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The Journal of Neuroscience, January 1, 2000, 20(1):206-218
Visualization of Cranial Motor Neurons in Live Transgenic
Zebrafish Expressing Green Fluorescent Protein Under the Control
of the Islet-1 Promoter/Enhancer
Shin-ichi
Higashijima1, 2,
Yoshiki
Hotta3, and
Hitoshi
Okamoto4
1 Inheritance and Variation Group, Precursory Research
for Embryonic Science and Technology, Japan Science and Technology
Corporation, Honmachi, Kawaguchi, Saitama 332-0012, Japan,
2 Division of Morphogenesis, National Institute for Basic
Biology, Myodaijicho, Okazaki, Aichi 444-8585, Japan,
3 National Institute of Genetics, Mishima, Shizuoka
411-8540, Japan, and 4 Laboratory for Developmental Gene
Regulation, Brain Science Institute, RIKEN (The Institute of
Physical and Chemical Research), Hirosawa, Wako, Saitama 351-0198, Japan
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ABSTRACT |
We generated germ line-transmitting transgenic zebrafish that
express green fluorescent protein (GFP) in the cranial motor neurons.
This was accomplished by fusing GFP sequences to Islet-1 promoter/enhancer sequences that were sufficient for neural-specific expression. The expression of GFP by the motor neurons in the transgenic fish enabled visualization of the cell bodies, main axons,
and the peripheral branches within the muscles. GFP-labeled motor
neurons could be followed at high resolution for at least up to day
four, when most larval neural circuits become functional, and larvae
begin to swim and capture prey. Using this line, we analyzed axonal
outgrowth by the cranial motor neurons. Furthermore, by selective
application of DiI to specific GFP-positive nerve branches, we showed
that the two clusters of trigeminal motor neurons in rhombomeres 2 and
3 innervate different peripheral targets. This finding suggests that
the trigeminal motor neurons in the two clusters adopt distinct fates.
In future experiments, this transgenic line of zebrafish will allow for
a genetic analysis of cranial motor neuron development.
Key words:
zebrafish; neuron-specific promoter; transgenic; Islet-1; motor neuron; GFP; live visualization
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INTRODUCTION |
Developing motor neurons in the
vertebrate hindbrain are an attractive system in which to study
mechanisms of segmentation and the processes regulating specific axonal
pathfinding (Guthrie, 1996 ; Lumsden and Krumlauf, 1996; Pfaff and
Kintner, 1998). Chick and mouse are the most frequently used
experimental model organisms to study motor neuron development in
vertebrates. Recently, the zebrafish has emerged as another useful
model system. Several features of zebrafish make them especially
amenable for developmental studies, including development of the
hindbrain. The embryos are transparent, making it possible to readily
visualize internal structures and cells in living zebrafish. The
embryonic hindbrain is relatively simple and manipulable (Chandrasekhar
et al., 1997, 1998), and the zebrafish is amenable to large-scale
genetic studies (Driever et al., 1996; Haffter et al., 1996) that have
generated interesting mutations in hindbrain motor neurons
(Chandrasekhar et al., 1999).
Despite these potential advantages of zebrafish for the study of motor
neuron differentiation in the hindbrain, this system has not yet been
fully exploited. No one has ever successfully visualized motor neurons
and their axons in live embryos, which would allow a dynamic analysis
of migration by differentiating motor neurons and pathfinding by their
extending growth cones. The ability to observe the dynamics of neuronal
differentiation may facilitate the detection of the effects of genetic
mutation or other molecular and cellular manipulations that might
otherwise be missed. In Drosophila melanogaster and
Caenorhabditis elegans, reproducible labeling of specific
types of neurons in vivo by expression of GFP under the
control of a cell-type-specific promoter has been used as a powerful
tool to study development of those neurons (Murray et al., 1998; Zallen
et al., 1998). In vertebrates, however, this approach has only
been successful under limited conditions (Dynes and Ngai, 1998; Okada
et al., 1999), partly because of a lack of appropriate promoters for
cell-type-specific expression of GFP or because of difficulty in
observation caused by opacity and complexity of the brain.
Recently, two groups have shown that transgenic zebrafish expressing
GFP in specific tissues can be reliably generated (Higashijima et al.,
1997b; Long et al., 1997). In the present study, we applied this
approach to generate zebrafish in which cranial motor neurons could be
selectively visualized to provide a new tool for studying motor neuron
development. Our strategy was to use the Islet-1 (Isl1) gene to drive GFP expression in cranial motor
neurons. Isl1 is a member of the LIM/homeobox gene
family and is expressed in all postmitotic motor neurons early in their
development (Ericson et al., 1992; Korzh et al., 1993; Inoue et al.,
1994; Tsuchida et al., 1994; Appel et al., 1995; Tokumoto et al., 1995;
Varela-Echavarría et al., 1996; Osumi et al., 1997). Thus, we
expected that the promoter/enhancer of the Isl1 gene would
be able to drive GFP expression in cranial motor neurons. We cloned
genomic fragments of the zebrafish Isl1 gene and identified
DNA sequences that could direct expression of GFP in the cranial motor
neurons of DNA-injected embryos. We then established a stable
transgenic line (Isl1-GFP) of zebrafish that expressed GFP in the
cranial motor neurons.
The intensity of GFP fluorescence by the cranial motor neurons in the
Isl1-GFP line was sufficiently high to enable clear visualization of
the cell bodies, main axons, and the peripheral branches in the target
muscles. In addition to cranial motor neurons, GFP was expressed in the
cranial sensory neurons, except for those in the trigeminal ganglion.
The generation of this transgenic line and the characterization of the
GFP-expressing neurons set the stage for a genetic dissection of the
development of these neurons in future experiments.
As an initial illustration of the usefulness of the Isl1-GFP line, we
characterized in detail the development of the trigeminal motor
neurons. We asked whether the rhombomeric location of the trigeminal
motor neurons correlated with the targets innervated by their axons.
This was analyzed by backlabeling trigeminal motor neurons with
selective DiI application to specific trigeminal nerve branches that
could be seen because of their GFP fluorescence. We found that
trigeminal neurons from rhombomeres 2 and 3 innervate different target
muscles. This result, together with our developmental analysis of the
trigeminal motor neurons, suggests that trigeminal neurons generated in
r2 and r3 adopt distinct fates, supporting the idea that segmental
origin dictates the fate of the two populations of trigeminal motor neurons.
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MATERIALS AND METHODS |
Cloning of the Isl1 genomic DNA, construction of plasmids,
and microinjection of DNA into zebrafish embryos. The
Isl1 cDNA was used to screen a series of zebrafish genomic
phage libraries. An initial screening and two rounds of genome walking
identified a genomic region of ~40 kb in total (Fig.
1A, LS1,
LS2, LS22). Screening of a zebrafish BAC
library was performed by Genome Systems, and one BAC clone (Fig.
1A, N21), ~90 kb in length, was isolated. To
examine the putative transcriptional start site of the Isl1 gene, RACE (rapid amplification of cDNA ends)-PCR was performed as described previously (Higashijima et al., 1997a) using two Isl1-specific primers. The results suggested that the
Isl1 cDNA (Inoue et al., 1994) was almost full-length.
Sequence analysis of the corresponding genomic DNA suggested that there
are no further introns other than the one shown in Figure
1B in the 5' region of the Isl1 gene. A
fragment of DNA corresponding to the 5' half of LS1 was PCR-amplified.
This fragment, termed the putative Isl1 core promoter (ICP),
contained 4.1 kb of 5' upstream region and ~30 bp of 5' untranslated
region of the Isl1 gene. The fragment had, at the 5' end, an
EcoRI site derived from the  DASHII (Stratagene, La
Jolla, CA) phage vector sequence, and a KpnI site at the 3' end, which was introduced with the PCR primer. The ICP-GFP plasmid was
generated in the following manner. The backbone plasmid was pBluescript
II SK (Stratagene). The NotI site was converted to an
NcoI site, and then, the KpnI site was converted
to an NotI site. Synthetic oligonucleotides were used in
these experiments. A fragment containing an SV40 poly(A) signal with an
intron was extracted from the pcDNA1 plasmid (Invitrogen, San Diego,
CA) and introduced between the XbaI and NcoI
sites of the modified pBluescript II SK. The resultant plasmid was
digested with SpeI and XbaI and self-ligated to
disrupt these sites. Then, the NcoI site at the 3' end of
the insert was converted to an XbaI site using a synthetic
oligonucleotide. The HindIII-BglII fragment encoding the modified GFP (codon-humanized, S65A, Y145F; kindly provided by K. Umesono, Kyoto University) was PCR-amplified, and introduced between the HindIII site and BamHI
site of the resultant plasmid. This GFP-encoding fragment carried a
KpnI site upstream of the initiation codon. Then, the
ClaI site within the remaining multiple cloning site of this
plasmid was converted to an EcoRI site using a synthetic
oligonucleotide. Finally, the ICP-GFP plasmid was created by inserting
the ICP fragment between the EcoRI and KpnI sites
immediately upstream of the GFP-encoding region. The ICP-GFP plasmid
therefore had unique NotI and EcoRI sites just 5'
to the ICP (Fig. 1C). All the recognizable EcoRI
fragments derived from the cloned region of the Isl1 genomic
DNA were individually subcloned into the EcoRI site of the
ICP-GFP plasmid. Each plasmid DNA was linearized by NotI,
which is located upstream of the EcoRI cloning site and used
for microinjection. Preparation of DNA and microinjection was performed
essentially as described previously (Higashijima et al., 1997b).
