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The Journal of Neuroscience, September 1, 2001, 21(17):6718-6731
Adenoviral Brain-Derived Neurotrophic Factor Induces Both
Neostriatal and Olfactory Neuronal Recruitment from Endogenous
Progenitor Cells in the Adult Forebrain
Abdellatif
Benraiss,
Eva
Chmielnicki,
Kim
Lerner,
Dongyon
Roh, and
Steven A.
Goldman
Department of Neurology and Neuroscience, Cornell University
Medical College, New York, New York 10021
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ABSTRACT |
Neural progenitor cells persist throughout the adult forebrain
subependyma, and neurons generated from them respond to brain-derived neurotrophic factor (BDNF) with enhanced maturation and survival. To
induce neurogenesis from endogenous progenitors, we overexpressed BDNF
in the adult ventricular zone by transducing the forebrain ependyma to
constitutively express BDNF. We constructed a bicistronic adenovirus
bearing BDNF under cytomegalovirus (CMV) control, and humanized green
fluorescent protein (hGFP) under internal ribosomal entry site (IRES)
control. This AdCMV:BDNF:IRES:hGFP (AdBDNF) was injected into the
lateral ventricles of adult rats, who were treated for 18 d
thereafter with the mitotic marker bromodeoxyuridine (BrdU). Three
weeks after injection, BDNF averaged 1 µg/gm in the CSF of
AdBDNF-injected animals but was undetectable in control CSF. In
situ hybridization demonstrated BDNF and GFP mRNA expression restricted to the ventricular wall. In AdBDNF-injected rats, the olfactory bulb exhibited a >2.4-fold increase in the number of BrdU+- III-tubulin+
neurons, confirmed by confocal imaging, relative to
AdNull (AdCMV:hGFP) controls. Importantly, AdBDNF-associated
neuronal recruitment to the neostriatum was also noted, with the
treatment-induced addition of
BrdU+-NeuN+-III-tubulin+
neurons to the caudate putamen. Many of these cells also expressed glutamic acid decarboxylase, cabindin-D28, and DARPP-32 (dopamine and
cAMP-regulated phosphoprotein of 32 kDa), markers of medium spiny
neurons of the neostriatum. These newly generated neurons survived at
least 5-8 weeks after viral induction. Thus, a single injection of
adenoviral BDNF substantially augmented the recruitment of new neurons
into both neurogenic and non-neurogenic sites in the adult rat brain.
The intraventricular delivery of, and ependymal infection by, viral
vectors encoding neurotrophic agents may be a feasible strategy for
inducing neurogenesis from resident progenitor cells in the adult brain.
Key words:
neurotrophic factors; neurogenesis; stem cells; gene
therapy; Huntington's disease; neostriatum
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INTRODUCTION |
Neural progenitor cells persist
throughout the adult forebrain subependyma and have been found in
species ranging from canaries to humans (Goldman and Nottebohm, 1983 ;
Alvarez-Buylla and Lois, 1995; Goldman et al., 1997b; Goldman and
Luskin, 1998). To the extent that neurogenesis and oligoneogenesis by
these endogenous progenitors may be induced or supported exogenously,
these cells may provide a cellular substrate for repair in the adult
CNS. In culture, adult-derived progenitors have been found to respond to mitogens, in particular epidermal growth factor (EGF) and fibroblast growth factor-2 (FGF-2), with increased division and neuronal mitogenesis (Reynolds and Weiss, 1992; Richards et al., 1992; Vescovi
et al., 1993; Palmer et al., 1995). Furthermore, neurons generated from
them respond to brain-derived neurotrophic factor (BDNF) with enhanced
migration, maturation, and survival in vitro (Kirschenbaum
and Goldman, 1995; Goldman et al., 1997a; Pincus et al., 1998).
Similarly, infusions of EGF and FGF-2 into the adult ventricular system
stimulate mitotic gliogenesis and neurogenesis, respectively (Craig et
al., 1996; Kuhn et al., 1997), whereas intraventricular infusions of
BDNF can enhance neuronal migration to the olfactory bulb, rostral
migratory stream (RMS), and adjacent forebrain (Zigova et al., 1998;
Pencea et al., 1999). Although intriguing, these studies have been
limited by the need for chronic intraventricular catheterization, with
its dependence on protein availability and stability, the uncertain
tissue bioavailability of intraventricularly administered proteins, and
the risks of infection and catheter loss inherent in chronic ventriculostomy.
On the basis of these studies, and of their limitations in practice, we
realized the need for an efficient means of delivering neurotrophic
differentiation agents to the adult subependyma. Previous studies had
reported that ependymal cells could express adenovirally delivered
genes after intraventricular injection of virus (Bajocchi et al., 1993;
Yoon et al., 1996). The high efficiency infection of, and transgene
expression by, the adult ependyma suggested to us that intraventricular
delivery of adenoviral vectors might be used for the sustained delivery
of neurotrophins not only to the ventricular zone but also to the CSF,
and hence throughout the neuroaxis. We therefore chose to use an
adenoviral vector to transduce the forebrain ependymal wall to
constitutively overexpress BDNF, with the goal of inducing neurogenesis
from endogenous progenitor cells. We report here that infection of the
adult rat ventricular lining with an adenoviral BDNF expression vector
resulted in the diffuse transduction of the adult ependymal wall, with
the effective subrogation of the ependyma into a source of secreted
BDNF protein to both the CSF and periventricular parenchyma. This
resulted in sustained and high-level BDNF secretion by the ventricular
wall and was associated with a >2.4-fold increase in the recruitment
of new neurons to the olfactory bulb in the 3 weeks after viral
administration. Importantly, AdCMV:BDNF:IRES:hGFP (AdBDNF) injection
was also associated with the heterotopic addition of new neurons to the
neostriatum, an otherwise non-neurogenic region of the adult brain.
These striatal neurons matured to express antigens typical of medium
spiny neurons and were found in undiminished numbers for at least 8 weeks after AdBDNF injection. Together, these results demonstrate that
viral delivery of neurotrophin genes may be a viable strategy for
modulating the induction, differentiation, and fate of ventricular zone
progenitor cells in the adult mammalian forebrain.
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MATERIALS AND METHODS |
Adenovirus construction
We constructed an adenoviral vector bearing BDNF under the
control of the constitutive cytomegalovirus (CMV) promoter, placed in
tandem sequence with humanized green fluorescent protein (hGFP), under
the control of an internal ribosomal entry site (IRES) (Morgan et al.,
1992). In brief, BDNF cDNA (Regeneron Pharmaceuticals, Tarrytown, NY)
was obtained in SpeI/HindIII. A
HindIII/SalI segment containing an IRES site
(Morgan et al., 1992) and hGFP were taken from pTRUFIII (Levy et al.,
1996). On digestion with SpeI/HindIII of
pBDNF, the 1.1 kb TRUFIII HindIII/SalI
fragment was ligated into the adenovirus shuttle vector pCMV:SV2,
digested with SpeI/SalI. The resultant construct
was designated pAdP/CMV:BDNF:IRES:hGFP. Established methods (Graham and
Prevec, 1991) were then used to construct a replication-defective
recombinant adenovirus via homologous recombination using the plasmid
pJM17, which contains the E1A-deleted type 5 adenovirus.
pAd5/CMV:BDNF:IRES:hGFP was cotransfected with pJM17 into human
embryonic kidney 293 (HEK293) cells, and viral plaques developed for 2 weeks. Crude viral lysates were then used for plaque purification.
Virus was propagated in HEK293 cells, purified by cesium chloride
density gradient centrifugation, and stored at  70°C. The resultant
titer of AdBDNF was between 1011 and
1012 pfu/ml; however, both AdBDNF and its
AdNull (AdCMV:hGFP) control were titered to 2.5 - 1010 pfu/ml before use to ensure that
experimental and control rats received equivalent viral loads (see
below). The efficacy of AdBDNF in driving expression of BDNF was
verified in HeLa cells by ELISA. In addition, the expression of GFP by
each virus was confirmed at 1 and 3 weeks after viral injection both in
sections of the adult ventricular wall using direct fluorescence
observation and by in situ hybridization of both BDNF and GFP.
