Departments of Ophthalmology and Physiology, Medical Scientist Training Program, Biomedical Sciences Program, Neuroscience Program, University of California San Francisco, CA94143, USA
* Author for correspondence (e-mail: dws{at}itsa.ucsf.edu)
Accepted 20 November 2002
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SUMMARY |
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Key words: Visual system, Retinal ganglion cell, Pathfinding, Semaphorin, Growth cone, Mouse
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INTRODUCTION |
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While semaphorins are best known for their inhibitory activity during
development, a number of reports have provided evidence for the opposite
function. Studies in grasshopper have shown that transmembrane Sema-1a
functions as an attractive guidance molecule in different regions of the limb
bud (Wong et al., 1999). In
the mammalian cortex, Sema3A has been reported to inhibit cortical axon growth
but attract dendritic growth from the same cell population
(Polleux et al., 2000
).
Similarly, growth cones can switch their response to a given guidance molecule
from attraction to repulsion, and vice versa, depending on signaling from a
second guidance molecule (Hopker et al.,
1999
; Song and Poo,
1999
). In vertebrates, L1, a guidance molecule of the Ig
superfamily, has been reported to switch growth cone response to secreted
Sema3A from inhibition to attraction
(Castellani et al., 2000
). It
is not clear whether a similar type of response switching occurs for
transmembrane semaphorins. If so, axon responses to transmembrane semaphorins
might continually change along a neural pathway as growth cones sequentially
encounter signals from a variety of axon guidance molecules.
Amongst the vertebrate semaphorins, Sema5A and Sema5B have an unusual
pairing of protein domains. The extracellular domain of these two semaphorins
contains seven thrombospondin (TSP) type-1 repeats in addition to the sema
domain (Adams et al., 1996).
Given that thrombospondin type-1 repeats have been reported to promote neurite
outgrowth and neuronal adhesion (Adams and
Tucker, 2000
), the pairing of a typically inhibitory sema domain
with TSP repeats poses an intriguing question as to how class V semaphorin
functions during neuronal development.
In the visual system, the optic nerve consists of the axons of retinal
ganglion cells (RGCs), and conveys retinal information to CNS targets. During
embryonic development, the optic nerve is formed as RGC axons extend from
their cell bodies centrally towards the optic disc, pass through the optic
disc, and travel down the optic stalk towards the brain. Some of the axon
guidance molecules contributing to this process have been identified. These
include L1, which is expressed by retinal axons, and is involved in axon
fasciculation in the retina (Brittis et
al., 1995). L1 is also highly expressed by retinal axons
traversing the optic nerve, chiasm and optic tract, suggesting that a large
number of retinal axon pathfinding tasks operate in the context of L1
signaling. A second retinal axon guidance molecule is netrin 1, which is
expressed by the group of neuroepithelial cells that form a collar surrounding
the optic disc. Netrin 1 is essential for promoting retinal axon growth
through the disc into the optic nerve
(Deiner et al., 1997
). In
approximately the same region, retinal axons are also thought to interact with
laminin 1, which co-operates with netrin 1 to help steer retinal axons into
the optic nerve (Hopker et al.,
1999
). Given that L1, netrin 1 and laminin 1 are all involved in
retinal axon exit at the optic disc leading to optic nerve formation, these
three guidance molecules can potentially modulate how retinal growth cones
respond to other guidance cues in the retinal pathway.
To identify additional guidance molecules mediating optic nerve development, we examined expression patterns of known guidance molecules including semaphorins. Of eight semaphorins studied, we found that Sema5A was specifically expressed at the optic disc, and along the optic nerve, in a pattern suggestive of a role in retinal axon pathfinding. Functional assays revealed that Sema5A consistently triggered an inhibitory response in embryonic retinal growth cones when tested in the presence of signaling from other relevant guidance molecules. Antibody mediated disruption of Sema5A function resulted in retinal axon defasciculation, and axons straying away from the optic nerve. Our results indicated that transmembrane Sema5A acts as a continually present inhibitory sheath, encasing the retinal pathway as RGC axons carry out multiple pathfinding tasks involving different sets of axon guidance molecules.
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MATERIALS AND METHODS |
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Full-length Sema5A cDNA was cloned into the pEX-myc vector, and a stably transfected HEK 293 cell line was isolated. Immunoblots using membrane preparations from transfected cells showed a single band of the expected size (140 kDa) by anti-myc staining, and by staining using an anti-Sema5A antibody (see below).