Linearized plasmid DNA was extracted using phenol-chloroform and then
chloroform, precipitated by ethanol, and dissolved in distilled water.
For injection of DNA solution, a holder supporting a glass micropipette
with a beveled opening was connected to a 10 ml disposable plastic
syringe through a plastic tube. A DNA solution of ~25 ng/ml was
injected into the cytoplasm of a one-cell-stage zebrafish embryo with
its chorion intact under dissecting microscope by manually adding air
pressure to the syringe. We adjusted the injection volume so that the
injected solution spread in a sphere with its diameter ranging from one quarter to one half that of the cytoplasm. For the transient expression assay, the injection volume was empirically adjusted such that, on
average, approximately one-fourth of the injected embryos died or
became malformed by the next day. When the injected embryos were raised
to adulthood to generate germ line-transmitting fish, the injection
volume was increased such that one-third to one-half of the injected
embryos died or were malformed by the next day. Expression of GFP was
examined on the first and second days of development. Three of 113 injected fish turned to be the founders for the transgenic progeny. The
frequency of transgenic zebrafish successfully generated using the
CMICP-GFP construct was significantly lower than in a previous study
when we used constructs that drive GFP expression under the control of
the  -actin promoter (20%; Higashijima et al., 1997b).
Although the exact reason for this remains unknown, we may have missed
transgenic lines with low-level GFP expression.
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Figure 1.
Genomic structure of the Islet-1
(Isl1) gene and the plasmid constructs.
A, EcoRI restriction map of the genomic
DNA flanking the Isl1 gene. Lines over
the map represent phage clones (LS1, LS2,
and LS22) and a BAC clone (N21). The
thick line, CM, includes the enhancer
elements for driving GFP expression in cranial motor neurons, whereas
SS includes the enhancer elements for driving GFP
expression in the trigeminal ganglion cells and Rohon-Beard cells.
Other EcoRI fragments were negative for enhancer
activity by our transient expression assay. B, Close-up
view of the genomic region around the Isl1 promoter.
Filled boxes are protein coding regions. The
hatched box represents the putative Isl1
promoter (ICP), which contains ~4.1 kb of the 5'
upstream region and an ~30 bp of the 5' untranslated region of the
Isl1 gene. It was used in all the constructs as a core
promoter. C, A map of the ICP-GFP, the core plasmid.
Every genomic EcoRI fragment was inserted into the
EcoRI site located in the immediate upstream of ICP.
NotI was used to linearize the plasmid DNA for
microinjection. D, A map of the CMICP-GFP or SSICP-GFP
(containing the SS-fragment) plasmid. The CMICP-GFP plasmid drove
expression of GFP in the cranial motor neurons, and it was used for
generating the Isl1-GFP line. The SSICP-GFP plasmid drove expression
of GFP both in Rohon-Beard neurons and the trigeminal sensory
neurons.
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Embryos and staging. Zebrafish were maintained as described
in Westerfield (1995). Most analyses were performed using homozygous transgenic embryos from the Isl1-GFP line. The embryos were collected after crossing homozygous parents. In the early phase of the
experiments, homozygous embryos were obtained by crossing heterozygous
parents. Homozygous fish exhibited no abnormality or retardation in the development of the nervous system. Embryos were collected within 30 min
after fertilization and were allowed to develop at 28.5°C to the
required age, in uncrowded conditions. The developmental age of the
embryos corresponds to the number of hours elapsed since fertilization.
Morphological features of the embryos in our experiments at a given
time stage were, in general, consistent with the zebrafish standard
staging table (Kimmel et al., 1995). Because repeated anesthetizations
are suggested to retard development (Kimmel et al., 1995), each embryo
was examined only once for most of the experiments. To reduce
pigmentation, embryos were transferred to fish water containing 0.002%
of phenylthiourea (PTU; Nakarai) between 12 and 22 hr (Burrill and
Easter, 1994). The concentration of PTU was reduced to 0.001% at 48 hr, to 0.0003% at 72 hr, and to 0.0001% at 96 hr. At this
concentration of PTU, no abnormality in development was observed.
Fluorescent microscopic observations. Initial examination
was performed using an epifluorescence dissecting microscope with a GFP
plus filter (Leica, Nussloch, Germany). A PlanApo 1.6× objective lens
was used. For detailed examination, fluorescent embryos were anesthetized using 0.01% ethyl-m-aminobenzoate
methanesulphonate (Sigma, St. Louis, MO) and mounted in 1.2%
agar (Difco, Detroit, MI) on a depression slide glass, as described in
Westerfield (1995). Embryos were either examined under a Zeiss
(Oberkochen, Germany) upright epifluorescence microscope with an FITC
or a GFP (Chroma 41015) filter cassette or under a Zeiss 510 confocal
microscope (510-CLSM, upright) with 488 nm excitation and a 505-550 nm
bandpass filter. Most observations, except for those of
rhodamine-phalloidin or antibody-labeled samples, were performed using
live material because visibility was best in living fish. A
Plan-Neofluar 20× [numerical aperture (NA) 0.5] objective lens was
used for most observations. For higher magnifications, water-immersion
lenses, Achroplan 63× (NA 0.9) and 100× (NA 1.0), were used. For
three-dimensional (3-D) reconstruction of the images, serial optical
sections at ~4 µm intervals (20× objective) or 0.5-1.5-µm
intervals (63 and 100× objective) were taken, and 3-D images were
reconstructed from the stacked confocal images by the software supplied
with the 510-CLSM.
For DiI-, Cy3- and rhodamine-labeled samples, observations were
performed using the 510-CLSM with 568 nm excitation and a 585 longpass
filter. For 2-p-dimethylaminostyrylpyridylethyl iodide (DASPEI)-labeled samples, 488 nm excitation and a 585 longpass filter were used. A DASPEI signal was also apparent during the collection of images for GFP (505-550 nm bandpass). For 3-D
reconstruction of images for signals from GFP and other dyes, serial
optical sections were obtained either simultaneously or sequentially. Each image was pseudocolored (GFP, green; others, red) and compiled.
Mosaic analysis. Cells derived from the homozygous Isl1-GFP
embryos were transplanted into wild-type hosts at the sphere stage as
in Westerfield (1995). Donor cells were transplanted near the animal
pole of host embryos to increase the chance that progeny of donor cells
would be distributed in the cranial region of the host embryo. Mosaic
embryos and larvae were examined between 48 and 90 hr.
Retrograde labeling of the trigeminal motor neurons. Larvae
were anesthetized at ~72-90 hr and embedded in 1.2% agar on a glass
slide in an orientation that allowed access to the nerve to be labeled.
The agar overlying the injection site was removed. The fluorescent
lipophilic dye DiI (Molecular Probes, Eugene, OR), at 2 mg/ml in
ethanol was pressure-injected (Eppendorf Transjector 5246) into a
region around a labeled nerve under an epifluorescent dissection
microscope with the longpass GFP filter (see above). Fluorescence
signals derived from both GFP (green) and DiI (orange) were
simultaneously observed under this condition. The injected larvae were
allowed to develop at room temperature for 4 hr so that the DiI would
retrogradely label the hindbrain neurons. DiI injection was also
performed in fixed embryos. In this case, the injected embryos were
incubated in 4% paraformaldehyde in PBS at room temperature for 12 hr.
In situ hybridization, antibody staining,
rhodamine-phalloidin staining, and DASPEI live staining. In
situ hybridization and antibody staining were performed according
to standard methods (Westerfield, 1995). Isl1 cDNA (Inoue et
al., 1994), zn5 antibody (Trevarrow et al., 1990), and Cy3-conjugated
anti-mouse antibody (Jackson ImmunoResearch, West Grove, PA) were used.