Cell culture and in vitro experiments
HeLa cells were plated at a density of 1 × 106/25 cm2 in
Ham's F12 with 10% FBS. After 24 hr, the cells were infected with 1, 10, or 100 multiplicities of infection (moi) of AdBDNF or AdCMV:GFP in
F12 with 1% FBS. After 24 hr, serum was added to achieve a 10%
concentration of FBS. After another 24 hr, the cells were washed and
switched to serum-free media for 3 d. The cells and their media
were then separately collected; the media was decanted to storage at
80°C for later ELISA of BDNF, and the cells were collected in
Ca/Mg-free HBSS-1 mM EDTA and pelleted. The cellular pellet was then resuspended in 10% FBS-containing media and subjected to viability assay; this was done to assess potential viral toxicity in
these same cultures. Triplicate 50 µl aliquots of resuspended cells
were diluted in trypan blue (1:1) to label dead cells; both live and
dead cells were separately counted 20 min later by a hemocytometer, and
their ratio was determined.
Experimental design and stereotaxic injection
Either the AdBDNF or AdNull viruses were delivered as single 3 µl injections into the lateral ventricles of seven adult rats. Both
viruses were established in the same backbone and titered to 2.5 × 1010 pfu/ml before use. Using a David Kopf Instruments
(Tujunga, CA) stereotactic frame, the rats were injected at the
following coordinates: anteroposterior, 0.3 mm; mediolateral, ±1.2
mm; dorsoventral, 3.6 mm (Paxinos and Watson, 1986). The rats were
injected daily for 18 d thereafter with the mitotic marker
bromodeoxyuridine (BrdU) (100 mg/kg, i.p.). Control animals were
injected with either AdCMV:GFP (AdNull; n = 5) or PBS
(n = 5). These animals were killed on the day after the
last BrdU injection (day 20). Among them, four each of the AdBDNF-,
AdNull-, and PBS-injected animals were used for the quantification of
BrdU+ cells in the olfactory bulb,
striatum, and other regions assessed; the remainder of the animals
killed on day 20 were used to supplement our assessment of the CSF BDNF levels.
An additional sample of three rats was injected with AdBDNF and BrdU as
noted but killed on the 35th day after the completion of BrdU
treatment, on day 56 after viral injection. These rats' brains were
examined solely with regards to the persistence of BrdU+ neurons in the neostriatum. In all
groups, daily weights were recorded beginning with the day of viral
injection, through the day of when the animal was killed.
ELISA
CSF. At 20 d after viral injection, rats were
injected with 0.6 ml of 65 mg/ml pentobarbital and perfused with HBSS
with
Mg2+/Ca2+
(Life Technologies, Gaithersburg, MD). CSF was collected from the
cisterna magna, aliquoted, and stored at 80°C. The BDNF in the CSF
of both PBS-injected and AdNull- or AdBDNF-injected rats was quantified
using a two-site ELISA (Emax Immunoassay System; Promega, Madison, WI)
(Mizisin et al., 1997), the use of which we have described previously
in detail (Leventhal et al., 1999) Briefly, the monoclonal anti-BDNF
capture antibody did not cross-react with other members of the
neurotrophin family at concentrations up to 10,000 times that used for
the standard curve, whereas the reporter antibody was a biotinylated
rabbit polyclonal anti-BDNF, similarly selective for BDNF. The dynamic
range of the ELISA was 10-1000 pg/ml for undiluted samples; all
samples were diluted in assay buffer to bring them into the linear
range of the standard curve of the assay. The CSF BDNF determinations
were derived from a total of seven AdBDNF-, five AdNull-, and three
PBS-injected animals. Total protein levels of each CSF sample were
assessed by BCA assay (Pierce).
Cells. For the supernatants of AdBDNF- and AdNull-infected
HeLa cell layers, BDNF levels were reported as the average of
triplicate samples
In situ hybridization
Probes. BDNF antisense and sense probes were generated from
pSK-rBDNF, a gift of Regeneron Pharmaceuticals. The BDNF plasmid DNA
was linearized with either BamHI for the antisense probe or EcoRV for the sense control and then transcribed in
vitro using either T7 RNA polymerase for the antisense probe or T3
RNA polymerase for the sense probe. The antisense GFP probe was
generated by linearizing pGFP with XbaI and transcribing
in vitro with T3 RNA polymerase. The probes were
non-isotopically labeled with digoxigenin-11-UTP (Boehringer Mannheim,
Mannheim, Germany).
Hybridization. A series of 15 µm cryostat sections were
permeabilized with 0.3% Triton X-100 in PBS for 15 min. The sections were dehydrated in ascending alcohols, cleared with xylene, rehydrated, treated with Proteinase K (1 µg/ml) for 30 min at 37°C, and
post-fixed with 4% paraformaldehyde for 5 min. To acetylate sections,
slides were incubated for 30 min in 0.1 M
triethanolamine buffer, pH 8.0, containing 0.25% acetic anhydride. The
sections were prehybridized with 4× SSC containing 50% formamide for
1 hr and then hybridized under coverslips for 15 hr at 42°C with
digoxygenin-labeled sense or antisense probes (300 ng/ml) in 40%
deionized formamide, 10% dextran sulfate, 1× Denhardt's solution,
4× SSC, 10 mM dithiothreitol, and 1 mg/ml salmon
sperm DNA. After hybridization, the sections were washed in 2× SSC for
5 min to remove the coverslips, washed with 50% formamide in 2× SSC
for 20 min at 52°C, washed in 2× SSC, and treated with RNase A (20 µg/ml) in 2× SSC for 30 min at 37°C. After four washes in 2× SSC,
the sections were washed with 0.2× SSC at 55°C for 1 hr.
Detection of digoxygenin-labeled probes. Slides were washed
in Tris-buffered saline (TBS) (0.1 M Tris-HCl
with 150 mM NaCl), three times for 5 min each,
blocked in 0.1% Triton X-100 and 2% sheep serum for 30 min, and then
incubated overnight at 4°C in alkaline phosphatase-conjugated
anti-digoxygenin (1:100; Boehringer Mannheim). After washing with TBS,
the sections were switched to detection buffer (100 mM Tris-HCl, pH 9.5, with 100 mM NaCl and 50 mM
MgCl2) for 10 min and incubated in
nitroblue-tetrazolium-chloride and 5-bromo-4-chlor-indolyl-phosphate
solution (Bio-Rad, Hercules, CA) with 1 mM
levamisole for 2-20 hr in the dark. During color development, the
reaction was terminated by washing (three times for 5 min each) in TBS
with 10 mM EDTA.
Immunohistochemistry
The animals were killed and perfusion fixed, and their
brains were removed on either the 20th or 56th day after viral
injection. Fixation was accomplished using 4% paraformaldehyde in 0.1 M phosphate buffer (PB), pH 7.4, with a 90 min post-fix
followed by immersion and sinking in 30% sucrose in PB. All brains
were cut as 15 µm sagittal sections that included the olfactory bulb
and rostral migratory stream rostrally; these were stained for BrdU
using immunoperoxidase detection when staining for BrdU alone or using double-immunofluorescence when staining for both BrdU and neuronal markers. Individual sections were denatured in 2N HCl for 1 hr and then
stained for BrdU using rat anti-BrdU antibody at 1:200 (Harlan Sprague
Dawley, Indianapolis, IN), followed serially by fluorescein-conjugated
anti-rat IgG at 1:150 (Jackson ImmunoResearch, West Grove, PA). The
sections were then washed and stained for the following:
III-tubulin, using the TuJ1 monoclonal antibody (Lee et al., 1990)
(a gift of Dr. A. Frankfurter, University of Virginia Medical School,
Charlottesville, VA); microtubule-associated protein-2 (MAP-2), using
rabbit anti-MAP-2 (Bernhardt and Matus, 1984) (Dr. S. Halpain, The
Scripps Institute, La Jolla, CA); NeuN (Eriksson et al., 1998)
(Chemicon, Temecula, CA); glutamic acid decarboxylase 67 (GAD67)
(Sigma, St. Louis, MO); calbindin-D28K (Guan et al., 1999) (Sigma); or
DARPP-32 (dopamine and cAMP-regulated phosphoprotein of 32 kDa )
(Ivkovic and Ehrlich, 1999) (Dr. H. Hemmings, Cornell University
Medical College, New York, NY), each as described previously (Goldman
et al., 1992; Menezes and Luskin, 1994; Eriksson et al., 1998; Guan et
al., 1999; Ivkovic and Ehrlich, 1999; Roy et al., 2000). All anti-mouse
secondary antibodies were preabsorbed against rat IgG to avoid
nonspecific staining.