In situ hybridization
E12-E18 wild-type (C57/B6) mouse embryo brains were fixed in 4%
paraformaldehyde for 60 minutes, and 10 µm cryostat sections cut for in
situ hybridization as previously described
(Birgbauer et al., 2000).
Digoxigenin-labeled sense and antisense RNA probes for mouse Sema3A, 3C, 3E,
Sema4A, 4C, Sema5A, 5B, and Sema6A between 250-400 bases in length were taken
from the 3' end of these genes. An additional Sema5A in situ probe (bp
201-2065) and Sema5B probe (bp 337-2497) were also used. These probes spanned
the Sema-domains and TSP repeats of both molecules.
Embryonic tissue culture
Retinal tissue was obtained from E14 mouse embryos harvested from
anesthetized timed pregnant C57/B6 mice (detection of vaginal plug was counted
as day 0). Laminin (Gibco) was coated onto polylysine covered dishes at 5
µg/ml for collapse assays, and at 2.5 µg/ml for netrin 1-dependent
neurite outgrowth assays (see below). To use L1 as a substratum,
polylysine-covered dishes were coated with anti-human Fc antibody (5 µg/ml;
Jackson Immunochemicals). Anti-human Fc-coated dishes were then blocked with
0.25% BSA, and L1-Fc (5 µg/ml) was applied. All coatings were performed at
37°C for 2 hours. L1-Fc coated dishes were washed with PBS three times and
used for explant cultures. Explants were maintained at 37°C, 5%
CO2 in F12 medium and N2 supplement (F12/N2 medium) (Gibco).
Retina-optic nerve preparations
The retinal eye cup and a length of optic nerve were removed from E14 mouse
embryos. Three quarters of the retina was cut away, leaving a retinal wedge
and the attached optic nerve stump (see
Fig. 4A). Retina-optic nerve
preparations were cultured overnight on L1-coated dishes, and held in place by
a flap of fine wire mesh (#203025-A, Small Parts Inc.) attached to the culture
dish by Sylgard (Dow Chemical).
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Growth cone collapse assays and substratum choice assays
Collapse assays were performed in 8-well coverglass chamberslides (Fisher),
ECD-Fc, Sema-Fc, TSR-Fc or Fc were diluted in F12/N2 medium, and added to
wells containing retinal explants at final concentrations of 2.5 nM-100 nM.
Anti-human Fc antibody (Jackson Immunochemical) was added at 7.5 µg/ml to
multimerize the Fc-tagged recombinant proteins. After exposure to reagents at
37°C in 5% CO2 for 30 minutes, retinal explants were fixed with
4% paraformaldehyde. Growth cones were stained using Texas Red-Phalloidin
(Molecular Probes), and scored for collapsed or expanded morphology.
Substratum choice assays were performed as previously described
(Birgbauer et al., 2001). The
responses of growth cones extending on laminin (5 µg/ml) encountering a
substratum region containing laminin (5 µg/ml) and 20 nM ECD-Fc were
analyzed. Growth cone stops or turning away were considered as positive
responses. A small amount of Cy3-labeled antibody was included along with
ECD-Fc as a fluorescent marker. ECD-Fc was substituted with 20 nM
heat-inactivated ECD-Fc (74°C for 20 minutes) in control experiments. E14
RGC axons show minimal response to Fc protein in substratum choice assays
(Birgbauer et al., 2001
).
Time-lapse microscopy
35 mm coverslip dishes (MakTek) containing retinal explants or retina-nerve
preparations were overlayed with pre-warmed mineral oil (Sigma) and maintained
at 37°C on a microscope stage incubator with CO2 influx.
Time-lapse images of growth cones were captured at 1 minute intervals with a
CCD camera (PXL2, Photometrics) using Hoffman optics and Deltavision image
acquisition software (API). Baseline growth was recorded for 20-45 minutes
before reagent application. Recombinant proteins and anti-Fc antibody were
diluted to a volume of 100 µl, and then added by gel-loading pipette to
cultures underneath the mineral oil to achieve a recombinant protein
concentration of 12.5 nM. Following reagent application, growth cone behavior
was recorded for an additional 45-80 minutes.