For rhodamine-phalloidin staining, larvae were fixed and treated in
acetone as described previously (Westerfield, 1995). The larvae were
washed in PBS containing 1% dimethylsulfoxide and 0.2% Triton-X 100, and incubated in 0.0002 U/ml rhodamine-phalloidin (Molecular Probes)
in the same solution for 1 hr at room temperature with shaking. They were observed after washing. For DASPEI staining, larvae were immersed
in 0.1 mM DASPEI (Molecular Probes) in E3 (in
mM: 5 NaCl, 0.17 KCl, 0.33 CaCl2, and 0.33 MgSO4) for
20 min, as in Balak et al. (1990) and Whitfield et al. (1996), and
observed after rinsing.
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RESULTS |
Identification of the Isl1 promoter/enhancer region and
generation of transgenic zebrafish
The Isl1 gene and its protein product have been used as
early markers for motor neurons in vertebrates. However, the
promoter/enhancer region that directs gene expression in motor neurons
has not yet been identified in any vertebrate species. To isolate the
promoter/enhancer of the Isl1 gene that is sufficient for
expression in zebrafish motor neurons, ~100 kb genomic sequences
flanking the Isl1 gene were isolated by screening both phage and BAC zebrafish genomic libraries (Fig. 1A).
The structure of the 5' region of the Isl1 gene is shown in
Figure 1B. The core plasmid, ICP-GFP, was generated by fusing 4.1 kb of the Isl1 promoter, ICP, to the gene
encoding a modified GFP (Fig. 1C). When the ICP-GFP DNA was
injected into embryos, GFP was expressed by hatching gland cells (data
not shown) whose precursors normally expresses the Isl1 gene
(Inoue et al., 1994), but not by motor neurons. This suggests that ICP
includes enhancer elements that regulate hatching gland expression of
the Isl1 gene.
To identify enhancer elements that control expression in motor neurons,
a series of constructs were generated by introducing genomic
EcoRI fragments into the ICP-GFP plasmid (Fig.
1C). All recognizable EcoRI fragments in the
cloned region (Fig. 1A) were tested for their
enhancer activity by injecting each construct into embryos. In the
injected embryos, GFP expression was frequently observed in the
hatching gland cells presumably because of the core promoter (ICP)
activity that was common to all the constructs (Fig.
2A, arrowhead). Thus,
hatching gland expression of GFP served as a positive control for the
injections. At least 50 surviving embryos were examined for each
construct. One construct, CMICP-GFP (Fig. 1D), which
carries a 15 kb EcoRI fragment (Fig. 1A,
CM), was found to drive GFP expression in branchiomotor
neurons innervating the pharyngeal arches in injected embryos (Fig.
2A, arrows). Additionally, we identified another
enhancer fragment (Fig. 1A, SS) that was capable of
driving GFP expression in the trigeminal ganglion cells and
Rohon-Beard cells in the spinal cord (Fig. 2B).
Isl1 is normally expressed by both of these cell types as
well as the motor neurons and the hatching gland (Inoue et al., 1994).
All of the other EcoRI fragments were negative: we carefully
looked for GFP expression in primary motor neurons in the spinal cord,
but expression was not detected in these cells that normally
express Isl1. Furthermore, Isl1 is
expressed in many other cells such as those in the epiphysis and the
nucleus of the posterior commissure, but no constructs gave GFP
expression in these cells. It should be noted that because transgenes
are mosaically expressed in the injected embryos, our negative results
should not be construed as conclusive.
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Figure 2.
Zebrafish Isl1
promoter/enhancer activity in transient expression assays.
A, GFP expression in the head of a 40 hr embryo injected
with the CMICP-GFP plasmid. The arrows indicate GFP
expression in branchial motor nerves. The arrowhead
indicates GFP expression in the hatching gland cells. Anterior is to
the left, dorsal is up. B,
A lateral view of GFP expression in a Rohon-Beard cell in the spinal
cord of a 36 hr embryo injected with the SSICP-GFP plasmid. Scale bar:
A, 200 µm; B, 230 µm.
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To establish stable transgenic zebrafish, CMICP-GFP-injected embryos
were raised to sexual maturity, and either incrossed with each other or
outcrossed with noninjected adult fish to generate F1 progeny. Of 113 fish, three produced embryos expressing GFP in a subset of
Isl1-expressing cells, including the cranial motor neurons
(Fig. 3A,B). The expression
patterns of GFP in embryos derived from the three founder fish were
identical, although expression levels varied. The line with the highest
GFP expression, referred to as Isl1-GFP hereafter, was chosen for
further analysis. In this study, we focused on GFP expression patterns
of the Isl1-GFP line in the cranial region. As predicted by the
transient expression analysis, GFP was also expressed in the hatching
gland cells (Fig. 3A, arrow). Additionally, some secondary
motor neurons in the spinal cord and a small number of interneurons in
the CNS also expressed GFP (data not shown).
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Figure 3.
GFP expression in cranial motor neurons in the
Isl1-GFP line. A, Lateral view of the head region of a
34 hr embryo. The arrow indicates GFP expression in the
hatching gland cells. B, Dorsal view of the midbrain and
the hindbrain of a 42 hr embryo. In A and
B, pictures were taken under a conventional
epifluorescence microscope. C-G, Close-up views of the
GFP-positive nerve endings and neurons in the Isl1-GFP line using a
confocal microscope. In panels C-F, composite pictures
were generated from the stacked confocal images. C,
Lateral view of the distal tips of the trigeminal motor axons at 30 hr.
Note the fine filopodial structures extending from the distal ends of
the axons. D, Lateral view of the neuromuscular junction
in the levator arcus palatini (lap) muscle at 96 hr. Note the fine
arborization of the nerve branches innervating individual muscle
fibers. E, F, GFP expression in the efferent component
of the lateral line nerves in a 96 hr embryo. Close-up view of their
endings at the neuromasts. The position of the neuromast corresponds to
h in Figure 7C. In F, the
larva was treated with the vital dye DASPEI, which stains hair cells.
DASPEI signals appear as orange. Note that the nerve endings
appear to terminate within the hair cells. G, A confocal
optical section showing the trigeminal motor neurons at 105 hr. Dorsal
view with medial to the top. A cluster of neurons situated on the
right correspond to those in the posterior (Vp) cluster
of the trigeminal motor neurons (Figs. 5-7). Note that individual
GFP-positive neurons are readily visualized. In all figures, anterior
is to the left. In lateral views, dorsal is
up. Scale bar: A, 110 µm;
B, 60 µm; C-F, 20 µm;
G, 10 µm.
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The Isl1-GFP line enables clear visualization of cranial
motor neurons
To examine how faithfully GFP expression reflects the expression
of the intrinsic Isl1 mRNA in the Isl1-GFP line, we compared the distribution of GFP mRNA and Isl1 mRNA.
GFP mRNA (Fig.
4A,C,E) is expressed in a majority of cranial motor neurons in a similar manner
to Isl1 mRNA (Fig. 4B,D,F). Outside
the CNS, GFP mRNA is also expressed in all the branchiomeric
sensory ganglion cells except for the trigeminal (V) ganglion cells
(Fig. 4E, fs, gs, vs). Branchiomeric
nerves (V, VII, IX, and X) are nerves innervating derivatives of the
pharyngeal arches and are known to include both motor and sensory
components. Besides, GFP is also expressed in the efferent neurons for
the lateral line and vestibuloacoustic nerves, as described in more
detail later.
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Figure 4.
Comparison of the expression patterns of
Islet-1 (Isl1) and GFP
mRNAs in the cranial motor and sensory neurons. A,
C, E, GFP mRNA expression
in embryos from the Isl1-GFP line. B, D,
F, Isl1 mRNA expression in wild-type
embryos. A, B, Dorsal views of 28 hr embryos.
GFP and Isl1 mRNAs are both expressed in
presumptive cranial motor neurons. Whereas Isl1 mRNA is
expressed in the trigeminal ganglion cells (tg),
GFP mRNA is not expressed in these cells. C,
D, Dorsal views of 40 hr embryos. Isl1 mRNA
expression in the nIII and nIV neurons is difficult to see because many
other neighboring cells also express Isl1 mRNA
(D, asterisk). Arrows in D
indicate cells that do not express GFP mRNA in the
Isl1-GFP line. The nVI and nIX neurons do not express GFP in the
Isl1-GFP zebrafish (see the following figures). E, F,
Lateral views of 40 hr embryos. GFP is expressed in cells in the facial
sensory ganglion (fs), glossopharyngeal sensory
ganglion (gs), and vagus sensory ganglions
(vs), but is not expressed in cells in the trigeminal
sensory ganglion (tg). Scale bar, 100 µm.