Confocal imaging
In sections double-stained for BrdU together for III-tubulin,
MAP-2, NeuN, DARPP-32, GAD67, or calbindin-D28, single
BrdU+ cells appeared to be double-labeled
for both the neuronal antigen and BrdU were identified and evaluated by
two-color confocal imaging. Using a Zeiss (Oberkochen, Germany) LSM510
confocal microscope, images were acquired in both red and green
emission channels using an argon-krypton laser. The images were then
viewed as stacked z-dimension images, both as series of
single 0.9 µm optical sections and as merged images thereof. The
z-dimension reconstructions were all observed in profile,
because every BrdU+ cell double-labeled
with a neuronal marker was then observed orthogonally in both the
vertical and horizontal planes. Only after three observers
independently deemed individual cells as double-labeled, with central
BrdU immunoreactivity surrounded by neuronal immunoreactivity at all
observation angles in every serial optical section and in each merged
and rotated composite, were the cells scored as double-labeled, newly
generated neurons.
Scoring and quantification
BrdU+ cell counts.
Unbiased counting was used to score the number, density, and
distribution of BrdU+ cells in the
injected brains using an optical dissector procedure (Sterio, 1984;
Kuhn et al., 1997; West, 1998). To estimate the number of BrdU-labeled
cells per region, we sampled 22 15 µm sections per animal for both
experimentals and controls; for each, every sixth section was analyzed
at 90 µm intervals. The first section of each sagittal series was
chosen randomly from a total sample that was accumulated beginning with
the first appearance of the olfactory cortex on cresyl violet-stained
alternate sections. Typically, the sampled region included that
subtended by the stereotaxic coordinates L0.3-L2.3 bilaterally. By
this means, we sampled a 2 mm mediolateral segment in the sagittal
plane, centered on the RMS.
Regions assessed. The absolute number of total
BrdU+ cells in every eighth 15 µm
sagittal section was counted in each of six regions: (1) the anterior
surface of the ventricular zone, (2) the olfactory subependyma of the
RMS; (3) the olfactory bulb, (4) the medial septum, (5) the
neostriatum, and (6) the frontal cortex overlying the corpus callosum,
rostral to the perpendicular extension of the rostral-most wall of the
lateral ventricle.
Imaging and scoring. In each sampled section, every
BrdU+ nucleus was counted in each scored
region; the positions of each of these cells were entered manually into
BioQuant image analysis software with its incorporated topography
reconstruction package, and the results were tabulated. For each
region, the results were reported as the mean number of
BrdU+ cells per section. In addition, for
the olfactory bulb and the neostriatum, these counts were converted
into BrdU+ cells per cubic millimeter
after determining the surface areas and hence volumes of each scored
region (Michel and Cruz-Orive, 1988). Statistical analysis was then
accomplished by ANOVA, followed by post hoc Boneferroni
t tests.
Striatal neuronal counts. To estimate total striatal
neuronal number, we counted the number of striatal neurons in each of six age- and sex-matched rats, three of which were treated with AdBDNF
and the other three with AdNull as a negative control
(n = 3). From each, we analyzed eight 15 µm sections,
representing every 32nd sequentially, thereby sampling at 480 µm
intervals beginning with the first appearance of rostrocaudally
oriented striatal fascicles on cresyl violet-stained alternate
sections. In these cresyl violet-stained sections, the number of
neurons in each striatum was counted under high magnification using
morphological criteria for neuronal identity by an observer blind as to
the experimental group. To this end, neurons were defined as large cells of >10 µm diameter, with pale central nuclei and central nucleoli, in an otherwise basophilic cytoplasm. To ensure the validity
of these criteria, two sections from each set of eight were destained
by acidified ethanol and then immunostained for calbindin. The number
of calbindin-defined striatal neurons was then counted and compared
with that obtained in the same section by cresyl violet. We found
>98% concordance in the neuronal counts obtained using these two methods.
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RESULTS |
Intraventricular delivery of adenoviral CMV:hGFP restricted
transgene expression to the adult ependyma and subependyma
To first assess the distribution of adenoviral transduction
after a single intraventricular injection of virus, we injected adenovirus bearing the gene encoding green fluorescent protein (hGFP),
placed under the control of the CMV promoter, into the lateral
ventricles of four adult Sprague Dawley rats. The rats were killed
either 1 or 3 weeks later, and their brains were prepared for
histology. We found that, in all four rats, most ependymal and
scattered subependymal cells labeled heavily to single viral injection,
with virtually the entire lining of the lateral ventricle noted to
express GFP after injection of 3 × 107 pfu adenovirus (3 µl of
1010 pfu/ml). Little parenchymal
expression of GFP was noted, despite the lack of specificity of the CMV
promoter, suggesting that viral penetration outside of the subependyma
was minimal (Fig. 1). The restriction of
transgene expression to the ventricular wall suggested that ependymal
cells might be targeted selectively on spatial grounds alone, even
without benefit of cell-specific promoters.
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Figure 1.
Ependymal restriction of intraventricular
adenoviral infection. A, A single intraventricular
injection of an adenoviral vector bearing GFP, expressed under the
control of the constitutive CMV promoter, shows the widespread
infection of the ventricular ependyma, bilaterally and throughout the
ventricular system 1 week after viral injection. B,
Along the striatal and septal walls, GFP expression was primarily
limited to the ventricular surface, with little subependymal and no
parenchymal extension. A, B, Sagittal
sections. C, A coronal section taken at the level of the
main body of the lateral ventricles again reveals GFP expression by the
infected striatal and callosal ventricular surfaces. Unlike the
striatal and septal walls, the callosal wall shows subependymal and
some parenchymal extension of labeled cells. Str,
Striatum; LV, lateral ventricle; CC,
corpus callosum; D, dorsal; V, ventral;
A, anterior; P, posterior.
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AdBDNF-infected cells expressed BDNF in vitro
We next sought to assess the effects of adenovirally
delivered BDNF on the adult ventricular zone pool. A  E1 type 5 adenovirus was thus constructed to express BDNF under the control of
the constitutively activated CMV promoter; the virus also included hGFP
as a reporter, placed under IRES promoter control. The resultant vector, AdBDNF, was characterized first by infecting HeLa cells, which
typically do not express BDNF. The production of BDNF by the infected
HeLa cells was assessed as a function of time after infection, using
ELISA of BDNF secreted to the culture media. BDNF release in response
to AdBDNF infection was thereby compared with that of both
untransfected and AdNull-infected control cells (Fig.
2A,B).
Within 2 d after infection with 10 pfu/cell AdBDNF, 234 ± 54.5 ng/ml BDNF protein was measured in the culture supernatant, ~250-fold greater than the levels observed in the uninfected
(0.8 ± 1.0 ng/ml) and AdNull-infected (1.0 ± 0.6 ng/ml)
control cultures. Thus, AdBDNF directed high-level expression of BDNF
by HeLa cells.
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Figure 2.
Adenoviral BDNF infection yielded high-level BDNF
expression in vitro and in vivo. A,
B, HeLa cells transduced with AdBDNF secreted BDNF in a
viral dose-dependent manner (n = 3).
