lateral ventricle,with just a few BrdU⁺ cells in the parenchyma surrounding the lateral and third ventricles.The pronounced discrepancy between the distribution of BrdU labelingin the brains of the intracerebroventricular infused and intraperitonealinjected animals underscores the limited ongoing proliferationthat ordinarily occurs in the parenchyma versus the subventricularzone of the adult brain.

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Figure 5. Density of newly generated BrdU⁺ cells in the striatum, septum, and hypothalamus after BDNF infusion relative to PBS infusion. For each structure analyzed, the gradient of the cell density is plotted from the wall of the ventricle (corresponding to the origin of axes) to 2.25 mm into the parenchyma. A, In the striatum, adjacent to the lateral ventricle, the density of the BrdU⁺ cells is two to three times higher after BDNF infusion than after PBS infusion, and in both cases the cell density declines gradually as a function of distance from the ventricular wall. Nevertheless, the newly generated cells extend farther into the parenchyma after BDNF infusion compared with PBS infusion. B, At each position in the septum, the cell density is ~1.5 times higher after BDNF infusion than after PBS infusion. In both groups, the cell density remains relatively constant in the septal parenchyma (~0.75 mm from the ventricular wall) and then decreases gradually in the fimbria fornix. C, In the proximal 0.5 mm adjacent to the third ventricle, the cell density in the hypothalamus is more than two times higher after BDNF administration than after PBS infusion. The number of the newly generated cells declines steeply beyond the hypothalamic border in both the BDNF- and PBS-infused brains. *p < 0.05; **p < 0.005.

The pattern of distribution of BrdU⁺ cells in the SVZ and parenchyma of the forebrain after intracerebroventricular administration of BDNF and BrdU

Our data indicated that there was a differential response to BDNF infusion in different regions along the ventricular lumen.In the SVZ lining the striatum, there was a prominent dorsal toventral gradient of BrdU⁺ cells (Fig. 2A). In the dorsal aspect of the striatal SVZ, BrdU⁺ cells formed a band multiple cell layers thick, whereas the ventralpart of the striatal SVZ was considerably thinner and containedwidely dispersed BrdU⁺ cells. Moreover, the BrdU⁺ cells in the dorsal aspect of the striatal SVZ often occurredin clusters (Fig. 3D), suggesting that there were "hot spots"of proliferation around the lateral ventricle, similar to thosedescribed in the telencephalon of the adult canary (Alvarez-Buyllaet al., 1990). The gradient in the BrdU labeling of the SVZ parallelsthe differences ordinarily observed in the relative thicknessand density of the SVZ, as described by Chiasson et al. (1999).

In the parenchyma of each structure containing BrdU⁺ cells, the density of the newly generated cells declines as a functionof distance from the ventricular wall (Fig. 4). However, therewas no apparent correlation between the extent and thickness ofthe SVZ and the number of newly generated cells present in theadjoining parenchyma. In some structures, such as the septum,there were numerous BrdU⁺ cells in the parenchyma, up to 1 mm from the ventricular wall(Figs. 2A, 3F, 5B), although there was only marginal labelingof the SVZ. Conversely, in some regions containing a prominentSVZ, such as the striatum, there was a high density of BrdU⁺ cells in the SVZ adjacent to the lateral ventricle (Figs. 2A,3D). Moreover, there were numerous BrdU⁺ cells in the adjacent striatal parenchyma, up to 2 mm away fromthe lateral ventricle (Figs. 2A, 3D, 5A). In addition, a considerablenumber of BrdU⁺ cells were observed in the parenchyma of the thalamus and hypothalamussurrounding the third ventricle, despite the absence of a distinguishableSVZ (Figs. 2B, 3H,J, 5C). Thus, the extent of the SVZ is not theonly determining factor for the production of new cells in theadultforebrain.