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We examined GFP expression in live zebrafish most often with a confocal
microscope (see Materials and Methods). After obtaining a series of
optical sections, composite pictures were generated from the stacked
images. The expression levels of GFP were high enough to visualize both
fine neuronal processes during development such as filopodia (Fig.
3C) and fine terminal arbors of the motor axons (Fig.
3D), suggesting that neuronal processes were visualizable in
their entirety in the Isl1-GFP line.
The expression of Isl1 in motor neurons begins early in
their development. Likewise, GFP expression was detected early in cranial motor/efferent neurons (Fig.
5A, see GFP expression in a 21 hr embryo). The transparent nature of zebrafish embryos and larvae
enabled visualization of GFP-labeled neurons and their processes at
high resolution in living animals. This was expected at early stages
such as 24 hr because the early hindbrain is relatively simple
(Chandrasekhar et al., 1997), but was also the case at much later
stages, such as day 4 when the hindbrain is much larger and much more
complex, and the larvae begin complex behaviors such as swimming. An
example is shown in Figure 3G (an optical section) in which
individual neurons in the trigeminal motor nucleus, which lie deep in
the hindbrain, were visualized even in a 4 d, live larva. Thus, it
is possible to observe development of the cranial motor neurons in
intact animals with a high level of resolution from early stages to
relatively mature stages in the Isl1-GFP line.
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Figure 5.
GFP expression early in the development of
the cranial motor neurons (21-36 hr) in the Isl1-GFP line. All
micrographs are confocal composite images generated from a series of
optical sections. E and F are
stereographic images. A, Dorsal view of a 21 hr embryo.
The arrow indicates the nVII/OLe axons. At this stage
most of the GFP-positive nVII/OLe neurons are located in r4 and r5.
Rhombomere boundaries were estimated by designating the hindbrain
region spanning the central half of the otocyst (oto) as
r5, and those spanning the anterior and posterior quarters of the
otocyst as parts of r4 and r6, respectively. B, Dorsal
view of a 24 hr embryo. The pioneering axons from the nVII/OLe neurons
are seen outside the hindbrain (arrow).
C, Dorsal view of a 26 hr embryo. *Longitudinal
processes that connect the nIII, nV, and nVII motor nuclei are visible
(for example, a and b). *The significance
of these early-forming axons is unknown. The majority of the nVII/OLe
axons exit from the hindbrain (c).
f indicates anteriorly projecting axons that
subsequently extend into the lateral line system (corresponding to
l in E). D, Dorsal view of
a 28 hr embryo. g indicates axons from the nIII neurons.
h indicates the peripherally extending axons from the Va
cluster of the nV neurons. d in C and
i in D indicate efferent axons extending
into the posterior lateral line. *Efferent axons for the posterior
lateral line also exit from the hindbrain via a posteriorly located
exit point (e in C and j
in D; Metcalfe et al., 1985). *Arrowheads
in A-D indicate GFP-positive cells located anteriorly
to the main nV cluster. *It is not clear whether these cells constitute
a part of the nV neurons. E, Lateral view of a 28 hr
embryo. k indicates the peripherally extending axons
from the nV neurons. l indicates diverging axons
extending into the lateral line system, whereas m
indicates the main nVII/OLe axons (mostly, the facial motor axons). It
should be noted that, viewed laterally, the efferent axons for the
posterior lateral line appear interrupted by the otocyst because of the
opaque nature of the otolith (also in Figs. 5F,
6B,E, 7C).
F, Lateral view of a 36 hr embryo. n
indicates dorsally extending axons from the nIV neurons.
o and p indicate the peripherally
extending axons from the nV and nVII/OLe neurons, respectively.
G, Dorsal view of a 36 hr embryo. The thick
arrow indicates axons from the Vp cluster of the nV neurons.
*Contralaterally projecting neurites from the nVII/OLe neurons are
visible (asterisk). H, A confocal
composite image of a 36 hr embryo in which hindbrain commissural axons
that are located at the rhombomere boundary are labeled with the zn5
antibody. Dorsal view. Numbers listed are rhombomere
numbers. Green is the GFP signal, whereas
red is the zn5 signal. VII and
VII', VII/OLe complex; oto, otocyst;
Va, Vp, anterior and posterior clusters of nV neurons,
respectively; fs, facial sensory ganglion;
pL, posterior lateral line; soL,
supraorbital lateral line; ioL, infraorbital lateral
line; gs, glossopharyngeal sensory ganglion;
hg, hatching gland. The sentences denoted by an
asterisk in this and all other legends describe
observations not detailed in Results. In lateral views, dorsal
is to the top. Scale bar, A-G,
100 µm; H, 50 µm.
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Overall development of the trigeminal motor (nV) neurons
Although axonal outgrowth by the nV neurons in zebrafish has been
examined by a variety of methods, including retrograde labeling or
immunohistochemistry (Hatta et al., 1990; Chandrasekhar et al., 1997;
Schilling and Kimmel, 1997), their overall development is still largely
obscure because of the limitation of these methods. Given below is a
description of the overall development of the nV neurons as gleaned
from observations of the Isl1-GFP line. Some of the figures (Figs.
5-7)
present micrographs in stereographic pairs.
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Figure 6.
GFP expression in the Isl1-GFP line on
days 2 and 3 of development. All panels except C are
confocal stereographic images. A, Dorsal view of a 48 hr
embryo. The asterisk indicates medially located nV
neurons that are presumably born later than laterally located nV
neurons. B, Lateral view of a 48 hr embryo.
C, Schematic illustration of GFP-labeled nerves in
B. ipsi and contra
indicate fourth nerves from the nIV neurons on the ipsilateral and the
contralateral sides, respectively. a and
b indicate the peripherally projecting axons from the
facial sensory ganglion cells. The axons of a take an
internal pathway, whereas those of b take an external
pathway. The axons indicated by a and b,
respectively, correspond to those indicated by in and
ex in Figure 9A-C. Thin arrows show
GFP-expressing cells that presumably do not correspond to motor
neurons. The thick arrow indicates an OLe nerve branch
extending into the hair cells in the otocyst. The
asterisk indicates branching processes of the OLe
nerves, which are added later to the major branches. The
arrowhead indicates the distal tip of the fifth motor
axons. D, Ventral view of a 62 hr embryo.
E, Lateral view of a 72 hr larva. The embryo in
D and the larva in E were treated with
the vital dye DASPEI, which stains hair cells in lateral line
neuromasts. DASPEI signals appear as yellow.
I, D, and P indicate the
intermediate, distal, and proximal branches of the fifth motor nerve,
respectively. Arrows in D and
E indicate peripherally projecting axons from the facial
sensory ganglion cells (equivalent to a and
b in C). Among them, in
indicates the axons that are distal tip of the axons indicated as
a in C. They take an internal pathway.
Most part of their tract is out-of-focus. The arrowhead
indicates the junction of the four motor nerves (both sides of the
fifth and seventh motor nerves). c and d
indicate nerve branches that innervate the intermandibularis anterior
and posterior (ima and imp), and the
hyohyal (hh), respectively (Fig. 7E).
e indicates the neuromuscular junction at the levator
arcus palatini (lap), whereas f indicates
the neuromuscular junctions at the abductor hyomandibulae
(ah) and the abductor operculi (ao) (Fig.
7D). g indicates distal branches of OLe
nerves from the main nVII/OLe nerve. Asterisks indicate
nerve endings of the OLe system in the ear (Fig. 7C).
*cn is likely to be the ciliary nerve innervating the
lens muscle for visual accommodation. *The lens muscle in teleost was
shown to be controlled by the postganglionic fibers of the oculomotor
(parasympathetic) nerve (Somiya, 1987), and thus, GFP should be
expressed in the parasympathetic ganglion cells corresponding to the
ciliary nerve. a-fs, centrally projecting afferent
facial sensory axons; pL, posterior lateral line;
vs, vagus sensory ganglion. Scale bar, 100 µm.
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Figure 7.