C, D, AdBDNF-injected animals showed
sustained expression of high levels of BDNF in CSF, as measured on day
20 (n = 5). A and C
show results in picograms per milliliter, and B and
D are given in picograms per microgram of protein.
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To ensure that transgene expression was not accomplished at the expense
of cell viability, we assessed trypan blue inclusion as a function of
viral dose over the range of 1-10 moi/cell and found that
adenovirus-associated toxicity was minimal and statistically insignificant over this dose range. In addition, to ensure that this dose range was no more toxic for primary brain cells than for HeLa
cells, we assessed the effect of increasing viral dose on the viability
of primary adult human astrocytes, obtained from temporal lobes
resected from adult epileptic patients (Leventhal et al., 1999). We
found that astrocytes exposed to 10 moi AdBDNF exhibited no significant
increment in lethal toxicity at 48 hr after infection.
CSF levels of BDNF rose markedly after intraventricular injection
of AdBDNF
To assess the level of release of BDNF protein into the CSF of
AdBDNF-treated rats, a total of 14 animals were injected with AdBDNF
(n = 7), AdNull (n = 5), or PBS
(n = 2); all were subjected to cisterna magna puncture
for CSF withdrawal at 3 weeks after viral infection. In the
AdBDNF-injected animals, ELISA revealed that CSF BDNF levels averaged
1.07 ± 0.3 µg/gm protein (mean ± SE) when assessed 3 weeks after injection (Fig. 2C,D). This
represented 2.02 ± 0.6 ng of BDNF per milliliter of ventricular
CSF, a level within the dose range appropriate for eliciting
TrkB-mediated biological effects in vitro (Lindsay et al.,
1994). In contrast, BDNF was undetectable in both the PBS and AdCMV:GFP
controls (p = 0.025 by ANOVA;
F(2,13) = 5.24). The absence of
detectable BDNF in the AdNull-injected controls indicated that the BDNF
levels achieved in the CSF of AdBDNF-treated animals was a product of the virally encoded BDNF transgene. Thus, adenoviral transduction of
the adult ventricular ependyma permitted high-level delivery of BDNF to
the brain and CSF, with expression that was sustained for at least 3 weeks after viral infection.
Adenoviral-transduced BDNF mRNA was restricted to the
ventricular wall
In situ hybridization, using RNA probes for BDNF and
hGFP, revealed that AdCMV:BDNF:IRES:GFP transduced expression of both BDNF and hGFP mRNA in vivo. Strikingly, BDNF and GFP mRNAs
were largely restricted to the wall of the lateral ventricular system (Fig. 3). Even when assessed 3 weeks
after viral injection, cells overexpressing BDNF and GFP were primarily
limited to the ventricular wall, with little or no infiltration of the
rostral migratory stream or bulb. Thus, at least rostrally along the
anterior face of the ventricle, the infected cell pool appeared to be
ependymal, with little or no direct infection of subependymal neuronal
migrants. This pattern appeared to be maintained along most of the
rostrocaudal extent of the ventricular system, throughout which virally
transduced BDNF and GFP mRNAs were limited to the ependymal surface,
except at the rostral tip of the lateral ventricles, in which scattered subependymal labeling was also noted.
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Figure 3.
AdBDNF transduced expression of BDNF and hGFP mRNA
in vivo. Serial sections of AdBDNF-GFP-injected brain
were treated with antisense probes for BDNF (A,
D) or GFP (B, E). mRNA
expression was restricted to the wall of the lateral ventricle.
C, Sense probe for BDNF, as control. D , dorsal; V , ventral; R , rostral;
C , caudal. Scale bar, 35 µm.
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AdBDNF infection of the ventricular wall increased substantially
the number of new neurons in both the rostral migratory stream and
olfactory bulb
To follow the generation and fates of new neurons generated from
the AdBDNF-treated ventricular zone, we injected an initial cohort of
rats with either AdBDNF or AdNull (n = 4 per group). These injections were followed with daily intraperitoneal injections of
BrdU at 100 mg/kg for the next 18 d. On day 20, the animals were
killed, CSF was extracted for BDNF ELISA, and the brains were fixed
along with the olfactory bulbs. The brains were then sectioned and
stained for BrdU in tandem with phenotype-specific markers (Fig.
4).
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Figure 4.
Strategy used to induce adult neuronal
recruitment. A, Delivery: schematic coronal section
showing site of injection of adenovirus into the lateral ventricle.
B, Vector: E1-deleted (E1) adenoviral type 5 constructs used to express a bicistronic transcript of BDNF and hGFP
(or hGFP alone, as a control vector) under the control of the
constitutive CMV early promoter. C, Experimental
protocol: adenovirus was injected on day 1, followed by intraperitoneal
injections of 100 mg/kg BrdU for the next 18 d. On day 20, CSF was
extracted for BDNF ELISA, and the brains were processed for BrdU
immunohistochemistry in tandem with phenotype-specific
immunolabeling.
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The effects of AdBDNF on neuronal recruitment were first assessed
in the region of the rostral migratory stream, as measured posteriorly
from the striatum and its ventricular wall up to, and including, the
internal granular layer of the olfactory bulb. Within this region, the
incidence of BrdU+ cells rose from
3398 ± 346 cells/mm3 (mean ± SE) in
the control animals to 8288 ± 1199 cells/mm3 in the AdBDNF-treated rats (Fig.
5). Within the olfactory bulb itself
(measured rostrally from the line connecting the dorsal and ventral
posterior borders of the olfactory cortex), we found that AdBDNF
treatment increased by 2.44 ± 0.1-fold the number of
BrdU+ cells relative to the AdNull
controls (p = 0.0006 by ANOVA;
F(1,7) = 42.1). This value reflected
the cell counts obtained from scoring entire sagittal sections of the
olfactory bulb; the values included both the internal and external
granular zones of the scored bulbs. These results indicated that the
number of cells migrating to the olfactory bulb was substantially
greater in the AdBDNF-treated animals than their AdNull controls.
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Figure 5.
AdBDNF injection increased recruitment to the
olfactory bulb. A, B,
BrdU+ cells in the olfactory bulbs of
AdBDNF:IRES:hGFP (A) AdNull:GFP
(B) injected brains, at day 20. C,
Stereological reconstruction of BrdU+ cells, viewed
here at different mediolateral levels of the olfactory bulb, revealed
substantially higher BrdU+ cell densities in the
olfactory subependyma and granular layers of AdBDNF-treated rats
(C) than in their AdGFP-injected controls
(D). Arrows denote entry to
rostral migratory stream in red. E, The
average number of BrdU+ cells/mm3
in the olfactory bulb (n = 4 per group), plotted as
a function of treatment, again revealed significantly higher numbers of
newly generated BrdU+ cells in AdBDNF-treated rats
than their controls.
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In both the AdBDNF and AdNull animals, the
BrdU+ cells were next double-immunostained
for III-tubulin and/or MAP-2 to establish the proportion of neurons
within the total BrdU+ cell pool (Fig.
6). In both groups, BrdU-incorporating
cells found within the olfactory stream almost invariably expressed III-tubulin immunoreactivity. The same was true in the olfactory bulb, within which double-labeled cells for MAP-2-BrdU were also frequent. Interestingly, MAP-2-labeled
BrdU+ cells were seen only in the bulb and
not in the olfactory subependyma or migratory stream. Instead, these
cells were first noted within the granular layer of the olfactory bulb
itself, consistent with the differentiation of mitotic
III-tubulin+ neuroblasts to postmitotic
MAP-2+ neurons during terminal migration
from the olfactory subependyma to the olfactory cortex (Lois et al.,
1996; Goldman and Luskin, 1998). Quantitatively, in the AdNull-treated
rats, 93.2 ± 0.5% of BrdU+ cells in
the olfactory bulb expressed III-tubulin. This proportion was
virtually identical to that obtained in the AdBDNF-treated olfactory
bulbs, in which an average of 93.0 ± 1.8 and 89.4 ± 2.4%
of BrdU+ cells coexpressed neuronal
III-tubulin or MAP-2, respectively. These data indicate that most
cells recruited to the olfactory bulbs were neurons and that AdBDNF
substantially promoted the addition of these new neurons to the adult
olfactory system.