Neurite outgrowth assays
Supernatant from netrin 1 expressing HEK 293 cells was concentrated using
centriprep-10 concentrator columns (Amicon). Netrin 1 concentration was
determined by Coomassie Blue staining and comparison with BSA standards. In
netrin 1-dependent outgrowth assays, laminin was used at 2.5 µg/ml
(threshold for reliable outgrowth was 4 µg/ml) and netrin 1 (100 ng/ml) was
added to the culture medium. Anti-DCC monoclonal antibody (Oncogene) was used
at 1:150 dilution.
Co-culture assays of retinal explants with either Sema5A-myc 293 cells or parental 293 cells were performed in laminin-coated 35 mm coverslip dishes (MakTek). 293 cells were grown to either 20% or 40% confluence. Retinal explants obtained from GFP-transgenic E14 mouse embryos (Jackson Lab) were cultured overnight on top of the laminin and 293 cells in F12/N2 medium with netrin 1 supplementation. Total neurite outgrowth was determined after fixation in 4% paraformaldehyde and tracing the fluorescent neurites on a video monitor. After conversion to digital images, total neurite length was quantified using Adobe Photoshop.
Antibody production and characterization
A rabbit polyclonal antibody was raised against bacterially expressed
Sema5A without the thrombospondin-type 1 repeats (aa 1-544 fused with
939-974). This coding sequence was inserted into pTrcHis 2B (Invitrogen), in
frame with a C-terminal myc epitope and a poly-histidine (His6)
tag. Recombinant protein was produced in E. coli (strain
BL21(DE3)pLysS) after IPTG induction for 3 hours at 30°C. Bacteria were
then lysed, and recombinant protein affinity purified on a NiNTA agarose
column (Pharmacia). Antigen was injected into rabbits by Covance Inc.
(Berkeley). Anti-Sema5A rabbit immune and pre-immune serum were precipitated
using ammonium sulfate, and dialyzed against F12 medium. Fab fragments were
made using papain digestion, and separated from Fc fragments and uncut
antibodies by protein A chromatography (Pierce).
Anti-Sema5A was used at 1:400 in western blots to demonstrate immunoreactivity against recombinant ECD-Fc. Live 293 cells expressing Sema5A-myc were stained for 1 hour at 37°C with anti-Sema5A (1:100) in culture medium. After 3 washes with pre-warmed culture medium, they were fixed in 4% paraformaldehyde, and visualized using a Cy3 donkey anti-rabbit antibody (Jackson Immunochemicals).
Retinal immunostaining
Live E14 retinas were isolated along with a short segment of optic nerve,
and incubated with anti-Sema5A antibody (1:100) in F12/N2 medium for 2-16
hours at 37°C. After three washes with warm culture medium, retinas were
incubated Cy2 donkey anti-rabbit antibody (1:500) (Jackson Immunochemicals)
for another 2-16 hours. Retinas were then washed three times, fixed in 4%
paraformaldehyde for 1 minute, and mounted whole. Control retinas were
processed in the same manner using pre-immune serum. The pattern of
immunoreactivity was analyzed using a confocal microscope (Pascal LSM,
Zeiss).
Sema5A function blocking experiments
For optic nerve experiments, live tissue preparations containing the
retinas, optic nerves, and the optic chiasm were dissected from E14 embryos
(Sretavan and Reichardt,
1993). Preparations were cultured for 8-10 hours at 37°C in
the presence of anti-Sema5A or pre-immune serum (1:100) in F12/N2 medium.
Tissue preparations were then transferred into 2 ml of antbody-free F12/N2
medium, cultured overnight, and fixed with 4% paraformaldehyde for 24 hours.
Retinas were removed, and a DiI crystal placed at the optic disc using a glass
micropipette. After overnight incubation in 4% paraformaldehyde at 37°C,
optic nerves were examined using rhodamine optics on a fluorescent microscope
(Microphot-SA, Nikon) or a confocal microscope (Pascal LSM, Zeiss).
For intra-retinal function blocking experiments, gestational day 14 pregnant mice were anesthetized with xylazine/ketamine mixture, and a mid-abdominal incision made to expose the uterine sacs. A small incision was made through the uterine wall to reveal one eye of an embryo. Micropipettes loaded with Fab fragments (1 µg/µl in F12 medium) were used for intraocular injections, and an estimated 2-4 µg of antibody was delivered into each eye. Up to four embryos were injected in each animal. Uterine incisions were closed with 8-0 sutures, and the abdominal wall and overlying skin closed with 4-0 sutures. After a further 24 hours of in utero development, injected embryos were harvested and fixed in 4% paraformaldehyde for 24 hours. A DiI crystal was placed in the peripheral retina of treated eyes, and after 6-8 hours at 37°C, retinas were mounted whole, and visualized using standard fluorescence optics.