GFP expression in the Isl1-GFP line on
days 3 and 4 of development. All figures are stereographic pictures
reconstructed from the stacked confocal images. A,
Dorsal view of a 72 hr larva. B, Dorsal view of a 96 hr
larva. GFP is also expressed in cells other than motor neurons in the
brain. The identities of these cells are not known. They are a cluster
of cells in the telencephalon (b) and a cluster
of cells in the mesencephalic region (d). Tracts
are formed between these two clusters (c). The
cluster of the mesencephalic region (d) also
sends processes posteriorly (e). a
in A corresponds to d in
B. For these cells and tracts, see also the legend to
Figure 9E. C, Lateral view of a 96 hr
larva. Five terminal-like structures are observed in the ear. These
appear to correspond to the anterior macula (ma)
accompanied by the anterior otolith (the anteriorly located triangle),
the medial macula (mm) accompanied by the posterior
otolith (the posteriorly located triangle), and the three crista
ampullarises (asterisks) associated with the anterior,
lateral, and posterior canals. Nomenclatures are according to Whitfield
et al. (1996). f indicates the largest vagus sensory
ganglion, which is likely to include neurons innervating visceral
organs. g indicates the vagus nerve extending into the
visceral organs. The nerve is likely to contain sensory components and
visceral motor (parasympathetic) components. h indicates
the endings of the OLe nerve at a lateral line neuromast. Higher
magnification views of the corresponding structures are shown in Figure
3, E and F. In B and
C, elaborated fine branches are visible at neuromuscular
junctions (for example, so and sr in
B, lap in C). D,
E, Fixed larvae were treated with rhodamine-phalloidin to
reveal actin filaments of muscles. Green is the GFP
signal, whereas red is the rhodamine-phalloidin signal.
D, Lateral view of a 96 hr larva. E,
Ventral view of a 105 hr larva. P, I, and
D in C-E indicate the proximal,
intermediate, and distal branches of the fifth motor nerve,
respectively. The proximal branch of the fifth nerve innervates the
lap and do muscles, the intermediate
branch innervates the am muscle, and the distal branch
innervates the ima and imp muscles. The
configuration is schematically summarized in Figure 8A.
Arrows indicate peripherally projecting axons from the facial
sensory ganglion cells. *The seventh motor nerves innervate surfacial
membranous muscles (indicated as m-m), which presumably
corresponds to the platysma in higher vertebrates. The
arrowhead indicates the junction of the four motor
nerves (both sides of the fifth and seventh motor nerves).
Abbreviations for muscles (so, sr,
io, ir, lap,
do, am, ima,
imp, ah, ao,
ih, and hh) are shown in Table 1.
*cn is likely to be the ciliary nerve (Fig.
6E, legend). Scale bar, 100 µm.
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GFP is expressed in the nV neurons, but not in the trigeminal sensory
ganglion cells (Isl1 is expressed in both; compare Fig. 4A,C,E with
B,D,F).
Thus, all the GFP-labeled axons in cranial nerve V are motor axons.
GFP-positive nV neurons are evident as early as 21 hr (Fig.
5A) and progressively increase in number with further
development (Fig. 5A-C). Thus, GFP is expressed early enough so that the entire time course of axonal outgrowth by the nV
neurons could be observed. By 28 hr, the motor axons derived from the
nV neurons (Fig. 5D, Va) have extended laterally to exit from the hindbrain into the periphery (Fig. 5D, h, E, k). At
about the same time, an additional more posterior cluster of nV neurons begins to express GFP (Fig. 5D, Vp). GFP-positive neurons in
the Vp cluster increase in number as development proceeds. At ~36 hr,
their axons (Fig. 5G, thick arrow) have extended laterally and then anteriorly to merge with the axons from the Va cluster. Our
observations showed that, throughout development, the Va and Vp
clusters lie discretely apart, and that their axons follow their own
pathways within the hindbrain until joining together at a common
hindbrain exit point (Figs. 5F,G,
6A-C,E, 7A,
8C,F,I).
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Figure 8.
Position of the trigeminal motor (nV)
neurons with respect to the peripheral nerve branches.
A, A diagram showing dye application sites and a summary
of the results. Trigeminal motor neurons were retrogradely labeled with
DiI. DiI application was performed at positions 1-5.
The results showed that Va solely consists of neurons projecting to the
intermediate branch (asterisk), whereas Vp consists of
neurons projecting to the either proximal (circle) or
distal branch (square). Abbreviations for the muscles
are the same as those shown in Table 1. In B-J, all
pictures are dorsal views (composite pictures made from stacked
confocal images) of larvae at ~90 hr with anterior to the
left and medial to the top.
B-D, DiI was applied at position 1.
Neurons belonging to the posterior cluster (Vp) of the
nV neurons were labeled with DiI. E-G, DiI was applied
at position 3. Neurons belonging to the anterior cluster
(Va) were labeled with DiI. H-J, DiI was applied at
position 4. Neurons belonging to the posterior cluster
(Vp) were labeled. Scale bar, 20 µm.
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We examined the locations of the Va and Vp clusters with respect to the
hindbrain rhombomeres using zn5 antibody, which labels hindbrain
commissural axons that are located at the rhombomere boundaries
(Trevarrow et al., 1990). Figure 5H shows that the Va and Vp
lie in r2 and r3, respectively. The hindbrain exit point of the fifth
motor nerve lies in r2 (Fig. 5G). The locations and distributions of the nV neurons are, in general, consistent with those
revealed by retrograde labeling with DiI (Chandrasekhar et al., 1997).
However, the number of neurons that are labeled at a given stage is
much larger in our analysis. Presumably, this is attributable to the
fact that DiI backlabeling from the target pharyngeal arch only labels
those neurons whose axons have reached the arch and that backlabeling
may be incomplete, whereas in the Isl1-GFP line, all the motor neurons,
even though they have not reached their targets, are labeled.
Furthermore, we found that cells in a medial position were labeled in
our Isl1-GFP line (Fig. 6A, asterisk), whereas at
similar stages backlabeling with DiI only labeled cells in a lateral
position (Chandrasekhar et al., 1997). Thus, it could be that the
earliest nV neurons are born medially and migrate laterally. This is
consistent with the possibility that nV neurons are arranged medial to
lateral within the hindbrain according to the time they are born and
differentiate with early ones laterally and later ones more medially. A
similar pattern of development of trigeminal motor neurons has also
been described in the chick embryo (Heaton and Moody, 1980; Simon et
al., 1994).
Once outside of the hindbrain, axons of the nV neurons extend ventrally
along the posterior edge of the eye (Fig. 5F, o), and by 48 hr the axons turn posteriorly (Fig. 6C, arrowhead). At 62 and 72 hr, nerve branches innervating the mandibular arch muscles are
clearly visible (I, D in Fig. 6D;
P in Fig. 6E). Among them, the distal branch of the
fifth nerve (D in Fig. 6D) runs in the
posteromedial direction to the midline, where it merges with both the
contralateral fifth nerve and the distal tip of the seventh (facial)
nerve (Figs. 6D, 7E,
arrowhead). As the zebrafish developed, the labeled fifth axons
progressively shifted anteriorly because of extension of the jaw
(compare Fig. 6D with 7E).
Correspondence between peripheral branches of the fifth nerve and
target muscles was determined by labeling of fixed sample with
rhodamine-phalloidin to show the configuration of the motor nerves and
their target mandibular muscles (Fig.
7D,E; see Table 1 for summary of the nomenclature of the
mandibular arch muscles and the extraocular muscles, the abbreviated
forms of their names, and their innervation patterns). The proximal
branch of the fifth nerve (P in Figs. 6E,
7C,D) innervates the levator arcus palatini (lap) and dilator operculi (do) muscles. The
intermediate branch (I in Figs. 6D,
7E) innervates the abductor mandibulae (am)
muscle. Finally, the distal branch (D in Figs.
6D, 7E) innervates the intermandibularis
anterior and posterior (ima and imp) muscles. This configuration is schematically shown in Figure
8A.
Trigeminal motor axons from different rhombomeres innervate
distinct target muscles
Because the trigeminal motor neurons innervate several different
muscles and they are organized into two clusters, Va in r2 and Vp in
r3, we wondered whether the two clusters of trigeminal motor neurons
innervated different target muscles. To examine this question, we took
advantage of the fact that nV nerve and branches are readily visible in
the Isl1-GFP line. We selectively backlabeled those motor neurons that
supply axons to a specific nerve branch by application of DiI to that
branch. In the periphery, there are three major branches, and DiI was
applied at five different positions along the branches in 72-90 hr
larvae (Fig. 8A, 1-5). DiI application at position
1, which contains axons innervating the lap and
do muscles, labeled Vp neurons (Fig.
8B-D; n = 5). DiI application at
position 2, which contains axons innervating the
am, ima, and imp muscles, labeled Va
and Vp neurons (data not shown; n = 2). Application of
DiI at position 3, which contains axons innervating the
am muscle, labeled Va neurons (Fig. 8E-G; n = 6). Finally, DiI application at position
4 or 5, which contains axons innervating the
ima and imp muscles, labeled Vp neurons (Fig.