The BrdU⁺ cells in the parenchyma were not evenly distributed. Rather, the distribution of BrdU⁺ cells was restricted by boundaries between and within structuresof the forebrain, similar to the restriction of newly generatedcells in the RMS (Luskin, 1993; Zigova et al., 1996, 1998). Forexample, although the BrdU⁺ cells in the septum on the infused side were widespread and numerous,they appeared to "avoid" the midline fimbria fornix and to forma dorsal and a ventral stream around the fimbria (Fig. 2A). Thepresence of BrdU⁺ cells in the septum adjacent to the uninfused lateral ventricle,combined with the absence of BrdU⁺ cells in the SVZ and striatum also lining the uninfused ventricle,suggests that some cells generated on the infused side may havemigrated across the midline to the contralateral septum. Alternatively,BrdU may have directly diffused across the midline in which itthen became incorporated in the septal cells on the contralateralside. The labeling pattern observed in the septum indicates thatthe distribution of BrdU⁺ cells is neither the result of the random migration of BrdU⁺ cells nor the effect of the passive diffusion of the BDNF-BrdU.

Prominent differences in the extent of BrdU incorporation were also observed surrounding the third ventricle. In particular,although there were numerous BrdU⁺ cells in the habenular nucleus of the thalamus, there were noBrdU⁺ cells in the part of the dentate gyrus immediately adjacent tothe third ventricle (Fig. 6B). However, after infusion of BDNF,there were newly generated cells in the subgranular layer of thedentate gyrus, as has been described previously in the normalbrain (Altman and Das, 1965; Schlessinger et al., 1975; Kaplanand Bell, 1984; Kuhn et al., 1996; Palmer et al., 1997). The restrictionof BrdU labeling to discrete regions surrounding the third ventricleis further illustrated by the paucity of BrdU⁺ cells in other thalamic nuclei adjacent to the habenula, althoughsome of them are also adjacent to the third ventricle (data notshown).

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Figure 6. The correlation between the distribution of newly generated cells and the expression of TrkB in the parenchyma surrounding the third ventricle. A-G, Representative fluorescent photomicrographs of 20 µm coronal sections demonstrating the relationship between TrkB expression and BrdU incorporation in structures surrounding the third ventricle, 16 d after a 12 d interval of BDNF and BrdU coinfusion. BrdU⁺ cells were identified with an antibody to BrdU and visualized by a rhodamine-conjugated secondary antibody (B, F), whereas TrkB expression was detected in adjacent sections with an antibody to TrkB and visualized by a fluorescein-conjugated secondary antibody (C, D, G). The cytoarchitecture of the structures analyzed was visualized by either their pattern of TuJ1 staining (A) or viewing sections stained with cresyl violet and viewed with a 4',6'-diamidino-2-phenylindole filter (E). A-D, Photomicrographs of the thalamic habenular nucleus and dentate gyrus adjacent to the dorsal lumen of the third ventricle stained with TuJ1 (A), anti-BrdU (B), and anti-TrkB (C, D). The habenular nucleus, with numerous BrdU⁺ cells, has a high level of TrkB expression (D), whereas the cells in the dentate gyrus, overlying the habenula, neither incorporate BrdU (B) nor express TrkB (D). E-G, Photomicrographs of the periventricular and paraventricular nuclei of the hypothalamus surrounding the ventral lumen of the third ventricle demonstrating their differential response to BDNF administration. The paraventricular nucleus has a much higher number of newly generated cells than the periventricular nucleus, despite its position farther away from the wall of the third ventricle. The TrkB expression (G) correlates with the level of BrdU expression; it is higher in the paraventricular nucleus than in the periventricular nucleus. The asterisks in E-G designate corresponding regions of the paraventricular nucleus. 3V, Third ventricle; DG, dentate gyrus; Hb, thalamic habenular nucleus; Pa, paraventricular hypothalamic nucleus; Pe, periventricular hypothalamic nucleus. Scale bars: A, B; 200 µm; C, D, 50 µm; E-G, 200 µm.