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Figure 6.
AdBDNF-associated newly generated olfactory cells
were neurons. Confocal imaging confirmed that BrdU+
cells added to the olfactory bulb were almost entirely neurons in rats
injected with virus 3 weeks before being killed and given BrdU daily
until the day before death. A-C, Merged
z-dimension stacks of confocal images of BrdU
(green) colabeling with
III-tubulin+ (A, B;
in red) and MAP-2+ (C;
red) neurons. This suggested that the AdBDNF-associated
increase in the olfactory bulb BrdU labeling index reflected enhanced
neurogenesis and/or recruitment to the bulb. Scale bars, 25 µm.
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Confocal imaging confirmed that cells added to the olfactory bulbs
were neurons
High-magnification confocal imaging confirmed the neuronal
antigenicity of the BrdU-labeled cells in both the rostral migratory stream and olfactory bulb. Representative sections were taken from four
brains, including two AdBDNF-treated experimentals and two AdNull
controls. Midsagittal sections derived from each of these were
double-immunostained for BrdU together with either III-tubulin or
MAP-2 and imaged via confocal laser scanning, with compositing and
reconstruction in the z-dimension to ensure the neuronal
immunoreactivity of BrdU+ cells. This
confirmed that those BrdU+ cells added to
the olfactory bulb were almost entirely neurons, in that they expressed
MAP-2 as well as III-tubulin, and did so in both the AdBDNF- and
AdNull-treated animals. Merged z-stacks of confocal images
of MAP-2+ and
III-tubulin+ neurons, colabeled for
BrdU, confirmed that >90% all BrdU+
nuclei in the olfactory bulb were harbored by
MAP-2+ or
III-tubulin+ cells (Fig. 6). This
indicated that the AdBDNF-associated increases in the olfactory bulb
BrdU labeling indices reflected enhanced neurogenesis and/or
recruitment in the treated animals.
Ventricular AdBDNF infection induced striatal
neuronal recruitment
Despite the extraordinary increase in olfactory neuronal
recruitment in AdBDNF-treated rats, this treatment was not associated with significantly increased cell division outside of the olfactory system. The mean numbers of BrdU+ cells
per section in the frontal cortex, septum, and striatum were all
approximately equivalent in the AdBDNF- and AdNull-injected brains when
assessed 20 d after viral injection (Fig.
7). Nonetheless, this left open the
possibility that AdBDNF might be influencing either the lineage choice
of mitotically active progenitors or the selective survival of their
neuronal daughters. To assess this possibility, we scored the incidence
of
III-tubulin+-BrdU+
cells in each non-olfactory region studied, in both AdBDNF- and AdNull-treated brains. When BrdU+ cells
were identified by epifluorescence microscopy, they were subjected to
two-color confocal imaging with serial sections in the z
plane, to estimate the incidence of double-labeled
III-tubulin+-BrdU+
cells and to ensure that the BrdU+ nuclei
indeed belonged to III-tubulin+ cell
profiles.
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Figure 7.
AdBDNF stimulation of BrdU+
cell addition was pronounced in the olfactory bulb but not appreciable
elsewhere. AdBDNF treatment promoted net BrdU+ cell
addition to the olfactory bulb but not to the septum, striatum, or
cortex. The difference between AdBDNF (red)- and AdNull
(blue)-treated olfactory bulb BrdU labeling indices was
significant to p < 0.001. No other comparisons
based on total BrdU+ cell counts were significant.
However, whereas BrdU+ cell addition to
non-olfactory regions was almost entirely non-neuronal in AdNull
control rats, the BrdU+ cell population included
newly generated neurons in several regions of the AdBDNF-injected
brains. Thus, when
BrdU+-III-tubulin+ neurons
were specifically compared between AdBDNF and AdNull treatment groups,
a significant effect of AdBDNF on neuronal recruitment to the striatum
was noted (see below). Red, AdBDNF treated;
blue, AdNull treated. VZ, Ventricular
zone; RMS, rostral migratory stream; OB,
olfactory bulb; Sep, septum; Str,
neostriatum; Ctx, neocortex.
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We found evidence of only very rare
BrdU+-III-tubulin+
neurons in the frontal cortex of AdBDNF-treated animals, too few to merit systematic comparison with null controls. We found no examples of
newly generated septal neurons in either the AdBDNF- or AdNull-injected animals. Surprisingly, however, we found that the AdBDNF-treated animals harbored a distinct population of newly generated neurons in
the neostriatum (Figs. 8,
9). These
BrdU+ neurons comprised a distinct
minority of the BrdU+ striatal cells in
these brains; they were scattered throughout the striatum, although
they were most often located in its periventricular third. Confocal
imaging confirmed examples of newly generated, BrdU+ striatal cells that expressed a
variety of independent markers of neuronal phenotype, which included
III-tubulin, NeuN, GAD67, DARRP-32, and
calbindin-D28K
(Figs. 9-11).
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Figure 8.
AdBDNF treatment was associated with neuronal
addition to the neostriatum. A shows sagittal
(left) and coronal (right) schematics of
the neostriatal region assessed for neuronal addition (indicated in
green) in AdBDNF-injected rats and their AdNull-injected
controls. B plots the mean density of
III-tubulin+-BrdU+ cells in
AdBDNF- and AdNull-injected striata and in PBS-injected controls at day
20 (n = 4).
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Figure 9.
AdBDNF induced the heterotopic addition of
BrdU+-III-tubulin+ neurons to
the striatum. Confocal images of BrdU-labeled neurons found in the
neostriata of AdBDNF-treated rats 3 weeks after virus injection. These
cells were identified by immunostaining for both BrdU
(green) and III-tubulin (red).
A-C, A representative
III-tubulin+-BrdU+ cell
(arrow). A shows a
z-dimension composite of serial 0.9 µm images, showing
III-tubulin+ (red) and BrdU
(green) immunoreactivities. B, A
z-dimension series of six separate 0.9 µm confocal
images taken 0.6 µm apart, displaying the concurrence of BrdU and
III-tubulin in the new neuron. C, A single optical
section with reconstructed orthogonal images, as viewed from the sides
in both the x-z and y-z planes.
D-F, Another newly generated,
III-tubulin+-BrdU+
neostriatal neuron (arrow), similarly viewed as a
z-stack composite (D). By way of
contrast, this field also includes both a non-neuronal
BrdU+ cell and a III-tubulin+
but BrdU-unlabeled resident neuron. Like A-C, this
field is also viewed as a series of optical sections
(E) and in orthogonal side views
(F). G-J, A pair of
III-tubulin+-BrdU+ striatal
neurons (arrows), composited in G with
split red and green images separately
indicating III-tubulin+ and BrdU, respectively.
H, I, An optical section with orthogonal
images taken at two different points to allow individual assessment of
the III-tubulin staining of each of these BrdU+
cells. Both BrdU+ nuclei are completely surrounded
by III-tubulin. J, A series of
z-dimension optical sections through these cells, again
confirming the coincident expression of BrdU and III-tubulin.
K, L, Low-power views of the fields shown
in A-C and G-J, respectively, to
visualize the range of morphologies of both resident (examples as
arrowheads) and newly added (arrows)
neurons. * in L shows a myelinated bundle passing
through the striatal matrix. Scale bars, 10 µm.
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Figure 10.