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RESULTS |
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A number of semaphorins were found in the developing mouse retina during
the period of active RGC neurogenesis and axon outgrowth through the optic
disc into the optic nerve (Table
1). The mRNAs corresponding to Sema3A, Sema3C, Sema3E and Sema6A
were found in the retinal ganglion cell layer. However, only mRNA
corresponding to Sema5A, a class V transmembrane semaphorin, was detected at
the developing optic disc and optic nerve. Sema5A mRNA was expressed by the
optic disc neuroepithelial cells, which as a group surrounded the RGC axons
exiting from the retina (Fig.
1A,B). Previous work has shown that this population of
neuroepithelial cells expresses netrin 1, which plays a major role in guiding
axons into the optic nerve (Deiner et al.,
1997). Sema5A mRNA was also found in neuroepithelial cells that
line the embryonic optic stalk connecting the retina to the ventral
diencephalon (Fig. 1A,E).
Expression was however absent at the midline region including the optic
chiasm, and absent within the diencephalon. Sema5A mRNA was present at the
optic disc and optic stalk from E12-E16, during the period of active retinal
axon growth through these areas, but was absent from these regions by E18
(data not shown). Sema5A mRNA expression was also observed in the lamina
propria under the olfactory epithelium
(Fig. 1G), and in the walls of
the lateral ventricles and developing striatum (data not shown). It is of
interest that mRNA for Sema5B, the other known vertebrate Class V semaphorin,
was not detected in the developing retinal pathway
(Fig. 1D). The pattern of
Sema5A mRNA expression placed this molecule in regions traversed by embryonic
retinal axons, and suggested a role in retinal axon guidance.
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The presence of Sema5A mRNA in the optic nerve and at the optic disc, a
major exit point for retinal axons, was at odds with the fact that vertebrate
semaphorins are generally considered inhibitory axon guidance molecules. Given
that growth cone responses have been reported to switch from inhibition to
attraction in the context of signaling from a second guidance molecule
(Castellani et al., 2000;
Hopker et al., 1999
), Sema5A
function during retinal pathway development needed to be determined. Since
axon pathfinding through the optic disc into the optic nerve is known to
involve L1, netrin 1 and laminin 1, we tested retinal axon responsiveness to
Sema5A in the context of signaling from each of these molecules.
Sema5A inhibits retinal growth cones on laminin
A secreted recombinant Sema5A protein was generated consisting of the
extracellular portion of Sema5A, encompassing both its semaphorin and
thrombospondin domains, fused to the human IgG Fc domain (ECD-Fc)
(Fig. 2A,B). Addition of 12.5
nM ECD-Fc, oligomerized with 7.5 µg/ml anti-Fc antibody, resulted in the
collapse of 68% of RGC growth cones cultured on laminin within 30 minutes
(Fig. 2C). Increases in ECD-Fc
concentration, or duration of exposure, did not further increase the response
rate (Fig. 2C and data not
shown). Oligomerization was required for maximal response, and was used in all
further collapse assays. In control experiments, axons treated with
oligomerized human Fc protein responded at a rate of 12% (n=89,
P<0.001) (Fig.
2C).
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Given that the extracellular domain of Sema5A collapsed retinal axons, we next tested whether this protein when used as a substratum could create a barrier to neurite growth. A substratum choice assay was used, in which growth cones extending on laminin (5 µg/ml) were confronted with a test substratum containing laminin (5 µg/ml) and either ECD-Fc (20 nM) or heat-inactivated ECD-Fc (20 nM). Growth cone responses upon reaching the test substratum included stopping at the border, turning to avoid the area, or growing freely across the border into the labeled region (Fig. 2D,E). We found that 58% of growth cones stopped at, or turned away from, ECD-Fc borders (n=105), while only 36% of growth cones (n=169) behaved similarly at heat-inactivated ECD-Fc borders (P<0.001) (Fig. 2F).
