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The Journal of Neuroscience, July 1, 2000, 20(13):5024-5036
Rapid Dendritic Remodeling in the Developing Retina: Dependence
on Neurotransmission and Reciprocal Regulation by Rac and Rho
Wai T.
Wong,
Beverly E.
Faulkner-Jones,
Joshua R.
Sanes, and
Rachel O. L.
Wong
Department of Anatomy and Neurobiology, Washington University
School of Medicine, St. Louis, Missouri 63110
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ABSTRACT |
We demonstrate that within the intact and spontaneously active
retina, dendritic processes of ganglion cells exhibit rapid and
extensive movements during the period of synaptogenesis. Marked restructuring occurs in seconds, but structural changes are relatively balanced across the dendritic arbor, maintaining overall arbor size and
complexity over hours. Dendritic motility is regulated by spontaneous
glutamatergic transmission. Both the rate and extent of the movements
are decreased by antagonists to NMDA and non-NMDA glutamate receptors
but are unaffected by tetrodotoxin, a sodium channel blocker. The
dendritic movements are actin dependent and are controlled by the Rho
family of small GTPases. Transfection of dominant-negative and
constitutively active mutants into ganglion cells showed that Rac and
Rho exert reciprocal effects on motility. We suggest that the Rho
family of small GTPases could integrate activity-dependent and
-independent signals from afferents, thereby adjusting target motility
and maximizing the chance for initial contact and subsequent synaptogenesis.
Key words:
dendritic development; process motility; synaptogenesis; Rho; Rac; spontaneous activity; retinal ganglion cells
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INTRODUCTION |
During embryogenesis, axons grow,
often over long distances, to reach their targets, after which their
growth cones form synapses. In this classic picture of synaptogenesis,
derived primarily from static images and studies in vitro,
the axon is viewed as the active partner, and the dendrite is viewed as
its passive target. Indeed, axonal growth cones are elaborate
sensorimotor structures that sense and integrate cues in their
environment, extend filopodia, form intercellular attachments, and
actively remodel as synapses form and mature (for review, see
Mueller, 1999 ). However, not only extending axons but also developing
dendrites bear filopodia (Vaughn et al., 1974; Berry and Bradley, 1976;
Vaughn, 1989). Moreover, S. J. Smith and colleagues have directly
visualized dendritic filopodia extending toward and initiating contact
with ingrowing afferents in hippocampal cell cultures in
vitro (Cooper and Smith, 1992; Dailey and Smith, 1996; Ziv and
Smith, 1996) and in zebrafish embryos in vivo (Jontes et
al., 2000). These observations raise the possibility that dendrites are
more active participants in synaptogenic interactions than imagined
previously. We therefore undertook studies aimed at obtaining a more
complete view of how dendrites move, particularly during the period of synaptogenesis, in active circuits.
We chose to examine dendritic remodeling in the developing vertebrate
retina. The retina is a suitable preparation for this study because it
can be isolated as an intact sheet of tissue without disrupting its
structure or function. In particular, we focused on the output neurons
of the retina, the ganglion cells, in embryonic chick retina at the
time that synapses are formed onto ganglion cell dendrites. By labeling
developing ganglion cells with green fluorescent protein (GFP), we were
able to follow dendritic remodeling within an intact circuit and to
characterize its dynamic nature. We also assessed the role of
intercellular communication in regulating dendritic remodeling.
Specifically, we examined the role of endogenous glutamatergic
neurotransmission during the time that glutamatergic synapses are
formed onto ganglion cell dendrites. Our results indicated that
dendritic remodeling in the developing retina is prominent and rapid,
with terminal processes moving at rates of up to 10 µm/min. These
rapid movements are regulated by afferent neurotransmission; blockade
of glutamatergic transmission suppresses dendritic motility and
decreases the total dendritic length and the number of branch points in
the dendritic tree. This indicated that glutamatergic signaling
occurring in developing retinal circuits is important in increasing the
rate of dendritic remodeling and maintaining the dendritic structure of
the arbor.
We were also interested in the intracellular mechanisms that underlie
rapid remodeling. Because terminal dendritic processes contain a dense
actin matrix (Matus et al., 1982; Markham and Fifkova, 1986), we
examined the involvement of actin, as well as the Rho family of small
GTPases, in the regulation of dendritic remodeling. This family of
molecules, of which Rac and Rho are members, is a group of prominent
intracellular regulators of signaling pathways that mediate changes in
actin organization in response to extracellular cues (Ridley and Hall,
1992; Ridley et al., 1992; Nobes and Hall, 1995). Our results here show
that rapid dendritic remodeling is an actin-dependent process and is
reciprocally regulated by Rac1 and RhoA that exert mutually
antagonistic effects. Thus, these molecules may serve as a nodal point
at which extracellular signals can be integrated to regulate precisely
dendritic behavior for the establishment and regulation of synaptic contacts.
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MATERIALS AND METHODS |
Retinal explant preparation. Embryonic day 12 (E12)-E13 chick embryos were decapitated and enucleated. Eyecups were
immersed in oxygenated, ice-cold Ringer's solution (2 mM
CaCl2, 5 mM KCl, 2 mM
MgCl2, 124 mM NaCl, 1.25 mM KH2PO4, 20 mM glucose, and 20 mM HEPES). Retinas were
dissected from the eyecups and then mounted on black Millipore filter
paper (HABP045) with the ganglion cell layer uppermost as described
previously (Wong et al., 1998).
