 |
 Previous Article | Next Article 
The Journal of Neuroscience, September 15, 1998, 18(18):7336-7350
TrkB and TrkC Signaling Are Required for Maturation and
Synaptogenesis of Hippocampal Connections
Albert
Martínez1,
Soledad
Alcántara1,
Víctor
Borrell1,
José A.
Del Río1,
Joan
Blasi2,
Raquel
Otal1,
Narciso
Campos3,
Albert
Boronat3,
Mariano
Barbacid4, 5,
Inmaculada
Silos-Santiago5, 6, and
Eduardo
Soriano1
1 Department of Animal and Plant Cell Biology,
University of Barcelona, Barcelona 08028, Spain,
2 Department of Cell Biology and Pathology, University of
Barcelona, L'Hospitalet de Llobregat, Barcelona 08907, Spain,
3 Department of Biochemistry and Molecular Biology,
University of Barcelona, Barcelona 08028, Spain, 4 Centro
Nacional de Investigaciones Oncológicas Carlos III, Instituto de
Salud Carlos III, 28220 Majalahonda, Madrid, Spain,
5 Department of Molecular Oncology, Bristol-Myers Squibb,
Pharmaceutical Research Institute, Princeton, New Jersey 08543-4000, and 6 Department of Neurobiology, Millennium
Pharmaceuticals Inc., Cambridge, Massachusetts 02139-4815
 |
ABSTRACT |
Recent studies have suggested a role for neurotrophins in the
growth and refinement of neural connections, in dendritic growth, and
in activity-dependent adult plasticity. To unravel the role of
endogenous neurotrophins in the development of neural connections in
the CNS, we studied the ontogeny of hippocampal afferents in trkB ( /) and trkC (/) mice.
Injections of lipophilic tracers in the entorhinal cortex and
hippocampus of newborn mutant mice showed that the ingrowth of
entorhinal and commissural/associational afferents to the hippocampus
was not affected by these mutations. Similarly, injections of biocytin
in postnatal mutant mice (P10-P16) did not reveal major differences in
the topographic patterns of hippocampal connections.
In contrast, quantification of biocytin-filled axons showed that
commissural and entorhinal afferents have a reduced number of axon
collaterals (21-49%) and decreased densities of axonal varicosities
(8-17%) in both trkB (/) and trkC
(/) mice. In addition, electron microscopic analyses showed that
trkB (/) and trkC (/) mice have
lower densities of synaptic contacts and important structural
alterations of presynaptic boutons, such as decreased density of
synaptic vesicles. Finally, immunocytochemical studies revealed a
reduced expression of the synaptic-associated proteins responsible for
synaptic vesicle exocytosis and neurotransmitter release (v-SNAREs and
t-SNAREs), especially in trkB (/) mice. We conclude
that neither trkB nor trkC genes are
essential for the ingrowth or layer-specific targeting of hippocampal
connections, although the lack of these receptors results in reduced
axonal arborization and synaptic density, which indicates a role for TrkB and TrkC receptors in the developmental regulation of synaptic inputs in the CNS in vivo. The data also suggest that
the genes encoding for synaptic proteins may be targets of TrkB and
TrkC signaling pathways.
Key words:
TrkB receptors; TrkC receptors; neurotrophic factors; mutant mice; neuronal connections; synaptogenesis; synaptic-associated
proteins; hippocampus
| |
INTRODUCTION |
The neurotrophins, including nerve
growth factor (NGF), brain-derived neurotrophic factor (BDNF),
neurotrophin 3 (NT3), and neurotrophin 4/5 (NT4/5), are essential for
the survival of populations of neurons in the PNS and CNS [Jones et
al. (1994) ; Minichiello and Klein (1996); Alcántara et al.
(1997); for review, see Snider (1994); Fariñas and Reichardt
(1996); Snider and Silos-Santiago (1996)]. Recent studies indicate
that neurotrophins may regulate dendritic and axonal growth (Cabelli et
al., 1995, 1997; Cohen-Cory and Fraser, 1995; McAllister et al., 1995,
1996, 1997; Bolz et al., 1997; Inoue and Sanes, 1997; Paves and Saarma,
1997) and the efficacy of synaptic transmission (Lohof et al., 1993;
Kang and Schuman, 1995; Korte et al., 1995; Thoenen, 1995; Figurov et
al., 1996; Prakash et al., 1996; Wang and Poo, 1997). Moreover, target-derived neurotrophins in the PNS may regulate the maturation of
synaptic contacts and the density of synaptic innervation (Miller et
al., 1994; Wang et al., 1995; Causing et al., 1997). In addition, a
role for BDNF and NT4/5 has been shown for the activity-dependent development of ocular dominance columns in the visual cortex (Cabelli et al., 1995, 1997; Galuske et al., 1996).
Most of the data on the effects of neurotrophins on axonal growth were
obtained in vitro or after application of exogenous neurotrophins. To our knowledge, the only study that has analyzed the
role of endogenous neurotrophins in the development of neural connections in the CNS was performed by infusion of neurotrophin receptors antagonists (TrkB-IgG) in the visual cortex (Cabelli et al.,
1997). To determine the contribution of endogenous neurotrophins to the
developmental pattern of neuronal connections and synaptogenesis in the
CNS, we studied the ontogeny of the main hippocampal afferents in mice
lacking trkB and trkC genes, which encode for the
receptors of BDNF and NT4/5, and NT3, respectively (Klein et al., 1991, 1992; Lamballe et al., 1991; Soppet et al., 1991). We chose the hippocampal area not only because neurotrophic factors and their receptors are abundantly expressed in this region (Gall and Isackson, 1989; Ernfors et al., 1990, 1991; Hofer et al., 1990; Gall et al.,
1991; Isackson et al., 1991; Rocamora et al., 1996), but also because
most studies on modulation of synaptic activity by neurotrophins have
been performed in this brain area (Kang and Schuman, 1995; Korte et
al., 1995; Figurov et al., 1996). In addition, the analysis of the
phenotype of hippocampal connections in trkB (/) and
trkC (/) mice allows us to assess the developmental functions of neurotrophins in a region where the main afferent connections are organized both in a layer-specific manner and in a
precise topographic order (Amaral and Witter, 1995).
| |
MATERIALS AND METHODS |
Mutant mice. Single-mutant trkB (/)
and trkC (/) mice and double-mutant homozygous mice were
generated by mating single and double heterozygous animals (Klein et
al., 1993, 1994; Fritzsch et al., 1997). Because no significant
differences were observed in the phenotype of wild-type and
heterozygous littermates, both groups of mice were used as controls for
the quantitative analyses.
In situ hybridization. Embryonic day (E14, E16, E18),
postnatal day (P0, P5, P10, P15, P21), and adult mice (NMRI strain; Iffa Credo, Lyon, France) were perfused with 4% paraformaldehyde in
0.1 M phosphate buffer, cryoprotected in 30% sucrose, and
frozen. Coronal sections (30-50 µm thick) were obtained and
hybridized as described elsewhere (Lecea et al., 1995, 1997). Briefly,
sections were deproteinized with 0.2 N HCl for 10 min, acetylated with 0.25% acetic anhydride in 0.1 M triethanolamine buffer, pH
8.0, and post-fixed for 10 min in 4% paraformaldehyde. Sections were then hybridized overnight at 60°C with digoxigenin-labeled antisense RNA probes to mouse BDNF and NT3 and to the tyrosine kinase domains of
mouse TrkB and TrkC in a solution containing 50% formamide, 20 mM PIPES, 5× Denhardt's solution, 10% dextran sulfate,
250 µg/ml yeast tRNA, 250 µg/ml salmon sperm DNA, 50 mM
dithiothreitol, 0.62 M NaCl, and 10 mM EDTA
solution. Sections were then digested with RNase A (37°C for 1 hr)
and washed in 0.5× SSC plus 50% formamide (55°C) and in 0.1× SSC
plus 0.5% sarcosyl (60°C). After hybridization, sections were
blocked with 10% sheep normal serum (2 hr), incubated overnight with
an alkaline phosphatase-labeled anti-digoxigenin antibody (1:2000), and
developed with a 5-bromo-4-chloro-3-idolyl phosphate (BCIP) and
nitroblue tetrazolium (NBT) substrate. After several washes, sections
were mounted onto slides and coverslipped with Mowiol. Sections
hybridized with sense riboprobes did not give signals above background
levels.
Anterograde tracing. Newborn and P5 mice were perfused with
4% paraformaldehyde in phosphate buffer, and their brains were dissected out. Crystals of
1-1'-dioctadecyl-3,3,3',3'-tetramethylindocarbocyanine perchlorate
(DiI) were injected into the entorhinal area or hippocampus as
described (Supèr and Soriano, 1994). Brains were stored in phosphate-buffered 4% paraformaldehyde for 5-8 weeks in the dark at
room temperature. Coronal sections were obtained with a vibratome, counterstained with the DNA-specific dye bisbenzimide, and mounted with
an antifading mounting medium. The sections were analyzed and
photodocumented in a Polyvar (Reichert) microscope equipped with
fluorescent filters. P10-P16 mice were injected by iontophoresis of
biocytin (20 min; positive current; 7 sec on/off cycle) in the
entorhinal cortex or the hippocampus. After 24 hr of survival, animals
were perfused with 4% paraformaldehyde, and brains were post-fixed in
the same fixative and sectioned at 50 µm using a vibratome.
Free-floating sections were then incubated with the avidin-biotin-peroxidase complex (ABC) (Vector Labs, Burlingame, CA),
developed with 0.05% diaminobenzidine (DAB) and 0.01% hydrogen peroxide in the presence of 0.02% nickel sulfate (Del Río et al., 1997), and counterstained with cresyl violet. A total of 97 postnatal mice were used (n = 11 trkB (+/+),
24 trkB (±), 23 trkB (/), 11 trkC
(+/+), 16 trkC (±), 12 trkC (/)). Five
newborn double-mutant trkB (/)/trkC
(/) mice were also injected with DiI. Selected entorhinal
and commissural fibers from trkB (/) and trkC
(/) mice (P13-P14) and from control littermates were drawn using a
40× oil-immersion objective lens (n = 2-4 animals per
group, 32-58 fibers). Length of fibers was measured using a
planimeter, and the branching index (Del Río et al., 1997) and
density of axonal varicosities (number of varicosities per 100 µm)
were calculated. Statistical analysis was performed using the
Student's t test.