The ability of Sema5A to inhibit retinal axons when expressed as a transmembrane molecule on cell surfaces was also tested. To do so, we measured RGC axon outgrowth in the presence of stably transfected cells expressing full-length Sema5A. Retinal explants placed on top of untransfected 293 cells growing at 20% confluence on a laminin substratum resulted in a mean total neurite length of 5.3 mm per explant (n=25 explants). In the presence of Sema5A-myc-transfected cells at the same confluence, the mean total length was reduced by 30% to 3.7 mm per explant (n=25 explants, P<0.001) (Fig. 2G-I). An increase in the density of 293 cells seeded onto the laminin-coated dishes to 40% confluence resulted in a mean total neurite length of 2.1 mm per explant for untransfected cells (n=9 explants), while Sema5A-myc-transfected cells resulted in a mean total neurite length of only 1.3 mm per explant (n=9 explants, P=0.011) (Fig. 2I). These results indicated that retinal axons extending on laminin were inhibited by Sema5A presented either as a soluble protein fragment in collapse assays, as immobilized protein in substratum choice assays, or as a cell surface protein in neurite outgrowth studies.
Sema5A inhibition is maintained on a L1 substratum
The extracellular fragment of human L1 was used as a substratum for retinal
axons in Sema5A growth cone collapse assays. After a 30 minute exposure to
12.5 nM ECD-Fc, 74% of growth cones extending on L1 collapsed
(n=148). By comparison, Fc treatment alone resulted in the collapse
of only 5% of retinal growth cones (n=178, P<0.001)
(Fig. 3B). Time lapse
microscopy confirmed that ECD-Fc-treated growth cones extending on L1
(n=30) underwent a loss of filopodia and lamellopdial structures
characteristic of growth cone collapse. Typical growth cone collapse involves
contraction from an open to a collapsed morphology, but interestingly, growth
cones extending on L1 displayed an intermediate stage in which growth cones
appeared to lose lamellopodia and consisted mainly of filopodial-like
structures (Fig. 3A). These
intermediate growth cones subsequently progressed to the fully collapsed,
stick-like morphology.
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Activities of the semaphorin and TSP domains
Class V semaphorins are unique in that they contain both a sema domain and
seven thrombospondin type-1 repeats in their extracellular domain. To
investigate the possible function of each sub-domain, recombinant proteins
consisting of the semaphorin domain alone fused to an Fc tag (Sema-Fc), or the
thrombospondin repeats fused to an Fc tag (TSP-Fc), were purified
(Fig. 1A,B) and used in
collapse assays. The ability of the sema domain alone to trigger growth cone
collapse appeared to be reduced compared to the intact extracellular domain.
12.5 nM Sema-Fc led to only 13% growth cone collapse (n=93), compared
to the 74% collapse response observed when 12.5 nM of the entire extracellular
fragment was used (Fig. 3C). An
increase of Sema-Fc to 100 nM resulted in a 62% collapse rate
(n=103), suggesting that the sema domain alone was approximately 8-10
fold less potent as an inhibitor (Fig.
3C).
Application of TSP-Fc up to 100 nM resulted in a collapse rate of only 12%
(n=146), which was not different to the 10% response rate seen after
application of recombinant Fc control protein (n=52)
(Fig. 3C). TSP-Fc was also
tested as a growth substratum at concentrations up to 20 mg/ml, but failed to
support axon outgrowth from embryonic retinal explants. This data indicated
that the inhibitory activity of transmembrane Sema5A lay within its sema
domain, as has been described for secreted Sema3A
(Koppel et al., 1997).
Additionally, the full inhibitory potential required activity supplied by
other regions in the extracellular domain.
Sema5A function in the presence of netrin 1
The mRNA expression pattern for Sema5A was remarkably similar to that of
netrin 1. To determine whether exposure to netrin 1 modified retinal growth
cone responses to Sema5A, we carried out Sema5A collapse assays in the
presence of soluble netrin 1, using retinal axons extending on either L1 or
laminin.
Retinal explants were cultured overnight on an L1 substratum in medium
containing 100 ng/ml netrin 1, a concentration previously shown to effectively
promote RGC axon outgrowth in collagen gels
(Deiner et al., 1997). ECD-Fc
was then added to a final concentration of 12.5 nM for 30 minutes, and the
resulting growth cone morphology was analyzed. Sema5A in the presence of
netrin 1 resulted in collapse of 74% of RGC growth cones (n=252),
same as the response rate of 74% following ECD-Fc treatment without netrin 1
in the culture medium (Fig.
3D). Addition of Fc alone in the presence of netrin 1 resulted in
the collapse of 11% of growth cones (n=116, P<0.001)
(Fig. 3D).