The hypothalamus, another structure bordering the third ventricle, also exhibits a well defined pattern of BrdU labeling afterBDNF infusion. Whereas in the rostral hypothalamus there was arelatively uniform density of BrdU⁺ cells surrounding the third ventricle (Fig. 2B), more caudally,the newly generated cells were concentrated in particular hypothalamicnuclei. For example, there was a relatively high density of BrdU⁺ cells in the parvocellular region of the paraventricular nucleus,although it is displaced from the wall of the third ventricle(Fig. 6F). Conversely, the periventricular nucleus immediatelysurrounding the third ventricle has a comparatively low numberof BrdU⁺ cells. Together, the pattern of BrdU labeling in the hypothalamussuggests that regions presumably exposed to the highest concentrationof BDNF (e.g., those closest to the ventricular lumen) do notnecessarily contain the highest density of newly generated BrdU⁺cells.

TrkB expression in the forebrain parenchyma of BDNF-infused brains correlates with sites of cell proliferation

To determine the correlation between the increased cell proliferation after intracerebroventricular infusion of BDNF and theexpression of TrkB, the high-affinity receptor for BDNF, we analyzedthe relationship between the BrdU incorporation and the patternof the full-length TrkB expression in the structures surroundingthe lateral and third ventricles. In a previous study (Zigovaet al., 1998), we found that the anterior part of the SVZ (SVZa)and the RMS of BDNF-infused adult brains contained a higher numberof BrdU⁺ cells and expressed higher levels of TrkB compared with the surroundingareas. In the present study, a similar correlation was observedin the areas surrounding the lateral (data not shown) and third(Fig. 6) ventricles. This correlation, such that the extent ofBrdU incorporation and TrkB expression parallel each other, canbe observed in the regions of the hypothalamus examined. Therewere numerous BrdU⁺ cells and a high level of TrkB expression in the paraventricularnucleus of the hypothalamus, whereas in the periventricular nucleus,the numbers of BrdU-labeled cells and TrkB expression were bothlow (Fig. 6E-G). Nevertheless, TrkB expression is not sufficientfor cell proliferation. For example, whereas TrkB is expressedat a uniformly high level throughout the habenular nucleus (Fig.6D), BrdU⁺ cells are much more numerous along the medial edge (Fig. 6B).This disparity cannot be accounted for by the differences in BDNFexposure, because the dorsal edge of the habenular nucleus, whichhas lower BrdU incorporation, also faces the thirdventricle.

To investigate whether the TrkB expression was influenced by the infusion of BDNF, we compared the pattern of TrkB expressionin the BDNF-infused hemispheres versus uninfused hemispheres orPBS-infused hemispheres. The levels of TrkB expression in differentstructures of the BDNF-infused hemispheres were similar to thosein the contralateral uninfused hemispheres and in the PBS-infusedbrains. These findings indicate that the infusion of BDNF or PBSdid not result in an overt change in the level of TrkB expressionin the regions containing BrdU⁺cells.

In the regions in which we observed both high levels of TrkB and numerous BrdU-labeled cells, we further investigated whetherthe cells expressing TrkB were able to incorporate BrdU duringthe administration of BDNF-BrdU. Our confocal analysis revealedthat the full-length TrkB receptor was not expressed by the BrdU⁺ cells in the parenchyma (Fig. 7). Nevertheless, the TrkB⁺ cells were frequently adjacent to the BrdU⁺ cells (Fig. 7C,D, insets), suggesting that BDNF may have an indirecteffect on the proliferation and/or survival of the newly generatedcells (see Discussion).

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Figure 7. The newly generated cells in the parenchyma of the adult rat forebrain do not express TrkB receptor after coinfusion of BDNF and BrdU. A-D, Representative fluorescent photomicrographs of coronal sections, captured by confocal microscopy, showing the distribution of the nuclei of newly generated BrdU⁺ cells and the cells expressing the full-length TrkB receptor in the striatum (A), septum (B), thalamus (C), and hypothalamus (D). The BrdU⁺ cells were identified with a rhodamine-conjugated secondary antibody (bright orange), and the TrkB was visualized with a fluorescein-conjugated secondary antibody (green). The sections were visualized with either a dual fluorescein-rhodamine filter or with only a fluorescein filter (insets). In none of the four regions analyzed did the BrdU⁺ cells (e.g., asterisks) express the TrkB receptor. Frequently, however, the BrdU⁺ cells were adjacent to TrkB⁺ cells. The absence of double-labeled cells suggests that the BDNF may have an indirect effect on the proliferation and/or survival of newly generated cells. Scale bar: A-D, 30 µm.