Electron microscopy. trkB (/) (P13,
n = 2), trkC (/) (P12-13,
n = 3), and control littermates [trkB
(+/+), n = 1; trkB (+/), n = 1; trkC (+/+), n = 1; trkC
(+/), n = 2] were perfused with 2%
glutaraldehyde-1% paraformaldehyde in 0.12 M phosphate buffer. Brains were removed from the skull and fixed in the same solution overnight. Tissue slices were post-fixed with 2% osmium tetroxide, stained with 2% uranyl acetate, and embedded in Araldite. Ultrathin sections were collected onto formvar-coated slot grids and
stained with lead citrate. Electron micrographs covering 100 µm2 (final magnification 19,000×) were randomly
taken from each hippocampal layer, and the number of synaptic contacts
was counted (n = 30-31 micrographs for each layer and
group). For the morphometric analysis of presynaptic boutons and
synapses, randomly selected synaptic contacts were micrographed at
58,000× final magnification (n = 81-170 axon
terminals and synapses per group and layer). The total number of
synaptic vesicles and vesicles clustered near the active zone [whose
membrane was closer than 50 nm (Rosahl et al., 1995)] was counted. The
area of axon terminals and the length and thickness of synaptic
specializations were calculated using the IMAT image analysis program
(Scientific-Technical Services, University of Barcelona). Statistical
analysis was performed using the Student's t test.
Organotypic slice cultures. Entorhinohippocampal cocultures
and hippocampus/hippocampus cocultures were prepared from newborn trkB (/), trkC (/), and double-mutant
trkB (/)/trkC (/) mice, as well as from
control littermates as described (Del Río et al., 1997).
Animals were anesthetized by hypothermia, their brains were removed,
and the hippocampus and entorhinal cortex were dissected out under a
microscope. Horizontal sections (350 µm thick) were obtained using a
McIlwain tissue chopper. Selected slices were cocultured using the
interphase membrane method (Stoppini et al., 1991). A total of 52 entorhinohippocampal and 50 hippocampus/hippocampus mixed slice
cocultures of mutant and control mice were prepared. In addition,
cultures from single-mutant mice were also prepared (n = 38). A crystal of biocytin was placed in the entorhinal cortex or the
hippocampus 24 hr before fixation. Cocultures were fixed with 4%
paraformaldehyde after 9-15 d in vitro (DIV). Horizontal sections (40 µm thick) were obtained, incubated with the ABC complex, and developed with diaminobenzidine/nickel and hydrogen peroxide as
described above. Cultures were then counterstained with cresyl violet
and coverslipped.
Immunocytochemistry and immunoblot. Mutant and control
littermates (P13; trkB (/), n = 2, trkB (+/+), n = 1; trkB (+/), n = 1; trkC (/), n = 2;
trkC (+/+), n = 1; trkC (+/),
n = 1) were perfused with 4% paraformaldehyde in
PBS, cryoprotected in 30% sucrose, and sectioned at 25 µm.
Sections from mutant and control mice were processed in bulk.
Free-floating sections were blocked with 15% fetal bovine serum
solution and incubated overnight at 4°C with one of the following
primary antibodies (diluted 1:1000-1500): anti- -tubulin (Sigma,
Poole Dorset, UK), anti-synapsin I [MAB 355, Chemicon, Temecula, CA
(recognizing the C-terminal fragment of synapsin I)],
anti-synaptophysin (MAB SVP-38, Sigma), anti-synaptotagmin I [MAB
41.1, gift from R. Jahn (Göttingen, Germany) (Brose et al., 1992)], anti-SNAP-25 (MAB SMI 81, Sternberger-Meyer,
Jarrettsville, MD), anti-synaptobrevin 2 [MAB 69.1, gift from R. Jahn
(Edelmann et al., 1995)], anti-syntaxin 1 [MAB HPC-1 recognizing
isoforms 1A and 1B; gift from G. Barnstable (New Haven, CT)
(Barnstable et al., 1985)], and anti-Rab3a [MAB 42.2, gift from R. Jahn (Matteoli et al., 1991)]. Thereafter, sections were incubated for
3 hr at room temperature in the dark with FITC-conjugated secondary
antibodies, mounted onto slides, and coverslipped with an antifading
mounting medium. Sections were viewed in a Leica TCS 4D confocal
scanning laser microscope. Two serial confocal images, 2 µm apart,
from each example were used to quantify the fluorescence intensity of
synaptic-associated protein immunolabeling. The intensities of
fluorescence (expressed as gray levels) were measured along vertical
strips extending from the stratum oriens to the hilar region, with the
aid of the IMAT image analysis program. Continuous linear profiles from
control and null-mutant mice were then averaged, and the fluorescence
intensities were calculated for each hippocampal layer. Statistical
analysis was performed using the Student's t test.
The forebrains of two trkB (/) and trkC
(/) mice and littermate controls were frozen and homogenized in
HEPES/NaOH 10 mM, pH 7.4, containing 0.32 M
sucrose, 1 µg/ml leupeptin, 5 µg/ml aprotinin, 1 mM
PMSF, and 1 mM EGTA. To remove nuclei and cellular debris,
the homogenates were centrifuged at 2000 rpm in a Beckman JA21 rotor
for 2 min followed by 12,000 rpm for 11 min in the same rotor.
Supernatants containing cytosolic and light membrane fractions were
subjected to SDS-PAGE and immunoblot analysis using 10 µg of protein
per lane. Gels were then electrotransferred to nitrocellulose membranes
using a semi-dry blotting system. Nitrocellulose membranes were blocked
with 5% nonfat milk in TBS (140 mM NaCl, 10 mM
Tris/HCl, pH 7.4, with 0.1% Tween-20) for 30 min at room temperature
and incubated overnight with the monoclonal antibodies described above.
After several washes, membranes were incubated with
peroxidase-conjugated anti-mouse antibodies for 1 hr at room temperature and developed using the ECL method (Amersham, Bucks, UK),
placed in contact with x-ray films for 10-60 sec, and quantified (Phoretix 1D Gel Analysis system). The values were normalized to
-tubulin to correct for possible inequalities in protein
content.
| |
RESULTS |
Expression of neurotrophic factors and their receptors in the
developing hippocampal region
In the mouse, developing entorhinal afferents reach the
hippocampus at embryonic day 15 (E15) and invade the appropriate target layer (stratum lacunosum-moleculare) by E16, whereas
commissural/associational afferents reach the target layers (stratum
oriens and stratum radiatum) 2-3 d later (Supèr and Soriano,
1994; Supèr et al., 1998). To investigate the role of
neurotrophins and their receptors in the development of these principal
hippocampal connections, we first analyzed the developmental expression
of trkB, trkC, bdnf, and
nt3 genes. At embryonic stages (E14-E18), both TrkB and
TrkC mRNAs were detected in postmitotic neurons of the entorhinal cortex, in the pyramidal neurons of the hippocampus proper (CA1-CA4 subfields), and in the granule cells of the dentate gyrus. At postnatal
stages (P0-P15), when hippocampal connections mature, levels of
expression for both transcripts increased steadily and were maximal
(Fig.
1A,B).
mRNA hybridization signals decreased to adult-like levels by P21. BDNF
mRNA was also widely expressed in the entorhinohippocampal system at
all ages (Fig. 1C), with levels of expression increasing
from P5 on to reach maximal expression levels in the adult. NT3
transcripts, which in the adult hippocampus are restricted to the
dentate gyrus and the CA2 region (Ernfors et al., 1990; Lindvall et
al., 1992; Isackson, 1995), were upregulated at prenatal and early
postnatal stages and were expressed in most neurons within the
hippocampus and entorhinal areas (data not shown). No remarkable
differences in the pattern of expression for either transcript were
observed between the medial and lateral fields of the entorhinal
cortex. These results show that TrkB and TrkC receptors and their
ligands, BDNF and NT3, are expressed in the hippocampal region at the
time of ingrowth and development of the main hippocampal afferents
(Supèr and Soriano, 1994; Del Río et al., 1997;
Supèr et al., 1998). Furthermore, TrkB and TrkC receptors are
expressed in entorhinohippocampal projection cells and in the neurons
of the CA3 subfield that give rise to the commissural/associational
pathway (Amaral and Witter, 1995).
View larger version (98K):
[in this window]
[in a new window]
|
Figure 1.
Expression of TrkB (A), TrkC
(B), and BDNF (C) mRNAs in
horizontal sections of P0 mice. Positive neurons are widely distributed
throughout the hippocampus (CA1, CA3), the dentate gyrus
(DG), and the entorhinal cortex (EC).
Scale bars: A-C, 300 µm.
|
|
Pattern of hippocampal connectivity in trkB (/) and
trkC (/) mice
Recently, it has been suggested that neurotrophins may be involved
in the attraction of the axonal growth cone (Paves and Saarma, 1997;
Song et al., 1997). To test whether TrkB or TrkC signaling is required
for the ingrowth and targeting of afferent fibers in the hippocampal
region we next examined the development of hippocampal connections in
trkB (/) and trkC (/) mice. Injections of
the anterograde tracer DiI in the entorhinal area at P0-P5 showed that
in trkB (/) and trkC (/) mice entorhinal axons innervated the appropriate target layers, the stratum
lacunosum-moleculare, and the dentate molecular layer, with a pattern
indistinguishable from that of wild-type and heterozygous littermates
(control mice) (Fig.
2A-C). Similarly,
tracer injections in the hippocampus of trkB (/) and
trkC (/) mice at P0-P5 resulted in a large number of
commissural fibers in the contralateral hippocampus innervating the
stratum oriens and stratum radiatum, which are the normal layers of
termination for these fibers (data not shown).
View larger version (119K):
[in this window]
[in a new window]
|
Figure 2.
Distribution of entorhinohippocampal and
commissural projections in trkB and trkC
(/)mice. A-C, Distribution of entorhinohippocampal
afferents in wild-type (A), trkB
(/) (B), and trkC (/)
(C) newborn mice after injections of DiI in the
entorhinal cortex. Labeled fibers (arrowheads) are
observed running in the stratum lacunosum-moleculare and in the white
matter in all three animal groups. Sections are counterstained with
bisbenzimide. D-F, Pattern of medial entorhinal
projections in wild-type (D), trkB
(/) (E), and trkC (/)
(F) P14 mice after iontophoresis of biocytin in
the entorhinal cortex. In all three groups, axons innervate the middle
tier of the molecular layer and two patches in the stratum moleculare,
in the CA2/CA1 and CA1/subiculum interphase
(arrowheads). G, H, Distribution of
lateral entorhinal projections in the hippocampus of wild-type (G) and
trkC (/) (H) P14 mice,
illustrating no major topographic differences in the innervation of the
outer molecular layer and stratum lacunosum-moleculare in the CA3
region (arrowheads). I, J, Distribution
of commissural fibers in the hippocampus of wild-type and
trkC (/) P14 mice after injections of biocytin in
the contralateral hippocampus. Commissural fibers innervate the stratum
radiatum and the inner molecular layer (arrowheads).