In a second set of experiments, we examined the effects of ECD-Fc on retinal neurites that were more directly dependent on netrin 1 for outgrowth. Retinal explants were cultured on a dish coated with 2.5 µg/ml laminin, a sub-optimal level for reliable axon outgrowth. However, the addition of 100 ng/ml netrin 1 to these cultures elicited reproducible retinal axon outgrowth. Netrin 1 dependence was demonstrated by the fact that addition of an antibody blocking the function of the Netrin receptor DCC attenuated this increased neurite outgrowth (Fig. 3E). In this netrin 1-dependent outgrowth assay, ECD-Fc collapsed 70% of RGC growth cones (n=135) compared to only 24% in Fc-treated controls (n=77, P<0.001) (Fig. 3F). Together, this data indicated that netrin 1 was not capable of modulating the inhibitory effects of Sema5A on RGC axons. Thus, Sema5A appeared to maintain its inhibitory function as RGC axons encountered the retinal pathfinding molecules L1, laminin or netrin 1.
Sema5A inhibition during navigation in the optic nerve
One feature of Sema5A mRNA expression was its presence along the entire
course of the developing optic nerve. Given that exposure to guidance
molecules at specific pathfinding regions can silence receptors and eliminate
the ability of a growth cone to respond to a different guidance molecule
(Stein and Tessier-Lavigne,
2001; Zou et al.,
2000
), we investigated whether RGC axons, after passing through
the optic disc, were altered in their responsiveness to Sema5A.
Retina-optic nerve preparations consisting of a portion of retina connected to the optic nerve were cultured on L1 (Fig. 4A). Retinal axons that had grown through the optic disc region readily extended from the cut end of the optic nerve (Fig. 4B) and their responsiveness to Sema5A was recorded using timelapse microscopy. Axons growing out of the optic nerve were sensitive to Sema5A, with 57% of growth cones collapsing in response to ECD-Fc (n=30), compared to only 12% of Fc-treated growth cones (n=24, P=0.002) (Fig. 4C). Additionally, we used video microscopy to test the response rate of axons from retinal explants. In this video-assay, growth cones from retinal explants had a 60% response rate, and there was no significant difference in the response rates between ECD-Fc-treated axons growing from retinal explants or retina-optic nerve preparations (60% versus 57%) (Fig. 4C). Results from these assays suggested that after growth through the optic disc, retinal axons remained sensitive to Sema5A during their course along the optic nerve.
Localization of Sema5A protein in retinal pathway
The results thus far indicated that Sema5A inhibited RGC axons, and that
this inhibition was maintained in the presence of co-impinging signals from
several relevant guidance molecules. To understand how this inhibition
contributed to retinal pathway development, we examined Sema5A protein
localization using a polyclonal antibody. This antibody recognized recombinant
ECD-Fc on western blots, and a single band of the appropriate size for Sema5A
(135 kDa) from embryonic retinal membrane preparations
(Fig. 5A). Furthermore, the
antibody also resulted in membrane staining of living cells transfected with
Sema5A-myc, but not of untransfected cells
(Fig. 5B and data not
shown).
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Retinal immunostaining using this anti-Sema5A antibody required the use of
unfixed tissues. In E14 mouse retinas, immunoreactivity was detected as a ring
at the perimeter of the optic disc, encircling RGC axons passing through the
optic disc (Fig. 5C,D).
Immunostaining was absent from the central region of the optic disc that
contained retinal axons and the neuroepithelial cell processes known to
display netrin 1 protein on their surfaces
(Deiner et al., 1997). This
pattern of protein localization, together with the inhibitory activity of
Sema5A on retinal axons, raised the possibility that Sema5A prevented RGC
axons from straying away from the optic disc and the optic nerve.
Perturbation of Sema5A function results in axon guidance errors
To test the role of Sema5A in development of the retinal pathway,
anti-Sema5A antibody, or Fab preparations, were applied intraocularly to
embryos in utero and to living embryonic tissue preparations containing the
optic nerve. In control experiments, anti-Sema5A antibody (1:100) was
effective in blocking Sema5A-mediated growth cone collapse of retinal axons
extending on L1 in vitro. In the presence of anti-Sema5A antibody, growth cone
collapse rates after ECD-Fc exposure dropped from 74% (n=148)
(Fig. 3A) to 32%
(n=121, P<0.001) (Fig.
6A). Pre-immune serum did not curb Sema5A-mediated growth cone
collapse, and resulted in a 70% response rate (n=95)
(Fig. 6A).