Newly recruited striatal neurons included
medium spiny neurons. The BrdU+ neurons found in
AdBDNF-treated striata expressed neuronal markers other than
III-tubulin, which included NeuN. They also expressed characteristic
antigenic markers of medium spiny neurons of the adult caudate putamen,
including calbindin-D28k, GAD67, and DARPP-32. A-C, A
typical NeuN+-BrdU+ striatal
neuron (arrow); local resident neurons
(NeuN+-BrdU ) shown by
arrowheads. A shows a
z-dimension composite of serial 1 µm images, with
split red (NeuN) and green (BrdU) images
on the right. B shows a single optical
section with reconstructed orthogonal images, as viewed from the sides
in both the x-z (top) and
y-z (right) planes. C
shows a z-dimension series, viewed as four separate 0.9 µm optical sections taken 0.6 µm apart. D, A
BrdU+
(green)-calbindin+
(red) neuron, with the split red and
green images of each to show calbindin
(arrow) and BrdU staining separately. E
and F show confocal images of a
GAD67+
(red)-BrdU+
(green) neuron in an AdBDNF-treated striatum.
E shows a confocal section with reconstructed orthogonal
side views. In the orthogonal side views, the green
BrdU+ nuclei remain completely surrounded by the
red GAD67 antigen. F shows a
z-dimension series of four separate 0.9 µm confocal
images taken 0.6 µm apart, displayed to reveal the correspondence of
BrdU and GAD67 in the same cell (arrow;
arrowheads indicate resident GAD67+ cells) at
multiple z-levels. G-I show analogous
images of a DARPP-32 (red)-BrdU+
(green) neuron in the same striatum
(arrowheads, show examples of BrdU-unlabeled resident
neurons). G shows the z-dimension
composite of serial 0.9 µm images, again with split
red and green images to show DARPP-32
(arrow) and BrdU staining individually. H
shows an optical section with reconstructed orthogonal side views, as
described. In both the x-z and y-z
planes, the BrdU+ nucleus is completely surrounded
by DARPP-32 signal. I shows a z-dimension
series through this cell. All images were taken of striatal
sections sampled from AdBDNF-treated rats killed 3 weeks after virus
administration. Scale bars, 10 µm.
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Figure 11.
AdBDNF-induced striatal neurons matured and
survived for at least 5-8 weeks.
III-tubulin+-BrdU+,
GAD67+-BrdU+, and
DARPP32+-BrdU+ striatal neurons
persisted in AdBDNF-injected rats. A-C, A typical
III-tubulin+-BrdU+ neuron
found in an AdBDNF-treated striatum 8 weeks after virus injection.
A, The z-dimension composite of serial 1 µm images, with split red and green
images to show III-tubulin+
(arrow) and BrdU, respectively. B, A
confocal section with reconstructed orthogonal images, as viewed from
the sides in both x-z (top) and
y-z (right) planes. C, A
z-dimension series of four separate 0.9 µm confocal
images taken 0.6 µm apart, confirming the III-tubulin
immunoreactivity of the BrdU+ cell.
D-F, Analogous images of a
GAD67+-BrdU+ neuron viewed in an
AdBDNF-treated striatum at 8 weeks. Only one of the two adjacent
GAD67+ neurons (arrow) is
BrdU-labeled; its neighbor is unlabeled (arrowhead).
G-I, A representative
DARPP-32+-BrdU+ neuron, again
found in an AdBDNF-treated striatum 8 weeks after virus injection.
G, A z-dimension composite of serial
optical sections, showing DARPP-32 (red) and BrdU
(green) immunoreactivities.
DARPP-32+-BrdU+ neurons are
indicated by arrows; BrdU-unlabeled resident neurons are
indicated by arrowheads. H, Orthogonal
views of the DARPP-32+-BrdU+
striatal neuron. I, Serial 0.9 µm optical sections
taken 0.6 µm apart confirm the coincidence of BrdU and DARPP-32 in
the same cell. Scale bars, 10 µm.
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Quantitatively, unbiased counting of all striatal
BrdU+ cells in sagittal sections of
AdBDNF-treated animals revealed an average of 1663 ± 748 BrdU+
cells/mm3. Among a randomly chosen sample
of 477 BrdU+ striatal cells located in
sections (n = 17) selected from three AdBDNF-treated
brains, 41 cells (8.3 ± 2.3%) could be confirmed as
double-labeled for both BrdU and III-tubulin by confocal imaging (Fig. 9) (see Materials and Methods for criteria used). This compared with the complete absence of double-labeled striatal neurons in the
PBS-injected rats (0 of 95 cells; n = 8 sections taken
from 3 rats) and with the relatively rare incidence of
BrdU+-III-tubulin+
neurons observed in the AdNull-injected rats (15 among 591 randomly chosen BrdU+ striatal cells; 2.1 ± 1.1%; n = 23 sections taken from 6 rats) (Fig.
8B; discussed below). ANOVA established that the
incidence of new striatal neurons in the AdBDNF-injected rats and their controls differed significantly (p = 0.006;
F(2,9) = 9.48). On a per animal basis,
8.3 ± 2.3% of the BrdU+ cells in
the AdBDNF-treated rat striata, or 143 ± 26.5 cells/mm3, were antigenically definable as
neurons (Fig. 8B). This represented only 0.34% (143 of 41,637) of the total striatal neuronal pool. However, because these
cells were generated in just 3 weeks, one might predict that
proportionately more neurons may be added to the striatum with longer
survival times (see below), provided that both viral BDNF expression
and progenitor cell competence are sustained.
No neurogenesis was noted in the untreated adult striatum
To assess the incidence, if any, of neuronal addition to the
normal untreated neostriatum, we examined control animals that were
injected intraventricularly with either PBS (n = 3) or
AdNull (n = 5), who received BrdU on days 2 through 19, and that were then killed on the next day (3 week time point). In the
PBS-injected rats, no
BrdU+-III-tubulin+
striatal neurons were found (Fig. 8). In these same rats, constitutive neurogenesis was observed in both the olfactory bulb and dentate gyrus,
as would be expected, although we made no attempt at quantifying baseline neuronal recruitment at these sites. Thus, we found no evidence of constitutive neurogenesis in the normal unstimulated neostriatum, in contrast to the robust neuronal recruitment observed in
the AdBDNF-treated striatum.
Adenoviral infection per se was associated with a minor induction
of neuronal recruitment
Interestingly, and in contrast to the absence of striatal neuronal
addition noted in the PBS-treated rats, the AdNull-injected controls
did exhibit a small amount of constitutive neuronal addition to the
striatum. As noted above, among 591 BrdU+
striatal cells identified in AdNull-injected rats killed at 3 weeks,
confocal analysis revealed that 15 cells (2.1 ± 1.1%)
double-labeled for BrdU and III-tubulin. This was determined using
the same criteria as in our concurrent analysis of AdBDNF-treated
striata, and the cells were assessed by the same individuals who were
blinded as to treatment group. As noted above, this incidence of
striatal neuronal addition in the AdNull-treated rats was significantly less (p = 0.006) than the 8.3 ± 2.2%
noted in their AdBDNF-treated counterparts (Fig. 8). Nonetheless, the
very presence of
BrdU+-III-tubulin+
neurons in the AdNull-treated striata was surprising, given the absence
of any new striatal neurons in the PBS-injected rats, and suggested
that adenoviral infection itself might have resulted in some
mobilization of neural progenitors. This raised the possibility that
virally induced ependymal cytokines may influence subependymal neuronal
production or migration; this in turn might allow otherwise heterotopic
neuronal recruitment. Nonetheless, the substantial increase in striatal
neuronal addition in the AdBDNF-treated rats relative to their
AdNull-treated controls argued that any adenovirus-associated mobilization of neural progenitor cells was minor relative to that
specifically attributable to BDNF. Together, these observations indicated that AdBDNF induced the addition of new neurons to the neostriatum, an otherwise atypical site for neuronal recruitment in the
adult brain.
AdBDNF-induced striatal neurons expressed antigens of medium
spiny neurons
To assess the neuronal phenotype induced by AdBDNF infection, we
immunostained sections of AdBDNF-treated brains for a number of markers
of striatal phenotype. We found that some
BrdU+ striatal cells expressed
calbindin-D28K, a marker of medium spiny neurons of the caudate putamen
(Waldvogel et al., 1991; Burke and Baimbridge, 1993) (Fig. 10).