EC, Entorhinal cortex; DG, dentate gyrus;
SG, stratum granulosum; SLM, stratum
lacunosum-moleculare; SM, stratum moleculare;
SO, stratum oriens; SP, stratum
pyramidale; SR, stratum radiatum. Scale bars:
A-H, 300 µm; I, J, 100 µm.
|
|
At later stages (P10-P16) the topography of lateral and medial
entorhinal projections in wild-type mice displayed adult-like patterns
of innervation, with distinct axons terminating in different hippocampal subdivisions and sublayers (Amaral and Witter, 1995). Thus,
medial entorhinal projections innervated the middle tier of the dentate
molecular layer and the stratum lacunosum-moleculare, where fibers
formed two patches of higher innervation in the subiculum and CA1 (Fig.
2D). Conversely, lateral entorhinal projections terminated in the outer tier of the dentate molecular layer and in the
stratum lacunosum-moleculare of the CA3/CA2 region and CA1/subicular
interphase (Fig. 2G). In trkB (/) and
trkC (/) mice, entorhinal afferents terminated in well
defined region-specific patches and sublayers indistinguishable from
those in wild-type mice in both the hippocampus proper and the dentate
gyrus (Fig. 2E,F,H).
Similarly, commissural afferents in these homozygous mutant mice were
targeted correctly to the stratum radiatum and stratum oriens in the
hippocampus proper and to the inner molecular layer in the dentate
gyrus (Fig. 2I,J). No aberrant innervation or
axonal trajectories were noted in these mutant mice. These findings
indicate that neither TrkB nor TrkC signaling is required for the
ingrowth of hippocampal afferents. Furthermore, the data indicate that these receptors are not essential for the layer-specific or
region-specific targeting of hippocampal connections.
Reduced axonal elaboration in trkB (/) and
trkC (/) mice
The injections of tracers in newborn and late postnatal mice
frequently resulted in a sparse innervation of the hippocampus in
trkB (/) and trkC (/) mice when compared
with wild-type littermates. To examine the possibility that
trkB and trkC genes may regulate the maturation
and elaboration of hippocampal connections, we quantified the branching
pattern of single, biocytin-filled axons in P10-P16 mutant and control
mice. This analysis showed that entorhinal and commissural fibers had
fewer axon collaterals in both trkB (/) and
trkC (/) mice in the hippocampus proper (CA1 and CA3
regions) and the dentate gyrus (Fig. 3).
In trkC (/) mice, this reduction was dramatic for
commissural and entorhinal axons innervating all the hippocampal
subregions (37-49%), except for entorhinal afferents present in CA1
subfield (26%). In contrast, trkB (/) mice showed a
20-36% reduction in the branching index of single axons, which was
more conspicuous for the commissural fibers innervating the hippocampus
proper. These findings indicate that TrkB and TrkC receptors may
regulate the elaboration and complexity of hippocampal afferents.
View larger version (25K):
[in this window]
[in a new window]
|
Figure 3.
Branching index (number of branching points/100
µm) and density of boutons (number of boutons/100 mm of fiber) of
commissural and entorhinal axons in trkB (/) mice, trkC (/)
mice, and control littermates (P12-P14; mean ± SEM). There are
significant differences between control and mutant mice
(*p < 0.05; **p < 0.01;
Student's t test). Abbreviations as in Figure 2.
|
|
We next estimated the number of putative presynaptic boutons formed by
trkB (/) and trkC (/) axons by
calculating the density of axonal varicosities present along
biocytin-labeled fibers. In both trkB (/) and
trkC (/) mice, commissural and entorhinal afferents
displayed significantly reduced densities of axonal varicosities
(8-17%), with the exception of commissural fibers in the CA3 region
of trkC (/) mice (Fig. 3).
Phenotype of hippocampal connections in trkB
(/)/trkC (/) mice
The above observations showed relatively mild alterations in the
topography of hippocampal afferents in trkB (/) and
trkC (/) mice. To determine whether these findings may
be attributable to redundancy of neurotrophin receptors, we generated
double-mutant trkB (/)/trkC (/) mice.
Injections of DiI in the entorhinal cortex and hippocampus of
double-mutant newborn mice did not reveal major differences in the
pattern of connections compared with control littermates or single
homozygous mutant mice (data not shown).
trkB (/)/trkC (/) animals die soon after
birth (Minichiello and Klein, 1996; Silos-Santiago et al., 1997). To
analyze the maturation of hippocampal connections in these
mice, we reconstituted the entorhinohippocampal and commissural
projections in organotypic slice cocultures (Del Río et al.,
1997) of newborn trkB (/)/trkC (/) mice,
which allowed us to monitor the development of hippocampal afferents
for up to 15 d in vitro. The hippocampal projections develop in slice cocultures with laminar and topographic specificity similar to that in vivo (Frotscher and Heimrich, 1993; Li et
al., 1993; Del Río et al., 1997). Thus, entorhinal afferents
densely innervate the stratum lacunosum-moleculare and the outer
molecular layer in the dentate gyrus in cocultures from wild-type mice
(Fig. 4A). A similar
pattern of entorhinal termination was observed in single
trkB (/) or trkC (/) cocultures (data not
shown), which is consistent with the above observations in
vivo.
View larger version (135K):
[in this window]
[in a new window]
|
Figure 4.
Formation of entorhinohippocampal connections in
organotypic slice cocultures of newborn double-mutant
trkB (/)/trkC (/) mice after 15 DIV. Control cocultures (A) and control
entorhinal slices cocultured with trkB
(/)/trkC (/) hippocampus
(C) resulted in a normal pattern of innervation
with fibers terminating into a thick zone covering the stratum
lacunosum-moleculare and the molecular layer. In contrast,
trkB (/)/trkC (/)cocultures
(B) and double-mutant entorhinal cortex
cocultured with control hippocampus (D) resulted
in a thinner layer of termination of entorhinal fibers. Injection sites
of the culture are indicated with asterisks.
Arrowheads point to labeled entorhinal fibers.
Abbreviations as in Figure 2. Scale bar, 300 µm.
|
|
In trkB (/)/trkC (/) slice cocultures,
the entorhinohippocampal pathway developed with correct layer
specificity (Fig. 4B) but with sparse innervation,
which led to a narrower afferent termination zone (84.28 ± 13.20 µm; n = 3, p < 0.01) than in
wild-type (161.25 ± 8.35 µm; n = 29) and
single-mutant cultures [139.33 ± 7.56 µm; n = 23, trkB (/); 159.00 ± 7.59 µm;
n = 15, trkC (/)]. In addition, the
patchy, region-specific distribution of fibers in the stratum
lacunosum-moleculare was less clearly discernible in these
trkB (/)/trkC (/) cultures. These
findings show that hippocampal connections develop even in the absence of both TrkB and TrkC receptors but form less elaborate innervations. This suggests a partial compensation of TrkB and TrkC receptors in the
normal development of hippocampal connections.
Analyses of mixed organotypic slice cocultures
Although neurotrophins are primarily considered to act as
retrograde factors derived from target neurons, recent investigations indicate that neurotrophic factors may also act in an autocrine manner
or even like anterograde factors released by nerve terminals (Davies,
1996; Von Bartheld et al., 1996; Altar et al., 1997; Liu et al., 1997;
Tonra et al., 1998).
The organotypic slice approach also allowed us to prepare mixed slice
cocultures of double-mutant and wild-type mice to determine the role of
neurotrophin receptors present in afferent (entorhinal) and target
(hippocampal) neurons. When wild-type entorhinal slices were cocultured
with double-mutant hippocampus, the pattern of entorhinal innervation
was similar to that of control cocultures (Fig. 4C)
(termination zone = 147.86 ± 10.47 µm; n = 8). In contrast, trkB (/)/trkC (/)
entorhinal slices cocultured with wild-type hippocampus (Fig.
4D) resulted in a reduced zone of innervation (92.73 ± 11.76 µm; n = 12, p < 0.01) reminiscent of that of double-mutant cocultures (Fig.
4B). These data indicate that abnormalities in hippocampal innervation are caused by the lack of TrkB and TrkC receptors in the afferent entorhinal neurons, with little contribution of the receptors present in the target hippocampal neurons.
trkB (/) and trkC (/) mice show
decreased synaptic innervation
The morphometric analysis of single axons has shown that the
number of axonal branches and varicosities is reduced in these homozygous mutant mice. To determine whether the decrease in axonal branching is accompanied by changes in synaptogenesis, we performed a
quantitative electron microscopic study in P12-P13 mice. Axon terminals in hippocampal plexiform layers in trkB (/)
and trkC (/) mice established synaptic contacts with
normal postsynaptic elements such as dendritic shafts and spines (Fig.
5A-C). However, the density
of synaptic contacts in homozygous mutants was lower in all hippocampal
layers of entorhinal and commissural afferent termination. This
decrease in synaptic innervation, compared with control littermates,
was more dramatic in trkB (/) mice (17-39%) than in
trkC (/) animals (11-17%) (Fig. 5D). In
addition, particularly in trkB (/) mice, differences
were more dramatic in the hippocampus proper (36-39% reduction in the
stratum radiatum and stratum lacunosum-moleculare, respectively) than
in the molecular layer of the dentate gyrus. These results show that
the lack of TrkB and TrkC signaling alters synaptogenesis in the CNS by
regulating the number of the synaptic inputs.
View larger version (71K):
[in this window]
[in a new window]
|
Figure 5.
Fine structure of synaptic boutons in
trkB (/) and trkC (/) mice at
P13-P14. A-C, Electron micrographs illustrating axon
terminals and synaptic contacts (arrowheads) in the
stratum radiatum of wild-type, trkB (/), and
trkC (/) mice. Note decreased densities of synaptic
vesicles and reduced thickness of postsynaptic specializations,
especially in trkB (/)mice. Scale bar, 0.5 µm.
D, Density of synaptic contacts in different hippocampal
layers in trkB (/), trkC (/), and
littermate controls (mean ± SEM; *p < 0.05;
**p < 0.01; Student's t test).
E-F, Histograms showing distributions of density of
synaptic vesicles (E) and numbers of synaptic
vesicles near the active zone (F) in axon
terminals in the stratum lacunosum-moleculare of trkB
(/) and trkC (/) mice and their littermate
controls. Note decreased density of synaptic vesicles in
trkB (/) but not in trkC (/)
mice, and reduced numbers of synaptic vesicles clustered near the
active zone in both mutant mice. AT, Axon terminal;
iml, inner molecular layer; mml, medial
molecular layer; oml, outer molecular layer;
slm, stratum lacunosum-moleculare; sr,
stratum radiatum.
|
|
Fine structural abnormalities of axon terminals in
trkB (/) and trkC (/) mice
To discern whether the remaining synaptic boutons may be affected
by the absence of TrkB or TrkC receptors, a detailed fine structural
analysis was performed. We observed that the majority of axon terminals
appeared to display a low density of synaptic vesicles, which were
distributed homogeneously throughout the axonal profile in the
homozygous mutant mice. Furthermore, there was little clustering of
synaptic vesicles near the active synaptic zone (Fig.