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Horizontal slice preparations of embryonic mouse brains, including the retinas and the optic nerves, were cultured in either anti-Sema5A antibody (1:100) or pre-immune serum (1:100) for 8-10 hours, and then grown overnight. In anti-Sema5A-treated optic nerves (n=26), 35% exhibited pathfinding errors compared with no occurrence of errors among optic nerves incubated in pre-immune serum (n=22, P=0.007) (Fig. 6B). The guidance errors ranged from mild cases in which a small number of axons were observed straying from the main optic nerve bundle (Fig. 6D) to more severe cases in which fascicles of axons were observed veering off from their normal path (Fig. 6E,F).
Anti-Sema5A Fab fragments injected into eyes of E14 mouse embryos in utero led to retinal axon guidance errors in 4 of 18 treated retinas. The phenotypes were mild, and consisted of stray axons leaving the optic disc region and projecting aberrantly for short distances within the retina itself (Fig. 6G,H). In sum, disruption of Sema5A function resulted in axons straying from the main retinal pathway, and this effect was more prominent in the optic nerve than at the optic disc.
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DISCUSSION |
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Sema 5A inhibition and L1, laminin, netrin 1 signaling
A major pathfinding task for retinal axons is exiting the retina by growing
through the optic disc into the optic nerve. This guidance event is mediated
by netrin 1 (Deiner et al.,
1997), and occurs in the presence of L1
(Deiner et al., 1997
) and
laminin (Hopker et al., 1999
).
Given that Sema5A was also present at the optic disc and nerve, we examined
how combinations of the axon guidance molecules L1, netrin 1 and laminin
affected the ability of retinal axons to respond to Sema5A. The results showed
that Sema5A clearly inhibited retinal growth cones in the presence of all
guidance molecule combinations tested, including laminin or L1 alone, and
pairings of netrin 1 with L1 or laminin. Thus, retinal growth cones reacted to
Sema5A as an inhibitory molecule even while receiving growth supporting
co-impinging signals from members of multiple families of attractive axon
guidance molecules.
Neurite outgrowth in the presence of laminin and netrin 1
The assay testing retinal axon responses to Sema5A under the influence of
both netrin 1 and laminin involved culturing retinal explants on a laminin at
a level that alone was too low to produce reliable axon outgrowth, but which
resulted in consistent neurite extension after the addition of soluble netrin
1. The dependence of this assay on both laminin and netrin 1 was demonstrated
by the fact that netrin 1 supplementation alone without the laminin substratum
supported no retinal axon outgrowth, and the fact that the outgrowth induced
by the laminin/netrin 1 combination was decreased by an antibody against the
Netrin receptor DCC (Fig. 2E).
The ability of this laminin/netrin 1 combination to augment neurite outgrowth
was somewhat unexpected given a previous study reporting that in the presence
of laminin 1, Xenopus retinal growth cone response to netrin 1 was
switched from attraction to repulsion
(Hopker et al., 1999). One
explanation for this difference is the micropipette delivery of a netrin 1
point source to Xenopus axons, while in the present study netrin 1
was bath applied, and did not expose neurites to a netrin 1 gradient. A second
possibility is a difference in laminin levels. The substratum laminin level in
the present study by itself did not reliably support retinal axon growth in
vitro. In contrast, Xenopus growth cones were first grown on
effective concentrations of laminin 1, and then tested with netrin 1
gradients. If this second explanation is correct, then whether switching
occurs in vivo may depend critically on the precise concentration of
particular axon guidance molecules to specific growth cones.
Effect of L1 on responses to Sema5A
Several aspects of Sema5A action on retinal axons such as effective
concentration, localization of inhibition to the sema domain, and increased
effectiveness after oligomerization, were consistent with previous studies of
semaphorin function (Koppel et al.,
1997; Koppel and Raper,
1998
; Xu et al.,
2000
). One difference, however, was the regulation of responses to
semaphorins by the Ig superfamily guidance molecule L1. Cortical axons, like
retinal axons, express abundant L1 on their surfaces in vivo, and likely carry
out numerous pathfinding tasks in the presence of L1 signaling. In a study in
which cortical axons were exposed to Sema3A in the presence of L1-Fc, growth
cones did not collapse, but instead maintained an open morphology
(Castellani et al., 2000
),
suggesting that growth cones responding to L1 signaling were freed of
Sema3A-mediated inhibition. This was not the case for Sema5A, as retinal
growth cones responded to Sema5A inhibition in the presence of L1.