Similarly, we found an abundance of BrdU+
striatal cells that coexpressed GAD67, a characteristic marker for
GABAergic neurons (Fig. 10).
Despite their expression by medium spiny neurons, both
calbindin and GAD67 are expressed by other cell types and even within the striatum may not be definitive markers of medium spiny neurons. Thus, to better ascertain the phenotype of AdBDNF-induced striatal neurons, we double-stained sections derived from the same animals for
DARPP-32, a highly selective marker of medium spiny neurons (Ivkovic
and Ehrlich, 1999). Among the rats killed 3 weeks after virus
injection, six of a random sample of 125 BrdU+ striatal cells (4.8%) were found to
be DARPP-32+ and were confirmed as such by
confocal imaging and serial reconstruction (Fig. 10). [This compared
with 41 of 477 BrdU+ cells (8.3%) in
adjacent sections of the same rats that expressed III-tubulin.]
Importantly, the percentage of DARPP-32+
cells among the BrdU+ striatal cell
population increased with time, such that when assessed in rats killed
8 weeks after AdBDNF injection, 10 of 128 BrdU+ cells (7.8%) were
DARPP-32+ (see below). Together, these
observations suggested that many, if not most, of the AdBDNF-induced
striatal cells matured to a phenotype characteristic of medium spiny
neurons. These data raise the possibility that AdBDNF treatment might
contribute to the restoration of this phenotype, a critical mediator of
striatopallidal communication, whose significance is underscored by its
selective loss in Huntington's Disease.
AdBDNF-induced striatal neurons matured and survived
The 3 week time point used to establish neuronal recruitment in
response to AdBDNF allowed the possibility that those cells generated
and detected at 3 weeks were merely transitional phenotypes, perhaps
transient in their very existence. To establish the more prolonged
survival of AdBDNF-associated striatal neurons, we thus set up a
distinct group of animals that were killed and assessed 8 weeks after
viral injection. Both
III-tubulin+-BrdU+
and
DARPP32+-BrdU+
double-labeled striatal cells persisted in these rats, with little apparent loss (Fig. 11). Among a sample of 106 BrdU+ cells in three 8 week rat striata
randomly sampled for confocal imaging, seven cells (6.6%) were found
to express III-tubulin. Similarly, 10 of 128 sampled
BrdU+ cells (7.8%) expressed DARPP-32.
The rough equivalency of the proportion of
BrdU+ striatal cells that were
III-tubulin+ and
DARPP+ argued that, by 8 weeks after
AdBDNF injection or 5 weeks after the last BrdU incorporation,
virtually all of the BrdU+ neurons, as
defined by III-tubulin, also would have been expected to express
DARPP-32. Thus, a substantial number of AdBDNF-induced striatal neurons
survived, depending on the time point of their generation during the
BrdU injection course, for at least 5-8 weeks after terminal mitosis.
Furthermore, these surviving neurons matured sufficiently to express
DARPP-32, a relatively mature marker of striatal neuronal phenotype. As
such, these AdBDNF-induced neurons did not appear to constitute
transitional phenotypes.
AdBDNF treatment was associated with systemic weight loss
The AdBDNF-injected animals were noted to experience a stereotypic
weight loss during the 3 week period between AdBDNF delivery and death.
This was not unexpected, because weight loss has been described
previously in rats receiving intraventricular BDNF infusions. This
syndrome appears to be central in origin and reflects BDNF-associated appetite suppression and hypophagia rather than any hypermetabolic state (Pelleymounter et al., 1995). We found that this was not an
effect of the virus in that neither AdNull- nor PBS-injected animals
experienced similar weight loss. Whereas AdNull-injected controls rose
from 300 ± 16 gm at the time of viral injection to 339 ± 6 gm at the time of being killed 3 weeks later (n = 4), a
matched set of AdBDNF-treated animals lost weight during that period,
falling from 328 ± 34 to 288 ± 17 gm per animal
(p = 0.016 by ANOVA, comparing the slopes of
weight gain as a function of time between AdBDNF-, AdNull-, and
PBS-treated rats; F(2,13) = 6.17)
The time course of weight loss in the AdBDNF-treated animals suggested
to us that virally delivered BDNF was exerting rapid and powerful
biological effects on the target nervous system, within the same time
frame as the BDNF-associated rise in neuronal recruitment. Whether this
anorexic phenotype was a consequence of olfactory neuronal addition and
altered olfactory perception or was instead an unrelated effect of
central BDNF overexpression remains to be established.
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DISCUSSION |
We report here that infection of the adult rat
ventricular lining with an adenoviral BDNF expression vector induced
the recruitment of new neurons from resident progenitor cells of the
forebrain ventricular zone. In particular, adenoviral infection
resulted in the diffuse transduction of the adult ventricular wall,
with the effective subrogation of the ependyma into a source of
secreted BDNF to both the CSF and periventricular parenchyma. This
resulted in the sustained, high-level secretion of BDNF by the
ventricular wall and was associated with a >2.4-fold increase in the
recruitment of new neurons to the rat olfactory bulb over the 3 weeks
after viral administration. Importantly, AdBDNF administration was also associated with the heterotopic addition of new neurons to the neostriatum, with the recruitment of BrdU-incorporating
III-tubulin+-DARPP-32+-NeuN+-GAD67+-calbindin-D28K+
neurons to the striata of the AdBDNF-treated animals. To the best of
our knowledge, these experiments comprise the first use of viral gene
delivery as a means to induce neurogenesis from resident progenitor
cells in the adult CNS. In addition, they present the first evidence
for induced neuronal addition to the mature neostriatum. Together,
these results indicate that viral transduction of the adult ependyma to
overexpress BDNF may be an effective means of inducing the recruitment
of new neurons to permissive regions of the mature brain.
We observed predominantly ependymal cell expression of
both BDNF and GFP mRNAs after intraventricular injection of
AdBDNF:IRES:GFP. Nonetheless, occasional subependymal labeling was
noted, particularly along the subcallosal and dorsolateral walls of the
lateral ventricles. When present, subependymal GFP fluorescence
appeared as rapidly as ependymal cell labeling; both were evident by
7 d after virus injection (Fig. 1).
GFP+ cells were limited to the ventricular
layers, however, and were never noted in either the olfactory
subependyma or striatal parenchyma, except for migrants into the corpus
callosum. Despite this restriction of virally expressed BDNF to the
ventricular wall, newly generated neurons, derived from uninfected
subependymal cells, were profoundly influenced by their genesis
adjacent to AdBDNF-infected ependymal cells. Thus, the effects of
ependymal BDNF on neurogenesis and neuronal recruitment to the
olfactory bulb and striatum likely derived from a paracrine effect of
BDNF on uninfected subependymal progenitors.
The effects of BDNF were presumably exerted early in the ontogeny of
newly generated neurons, before their departure from the ventricular
wall, because it is unlikely that ependymal secretion of BDNF to the
CSF and periventricular parenchyma would have influenced BDNF levels in
the olfactory bulb or striatal parendyma. Indeed, the mature olfactory
bulb harbors high levels of BDNF, whereas the neurotrophin appears
relatively sequestered from the adult ventricular zone and olfactory
subependyma. Thus, a likely scenario is that ependymal BDNF acts to
promote the early differentiation and survival during migration of
newly generated, subependymally derived neurons, and that these cells
survive to migrate into an already BDNF-rich environment in the
olfactory bulb. As such, neuronal mitogenesis and departure from the
ventricular wall may be viewed as the initial rate-limiting steps for
neuronal recruitment, with the cells finding a permissive environment
for survival once in the bulb.