5E,F). These abnormalities were more dramatic in
trkB (/) than in trkC (/) mice. In
addition, synaptic specializations were less conspicuous in these
homozygous mutant mice.
To substantiate these observations we performed a morphometric study of
presynaptic boutons and synaptic contacts in the different termination
layers of the hippocampus (Table 1; Fig.
5E,F). Within all the termination fields, presynaptic
boutons were larger in trkB (/) mice (28-38%) and
displayed a lower density of synaptic vesicles (19-41%) than in
control littermates. In contrast, no significant differences for these
parameters were observed in trkC (/) animals. In
addition, the number of synaptic vesicles clustered near the active
zone (Rosahl et al., 1995) was much lower in both trkB
(/) (19-40%) and trkC (/) (23-30%) mice (Table
1; Fig. 5F) than in their control littermates.
Moreover, the thickness of the postsynaptic zone was reduced in both
homozygous mutants, whereas the synaptic cleft was slightly thinner
only in trkB (/) mice. Finally, we did not find
significant differences in the length of synaptic contacts in
trkB (/) and trkC (/) mice (Table 1).
These findings were similar for all hippocampal laminae, including the
layers of termination of entorhinal and commissural afferents. These
data show major structural alterations of presynaptic axon terminals
and synapses in mice lacking TrkB receptors, and to a lesser extent, in
those lacking TrkC, which supports a role of neurotrophic factors in
the functional maturation of CNS synapses.
Expression of synaptic-associated proteins in trkB
(/) and trkC (/) mice
Some of the synaptic abnormalities reported above are similar to
those described in null-mutant mice for genes encoding
synaptic-associated proteins (Rosahl et al., 1993; Li et al., 1995;
Takei et al., 1995). To examine whether the distribution and expression
of these proteins were altered in trkB (/) and
trkC (/) mice, we performed an immunocytochemical
analysis. Consistent with the electron microscopic observations,
confocal microscopy analysis of immunoreacted sections showed that the
synaptic vesicle proteins synapsin I and synaptophysin were markedly
reduced in trkB (/) mice among all hippocampal layers
(38-71%), especially in the stratum radiatum (Figs.
6, 7).
These proteins are considered to be integral proteins of synaptic vesicles and thus markers of synaptic vesicle populations. A dramatic decrease was also observed in trkB (/) animals in the
immunolabeling for the synaptic vesicle protein synaptotagmin I
(31-56% reduction) (Figs. 6, 7), a v-SNARE essential for
neurotransmitter release (Geppert et al., 1994b). In contrast,
immunostaining for synaptobrevin 2, another v-SNARE protein, was not
decreased in trkB (/) animals but showed a slight
increase in some layers (16%). We next examined the distribution of
the synaptic membrane proteins SNAP-25 and syntaxin 1, which are
essential t-SNAREs for calcium-dependent exocytosis and
neurotransmitter release (Blasi et al., 1993; Südhof, 1995;
Hay and Scheller, 1997). Although syntaxin 1-immunostaining was
dramatically reduced (60-68% reduction), the immunolabeling for
SNAP-25 was decreased notably in the hippocampus proper (40-56% reduction) but not in the dentate gyrus (20% reduction) (Figs. 6,
7). Similarly, the small GTP-binding protein Rab3a, which is believed
to regulate synaptic vesicle fusion (Geppert et al., 1994a, 1997), was
also significantly reduced in these mutant mice (53-63%) (Fig. 7). We
conclude that most synaptic-associated proteins, except synaptobrevin
2, are differentially downregulated in trkB (/) mice
with distinguishing patterns of laminar changes. In addition, the
profiles of reductions were different for each protein and in general
were more dramatic in the hippocampus proper than in the dentate
gyrus.
View larger version (174K):
[in this window]
[in a new window]
|
Figure 6.
Immunolabeling for different synaptic-associated
proteins in hippocampal sections of wild-type (left
column), trkB (/) (middle
column), and trkC (/) (right
column) mice (P14) (SYNTG, synaptotagmin I;
SYTPH, synaptophysin; and SNAP-25). Laser confocal
microscopy photomicrographs are reconstructions of two 2-µm-thick
confocal sections. To allow comparison of mutant and control
littermates, sections were immunolabeled in bulk and photographed in
identical conditions. Abbreviations as in Figure 2. Scale bar, 150 µm.
|
|
View larger version (29K):
[in this window]
[in a new window]
|
Figure 7.
Quantitative determination of immunofluorescence
signals in trkB (/) and trkC (/)
mice and in control littermates. Diagrams show continuous linear
profiles of fluorescence intensity in vertical stripes of hippocampal
sections from the stratum pyramidale to the stratum granulare, for
different synaptic-associated protein immunolabeling
(SYN1, synapsin 1; SYTPH, synaptophysin;
SYNTG, synaptotagmin; SBV2, synaptobrevin
2; SYTX1, syntaxin 1; SNAP-25;
Rab3a). The correspondence with hippocampal layers is
indicated on the x-axis. The intensities of fluorescence
are represented in gray levels
(y-axis). The profiles of null-mutant (red
lines) and their control littermates (black
lines) are displayed in the same diagram to allow
comparison.
|
|
In trkC (/) mice, in contrast, only the
immunocytochemical signal for synapsin 1 was dramatically reduced
(52-64% reduction) (Fig. 7), whereas the v-SNAREs synaptotagmin I and
synaptobrevin 2 and the t-SNARE syntaxin 1 showed moderate decreases
(19-45%). None of the remaining synaptic proteins studied, including
synaptophysin, SNAP-25, and Rab3a, showed major changes in these
mutants compared with wild-type littermates (Figs. 6, 7).
To further support the view that synaptic-associated proteins were
downregulated in these mutants, we performed biochemical studies.
Western blot analyses confirmed a marked reduction (27-46%) of
synaptic-associated protein levels in the forebrain of trkB (/) mutant mice compared with control littermates (Fig.
8). trkC (/) mice, in
contrast, showed moderate reduction of protein levels. Taken together,
these findings show that the lack of TrkB and, to a lesser extent, TrkC
signaling leads to downregu-lation of both synaptic vesicle and
synaptic membrane proteins responsible for synaptic vesicle docking and
fusion, and neurotransmitter release at synaptic sites (Südhof,
1995; Hay and Scheller, 1997).
View larger version (111K):
[in this window]
[in a new window]
|
Figure 8.
Immunoblot analysis of the synaptic proteins
synaptotagmin I (SYNTG), synaptophysin
(SYTPH), syntaxin 1 (SYTX1),
SNAP-25, and of -tubulin (TUB) in
trkB (/) and trkC (/) mice and
control littermates. Densitometric analysis (n = 2 animals per group, considering -tubulin levels as reference)
revealed decreases of 27% (SYNTG), 44% (SYTPH), 39% (SYTX1), and
46% (SNAP-25) in trkB (/) mice compared with
control littermates. trkC (/) mice showed moderate
reductions in SNAP-25 (24%) and synaptotagmin (22%), and slight
reductions (7-5%) in synaptophysin and syntaxin 1.
|
|
| |
DISCUSSION |
TrkB and TrkC receptors are not required for the development of
layer-specific connections in the hippocampus
Studies in the PNS have implicated target-derived neurotrophins in
the guidance and growth of developing axons and in the regulation of
the density of innervation (Edwards et al., 1989; Diamond et al., 1992;
Miller et al., 1994; Causing et al., 1997; Fritzsch et al., 1997; Paves
and Saarma, 1997; Song et al., 1997). In the CNS, several studies
in vitro and in vivo have shown that exogenous
neurotrophins may regulate axonal and collateral branching in several
brain regions (Cabelli et al., 1995; Cohen-Cory and Fraser, 1995;
Galuske et al., 1996; Bolz et al., 1997; Inoue and Sanes, 1997). A
recent study, using infusion of blocking TrkB-IgG fusion proteins, has
shown that endogenous BDNF or NT4 is necessary for the formation of
ocular dominance columns in the visual cortex of kittens (Cabelli et
al., 1997).
The present study has analyzed, for the first time, the development of
neuronal connections in the CNS in vivo in the absence of
endogenous TrkB and TrkC signaling and in the absence of both receptors. We show that in trkB (/) and trkC
(/) mice, the main afferents to the hippocampus, the commissural
and entorhinal axons, grow into the target hippocampal region with a
timing and pattern of termination similar to that in wild-type animals
(Supèr and Soriano, 1994; Del Río et al., 1997;
Supèr et al., 1998). Most notably, the highly precise laminated
connections of the hippocampal region are preserved in these mutant
mice. Because both TrkB and TrkC receptors are expressed in the neurons
of origin of entorhinal and commissural afferents during development,
we conclude that these receptors and their cognate ligands BDNF/NT4 and
NT3 are not essential for the ingrowth or layer-specific targeting of
hippocampal afferents. This conclusion is supported by our observations
in double-mutant mice showing that the lack of both TrkB and TrkC
signaling does not alter the ingrowth or laminated pattern of
hippocampal connections.
Neurotrophins, formation of topographic maps, and
neuronal activity
As in other brain regions, the development of topographic
projections from the medial and lateral entorhinal cortex to the hippocampus passes through a period of exuberancy followed by refinement and final shaping of adult connections. Thus, axons from
both the lateral and medial entorhinal cortex initially innervate the
entire stratum lacunosum-moleculare from CA3 to the subiculum; the
characteristic patches of medial and lateral entorhinal innervation attain an adult-like appearance by P10-P12 (Supèr and Soriano, 1994; Del Río et al., 1997; Supèr et al., 1998). The
present findings suggest that neurotrophins do not play a role in the shaping of topographic connections in the hippocampus because trkB (/) and trkC (/) mice have normal
patterns of projections from the lateral and medial entorhinal cortex.
Because double-mutant mice die soon after birth, we cannot determine
whether the lack of both TrkB and TrkC receptors influences the
formation of lateral and medial projections, because the topography of
these projections is not well preserved in vitro.
In the visual system, application of exogenous BDNF and NT4 or infusion
of TrkB-IgG fusion proteins in the postnatal period prevents the
formation of ocular dominance columns (Cabelli et al., 1995, 1997;
Galuske et al., 1996; Hata et al., 1996). These observations suggest
that neuronal activity by thalamocortical axons may control the
expression of neurotrophins in target neurons in layer IV, which in
turn may act as retrograde signals for axonal growth and synaptic
stabilization through a Hebbian mechanism (Katz and Shatz, 1996;
Cabelli et al., 1997). In addition, neurotrophins present in limited
amounts may also be responsible for the retraction of thalamocortical
collaterals that accompanies the formation of ocular dominance
columns.