Numerous newly generated neurons appear in the SVZ and parenchyma of the forebrain after BDNF infusion

We analyzed the phenotype of the BrdU⁺ cells in the SVZ and parenchyma after intracerebroventricular infusion of BDNF to determinewhat proportion of the newly generated cells were neurons. Thephenotype of the newly generated BrdU⁺ cells was identified using cell type-specific markers. In allregions examined, a significant proportion of BrdU⁺ cells colocalized TuJ1 (Fig. 8A-G), an antibody against neuron-specific $beta$ III-tubulin, expressed by immature neurons (Lee et al., 1990;Easter et al., 1993). The percentage of double-labeled TuJ1⁺-BrdU⁺ cells in the SVZ was ~27% (Table 1). A similar percentage ofthe BrdU⁺ cells in the parenchyma of the striatum and septum were neurons;the percentage was slightly higher (~42%) in the hypothalamus(Table 1). In each of the regions containing TuJ1⁺-BrdU⁺ cells, we also observed that a small percentage of the newlygenerated cells expressed MAP-2⁺, a marker for mature neurons (Bernhardt et al., 1985; Johnsonand Jope, 1992) (Fig. 8H-K). This discrepancy between the percentageof TuJ1⁺ and anti-MAP-2⁺ cells suggests that the majority of the newly generated neuronsmay not have sufficiently matured to express MAP-2.

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Figure 8. After the coinfusion of BDNF and BrdU into the lateral ventricle of the adult rat brain, newly generated cells in the SVZ and within the parenchyma express a neuronal phenotype. A-K, To analyze the phenotype of the newly generated cells, 20 µm coronal sections were immunostained with anti-BrdU (red) and the neuronal antibody TuJ1 (green) (A-G) or anti-MAP-2 (green) (H-K) and then visualized with either conventional (A, F, G, J, K) or confocal (B-E, H, I) microscopy. A, A representative photomicrograph viewed with a dual fluorescein-rhodamine filter, demonstrating the presence of numerous BrdU⁺ cells in the SVZ and the absence of BrdU⁺ cells in the ependyma lining the lateral ventricle. The arrow designates a double-labeled BrdU⁺/TuJ1⁺ cell with the typical bipolar morphology of a migrating neuron. B-E, Representative photomicrographs of the striatal parenchyma visualized by confocal microscopy and viewed with either a dual fluorescein-rhodamine filter (B, D) or with only a fluorescein filter (C, E). In B and C, the two large cells, with morphology typical of striatal neurons (e.g., arrowheads), display prominent cytoplasmic TuJ1 staining surrounding their nucleus. The lower cell (arrows) is double-labeled (BrdU⁺/TuJ1⁺). Several cells in the striatal parenchyma adjacent to the subventricular zone, shown in D and E, are BrdU⁺. The neuronal phenotype of one of these cells (arrows) is established by the TuJ1⁺ cytoplasm (E) surrounding its nucleus. The upper BrdU⁺ cells (arrowheads) also colocalize TuJ1, but because of the plane of focus, the TuJ1 staining is not limited to the periphery of the nuclei, and therefore their neuronal phenotype cannot be definitively established. F, G, Representative photomicrographs of the septal parenchyma viewed with a dual fluorescein-rhodamine filter (F) or with a fluorescein filter (G). The BrdU⁺/TuJ1⁺ newly generated neuron (arrows) is flanked by numerous TuJ1⁺ fibers (e.g., arrowheads). H-K, Representative photomicrographs of the hypothalamic parenchyma visualized by confocal (H, I) or conventional (J, K) microscopy and viewed with either a dual fluorescein-rhodamine filter (H, J) or with only a fluorescein filter (I, K). In H and I, two cells with a neuronal morphology display prominent MAP-2 staining of their somata and proximal processes (e.g., arrowheads). The lower cell (arrows) is a double-labeled (BrdU⁺/MAP-2⁺) neuron. In J and K, one of the MAP-2⁺ hypothalamic neurons is also BrdU⁺. ep, Ependyma; LV, lateral ventricle; ST, striatum; SVZ, subventricular zone. Scale bars: A, 25 µm; B, C, 10 µm; D, E, 10 µm; F, G, 10 µm; H, I, 10 µm; J, K, 10 µm.