8H-J; n = 7 for 4 and
n = 4 for 5). These results indicate that
the Va neurons exclusively innervate the am muscle, whereas the Vp neurons innervate the lap, do,
ima, and imp muscles. Thus, the two clusters of
trigeminal motor neurons innervate distinct target muscles, and this
can be seen at early larval stages. These results confirm the pattern
of innervation found in adult fish (Song and Boord, 1993). Because Va
and Vp are located in different rhombomeres and appear not to
intermingle during development, our results are consistent with the
notion that nV neurons born in r2 and r3 adopt distinct fates, and this
suggests that the segment of origin determines the identity of the nV neurons.
Characterization of GFP-positive cranial nerves other than the
trigeminal nerve
Below we describe the GFP-positive cranial motor and sensory
neurons because many of them have not yet been fully characterized in
developing zebrafish. To keep the text concise, some minor observations
are described only in the figure legends (Figs. 5-7, see the comments
denoted by asterisks). Some of our findings overlap with previously
reported results (Chandrasekhar et al., 1997).
Facial (VII) and octavolateralis efferent (OLe) nerves
In addition to motor neurons, GFP is expressed in the efferent
neurons for the lateral line and the vestibuloacoustic nerves. The
lateral line, which is unique to aquatic vertebrates, is a sensory
system mainly responsible for detection of water displacement (Coombs
et al., 1989). The lateral line nerve as well as the vestibulo-acoustic nerve terminates at hair cells that are innervated by both sensory and
efferent (octavolateralis efferent, OLe) nerves (Roberts and Meredith,
1989; 1992; Highstein, 1991). The facial motor (nVII) and OLe neurons
are located in close proximity, and the efferent axons from both cell
types extend together in the hindbrain. Therefore, we have combined the
description of axonal outgrowth by both sets of efferent neurons.
GFP-positive nVII/OLe neurons (Fig. 5A, VII) and
their axons (Fig. 5A, arrow) are evident by 21 hr. At ~24
hr, the pioneering axons among the nVII/OLe axons exit from the
hindbrain (Fig. 5B, arrow), and by 26 hr, most of the
nVII/OLe axons have left the hindbrain (Fig. 5C, c). The
thick, main bundle of nVII/OLe axons (Fig. 5E, m) grows
toward the facial ganglion (Fig. 5E, fs), which becomes
discernible at ~27-28 hr. By the facial ganglion, the main bundle
grows ventrally (Fig. 5F, p). At 48 hr, the main bundle (Fig. 6A-C, purple) is mainly composed of
the facial motor axons (see below for the sensory and OLe fibers).
Projection of motor nerves to target muscles was confirmed by labeling
muscles with rhodamine-phalloidin at later stages (Fig.
7D,E). The labeled seventh motor
nerve innervates the ah, ao, ih, and
hh muscles (see Table 1 for abbreviations for the names of
the muscles).
The nVII/OLe motor neurons appear to migrate caudally during
development. At early stages (21 hr), most of the nVII/OLe neurons are
localized in r4 and r5, as judged by comparison with the location of
the otocyst (Fig. 5A, see its legend for assignment of
rhombomere). In the next 15 hr, the nVII motor neurons were seen to
migrate caudally such that by 36 hr most of the motor neurons (Fig.
5H, VII, VII') were located in r6 with some in
r7. Our findings confirm the hypothesis that the nVII/OLe motor neurons
migrate caudally, as first suggested by Chandrasekhar et al. (1997)
based on a caudal shift of cells expressing the Isl1 protein and
tag1 mRNA (cranial motor neuron markers) from r4 and r5 to
r6 and r7. In this earlier study, however, there remained the
possibility that the apparent caudal shift of the
Isl1/tag1-positive cells was not caused by migration of
neurons, but was caused by changes in gene expression by neurons in
these rhombomeres. Because the nVII/OLe neurons (identified by their
axonal trajectories) were seen to shift caudally in Isl1-GFP embryos by
observing them at several different time points, it is clear that these
neurons indeed do migrate caudally.
To get a clearer description of axonal outgrowth by the motor and
sensory components, we made mosaic embryos, by isochronically transplanting cells of the Isl1-GFP line into wild-type embryos at the
sphere stage. In the resultant embryos, GFP was expressed by only a
small number of cranial motor and sensory neurons, making it possible
to unambiguously follow axonal outgrowth in these cells. Interestingly,
observations of facial sensory neurons in mosaic embryos showed that
their centrally projecting axons (a-fs in Figs.
6A,E, 7A,
9A, C,
D; green in Fig. 6C) take a distinct pathway from the outgrowing nVII/OLe motor axons. In amniotes, the
motor/efferent axons and the centrally projecting sensory axons follow
the same pathway. The centrally projecting axons initially extend
dorsoposteriorly, turn medially into the hindbrain, and then
posteriorly within the hindbrain (Figs. 7A, a-fs;
9C,D) to terminate in the dorsoposterior
part of the hindbrain by day 3 (Fig. 9C,D,
arrowheads). The peripherally extending axons of the sensory nVII
neurons diverge into two nerves as they extend in a ventroanterior
direction (Fig. 6C, a, b), but they all
eventually terminate around the mouth (Figs.
6D,E, 7E, arrows;
9A,B). This outgrowth pattern is
consistent with the notion that the facial sensory nerves in
vertebrates mostly convey gustatory information (Fig. 9A-C,
see the legend to for further details on the peripheral trajectories).
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Figure 9.
Mosaic analysis of the Isl1-GFP line.
Mosaic animals were made by isochronically transplanting cells of the
Isl1-GFP line into the normal embryo at the sphere stage to obtain
stochastic labeling of cranial motor and sensory neurons. All images
except for C are taken from larvae at ~75 hr.
C is from a larva at ~90 hr. All figures are composite
pictures made from the stacked confocal images. A,
Lateral (slightly ventral) view of a mosaic larva in which GFP is
expressed in the facial sensory ganglion cells
(fs). B, C, Ventral
(B) and dorsal (C) views of
the same larva shown in A. a-fs shows the
centrally projecting afferent facial sensory axons, which terminate in
the dorsoposterior part of the hindbrain (arrowhead).
The asterisk indicates signals derived from
GFP-expressing cells in the mesencephalic region (Fig. 7A, a; B,
d; see also single and double
asterisks in E). Peripherally extending axons
from the facial sensory ganglion cells take internal
(in) and external (ex) pathways. Axons of
both internal and external pathways terminate near the mouth. The
internal fibers (correspond to a in Fig.
6C) take a deep route, and most of the parts of the
fibers are not visible, partly because they run out of the focal plane,
and partly because of the opaque nature of the eye (lateral view) and
cartilages (ventral view). The external fibers initially take the same
superficial pathway as the seventh motor nerve and then diverge (Fig.
6C, b;
D,E, 7E,
arrows). D, Lateral view of a mosaic larva in
which GFP is expressed in neurons in the facial sensory ganglion
(fs), in the glossopharyngeal sensory ganglion
(gs), and the vagus sensory ganglion
(short arrows). a-fs shows the centrally
projecting afferent facial sensory axons, which terminate in the
dorsoposterior part of the hindbrain (arrowhead). The
long thin arrow indicates the faintly fluorescent
centrally projecting axons from the glossopharyngeal sensory neurons.
Terminals of the centrally projecting axons from the facial,
glossopharyngeal, and vagus ganglion cells are located near one another
in the dorsoposterior part of the hindbrain. The terminal region is
likely to correspond to the nucleus tractus solitarii in the adult
fish. We have examined a number of mosaic embryos in which GFP was
expressed in the facial sensory neurons (n > 15).
In all cases, centrally projecting fibers took the same pathway (Figs.
6A,E, 7A,
a-fs; 6C, green), and peripherally
projecting fibers eventually terminated around the mouth.
E, Dorsal view of a mosaic embryo in which GFP is
expressed in a number of cells other than the motor neurons in the
brain. The double-headed arrow marks the midline. The
double asterisks and the single asterisk
indicate the GFP-positive cells in the mesencephalic region (Fig.
7A, a; B, d). Anteriorly projecting processes from these
cells (probably from the cells marked by the double
asterisk) correspond to the tracts marked by c
in Figure 7B, whereas posteriorly projecting processes
from these cells (probably from the cells marked by the single
asterisk) correspond to the tracts marked by e
in Figure 7B. The posteriorly projecting axons may
terminate around the trigeminal motor nucleus and facial motor nucleus
(arrows). Scale bar, 100 µm.