Several differences may be considered between the development of
hippocampal connections and that of ocular dominance columns. For
instance, it is not known whether the refinement of hippocampal connections depends on neuronal activity. Another difference is that
the medial and lateral entorhinal projections terminate onto distinct
classes of pyramidal neurons (CA1, CA2, CA3, and subicular cells),
which have different developmental histories, afferent and efferent
connections, electrophysiological properties, and patterns of gene
expression (Stanfield and Cowan, 1988; Amaral and Witter, 1995; Freund
and Buzsaki, 1996). This allows a scenario in which different pyramidal
neurons may express distinct molecules influencing axonal growth, which
is unlikely to occur in early columns of neurons in layer IV of the
visual cortex. Thus, all the available evidence suggests that the
building of neural connections in the hippocampus depends on the
expression of selective molecules (such as ephrins and semaphorins) in
subsets of pyramidal neurons.
Neurotrophins regulate axonal branching of
hippocampal connections
Exogenous BDNF and NT3 have been shown to enhance axonal growth
and branching in a number of brain regions (Cabelli et al., 1995, 1997;
Cohen-Cory and Fraser, 1995; Bolz et al., 1997; Inoue and Sanes, 1997).
Neurotrophins also regulate the growth and maturation of dendritic
trees in the developing cerebral cortex in an activity-dependent manner
(McAllister et al., 1995, 1996, 1997). The present data provide
evidence that axonal branching of both commissural and entorhinal
fibers is decreased in trkB (/) and trkC
(/) animals, which supports a role for the endogenous neurotrophins
BDNF/NT4 and NT3 in the elaboration and maturation of hippocampal
afferent fibers.
The above studies have often reported specific, and even opposing,
effects of BDNF/NT4 and NT3 on axonal growth. The present observations
show consistent reductions of axonal arbors in both trkC
(/) (26-49% reduction) and trkB (/) (20-36%
reduction) animals, which suggests that ligands of both TrkB and TrkC
receptors cooperate in the elaboration and branching of hippocampal
afferents. This notion is consistent with the coexpression of
trkB and trkC transcripts in the hippocampal
afferent neurons during development.
Neurotrophins and synaptogenesis in the CNS
We show here for the first time that the lack of endogenous TrkB
and TrkC receptors alters synaptogenesis in the CNS by reducing the
density of synaptic contacts, which supports a role for neurotrophic factors in the regulation of the number of synapses during development (Snider and Litchman, 1996). The reduction in synaptic density (number
of synapses per unit area) was more dramatic in trkB (/) mice (17-39%) than in trkC (/) animals (11-17%).
Because the size and area of the afferent termination layers in the
hippocampus of these homozygous mutant mice are smaller than those of
control littermates [21% and 18% reduction of layers in
trkB (/) and trkC (/) mice, respectively,
as estimated in Nissl-stained sections], the reduction in the total
number of synaptic inputs is higher. This reduction in the total number
of hippocampal synapses can be estimated as 34-52% and 25-30% for
trkB (/) and trkC (/) mice,
respectively.
Postnatal trkB (/) mice show increased neuronal cell
death in some of the populations of hippocampal afferent neurons, such as the CA3 pyramidal cells (Alcántara et al., 1997). The
decreased synaptic innervation in part may be the result of a reduction in the number of neurons. Although neuronal cell death may account for some of the reduction in synaptic innervation, our findings show
that homozygous mutant mice display decreased branching and elaboration
of single axonal arbors and reduced densities of axonal varicosities
along axon collaterals (Fig. 3). These results indicate that the
reduced synaptic innervation is also attributable to an effect of the
mutations on developing afferent axons.
Neurotrophins and the functional maturation of synapses:
regulation of v-SNAREs and t-SNAREs
This study reports for the first time that the axon terminals of
trkB and trkC kinase-deficient mice display
dramatic fine structural abnormalities, such as decreased density of
synaptic vesicles and less prominent clustering of synaptic vesicles
near the active zone. These findings suggest that the absence of TrkB and TrkC signaling interferes with the functional maturation of the
presynaptic machinery, in particular by altering the number of synaptic
vesicles or their exocytotic/endocytotic cycle or both. In
agreement with this notion, we report here a dramatic and specific
downregulation of presynaptic proteins, including t-SNARE and v-SNARE
proteins, responsible for synaptic vesicle fusion (Blasi et al., 1993;
Südhof, 1995; Geppert et al., 1997; Hay and Scheller, 1997;
Martin, 1997). Such a downregulation is unlikely to be solely the
consequence of a decreased synaptic density because the reductions of
protein levels are very heterogeneous (Figs. 6, 7). For instance,
decreased immunocytochemical signals in trkB (/) mice
range from the virtual disappearance of syntaxin 1-immunostaining to no
detectable changes in synaptobrevin 2. This is more evident in
trkC (/) animals, which show a selective reduction in
the immunological signals of only three synaptic proteins. Taken
together these observations support a role of neurotrophins in the
developmental maturation of synaptic structure and function by
regulating the levels of some, but not all, presynaptic proteins (Wang
et al., 1995; Takei et al., 1997).
Because similar structural and biochemical changes in mice lacking
synaptic-associated proteins are linked to altered synaptic function
and neurotransmitter release (Rosahl et al., 1993; Li et al., 1995;
Takei et al., 1995; Castillo et al., 1997), it is tempting to speculate
that Ca2+-dependent synaptic vesicle dynamics and
neural transmission may be altered in trkB and
trkC-deficient mice. Neurotrophins and presynaptic Trk
receptors have been shown to potentiate neurotransmitter release (Lohof
et al., 1993; Kang and Schuman, 1995; Korte et al., 1995; Wang and Poo,
1997), and BDNF is necessary for induction of LTP (Korte et al., 1995).
These actions are thought to be mediated by presynaptic Trk activation
and phosphorylation of some synaptic proteins, such as synapsin I
(Jovanovic et al., 1996). We propose that TrkB and TrkC receptors not
only modify the presynaptic machinery locally, but they also regulate
synaptic protein levels during development. This may suggest that
transcriptional regulation of v-SNAREs and t-SNAREs is one of the
mechanisms by which neurotrophins contribute to the activity-dependent
plasticity of the developing and adult CNS.
| |
FOOTNOTES |
Received April 8, 1998; revised July 1, 1998; accepted July 6, 1998.
This work was supported by grants from Comisión Interministerial
de Ciencia y Tecnología, Spain (SAF98-0106), and
Dirección General de Investigaciones Científicas y
Técnicas (P.M.95-102), and by the Ramón Areces Foundation
(Spain), the International Institute for Research in Paraplegia
(Switzerland), and the Marató of TV3 to E.S. We thank Robin
Rycroft for editorial assistance, and G. Barnstable and R. Jahn for
generously providing antibodies to synaptic proteins.
A.M. and S.A. contributed equally to this work.
Correspondence should be addressed to Dr. Eduardo Soriano, Department
of Animal and Plant Cell Biology, Faculty of Biology, University of
Barcelona, Diagonal 645, Barcelona 08028, Spain.
| |
REFERENCES |
-
Alcántara S,
Frisén J,
Del Río JA,
Soriano E,
Barbacid M,
Silos-Santiago I
(1997)
TrkB signaling is required for postnatal survival of CNS neurons and protects hippocampal and motor neurons from axotomy-induced cell death.
J Neurosci
17:3623-3633[Abstract/Free Full Text].
-
Altar CA,
Cai N,
Bliven T,
Juhasz M,
Conner JM,
Acheson AL,
Lindsay RM,
Wiegand SJ
(1997)
Anterograde transport of brain-derived neurotrophic factor and its role in the brain.
Nature
386:856-860.
-
Amaral DG,
Witter MP
(1995)
Hippocampal formation.
In: The rat nervous system (Paxinos G,
ed), pp 433-493. San Diego: Academic.
-
Barnstable CJ,
Hofstein R,
Akagawa K
(1985)
A marker for amacrine cell development in rat retina.
Dev Brain Res
20:286-290.
-
Blasi J,
Chapman ER,
Link E,
Binz T,
Yamasaki S,
DeCamilli P,
Südhof TC,
Niemann H,
Jahn R
(1993)
Botulinum neurotoxin A selectively cleaves the synaptic protein SNAP-25.
Nature
365:160-163[Medline].
-
Bolz J,
Castellani V,
Batardière A
(1997)
Neurotrophic factors play a role in the elaboration of local cortical circuits.
Soc Neurosci Abstr
23:1433.
-
Brose N,
Petrenko AG,
Südhof TC,
Jahn R
(1992)
Synaptotagmin: a calcium sensor on the synaptic vesicle surface.
Science
256:1021-1025[Abstract/Free Full Text].
-
Cabelli RJ,
Hohn A,
Shatz T
(1995)
Inhibition of ocular dominance column formation by infusion of NT-4/5 or BDNF.
Science
267:1662-1666[Abstract/Free Full Text].
-
Cabelli RJ,
Shelton DL,
Segal RA,
Shatz CJ
(1997)
Blockade of endogenous ligands of TrkB inhibits formation of ocular dominance columns.
Neuron
19:63-76[Web of Science][Medline].
-
Castillo PE,
Janz R,
Südohf TC,
Tzounopoulos T,
Malenka RC,
Nicoll RA
(1997)
Rab3a is essential for mossy fibre long-term potentiation in the hippocampus.
Nature
388:590-593[Medline].
-
Causing CG,
Gloster A,
Aloyz R,
Bamji SX,
Chang E,
Fawcett J,
Kuchel G,
Miller FD
(1997)
Synaptic innervation density is regulated by neuron-derived BDNF.
Neuron
18:257-267[Web of Science][Medline].
-
Cohen-Cory S,
Fraser SE
(1995)
Effects of brain-derived neurotrophic factor on optic axon branching and remodelling in vitro.
Nature
378:192-196[Medline].
-
Davies AM
(1996)
Paracrine and autocrine actions of neurotrophic factors.
Neurochem Res
21:749-753[Web of Science][Medline].
-
Del Río JA,
Heimrich B,
Borrell V,
Förster E,
Drakew A,
Alcántara S,
Nakajima K,
Miyata T,
Ogawa M,
Mikoshiba K,
Derer P,
Frotscher M,
Soriano E
(1997)
A role of Cajal-Retzius cells and reelin in the development of hippocampal connections.
Nature
385:70-74[Medline].
-
Diamond J,
Holmes M,
Coughlin M
(1992)
Endogenous NGF and nerve impulses regulate the collateral sprouting of sensory axons in the skin of the adult rat.
J Neurosci
12:1454-1466[Abstract].
-
Edelmann L,
Hanson PI,
Chapman ER,
Jahn R
(1995)
Synaptobrevin binding to Synaptophysin: a potential mechanism for controlling the exocytotic fusion machine.