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Table 1. Percentage of neurons and astrocytes in the SVZ and parenchyma

The percentages of the newly generated cells that were TuJ1⁺ were similar in the BDNF- and PBS-infused brains in the SVZ, striatum,and septum but not in the hypothalamus, indicating that, in mostregions, the in vivo administration of BDNF did not alter thephenotype of the newly generated cells. In all regions, however,the total number of new neurons was significantly higher afterBDNF infusion than PBS infusion. In the hypothalamus, there wasa higher percentage of newly generated neurons in the BDNF-infusedthan in the PBS-infused brains (e.g., ~41% after BDNF vs ~21%after PBS), suggesting that the cells of the hypothalamus mayrespond differently than other forebrain structures to the BDNFadministration. In contrast to the BDNF- or PBS-infused brains,no new neurons were found outside the subventricular zone in thebrains of the animals that had received only intraperitoneal injectionsof BrdU (data notshown).

Because the multipotential progenitor cells in the adult SVZ ordinarily give rise to glia (Reynolds et al., 1992; Chiassonet al., 1999), we investigated what percentage of the newly generatedBrdU⁺ cells are astrocytes or oligodendrocytes after BDNF infusion.We used an antibody to GFAP to identify astrocytes and antibodiesagainst GalC and PLP to identify oligodendrocytes. In both theBDNF- and PBS-infused brains, the parenchyma of the striatum (Fig.9A), septum, and hypothalamus (Fig. 9B) contained a low percentage(2-7%) of newly generated GFAP⁺ cells (Table 1). The percentage of BrdU⁺ astrocytes was similar (~3%) in the hypothalamus in the BDNF-and PBS-infused brains, whereas in the striatum and septum, thepercentage of BrdU⁺ astrocytes was higher in the BDNF-infused brains (Table 1).In both the BDNF- and PBS-infused brains, however, the percentageof newly generated astrocytes was much higher (17-19%) in theSVZ than in the parenchyma. In each of the areas examined, thepercentage of BrdU⁺ oligodendrocytes was negligible and not quantified.

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Figure 9. After coinfusion of BDNF and BrdU, most of the newly generated cells in the parenchyma of the adult rat forebrain do not express GFAP. A, B, Coronal sections (20 µm) were immunostained with anti-BrdU (bright orange) and anti-GFAP (green) and visualized with a dual fluorescein-rhodamine filter. A, A representative fluorescent photomicrograph of the striatal parenchyma showing that the GFAP⁺ cells (e.g., arrowheads) and the BrdU⁺ nuclei (e.g., arrows) do not overlap. The absence of double-labeled BrdU⁺/GFAP⁺ cells indicates that the newly generated cells are not astrocytes. B, Representative photomicrograph of the hypothalamus adjacent to the third ventricle demonstrating that, although the GFAP⁺ cells (e.g., arrowheads) with the appearance of radial glia are intermingled with BrdU⁺ cells, the newly generated cells are not astrocytes. 3V, Third ventricle. Scale bar: A, B, 50 µm.

The SVZ of the adult brain contains cells that express the intermediate neurofilament protein nestin, characteristic of undifferentiatedneuroepithelial and radial glial cells (Hockfield and McKay, 1985;Lendahl and McKay, 1990). Because nestin⁺ SVZ cells have the ability to incorporate BrdU and proliferate(Morshead et al., 1994), we sought to determine whether therewas an increase in the percentage of nestin⁺-BrdU⁺ cells after the administration of BDNF. Although we observeda few nestin⁺ cells in the SVZ surrounding the lateral ventricle as well asaround the cortical lesion made by the infusion catheter, theywere absent from the parenchyma. Moreover, only a low percentageof the nestin⁺ cells in the SVZ incorporated BrdU. The low percentage of nestin⁺-BrdU⁺ cells, in conjunction with the relatively high percentage ofBrdU⁺ cells expressing neuronal or astrocytic markers, suggests thatthe majority of the newly generated cells undergodifferentiation.