Importantly, AdBDNF injection was also associated with the
addition of new neurons to the neostriata of treated animals. Such neuronal addition to non-granule cell populations has only rarely been
reported in the adult mammalian brain, specifically in the visual
cortex (Kaplan, 1981) and macaque frontal cortex (Gould et al., 1999),
as well as in response to injury in the adult mouse frontal cortex
(Magavi et al., 2000). More generally, however, reports of neurogenesis
in the adult mammalian brain have been limited to olfactory,
hippocampal, and cerebellar granule cell populations (for review, see
Goldman and Luskin, 1998). Nonetheless, careful analysis of serially
reconstructed confocal images revealed that our AdBDNF-injected animals
harbored a discrete cohort of antigenically confirmed neurons, which
colabeled with BrdU and were scattered throughout the neostriatum.
Because the adult neostriatum typically does not add new neurons, the
induced neuronal addition associated with AdBDNF treatment may be
viewed as heterotopic in nature.
Although their numbers were small relative to the much
larger pool of AdBDNF-induced olfactory neurons, the recruitment
kinetics of the induced striatal pool were surprisingly robust. Given
an average striatal neuronal BrdU labeling index of 0.34% and an average of 1.03 × 106 ± 6.56 × 104 neurons per striatum, ~3.5 × 103 neurons may be added to each
striatum over an 18 d period of BrdU injection, or ~195 neurons
per striatum per day. This estimate is crude and likely an
underestimate in that it is predicated on the assumptions that daily
BrdU injections label the entire mitotic pool and that no striatal
cells die during this period. In addition, these numbers reflect but
one point on the dose-response curve relating neuronal recruitment to
BDNF expression levels; it is important to remember that in this study
we have not perturbed either the dose of adenovirus or that of its
expressed BDNF. Nonetheless, these numbers suggest that AdBDNF-induced
neuronal addition may be sufficiently robust to contribute meaningfully
to striatal function, if not architecture. Furthermore, the
identification of many AdBDNF-induced neurons as
DARPP-32+-GAD67+-calbindin-D28K+
suggests that at least a significant fraction of these neurons may be
homologous to the medium spiny neuron population of the adult
neostriatum. Because this is the neuronal population lost in
Huntington's disease and the striatonigral degenerations, transduction of the ventricular wall with BDNF expression vectors might be envisaged
as a feasible strategy for restoring diminished neuronal populations in
the striatal degenerations, as well as in other conditions of acquired
striatal neuronal loss.
Interestingly, we noted that the AdNull-injected controls
exhibited a small amount of constitutive neuronal addition to the striatum. This did not appear to reflect neurogenesis in the normal striatum, because PBS-injected rats exhibited no striatal neuronal addition whatsoever. Rather, these results suggested that adenoviral infection per se might have been sufficient to instigate mobilization of neural progenitors. Although minor in extent and significantly less
robust than AdBDNF-induced neuronal recruitment, the AdNull induction
of striatal neuronal addition may represent a hitherto unrecognized
feature of central viral infection, especially of the
ependyma-subependyma. Presumably, virally induced ependymal cytokines
might stimulate subependymal neurogenesis and thereby permit otherwise
heterotopic neuronal recruitment. This possibility is strengthened by
reports that adenovirally induced cytokines include interleukin-6
(IL-6) and IL-8, both of which have been found to be neurotrophic
in vitro (Driesse et al., 2000). Indeed, such paracrine
activation of neurotrophic cytokines might explain recent observations
of both inflammation and apoptosis-related neuronal recruitment in the
adult brain (Wang et al., 1998; Magavi et al., 2000). In any event, the
significant increase in neuronal recruitment to the striatum in the
AdBDNF-treated rats, relative to their AdNull-treated controls, argued
that any virus-associated cell genesis paled beside that specifically
associated with BDNF.
It is worth noting that, despite the frequent observation
of BrdU-incorporating cells in the septa, striata, and frontal cortices of these animals, no significant differences were noted between the
AdBDNF and AdNull control animals in their BrdU-labeled cell numbers
(Fig. 7). To be sure, AdBDNF treatment was associated with an increase
in the relative proportion of neurons among the BrdU+ cells of the neostriatum (Figs. 8,
9). Nonetheless, the percentage of confocal-validated new neurons in
the overall striatal BrdU+ cell population
was so small (just 8% of the BrdU+
population) that AdBDNF would not have been expected to yield readily
demonstrable treatment-related differences in either the total
BrdU+ cell number or overall striatal
neuronal number. The induction of striatal neurogenesis by AdBDNF might
therefore reflect either the neuronal differentiation of postmitotic
daughters that might otherwise have become glia or the postmitotic
rescue of daughters otherwise destined to die. Indeed, although a
number of studies have failed to observe any mitogenic effect of BDNF
on ventricular zone progenitor cells (Ahmed et al., 1995; Kirschenbaum
and Goldman, 1995), these data do not allow us to rule out a direct
mitogenic effect in vivo.
It is important to also consider the possibility that BDNF
might act not only to recruit a ventricular zone-derived population but
also to activate resident parenchymal glial progenitors to differentiate as neurons. Studies of both adult rat (Palmer et al.,
1999) and human (Roy et al., 1999) brain have indicated the ability of
white matter progenitor cells to differentiate as neurons in
vitro. In the AdBDNF-treated neostriata in particular, the possibility of AdBDNF-induced neurogenesis from parenchymal progenitors is suggested by the frequent observation of clustered pairs of BrdU+ neurons (Fig. 9G),
although continued division of ventricular zone migrants might also
explain this observation (Menezes et al., 1995). Thus, although the
possibility that AdBDNF might stimulate neuronal recruitment from
parenchymal as well as ventricular zone progenitors is intriguing, our
data do not yet allow us to address the source or migration routes of
AdBDNF-induced striatal neurons.
The implications of AdBDNF-induced striatal neurogenesis may be
profound, particularly for disorders such as Huntington's disease and
striatonigral degeneration, in which the loss of striatal neurons may
dictate the pathology. The apparent assumption of a medium spiny
neuronal phenotype by many, and perhaps most, AdBDNF-induced neostriatal neurons is especially intriguing, in that it suggests the
potential therapeutic utility of this neuronal population. Axiomatically, our hope is that if these cells prove functional and
able to survive, then AdBDNF-induced striatal neurons might be able to
delay, abrogate, or reverse striatal neurodegenerative disease.
Nonetheless, it remains to be seen whether these AdBDNF-induced neurons
can functionally integrate, both with resident striatal neurons and
nigrostriatal afferents, whether they can survive longer than the 5-8
weeks that we have noted, and whether they can survive the primary
disease process better than the cells they are intended to replace.
These uncertainties notwithstanding, the adenoviral BDNF-mediated
induction of neuronal addition to the adult brain expands our
conception of cellular plasticity in the adult CNS and lends a new
perspective to the potential for gene therapy in the treatment of
structural neurological disease.
| |
FOOTNOTES |
Received Dec. 13, 2000; revised March 12, 2001; accepted April 6, 2001.
This work was supported by the National Multiple Sclerosis Society,
Project ALS, the G. Harold and Leila Y. Mathers Charitable Foundation,
and National Institutes of Health Grants P50HL59312, R01NS29813, and
R01NS33106. We are grateful to Drs. Ron Crystal and Neil Hackett for
their advice in the construction of our viral vectors, to Drs. George
Yancopoulos and Stan Wiegand of Regeneron Pharmaceuticals for BDNF
cDNA, and to Dr. Anne Acheson of Regeneron for help with BDNF ELISA. We
thank Dr. A. Frankfurter for monoclonal antibody TuJ1, Dr. Shelley
Halpain for anti-MAP-2, and Dr. Hugh Hemmings for anti-DARPP-32.
A.B. and E.C. contributed equally to this work.
Correspondence should be addressed to Dr. Steven A. Goldman, Department
of Neurology and Neuroscience, Cornell University Medical Center, 1300 York Avenue, Room E607, New York, NY 10021. E-mail:
sgoldm{at}mail.med.cornell.edu.
| |
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TOP
ABSTRACT
INTRODUCTION
Compound via MeSH