Furthermore, concentrations of Sema5A required to trigger growth cone collapse
were similar for retinal axons grown on laminin or L1. These results raise the
possibility that the growth cone signaling cascades triggered by Sema3A and
Sema5A are different, and cross-talk with L1 signaling exists in the case of
Sema3A but not Sema5A. Interestingly, it appears that L1 influences Sema3A
signaling by interacting directly with the Sema3A receptor neuropilin 1
(Castellani et al., 2000
).
Currently, known families of semaphorin receptors include the neuropilins and
the plexins (Raper, 2000
),
however, specific receptors for transmembrane semaphorins have not yet been
identified.
Function of thrombospondin type-1 repeats
A unique aspect of class V semaphorins is the seven thrombospondin type-1
repeats in their extracellular domains. While TSP repeats in other molecules
have been shown to promote axon growth and to mediate neural attachment
(Adams and Tucker, 2000), these
results showed that TSP repeats combined with a semaphorin domain clearly
resulted in a molecule with overall inhibitory activity for retinal neurite
outgrowth. In addition, the TSP repeat domain by itself did not trigger growth
cone collapse, nor did it support retinal axon outgrowth. Given that the
intact Sema5A extracellular domain, which included the TSP region, was a more
potent inhibitor of retinal axons than the sema domain alone, it is possible
that TSP repeats contribute to ligand-receptor binding, a known function for
the non-sema domains of other semaphorins
(Feiner et al., 1997
). However,
given that TSP repeats have also been implicated in protein binding
(Adams and Tucker, 2000
), an
additional possibility is that Sema5A associates with other proteins through
the TSP repeats and these protein complexes represent an as yet unrecognized
aspect of Sema5A function.
Localization of Sema5A
In situ hybridization and immunostaining showed that Sema5A was expressed
by the group of optic disc neuroepithelial cells that surround the retinal
axon bundle exiting the retina. These same cells are known to extend netrin
1-bearing processes radially towards the center of the optic disc
(Deiner et al., 1997). Although
expressed by the same cell population, Sema5A protein was localized mostly to
the cell bodies of the neuroepithelial cells arrayed at the periphery of the
optic disc, and Sema5A protein was not detected on the netrin 1-bearing
processes. This suggested that Sema5A may be specifically excluded from
neuroepithelial cell processes, possibly through anchoring of transmembrane
Sema5A via its cytoplasmic domain.
An inhibitory sheath for optic nerve development
Blocking Sema5A function resulted in retinal axon defasciculation from the
main axon bundle of the optic nerve. Although some cases showed sizable
retinal axon bundles leaving the optic nerve, other preparations had only a
few stray axons, and in many anti-Sema5A-treated nerves, no errors were noted.
This variation in occurrence and severity of pathfinding errors could be due
to the use of a function-blocking antibody over a relatively short time
period; a necessary limitation to maintain the health of tissue preparations.
A second possibility is the presence of other inhibitory molecules such as
Slit proteins in the developing optic nerve
(Niclou et al., 2000) serving
a similar ensheathing function.
In principle, axon defasciculation from the optic nerve in the face of
anti-Sema5A antibodies could be interpreted as a loss of growth
promoting/fasciculation activity rather than loss of Sema5A-mediated
inhibition. However, given the in vitro evidence that Sema5A inhibited retinal
axon outgrowth and caused growth cone collapse, combined with the evidence
that Sema5A mRNA and protein were found surrounding the optic nerve bundle, we
favor the model that Sema5A served as an inhibitory sheath. Furthermore, since
new retinal growth cones entering the optic nerve generally extend along the
external surface of the axon bundle (Reese
et al., 1991; Williams et al.,
1991
), a Sema5A sheath places this inhibitory molecule in a direct
position to contain the growth of newly arriving axons.
Maintaining inhibition during pathfinding
Previous studies have shown that receptor signaling cascades activated by
guidance molecules can interact and modulate growth cone responses. These
interactions set up a logic system in which a growth cone's response to
multiple cues presented simultaneously is not merely the sum of the individual
guidance forces, and creates increased functionality given a limited
repertoire of guidance molecules. During pathfinding however, there are
instances, as axons grow over long distances, where it may be useful to
maintain a constant responsiveness to a single guidance molecule while
accomplishing sequential pathfinding tasks involving various others. In such
cases, the nervous system could utilize molecules such as Sema5A that appear
to trigger a conserved response in growth cones in the face of co-impinging
signals from multiple families of guidance molecules.
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ACKNOWLEDGMENTS |
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