Infusion of BDNF and PBS results in the formation of "polyp-like" hyperplasias of the ventricular wall

To determine whether the infusion of BDNF or PBS induces the formation of "polyps" similar to those described after intracerebroventricularinfusion of EGF (Kuhn et al., 1997), we analyzed the BDNF- andPBS-infused brains for the incidence of polyp formation and theirphenotypic composition. Intraventricular polyps were observedprotruding into the infused lateral ventricle in both the BDNF-and PBS-infused brains. These polyps were not present in the uninfusedlateral or third ventricles. After BDNF infusion, several small(<200 µm in diameter) polyps were found emanating from the wallof the lateral ventricle lining the striatum (Fig. 10B), septum,and corpus callosum. These hyperplasias consisted of cells thatwere predominantly TuJ1⁺; very few of the cells were GFAP⁺ (data not shown). A low proportion of the cells within the polypwere BrdU⁺, but the underlying ventricular wall usually contained a highproportion of BrdU⁺ cells. In contrast, the PBS-infused brains contained considerablylarger polyps (up to 600 µm in diameter) that were devoid of astrocyticand neuronal markers, except for a central core containing predominantlyneurons (Fig. 10A) and a low number of glia (data not shown). Thepolyps formed after PBS-infusion consist of a much higher densityof BrdU⁺ undifferentiated cells. The characteristics of the polyps observedafter BDNF-infusion suggest that the BDNF promotes the differentiation,but perhaps not the formation, of these polyps.

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Figure 10. The protrusion of hyperplastic polyps into the lateral ventricle of the brain of an adult rat after the intracerebroventricular administration of BDNF-BrdU or PBS-BrdU. A, B, Coronal sections (20 µm) stained with anti-BrdU (bright orange) and TuJ1 (green) and visualized by a dual fluorescein-rhodamine filter. A, A representative hyperplastic polyp situated along the striatal wall formed 16 d after a 12 d interval of intracerebroventricular PBS-BrdU administration. The polyp consists of multiple layers of BrdU⁺/TuJ1 cells surrounding a central TuJ1⁺/BrdU core. Notice the abundance of BrdU⁺ cells in the polyp compared with the low number of BrdU⁺ cells in the adjacent striatal SVZ (e.g., arrows). B, A representative hyperplastic polyp from the striatal wall after intracerebroventricular administration of BDNF and BrdU. The polyp contains cells with a high level of TuJ1 immunoreactivity and a low level of BrdU incorporation and is considerably smaller than the polyp in A resulting from the PBS infusion, indicating that the hyperplastic polyp formed after BDNF administration is more differentiated than that after PBS infusion. Also note that, in B, there are numerous BrdU⁺ cells in the striatal SVZ immediately underlying the polyp. LV, Lateral ventricle; SPT, septum; ST, striatum. Scale bars: A, 100 µm; B, 50 µm.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Our study disputes the belief that the SVZ and hippocampus are the only areas of the forebrain that generate new neurons throughoutlife. In this study, we demonstrate that, 16 d after a 12 d intervalof BDNF-BrdU administration, new neurons occur not only in theSVZ lining the lateral ventricle but also in the striatum, septum,thalamus, and hypothalamus. After BDNF infusion, numerous BrdU-labeledneurons were identified in restricted regions bordering the rostrocaudalextent of the lateral and third ventricles. The BrdU-immunoreactivecells were only present in regions expressing TrkB, the high-affinityreceptor for BDNF. However, the TrkB⁺ cells were not themselves BrdU⁺. Our study demonstrates that the adult forebrain has a greatercapacity to produce new neurons than recognized previously andthat exogenous BDNF can trigger an immense proliferation and appearanceof new neurons in the parenchyma of theforebrain.