EMBO J
14:224-231[Web of Science][Medline].
-
Edwards RM,
Rutter WJ,
Hanahan D
(1989)
Directed expression of NGF to pancreatic
 cells in transgenic mice leads to selective hyperinnervation of the islets.
Cell
58:161-170[Web of Science][Medline]. -
Ernfors P,
Wetmore C,
Olson L,
Persson H
(1990)
Identification of cells in rat brain and peripheral tissues expressing mRNA for members of the nerve growth factor family.
Neuron
5:511-526[Web of Science][Medline].
-
Ernfors P,
Bengzon J,
Kokaia Z,
Persson H,
Lindvall A
(1991)
Increased levels of messenger RNAs for neurotrophic factors in the brain during kindling epileptogenesis.
Neuron
7:165-176[Web of Science][Medline].
-
Fariñas I,
Reichardt LF
(1996)
Neurotrophic factors and their receptors: implications of genetic studies.
Semin Neurosci
8:133-143.
-
Figurov A,
Pozzo-Miller LD,
Olaffson P,
Wang T,
Lu B
(1996)
Regulation of synaptic responses to high-frequency stimulation and LTP by neurotrophins in the hippocampus.
Nature
381:706-709[Medline].
-
Freund TF,
Buzsaki G
(1996)
Interneurons of the hippocampus.
Hippocampus
6:345-470.
-
Fritzsch B,
Silos-Santiago I,
Bianchi LM,
Fariñas I
(1997)
The role of neurotrophic factors in regulating the development of inner ear innervation.
Trends Neurosci
20:159-164[Web of Science][Medline].
-
Frotscher M,
Heimrich B
(1993)
Formation of layer-specific fiber projections to the hippocampus in vitro.
Proc Natl Acad Sci USA
90:10400-10403[Abstract/Free Full Text].
-
Gall CM,
Isackson PJ
(1989)
Limbic seizures increase neuronal production of messenger RNA for nerve growth factor.
Science
245:758-761[Abstract/Free Full Text].
-
Gall CM,
Murray K,
Isackson PJ
(1991)
Kainic acid-induced seizures stimulate increased expression of nerve growth factor mRNA in rat hippocampus.
Mol Brain Res
9:113-123[Medline].
-
Galuske RAW,
Kim D-S,
Castren E,
Thoenen H,
Singer W
(1996)
Brain-derived neurotrophic factor reverses experience-dependent synaptic modifications in kitten visual cortex.
Eur J Neurosci
8:1554-1559[Web of Science][Medline].
-
Geppert M,
Bolshakov VY,
Siegelbaum SA,
Takel K,
De Camilli P,
Hammer RE,
Südhof TC
(1994a)
The role of Rab3A in neurotransmitter release.
Nature
369:493-497[Medline].
-
Geppert M,
Goda Y,
Hammer RE,
Li C,
Roshal TW,
Stevens CF,
Südhof TC
(1994b)
Synaptotagmin I: a major Ca2+ sensor for transmitter release at a central synapse.
Cell
79:717-727[Web of Science][Medline].
-
Geppert M,
Goda Y,
Stevens CF,
Südhof TC
(1997)
The small GTP-binding protein Rab3a regulates a late step in synaptic vesicle fusion.
Nature
387:810-814[Medline].
-
Hata Y,
Katsuyama N,
Fukuda M,
Ohshima M,
Tsumoto T,
Hatanaka H
(1996)
Brain-derived neurotrophic factor disrupts effects of monocular deprivation in kitten visual cortex.
Soc Neurosci Abstr
22:1728.
-
Hay JC,
Scheller RH
(1997)
SNAREs and NSF in targeted membrane fusion.
Curr Opin Cell Biol
9:505-512[Web of Science][Medline].
-
Hofer M,
Pagliusi SR,
Hohn A,
Leibrok J,
Barde Y-A
(1990)
Regional distribution of brain-derived neurotrophic factor RNA in the adult mouse brain.
EMBO J
9:2459-2464[Web of Science][Medline].
-
Inoue A,
Sanes JR
(1997)
Lamina-specific connectivity in the brain: regulation by N-cadherin, neurotrophins, and glycoconjugates.
Science
276:1428-1431[Abstract/Free Full Text].
-
Isackson PJ
(1995)
Trophic factor response to neuronal stimuli or injury.
Curr Opin Neurobiol
5:350-357[Web of Science][Medline].
-
Isackson PJ,
Huntsman MM,
Murray KD,
Gall CM
(1991)
BDNF mRNA expression is increased in adult rat forebrain after limbic seizures: temporal patterns of induction distinct from NGF.
Neuron
6:937-948[Web of Science][Medline].
-
Jones KR,
Fariñas I,
Backus C,
Reichardt LF
(1994)
Targeted disruption of the BDNF gene perturbs brain and sensory neuron development but not motor neuron development.
Cell
76:989-999[Web of Science][Medline].
-
Jovanovic JN,
Benfenati F,
Siow YL,
Sihra TS,
Sanghera JS,
Pelech SL,
Greengard P,
Czernik J
(1996)
Neurotrophins stimulate phosphorylation of synapsin I by MAP kinase and regulate synapsin I-actin interactions.
Proc Natl Acad Sci USA
93:3679-3683[Abstract/Free Full Text].
-
Kang H,
Schuman EM
(1995)
Long-lasting neurotrophin induced enhancement of synaptic transmission in the adult hippocampus.
Science
267:1658-1662[Abstract/Free Full Text].
-
Katz LC,
Shatz CJ
(1996)
Synaptic activity and the construction of cortical circuits.
Science
274:1133-1138[Abstract/Free Full Text].
-
Klein R,
Nanduri V,
Jing S,
Lamballe F,
Tapley P,
Bryant S,
Cordon-Cardo C,
Jones KR,
Reichardt LF,
Barbacid M
(1991)
The trkB tyrosine protein kinase is a receptor for brain-derived neurotrophic factor and neurotrophin-3.
Cell
66:395-403[Web of Science][Medline].
-
Klein R,
Lamballe F,
Bryant S,
Barbacid M
(1992)
The trkB tyrosine protein kinase is a receptor for neurotrophin-4.
Neuron
8:947-956[Web of Science][Medline].
-
Klein R,
Smeyne RJ,
Wurst W,
Long LK,
Auerbach BA,
Joyner AL,
Barbacid M
(1993)
Targeted disruption of the trkB neurotrophin receptor gene results in nervous system lesions and neonatal death.
Cell
75:113-122[Web of Science][Medline].
-
Klein R,
Silos-Santiago I,
Smeyne RJ,
Lira S,
Brambilla S,
Bryant S,
Zhang L,
Snider WD,
Barbacid M
(1994)
Disruption of the neurotrophin receptor gene trkC eliminates muscle afferents and results in abnormal movements.
Nature
368:249-251[Medline].
-
Korte M,
Carroll P,
Wolf E,
Brem G,
Thoenen H,
Bonhoeffer T
(1995)
Hippocampal long-term potentiation is impaired in mice lacking BDNF.
Proc Natl Acad Sci USA
92:8856-8880[Abstract/Free Full Text].
-
Lamballe F,
Klein R,
Barbacid M
(1991)
trkC, a new member of the trk family of tyrosine protein kinases, is a receptor for neurotrophin-3.
Cell
66:967-979[Web of Science][Medline].
-
Lecea L,
Del Río JA,
Soriano E
(1995)
Developmental expression of parvalbumin mRNA in the cerebral cortex and hippocampus of the rat.
Mol Brain Res
32:1-13[Medline].
-
Lecea L,
Del Río JA,
Alcántara S,
Criado JR,
Morales M,
Henriksen S,
Soriano E,
Sutcliffe G
(1997)
Cortistatin is expressed in a distinct subset of cortical interneurons.
J Neurosci
17:5868-5880[Abstract/Free Full Text].
-
Li D,
Field PM,
Starega U,
Li Y,
Raisman G
(1993)
Entorhinal axon project to dentate gyrus in organotypic slice co-culture.
Neuroscience
52:799-813[Web of Science][Medline].
-
Li L,
Chin LS,
Shupliakov O,
Brodin L,
Shira TS,
Hvalby O,
Jensen V,
Zheng D,
McNamara JO,
Greengard P,
Andersen P
(1995)
Impairment of synaptic vesicle clustering and of synaptic transmission, and increased seizure propensity, in synapsin I-deficient mice.
Proc Natl Acad Sci USA
92:9235-9239[Abstract/Free Full Text].
-
Lindvall O,
Ernfors P,
Bengzon J,
Kokaia Z,
Smith ML,
Siesjö BK,
Persson H
(1992)
Differential regulation of mRNAs for nerve growth factor, brain-derived neurotrophic factor, and neurotrophin-3 in the adult rat brain following cerebral ischemia and hypoglycemic coma.
Proc Natl Acad Sci USA
89:648-652[Abstract/Free Full Text].
-
Liu ZZ,
Zhu LQ,
Eide FF
(1997)
Critical role of TrkB and brain-derived neurotrophic factor in the differentiation and survival of retinal pigment epithelium.
J Neurosci
17:8749-8755[Abstract/Free Full Text].
-
Lohof AM,
Ip NY,
Poo M
(1993)
Potentiation of developing neuromuscular synapses by the neurotrophins NT-3 and BDNF.
Nature
363:350-353[Medline].
-
Martin TFJ
(1997)
Stages of regulated exocytosis.
Trends Cell Biol
7:271-276.[Medline]
-
Matteoli M,
Takei K,
Cameron R,
Hurlbut P,
Johnston PA,
Sudhof TC,
Jahn R,
De Camilli P
(1991)
Association of Rab3a with synaptic vesicles at the late stages of the secretory pathway.
J Cell Biol
115:625-633[Abstract/Free Full Text].
-
McAllister AK,
Lo DC,
Katz LC
(1995)
Neurotrophins regulate dendritic growth in developing visual cortex.
Neuron
15:791-803[Web of Science][Medline].
-
McAllister AK,
Katz LC,
Lo DC
(1996)
Neurotrophin regulation of cortical dendritic growth requires activity.
Neuron
17:1057-1064[Web of Science][Medline].
-
McAllister AK,
Katz LC,
Lo DC
(1997)
Opposing roles for endogenous BDNF and NT-3 in regulating cortical dendritic growth.
Neuron
18:767-778[Web of Science][Medline].
-
Miller FD,
Speelma A,
Mathew TC,
Fabian J,
Chang E,
Pozniak C,
Toma JG
(1994)
Nerve growth factor derived from terminals selectively increases the ratio of p75 to trkA NGF receptors on mature sympathetic neurons.
Dev Biol
161:206-217[Web of Science][Medline].