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Because GFP is not expressed in the sensory neurons related to the
octavolateralis system, all of the GFP-labeled octavolateralis nerves
in the periphery are efferent axons. Thus, it was possible to
systematically follow the axonal outgrowth of the lateral line efferents. As described earlier, the pioneering axons among the nVII/OLe axons exit from the hindbrain at ~24 hr (Fig. 5B,
arrow). In vivo, time-lapse microscopic observations of
these embryos suggested that these pioneering axons correspond to the
OLe axons (data not shown). These axons extend both anteriorly (Fig.
5C, f ) and posteriorly (Fig. 5C, d; D,
i) from the exit point. Posteriorly extending axons are likely to
project to the posterior lateral line (Metcalfe et al., 1985). The
anteriorly extending nerve takes a superficial pathway (Fig. 5E,
l), and subsequently, branches with one branch extending
anteriorly [supraorbital lateral line (soL)] and the other extending
ventrally [infraorbital lateral line (ioL)] (Figs. 5F,
6B,C). Later in development, other
branching processes can also be recognized (Fig. 6C,
asterisks; E, g). Vital staining of hair cells in the
lateral line neuromasts by DASPEI revealed that the OLe axons were
found near the neuromasts as expected (Fig.
6D,E). Their endings spread into
fine branches terminating in the circumference of the individual hair
cells (Fig. 3E,F). Branches
of the OLe nerves were also seen to project to the hair cells in the
otocyst (Fig. 7C, mm, ma, asterisks). Thus, OLe nerves project to hair cells in the lateral line and otocyst
quite early in their development, suggesting that hair cells receive
efferent input from the onset of their function.
Other cranial nerves
Among the motor neurons innervating the extraocular muscles, GFP
is expressed in the oculomotor (nIII) and the trochlear motor (nIV)
neurons, but not in the abducens motor (nVI) neurons. GFP-positive nIII
neurons are visible at 26 hr (Fig. 5C), and subsequently, they extend axons toward the extraocular muscles (Fig. 5D,
g; 6B,C). The projection
pattern of the GFP-labeled axons to target extraocular muscles are
described in Table 1. GFP-positive nIV neurons appear at 30-32 hr
(data not shown). Their axons extend dorsally within the midbrain (Fig.
5F, n), cross the dorsal midline (Fig. 7A) before
they exit the CNS, extend ventrally in the periphery (Fig.
6B,C), and then turn anteriorly
toward their target, the superior oblique (so) muscle (Fig.
7A,B).
In the glossopharyngeal (IX) and vagus (X) cranial systems, GFP is
expressed in the glossophayngeal sensory ganglion cells (Fig.
4E, gs), the vagus motor (nX) neurons, and the vagus
sensory ganglion cells, which form clusters associated with each gill (vs; Figs. 4E, 9D). No GFP expression is
detected in the glossopharyngeal motor (nIX) neurons. By 36 hr,
GFP-expressing cells in the glossopharyngeal ganglion along with their
centrally projecting axons can be observed (Fig. 5F, gs).
Later in development, peripherally extending axons into the first gills
are also observed (Figs. 6B,C,E,
7C, IX ). The nX motor neurons form a large cluster in the
posterior part of the hindbrain (Fig. 4C,E;
Chandrasekhar et al., 1997) and extend thick axon bundles into the
periphery (Fig. 5F). The pathways of the vagus
sensory axons extending in both central and peripheral directions
appear to coincide with the branchial (to gills) and visceral motor
pathways (Fig. 7C; g shows fibers extending into the visceral organs). Thus, the labeled tenth nerves are likely to
include both motor and sensory components. Later in development, GFP is
also expressed in cells other than motor neurons in the brain (Figs.
6C, thin arrows; 7A, a, B, b,
d; 9E, single and double asterisks).
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DISCUSSION |
This study reports the generation of a line of transgenic
zebrafish, the Isl1-GFP fish, that expresses GFP in the cranial motor
neurons, some of the cranial sensory neurons, and several other groups
of cells. The transparency of zebrafish embryos and larvae enabled us
to obtain high-resolution images of cranial motor neurons and their
axonal trajectories in intact animals throughout development.
Observations of the development of the cranial motor and sensory
neurons in the transgenic zebrafish were easy and reproducible. Taking
advantage of these features, we first followed overall development of
the nV neurons. Next, we have examined whether the segmental origin of
the nV neurons correlates with target selection. Additionally, we
characterized several other groups of GFP-positive neurons. The
generation of this transgenic line and the description of axonal
outgrowth by the GFP-positive neurons derived from analysis of this
line set the stage for future experimental and genetic examination
of the development of these neurons.
Identification of the promoter/enhancer region of the Isl1 gene and
generation of the transgenic fish
In transient expression assays, we identified two enhancer
elements of the Isl1 gene: one for expression in cranial
motor neurons and the other for expression in Rohon-Beard cells and the trigeminal ganglion cells. Using the former element, we generated a
stable transgenic line. Our strategy in dissecting the enhancer regions
was as follows. First, we prepared a core plasmid that has a minimum
promoter of the Isl1 gene sufficient only for expression in
hatching gland cells. Next, we generated a series of DNA constructs in
which different genomic fragments near the Isl1 gene were
inserted into the core plasmid and examined enhancer activity by
injecting each construct into zebrafish embryos. The ease of transient
expression assays in zebrafish embryos made it feasible to test a
number of DNA constructs. This approach should be generally applicable to the identification of enhancer elements of any gene that controls tissue-specific gene expression and to the subsequent generation of
stable transgenic fish lines.
Segmental origins within the nV neurons define their
target fields
Our analysis of the fifth nerve by branch-specific DiI labeling
revealed that neurons supplying axons into an intermediate branch
(innervating the am) are located in the anterior cluster of the nV, and
neurons supplying axons into proximal (innervating the lap and do) and
distal (innervating the ima and imp) branches are located in the
posterior cluster of the nV. The am, the only muscle innervated by the
anteriorly located neurons, functions as a jaw "closer" acting
antagonistically with the rest of jaw "openers". Thus, the closer
and opener motor neurons are located in different rhombomeres.
The organization of the trigeminal motor neurons in the CNS with
respect to the peripheral nerve branches has been examined in many
adult vertebrates (for references, see Song and Boord, 1993). These
studies suggested that, despite the wide range of morphological
differences, the organization of the trigeminal system is conserved
among vertebrates. All vertebrates examined so far contain equivalent
proximal, intermediate, and distal branches of nV, with motor neurons
that project into the intermediate branch located as a discrete cluster
at the anterior part of the trigeminal nucleus. Our results support
such previous observations and reveal that the stereotyped connections
between subpopulations of the trigeminal motor neurons and the opener
and closer muscles are established early in development. Because
GFP-positive clusters of trigeminal neurons, from the beginning, start
out as discrete clusters in r2 and r3, it is likely that the neurons of
the anterior and posterior clusters are born in r2 and r3,
respectively. Thus, the differences between the two clusters of
trigeminal motor neurons can be attributed to the segmental origin of
the motor neurons; i.e., neurons born in r2 and r3 will eventually
project to distinct target muscles of different physiological
functions. It is possible that the anterior cluster (r2) and the
posterior cluster (r3) are distinct in nature at birth, presumably
under the control of the regulatory genes expressed in a
rhombomere-specific manner (Lumsden and Krumlauf, 1996). Conservation
of both the adult trigeminal pattern (Song and Boord, 1993) and
hindbrain segmentation processes during development among vertebrates
(Gilland and Baker, 1993; Lumsden and Krumlauf, 1996) suggests that
this idea applies to other vertebrates, including chick and mouse.
Potential use of the Isl1-GFP line for neurobiology
The Isl1-GFP zebrafish will be useful for several types of
studies. For instance, it could be used to analyze the function of
genes regulating motor neuron development. By injecting DNA constructs,
such as dominant negative alleles of genes normally expressed by the
cranial motor neurons into Isl1-GFP embryos, one could potentially
examine loss of function effects on outgrowth and pathfinding by the
motor axons. Live visualization of motor neurons and their axons would
allow for a dynamic analysis of the effects of such molecular
manipulations on pathfinding by growth cones. The ability to assay
effects dynamically would increase the detectability of phenotypes
because the effect of some molecular manipulations may be most apparent
and informative in a dynamic analysis. Similarly, the Isl1-GFP line
would be useful for cellular manipulations such as laser ablation
experiments, which could ablate specific groups of trigeminal neurons
or other cell types. Furthermore, the transgenic fish might be also
useful for electrophysiological studies because it would allow
researchers to record the activity of a GFP-labeled neuronal type reproducibly.