BDNF leads to the production of newly generated cells in the adult forebrain

Previous experiments have suggested that BDNF can promote the survival and/or differentiation of cells in vitro and in vivo.In the adult forebrain, BDNF can rescue newly formed cells thatwould otherwise undergo cell death (Morshead and van der Kooy,1992). Moreover, in vitro studies have demonstrated that BDNFcan promote the survival of SVZ cells in both young and senescentrats (Kirschenbaum and Goldman, 1995; Goldman et al., 1997). However,in our study, simply the prevention of cell death seems insufficientto account for the immense number of BrdU-immunoreactive cellsin the SVZ, striatum, and septum, as well as in regions in whichcell proliferation has never been described previously, such asthe thalamus andhypothalamus.

Our data suggests that the BDNF infusion triggers cell proliferation in the adult forebrain. The BDNF effects, however, mustbe distinguished from those of the implantation of a cannula andthe infusion of the vehicle (PBS) used for BDNF delivery. Weinsteinet al. (1996) showed that the insertion of a cannula into thelateral ventricle increases the proliferation of SVZ cells, suggestingthat a low rate of proliferation might be induced by the mechanicaldisruption of the SVZ. Whether SVZ "trauma" releases neurotrophinsor cytokines that cause a proliferative response remains to bedetermined. However, the level of proliferation after PBS-BrdUinfusion is much lower than that after BDNF-BrdU administration.This discrepancy indicates that the BDNF actions are above andbeyond those attained by PBS alone. Therefore, we conclude thatBDNF profoundly increases the cell proliferation and/or survivalof progenitor cells and theirprogeny.

Presumptive subventricular and nonsubventricular origins of the newly generated cells in the adult forebrain

In our study, numerous newly generated cells were found in several parenchymal structures after BDNF infusion. One hypothesisto account for this distribution is that the SVZ cells divideand their progeny migrate into the nearby parenchyma, much likeafter the intracerebroventricular infusion of EGF (Craig et al.,1996). This scenario is also similar to the generation of newneurons in the adult primate brain reported by Gould et al. (1999).However, in our study, in contrast to that of Craig et al. (1996),we did not observe an expansion of the SVZ, with the exceptionof the anterior part of the SVZ and the RMS leading to the olfactorybulb. Moreover, in restricted regions such as the hypothalamus,we observed a significant number of new BrdU⁺ cells in the apparent absence of a SVZ. This suggests that, inagreement with Magavi et al. (2000), the SVZ may not be the onlysource of new neurons in the adult forebrain. Furthermore, theoccurrence of newly generated cells in the parenchyma may indicatethat progenitor cells are normally present in situ and are inducedto divide after BDNF exposure. In fact, multipotent progenitorcells have been shown to reside in parenchymal structures of theadult forebrain (Reynolds et al., 1992; Palmer et al., 1995; Marmuret al., 1998; Laywell et al., 2000). These progenitor cells exhibita robust proliferation in response to the in vitro exposure toparticular growth factors. Furthermore, Magavi et al. (2000) demonstratedthat newly generated neurons can be observed in the adult mousecerebral cortex after lesion of layer VI neurons. The authorsconcluded that at least some neurons were generated in situ. Inour study, a high percentage of the newly generated parenchymalcells occurred in pairs. This could arise by a number of mechanisms,including the division of "activated" cells residing in the parenchymaor, alternatively, the division within the parenchyma of progenitorcells that originated in the SVZ. Additional experiments are neededto distinguish between these possibilities. The sparse ongoingproliferation present in the adult mammalian brain may thereforebe attributable to a limitation in the availability of certaingrowth factors and regulatory signals rather than an absence ofprogenitorcells.

Although the division of parenchymal progenitor cells in situ could explain the occurrence of newly generated cells in theparenchymal structures lacking a distinguishable SVZ, it is notclear whether BDNF can diffuse more than a few hundred micrometersaway from the ventricular wall to directly affect distant progenitors.Previous studies have shown a negligible parenchymal diffusionof BDNF after its administration into the lumen of the lateralventricle for 14 d (Yan et al., 1994; Anderson et al., 1995).Because TrkB is abundantly expressed in the SVZ surrounding thelateral ventricle (Yan et al., 1994; Zigova et al., 1998), theBDNF binding to TrkB receptors might limit the diffusion of BDNF.Therefore, the actions of BDNF could be restricted to progenitorcells situated in proximity to the ventricle, and the migrationof progenitor cells into the depth of the parenchyma might beat least partially responsible for the extensive distributionof the newly generatedcells.