-
Minichiello L,
Klein R
(1996)
TrkB and TrkC neurotrophin receptors cooperate in promoting survival of hippocampal and cerebellar granule neurons.
Genes Dev
19:2849-2858.
-
Paves H,
Saarma M
(1997)
Neurotrophins as in vitro growth cone guidance molecules for embryonic sensory neurons.
Cell Tissue Res
290:285-298[Web of Science][Medline].
-
Prakash N,
Cohen-Cory S,
Frostig RD
(1996)
Rapid and opposite effects of BDNF and NGF on the functional organization of the adult cortex "in vivo".
Nature
381:702-706[Medline].
-
Rocamora N,
Pascual M,
Ascady L,
de Lecea L,
Freund T
(1996)
Expression of NGF and NT3 mRNAs in hippocampal interneurons innervated by the GABAergic septohippocampal pathway.
Neuron
16:3991-4004.
-
Rosahl TW,
Geppert M,
Spillane D,
Herz J,
Hammer RE,
Malenka RC,
Südhof TC
(1993)
Short-time synaptic plasticity is altered in mice lacking synapsin I.
Cell
75:661-670[Web of Science][Medline].
-
Rosahl TW,
Spillane D,
Missler M,
Herz J,
Selig DK,
Wolff JR,
Hammer RE,
Malenka RC,
Südhof TC
(1995)
Essential function of synapsins I and II in synaptic vesicle regulation.
Nature
375:488-493[Medline].
-
Silos-Santiago I,
Fagan AM,
Garber M,
Fritzsch B,
Barbacid M
(1997)
Severe sensory deficits but normal CNS development in newborn mice lacking TrkB and TrkC tyrosine protein kinase receptors.
Eur J Neurosci
9:2045-2056[Web of Science][Medline].
-
Snider WD
(1994)
Functions of the neurotrophins during nervous system development: what are knockouts teaching us.
Cell
77:627-638[Web of Science][Medline].
-
Snider WD,
Litchman J
(1996)
Are neurotrophins synaptotrophins?.
Mol Cell Neurosci
7:433-442[Web of Science][Medline].
-
Snider WD,
Silos-Santiago I
(1996)
Dorsal root ganglion neurons require functional neurotrophin receptors for survival during development.
Philos Trans R Soc Lond B Biol Sci
351:395-403[Web of Science][Medline].
-
Song H-J,
Ming G-L,
Poo M-M
(1997)
cAMP-induced switching in turning direction of nerve growth cones.
Nature
388:275-279[Medline].
-
Soppet D,
Escandon E,
Maragos J,
Middlemas DS,
Reid SW,
Blair J,
Burton LE,
Stanton BR,
Kaplan DR,
Hunter T,
Nickolics K,
Parada LF
(1991)
The neurotrophic factors brain-derived neurotrophic factor and neurotrophin-3 are ligands for the trkB tyrosine kinase receptor.
Cell
65:895-903[Web of Science][Medline].
-
Stanfield BB,
Cowan WM
(1988)
The development of the hippocampal region.
In: Development and maturation of cerebral cortex. Cerebral Cortex. Vol VII (Peters A, Jones EG), pp 91-122. New York: Plenum.
-
Stoppini L,
Buchs PA,
Muller D
(1991)
A simple method for organotypic cultures of nervous tissue.
J Neurosci Methods
37:173-182[Web of Science][Medline].
-
Südhof TC
(1995)
The synaptic vesicle cycle: a cascade of protein-protein interactions.
Nature
375:645-653[Medline].
-
Supèr H,
Soriano E
(1994)
. The organization of the embryonic and early postnatal murine hippocampus. II. Development of entorhinal, commissural, and septal connections studied with the lipophilic tracer DiI.
J Comp Neurol
344:101-120[Web of Science][Medline].
-
Supèr H,
Martínez A,
Del Río JA,
Soriano E
(1998)
Involvement of distinct pioneer neurons in the formation of layer-specific connections in the hippocampus.
J Neurosci
18:4616-4626[Abstract/Free Full Text].
-
Takei Y,
Harada A,
Takeda S,
Kobayashi K,
Terada S,
Noda T,
Takahashi T,
Hirokawa N
(1995)
Synapsin I deficiency results in the structural change in the presynaptic terminals in the murine nervous system.
J Cell Biol
131:1789-1800[Abstract/Free Full Text].
-
Takei N,
Sasaoka K,
Inoue K,
Takahashi M,
Endo Y,
Hatanaka H
(1997)
Brain-derived neurotrophic factor increases the stimulation-evoked release of glutamate and the levels of exocytosis-associated proteins in cultured cortical neurons from embryonic rats.
J Neurochem
68:370-375[Web of Science][Medline].
-
Thoenen H
(1995)
Neurotrophins and neuronal plasticity.
Science
270:593-598[Abstract/Free Full Text].
-
Tonra JR,
Cutis R,
Wong V,
Cliffer KD,
Park JS,
Timmes A,
Nguyen T,
Lindsay RM,
Acheson A,
DiStefano PS
(1998)
Axotomy upregulates the anterograde transport and expression of BDNF by sensory neurons.
J Neurosci
18:4374-4383[Abstract/Free Full Text].
-
Von Bartheld CS,
Byers MR,
Williams R,
Bothwell M
(1996)
Anterograde transport of neurotrophins and axodendritic transfer in the developing visual system.
Nature
379:830-833[Medline].
-
Wang T,
Xie K,
Lu B
(1995)
Neurotrophins promote maturation of developing neuromuscular synapses.
J Neurosci
15:4796-4805[Abstract].
-
Wang X-H,
Poo M-M
(1997)
Potentiation of developing synapses by postsynaptic release of neurotrophin-4.
Neuron
19:825-835[Web of Science][Medline].
Copyright © 1998 Society for Neuroscience 0270-6474/98/18187336-15$05.00/0
This article has been cited by other articles:
|
|
|
|
 
F. Xu, D. A. Hennessy, T. K. M. Lee, and N. I. Syed
Trophic Factor-Induced Intracellular Calcium Oscillations Are Required for the Expression of Postsynaptic Acetylcholine Receptors during Synapse Formation between Lymnaea Neurons
J. Neurosci.,
February 18, 2009;
29(7):
2167 - 2176.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
K. J. M. Marler, E. Becker-Barroso, A. Martinez, M. Llovera, C. Wentzel, S. Poopalasundaram, R. Hindges, E. Soriano, J. Comella, and U. Drescher
A TrkB/EphrinA Interaction Controls Retinal Axon Branching and Synaptogenesis
J. Neurosci.,
November 26, 2008;
28(48):
12700 - 12712.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
M. D. David, A. Yeramian, M. Dunach, M. Llovera, C. Canti, A. G. de Herreros, J. X. Comella, and J. Herreros
Signalling by neurotrophins and hepatocyte growth factor regulates axon morphogenesis by differential {beta}-catenin phosphorylation
J. Cell Sci.,
August 15, 2008;
121(16):
2718 - 2730.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
W Boesmans, P Gomes, J Janssens, J Tack, and P V. Berghe
Brain-derived neurotrophic factor amplifies neurotransmitter responses and promotes synaptic communication in the enteric nervous system
Gut,
March 1, 2008;
57(3):
314 - 322.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
K. Bartkowska, A. Paquin, A. S. Gauthier, D. R. Kaplan, and F. D. Miller
Trk signaling regulates neural precursor cell proliferation and differentiation during cortical development
Development,
December 15, 2007;
134(24):
4369 - 4380.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
J.-Y. Hu, Y. Chen, and S. Schacher
Multifunctional Role of Protein Kinase C in Regulating the Formation and Maturation of Specific Synapses
J. Neurosci.,
October 24, 2007;
27(43):
11712 - 11724.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
S. Marshak, A. M. Nikolakopoulou, R. Dirks, G. J. Martens, and S. Cohen-Cory
Cell-Autonomous TrkB Signaling in Presynaptic Retinal Ganglion Cells Mediates Axon Arbor Growth and Synapse Maturation during the Establishment of Retinotectal Synaptic Connectivity
J. Neurosci.,
March 7, 2007;
27(10):
2444 - 2456.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
T. Sadakata, W. Kakegawa, A. Mizoguchi, M. Washida, R. Katoh-Semba, F. Shutoh, T. Okamoto, H. Nakashima, K. Kimura, M. Tanaka, et al.
Impaired Cerebellar Development and Function in Mice Lacking CAPS2, a Protein Involved in Neurotrophin Release
J. Neurosci.,
March 7, 2007;
27(10):
2472 - 2482.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
H.-T. Zhang, L.-Y. Li, X.-L. Zou, X.-B. Song, Y.-L. Hu, Z.-T. Feng, and T. T.-H. Wang
Immunohistochemical Distribution of NGF, BDNF, NT-3, and NT-4 in Adult Rhesus Monkey Brains
J. Histochem. Cytochem.,
January 1, 2007;
55(1):
1 - 19.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
R. A. Gomes, C. Hampton, F. El-Sabeawy, S. L. Sabo, and A. K. McAllister
The Dynamic Distribution of TrkB Receptors before, during, and after Synapse Formation between Cortical Neurons.
J. Neurosci.,
November 1, 2006;
26(44):
11487 - 11500.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
E. Vergano-Vera, M. J. Yusta-Boyo, F. de Castro, A. Bernad, F. de Pablo, and C. Vicario-Abejon
Generation of GABAergic and dopaminergic interneurons from endogenous embryonic olfactory bulb precursor cells
Development,
November 1, 2006;
133(21):
4367 - 4379.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
W. J. Tyler, X.-l. Zhang, K. Hartman, J. Winterer, W. Muller, P. K. Stanton, and L. Pozzo-Miller
BDNF increases release probability and the size of a rapidly recycling vesicle pool within rat hippocampal excitatory synapses
J. Physiol.,
August 1, 2006;
574(3):
787 - 803.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
S. X. Bamji, B. Rico, N. Kimes, and L. F. Reichardt
BDNF mobilizes synaptic vesicles and enhances synapse formation by disrupting cadherin-{beta}-catenin interactions
J. Cell Biol.,
July 17, 2006;
174(2):
289 - 299.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
K. Shimazu, M. Zhao, K. Sakata, S. Akbarian, B. Bates, R. Jaenisch, and B. Lu
NT-3 facilitates hippocampal plasticity and learning and memory by regulating neurogenesis
Learn. Mem.,
May 1, 2006;
13(3):
307 - 315.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
M. A. Carmona, E. Pozas, A. Martinez, J. F. Espinosa-Parrilla, E. Soriano, and F. Aguado
Age-dependent Spontaneous Hyperexcitability and Impairment of GABAergic Function in the Hippocampus of Mice Lacking trkB
Cereb Cortex,
January 1, 2006;
16(1):
47 - 63.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
B. Hu, A. M. Nikolakopoulou, and S. Cohen-Cory
BDNF stabilizes synapses and maintains the structural complexity of optic axons in vivo
Development,
October 1, 2005;
132(19):
4285 - 4298.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
B. W. Luikart, S. Nef, T. Virmani, M. E. Lush, Y. Liu, E. T. Kavalali, and L. F. Parada
TrkB Has a Cell-Autonomous Role in the Establishment of Hippocampal Schaffer Collateral Synapses
J. Neurosci.,
April 13, 2005;
25(15):
3774 - 3786.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
K. N. Robinson, K. Manto, R. J. Buchsbaum, J. I. S. MacDonald, and S. O. Meakin
Neurotrophin-dependent Tyrosine Phosphorylation of Ras Guanine-releasing Factor 1 and Associated Neurite Outgrowth Is Dependent on the HIKE Domain of TrkA
J. Biol. Chem.,
January 7, 2005;
280(1):
225 - 235.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
J.-Y. Hu, J. Goldman, F. Wu, and S. Schacher
Target-Dependent Release of a Presynaptic Neuropeptide Regulates the Formation and Maturation of Specific Synapses in Aplysia
J. Neurosci.,
November 3, 2004;
24(44):
9933 - 9943.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
T. Numakawa, T. Ishimoto, S. Suzuki, Y. Numakawa, N. Adachi, T. Matsumoto, D. Yokomaku, H. Koshimizu, K. E. Fujimori, R. Hashimoto, et al.