Because the zebrafish is genetically manipulable, the Isl1-GFP
zebrafish provides an opportunity for genetic analyses of the development of neurons such as the cranial motor neurons. Recent large-scale mutant screens have identified many mutations that cause
defects in CNS or craniofacial development (Driever et al., 1996;
Haffter et al., 1996). The Isl1-GFP fish will enable further examination of these mutations after introduction of the Isl1-GFP transgene into the mutant background by crossing mutant with Isl1-GFP lines. Our detailed characterization of GFP-labeled motor and sensory
neurons along with their fibers provides an anatomical basis for these
studies. Finally, the Isl1-GFP line can be used as a starting strain
for mutational analysis of GFP-positive neurons. The line affords the
possibility of screening for new mutations that affect hindbrain
segmentation and determination of specific neuronal types. Furthermore,
the fact that axon outgrowth can be so readily assayed in these embryos
should make it possible to screen directly for mutations that affect
outgrowth, pathfinding, and synapse formation by the GFP-positive neurons.
| |
FOOTNOTES |
Received July 14, 1999; revised Oct. 6, 1999; accepted Oct. 14, 1999.
This work was supported by grants from the Japan Science and Technology
Corporation, the Ministry of Education, Science, and Culture of Japan,
and Special Coordination Fund from Science and Technology Agency of
Japan. We especially thank N. Ueno, in whose laboratory the majority of
this study was performed. We thank G. Eguchi and G. Mandel for generous
support. We thank Y. Ishikawa, K. Kawamura, and S. Kuratani for
their suggestions on the anatomy of cranial motor and sensory neurons.
We thank G. Mandel, J. Fetcho, K. Cho, A. Thomson, Y. Ishikawa,
and J. Y. Kuwada for comments on this manuscript. We thank M. Sugiura for assistance with the experiments; K. Takamatsu and Y. Katoh
for maintaining our fish colony; M. Nikaido for instruction in the
technique of mosaic analysis; K. Umesono for the donation of a modified
GFP; M. Petkovich, A. Picker, and H. Takeda for the donation of
zebrafish genomic libraries; and members of the Ueno laboratory for
encouragement and discussion. The zn8 (= zn5) antibody was obtained
from the Developmental Studies Hybridoma Bank maintained by the
Department of Biology at the University of Iowa.
Correspondence should be addressed to Hitoshi Okamoto, Laboratory for
Developmental Gene Regulation, Brain Science Institute, RIKEN (The
Institute of Physical and Chemical Research), 2-1 Hirosawa, Wako,
Saitama 351-0198, Japan. E-mail: hitoshi{at}brain.riken.go.jp.
Dr. Higashijima's present address: Department of Neurobiology and
Behavior, State University of New York at Stony Brook, Stony Brook, NY
11794. E-mail: shigashijima{at}notes.cc.sunysb.edu.
| |
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C. T. Miller, L. Maves, and C. B. Kimmel
moz regulates Hox expression and pharyngeal segmental identity in zebrafish
Development,
May 15, 2004;
131(10):
2443 - 2461.
[Abstract]
[Full Text]
[PDF]
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Y. Murakami, M. Pasqualetti, Y. Takio, S. Hirano, F. M. Rijli, and S. Kuratani
Segmental development of reticulospinal and branchiomotor neurons in lamprey: insights into the evolution of the vertebrate hindbrain
Development,
March 1, 2004;
131(5):
983 - 995.
[Abstract]
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[PDF]
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J. R. Fetcho and S.-i. Higashijima
Optical and Genetic Approaches Toward Understanding Neuronal Circuits in Zebrafish
Integr. Comp. Biol.,
February 1, 2004;
44(1):
57 - 70.
[Abstract]
[Full Text]
[PDF]
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G. Deflorian, N. Tiso, E. Ferretti, D. Meyer, F. Blasi, M. Bortolussi, and F. Argenton
Prep1.1 has essential genetic functions in hindbrain development and cranial neural crest cell differentiation
Development,
February 1, 2004;
131(3):
613 - 627.
[Abstract]
[Full Text]
[PDF]
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S.-i. Higashijima, M. A. Masino, G. Mandel, and J. R. Fetcho
Imaging Neuronal Activity During Zebrafish Behavior With a Genetically Encoded Calcium Indicator
J Neurophysiol,
December 1, 2003;
90(6):
3986 - 3997.
[Abstract]
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A. Tallafuss and L. Bally-Cuif
Tracing of her5 progeny in zebrafish transgenics reveals the dynamics of midbrain-hindbrain neurogenesis and maintenance
Development,
September 15, 2003;
130(18):
4307 - 4323.
[Abstract]
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M. L. McWhorter, U. R. Monani, A. H.M. Burghes, and C. E. Beattie
Knockdown of the survival motor neuron (Smn) protein in zebrafish causes defects in motor axon outgrowth and pathfinding
J. Cell Biol.,
September 1, 2003;
162(5):
919 - 932.
[Abstract]
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[PDF]
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F. Carreira-Barbosa, M. L. Concha, M. Takeuchi, N. Ueno, S. W. Wilson, and M. Tada
Prickle 1 regulates cell movements during gastrulation and neuronal migration in zebrafish
Development,
September 1, 2003;
130(17):
4037 - 4046.
[Abstract]
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S. A. Lee, E. L. Shen, A. Fiser, A. Sali, and S. Guo
The zebrafish forkhead transcription factor Foxi1 specifies epibranchial placode-derived sensory neurons
Development,
June 15, 2003;
130(12):
2669 - 2679.
[Abstract]
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T. Xiao, W. Shoji, W. Zhou, F. Su, and J. Y. Kuwada
Transmembrane Sema4E Guides Branchiomotor Axons to Their Targets in Zebrafish
J. Neurosci.,
May 15, 2003;
23(10):
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[Abstract]
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L. Maves, W. Jackman, and C. B. Kimmel
FGF3 and FGF8 mediate a rhombomere 4 signaling activity in the zebrafish hindbrain
Development,
March 10, 2003;
129(16):
3825 - 3837.
[Abstract]
[Full Text]
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J. M. McClintock, M. A. Kheirbek, and V. E. Prince
Knockdown of duplicated zebrafish hoxb1 genes reveals distinct roles in hindbrain patterning and a novel mechanism of duplicate gene retention
Development,
March 7, 2003;
129(10):
2339 - 2354.
[Abstract]
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K. R. Svoboda, S. Vijayaraghavan, and R. L. Tanguay
Nicotinic Receptors Mediate Changes in Spinal Motoneuron Development and Axonal Pathfinding in Embryonic Zebrafish Exposed to Nicotine
J. Neurosci.,
December 15, 2002;
22(24):
10731 - 10741.
[Abstract]
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F. Ono, A. Shcherbatko, S.-i. Higashijima, G. Mandel, and P. Brehm
The Zebrafish Motility Mutant twitch once Reveals New Roles for Rapsyn in Synaptic Function
J. Neurosci.,
August 1, 2002;
22(15):
6491 - 6498.
[Abstract]
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R. A. Cornell and J. S. Eisen
Delta/Notch signaling promotes formation of zebrafish neural crest by repressing Neurogenin 1 function
Development,
January 6, 2002;
129(11):
2639 - 2648.
[Abstract]
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D. A. Ritter, D. H. Bhatt, and J. R. Fetcho
In Vivo Imaging of Zebrafish Reveals Differences in the Spinal Networks for Escape and Swimming Movements
J. Neurosci.,
November 15, 2001;
21(22):
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[Abstract]
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F. Ono, S.-i. Higashijima, A. Shcherbatko, J. R. Fetcho, and P. Brehm
Paralytic Zebrafish Lacking Acetylcholine Receptors Fail to Localize Rapsyn Clusters to the Synapse
J. Neurosci.,
August 1, 2001;
21(15):
5439 - 5448.
[Abstract]
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J. M. McClintock, R. Carlson, D. M. Mann, and V. E. Prince
Consequences of Hox gene duplication in the vertebrates: an investigation of the zebrafish Hox paralogue group 1 genes
Development,
July 1, 2001;
128(13):
2471 - 2484.
[Abstract]
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[PDF]
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M. Kobayashi, K. Nishikawa, and M. Yamamoto
Hematopoietic regulatory domain of gata1 gene is positively regulated by GATA1 protein in zebrafish embryos
Development,
June 15, 2001;
128(12):
2341 - 2350.
[Abstract]
[Full Text]
[PDF]
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TOP
ABSTRACT
INTRODUCTION