The possible direct and indirect involvement of TrkB receptors in the production of newly generated neurons in the adult forebrain

An unexpected finding of this study was the variable level of BrdU incorporation in structures presumably exposed to a uniformconcentration of BDNF-BrdU. For example, although there were numerousBrdU⁺ cells in the thalamic habenular nuclei, there were no BrdU⁺ cells in the overlying part of the dentate gyrus, also adjacentto the third ventricle. Moreover, the structures closest to theventricle did not always exhibit the highest level of BrdU incorporation.For example, in the hypothalamus, there is a higher density ofBrdU⁺ cells in the paraventricular nucleus, despite its location fartheraway from the ventricle. An explanation for the difference inthe density of BrdU⁺ cells is that the regions with high cell proliferation have highTrkB expression, whereas the regions with a very low level ofcell proliferation have low TrkB expression. Together, these findingssuggest that the distribution of newly generated cells after BDNFinfusion may be at least partially influenced by the pattern ofBDNFexpression.

Although the regions with increased cell proliferation coincide with areas of high TrkB expression, the newly generated BrdU⁺ cells were not TrkB⁺. The absence of the TrkB receptor from the membrane of the BrdU⁺ cells may indicate that BDNF does not act directly on progenitorcells but rather initially influences the cells surrounding them.This notion is supported by our confocal analysis in which TrkB⁺ cells were frequently adjacent to BrdU⁺ cells. The possibility that TrkB⁺ cells exert a paracrine influence on progenitors cannot be ruledout. Another hypothesis to account for the absence of TrkB receptorfrom the membrane of the newly generated cells is the downregulationof the TrkB receptor after BDNF exposure. Alternatively, afterbinding BDNF, the progenitor cells may internalize their TrkBreceptor, which results in the masking of the antigenic sitesrecognized by our antibody. Previous studies have shown that internalizationand transport of the ligand-receptor complex are required to initiatesome responses to neurotrophins (Bergeron et al., 1995; Zhanget al., 2000). Hence, it will be important to elucidate whetherthe internalization of the BDNF-TrkB complex plays a role in thesurvival and/or differentiation of the newly generated cells afterBDNF infusion of the adultforebrain.

Concluding remarks on the potential relevance of BDNF infusion to strategies for neuronal replacement

Recent studies have demonstrated that, in brains affected by neurodegenerative diseases, discrete regions characterized byloss of neurons have abnormally low levels of BDNF expression.In particular, Ferrer et al. (2000) have shown that, in Huntington'sdisease, BDNF is reduced by 53-82% in the caudate and putamen,two regions exhibiting neuronal loss. Similar studies also suggestthat, in Alzheimer's disease, decreased levels of BDNF leads tolack of trophic support for susceptible neurons, and thus, contributesto the degeneration of specific neuronal populations (Hock etal., 2000). Collectively, these findings indicate that BDNF isimportant for the survival of certain neuronal populations inthe adult forebrain. Thus, if BDNF could be provided exogenously,it could potentially serve to promote the formation of numerousnew neurons in extensive regions of the mammalian brain. Our futurestudies will seek to reveal whether BDNF can rescue degeneratedneurons or help achieve replacement of neurons already lost asa result of a diseaseprocess.

  FOOTNOTES

Received Feb. 20, 2001; revised June 5, 2001; accepted June 7, 2001.

This work was supported by National Institute of Deafness and Other Communicative Disorders Grant RO1 DC03190 (M.B.L.) andby Regeneron Pharmaceuticals, Inc. We are grateful to Dr. GiriVenkatraman, Dr. Volkan Coskun, and Joanna Bonsall for their criticaland helpful comments on this manuscript and to Dr. Stuart C. Feinsteinfor his generous gift of anti-TrkB.
Correspondence should be addressed to Dr. Marla B. Luskin, Department of Cell Biology, Emory University School of Medicine,1648 Pierce Drive, Atlanta, GA 30322. E-mail: luskin{at}cellbio.emory.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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