Neuronal Roles of the Integrin-associated Protein (IAP/CD47) in Developing Cortical Neurons
J. Biol. Chem.,
October 8, 2004;
279(41):
43245 - 43253.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
L. Tong, R. Balazs, P. L. Thornton, and C. W. Cotman
{beta}-Amyloid Peptide at Sublethal Concentrations Downregulates Brain-Derived Neurotrophic Factor Functions in Cultured Cortical Neurons
J. Neurosci.,
July 28, 2004;
24(30):
6799 - 6809.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
S. B. Elmariah, M. A. Crumling, T. D. Parsons, and R. J. Balice-Gordon
Postsynaptic TrkB-Mediated Signaling Modulates Excitatory and Inhibitory Neurotransmitter Receptor Clustering at Hippocampal Synapses
J. Neurosci.,
March 10, 2004;
24(10):
2380 - 2393.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
H. Golan, T. Levav, A. Mendelsohn, and M. Huleihel
Involvement of Tumor Necrosis Factor Alpha in Hippocampal Development and Function
Cereb Cortex,
January 1, 2004;
14(1):
97 - 105.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
F. M. Smart, G. M. Edelman, and P. W. Vanderklish
BDNF induces translocation of initiation factor 4E to mRNA granules: Evidence for a role of synaptic microfilaments and integrins
PNAS,
November 25, 2003;
100(24):
14403 - 14408.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
C. Itami, F. Kimura, T. Kohno, M. Matsuoka, M. Ichikawa, T. Tsumoto, and S. Nakamura
Brain-derived neurotrophic factor-dependent unmasking of """silent""" synapses in the developing mouse barrel cortex
PNAS,
October 28, 2003;
100(22):
13069 - 13074.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
D. W Munno and N. I Syed
Synaptogenesis in the CNS: An Odyssey from Wiring Together to Firing Together
J. Physiol.,
October 1, 2003;
552(1):
1 - 11.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
F. Barnabe-Heider and F. D. Miller
Endogenously Produced Neurotrophins Regulate Survival and Differentiation of Cortical Progenitors via Distinct Signaling Pathways
J. Neurosci.,
June 15, 2003;
23(12):
5149 - 5160.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
F. Aguado, M. A. Carmona, E. Pozas, A. Aguilo, F. J. Martinez-Guijarro, S. Alcantara, V. Borrell, R. Yuste, C. F. Ibanez, and E. Soriano
BDNF regulates spontaneous correlated activity at early developmental stages by increasing synaptogenesis and expression of the K+/Cl- co-transporter KCC2
Development,
April 1, 2003;
130(7):
1267 - 1280.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
W. J. Tyler, S. P. Perrett, and L. D. Pozzo-Miller
The Role of Neurotrophins in Neurotransmitter Release
Neuroscientist,
December 1, 2002;
8(6):
524 - 531.
[Abstract]
[PDF]
|
|
|
|
|
|
|
S. Cohen-Cory
The Developing Synapse: Construction and Modulation of Synaptic Structures and Circuits
Science,
October 25, 2002;
298(5594):
770 - 776.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
W. J. Tyler, M. Alonso, C. R. Bramham, and L. D. Pozzo-Miller
From Acquisition to Consolidation: On the Role of Brain-Derived Neurotrophic Factor Signaling in Hippocampal-Dependent Learning
Learn. Mem.,
September 1, 2002;
9(5):
224 - 237.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
V. Borrell and E. M. Callaway
Reorganization of Exuberant Axonal Arbors Contributes to the Development of Laminar Specificity in Ferret Visual Cortex
J. Neurosci.,
August 1, 2002;
22(15):
6682 - 6695.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
A. R. Carter, C. Chen, P. M. Schwartz, and R. A. Segal
Brain-Derived Neurotrophic Factor Modulates Cerebellar Plasticity and Synaptic Ultrastructure
J. Neurosci.,
February 15, 2002;
22(4):
1316 - 1327.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
X. Wang, R. Butowt, M. R. Vasko, and C. S. von Bartheld
Mechanisms of the Release of Anterogradely Transported Neurotrophin-3 from Axon Terminals
J. Neurosci.,
February 1, 2002;
22(3):
931 - 945.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
R. Kyin, Y. Hua, M. Baybis, B. Scheithauer, D. Kolson, E. Uhlmann, D. Gutmann, and P. B. Crino
Differential Cellular Expression of Neurotrophins in Cortical Tubers of the Tuberous Sclerosis Complex
Am. J. Pathol.,
October 1, 2001;
159(4):
1541 - 1554.
[Abstract]
[Full Text]
|
|
|
|
|
|
|
H. W. Tao and M.-m. Poo
Retrograde signaling at central synapses
PNAS,
September 25, 2001;
98(20):
11009 - 11015.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
W. J. Tyler and L. D. Pozzo-Miller
BDNF Enhances Quantal Neurotransmitter Release and Increases the Number of Docked Vesicles at the Active Zones of Hippocampal Excitatory Synapses
J. Neurosci.,
June 15, 2001;
21(12):
4249 - 4258.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
M. Bibel and Y.-A. Barde
Neurotrophins: key regulators of cell fate and cell shape in the vertebrate nervous system
Genes & Dev.,
December 1, 2000;
14(23):
2919 - 2937.
[Full Text]
|
|
|
|
|
|
|
B. H. Han and D. M. Holtzman
BDNF Protects the Neonatal Brain from Hypoxic-Ischemic Injury In Vivo via the ERK Pathway
J. Neurosci.,
August 1, 2000;
20(15):
5775 - 5781.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
A. F. Ernst, G. Gallo, P. C. Letourneau, and S. C. McLoon
Stabilization of Growing Retinal Axons by the Combined Signaling of Nitric Oxide and Brain-Derived Neurotrophic Factor
J. Neurosci.,
February 15, 2000;
20(4):
1458 - 1469.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
M. Barallobre, J. Del Rio, S Alcantara, V Borrell, F Aguado, M Ruiz, M. Carmona, M Martin, M Fabre, R Yuste, et al.
Aberrant development of hippocampal circuits and altered neural activity in netrin 1-deficient mice
Development,
January 11, 2000;
127(22):
4797 - 4810.
[Abstract]
[PDF]
|
|
|
|
|
|
|
J. P. Fawcett, M. A. Alonso-Vanegas, S. J. Morris, F. D. Miller, A. F. Sadikot, and R. A. Murphy
Evidence that Brain-Derived Neurotrophic Factor from Presynaptic Nerve Terminals Regulates the Phenotype of Calbindin-Containing Neurons in the Lateral Septum
J. Neurosci.,
January 1, 2000;
20(1):
274 - 282.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
R. Tyzio, A. Represa, I. Jorquera, Y. Ben-Ari, H. Gozlan, and L. Aniksztejn
The Establishment of GABAergic and Glutamatergic Synapses on CA1 Pyramidal Neurons is Sequential and Correlates with the Development of the Apical Dendrite
J. Neurosci.,
December 1, 1999;
19(23):
10372 - 10382.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
B. Rohrer, J. I. Korenbrot, M. M. LaVail, L. F. Reichardt, and B. Xu
Role of Neurotrophin Receptor TrkB in the Maturation of Rod Photoreceptors and Establishment of Synaptic Transmission to the Inner Retina
J. Neurosci.,
October 15, 1999;
19(20):
8919 - 8930.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
G. Chen, R. Kolbeck, Y.-A. Barde, T. Bonhoeffer, and A. Kossel
Relative Contribution of Endogenous Neurotrophins in Hippocampal Long-Term Potentiation
J. Neurosci.,
September 15, 1999;
19(18):
7983 - 7990.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
L. D. Pozzo-Miller, W. Gottschalk, L. Zhang, K. McDermott, J. Du, R. Gopalakrishnan, C. Oho, Z.-H. Sheng, and B. Lu
Impairments in High-Frequency Transmission, Synaptic Vesicle Docking, and Synaptic Protein Distribution in the Hippocampus of BDNF Knockout Mice
J. Neurosci.,
June 15, 1999;
19(12):
4972 - 4983.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
R. Aloyz, J. P. Fawcett, D. R. Kaplan, R. A. Murphy, and F. D. Miller
Activity-Dependent Activation of TrkB Neurotrophin Receptors in the Adult CNS
Learn. Mem.,
May 1, 1999;
6(3):
216 - 231.
[Abstract]
[Full Text]
|
|
|
|
|
|
|
V. Borrell, J. A. Del Rio, S. Alcantara, M. Derer, A. Martinez, G. D'Arcangelo, K. Nakajima, K. Mikoshiba, P. Derer, T. Curran, et al.
Reelin Regulates the Development and Synaptogenesis of the Layer-Specific Entorhino-Hippocampal Connections
J. Neurosci.,
February 15, 1999;
19(4):
1345 - 1358.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
A. Shimada, C. A. Mason, and M. E. Morrison
TrkB Signaling Modulates Spine Density and Morphology Independent of Dendrite Structure in Cultured Neonatal Purkinje Cells
J. Neurosci.,
November 1, 1998;
18(21):
8559 - 8570.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
Y. Yin, G. M. Edelman, and P. W. Vanderklish
The brain-derived neurotrophic factor enhances synthesis of Arc in synaptoneurosomes
PNAS,
February 19, 2002;
99(4):
2368 - 2373.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
Top
Abstract
Introduction