Particle-mediated gene transfection. The mounted retinas
were transfected immediately after dissection using the Helios Gene Gun
(Bio-Rad, Hercules, CA). In this method, DNA to be transfected is
precipitated onto tiny gold particles that are then propelled into the
nuclei of cells using a high-pressure helium stream (Lo et al., 1994).
The preparation of DNA-coated gold particles was performed according to
the manufacturer's recommendations. Typically, for transfections, a
total of 1 µg of DNA, coated onto 0.5 mg of gold particles (diameter,
1.0 µm), was used in the transfection of each retinal piece. For
cotransfection of GFP with the Rac and Rho mutants, DNA coding for
GFP (or yellow fluorescent protein; Clontech, Cambridge,
UK) and for the small GTPase was mixed in a 1/2.3 ratio and
coprecipitated onto the gold particles. The myc-tagged
dominant-negative and constitutively active mutants of Rac and Rho were
obtained from Dr. Alan Hall (University College, London, UK).
Transfections into the ganglion cell layer of the retina were performed
at pressures of 30-40 psi, and the retinal explants were subsequently
incubated in oxygenated Ringer's solution at 30°C overnight. GFP
expression was first detected after 6 hr, and complete labeling of
ganglion cell arbors occurred by 10 hr. The retinae remained viable for
>36 hr after transfection, as assessed by dendritic morphology and
spontaneous activity. The morphologies of cells obtained with GFP
labeling were comparable with those obtained by
1,1'-dioctadecyl-3,3,3',3'-tetramethylindocarbocyanine perchlorate
(DiI; Molecular Probes, Eugene, OR). This indicates that GFP in the
cytoplasm is unlikely to be compartmentalized but is instead
distributed throughout the dendritic tree.
Time-lapse imaging. Transfected retinas with labeled cells
were transferred to a stage-mounted, temperature-controlled (34°C) chamber through which oxygenated Ringer's solution was continuously superfused (30-60 ml/hr). Ganglion cells with well resolved arbors were chosen for time-lapse confocal imaging using the Bio-Rad Multiphoton Imaging System (MRC 1024M). GFP-labeled cells were excited
using the 488 nm line of a krypton-argon laser (1-3% output), and
the emitted light was viewed through a 522/35 nm filter. Images of live
cells were typically viewed using 40× [numerical aperture (NA), 0.8] and 60× (NA, 0.9) water-immersion objectives
(Olympus). Time-lapse images of entire dendritic arbors were
reconstructed as a sequence of z-projections from stacks of
optical sections spanning the entire z-dimension of the cell
captured every 20-30 min. Rapid time-lapse imaging to follow the
continuous movement of individual processes was performed by capturing
single-plane images every 3-5 sec with additional electronic zoom
factors of two to eight that result in an overall pixel size of ~0.2
µm (40× water objective; NA, 0.8; Olympus). In these recordings,
however, the confocal aperture was fully open, so that it was possible to distinguish between processes that moved within the
x-y plane versus those that traversed out of the
plane of focus.
Several observations indicate that the structural changes we describe
are not movement artifacts. First, because stacks of confocal images
spanning the entire dendritic arbor in all three dimensions were
analyzed at each time point, we could reliably determine whether a new
terminal dendrite was added, eliminated, extended, or retracted in
length. Second, in the fast time-lapse recordings in which a section of
the dendritic arbor was imaged with a wide-open aperture, we did not
detect significant focal drift in any direction. In these recordings,
the primary and secondary branches always remained within the focal
plane and exhibited little structural change, whereas small terminal
processes showed considerable movements within the
x-y plane. There are a few processes that show
movements in the z-direction and may even move out of the
plane of focus, but these can be clearly identified and are not
included in our quantitations. In addition, there were also adjacent
processes that showed differing movements; one may remain stable,
whereas another a few micrometers away shows marked motility. These
observations cannot be accounted for by a focus drift in the
z-direction, as evident from a simple inspection of the
movies of such time-lapse recordings (see Fig. 2 for example). Third, the stability of our recordings is also evident in situations in which
motility is completely arrested and the processes remained in focus,
without any focal readjustments, after superfusion of agents preventing
actin polymerization and depolymerization (see results in Fig. 7).
The dendritic movements that we have observed using these imaging
methods are also unlikely to arise from deleterious cellular effects
resulting from the axotomy of the ganglion cells because we did not
observe deterioration in their spontaneous activity or dendritic
motility over hours in vitro. In addition, interneurons (amacrine cells) that do not project into the optic nerve also exhibited similar morphological dynamics. The dendritic movements are
also unlikely to be induced by phototoxicity. We typically captured
images using a laser intensity at least 10 times less than that that
results in blebbing changes in dendrites. In addition, the movements
occurred immediately after laser scanning and continued at a similar
rate throughout the recording period. Importantly, addition of new
dendritic processes continued until the end of the recording periods
(typically ~3 hr or more in duration). Single images taken at widely
spaced times also suggest that morphological changes continue to occur
in the absence of frequent irradiation. In addition, the dynamics
observed using confocal microscopy were similar to that observed using
two-photon microscopy that produces little photodamage (data not
shown). We chose to use confocal microscopy to image rapid dynamics
because single-plane confocal images captured with a widely open
aperture afforded a deeper plane of sectioning than did those obtained
using two-photon microscopy. This enabled us to follow more
successfully dendritic movements that have a significant length
component in the z-direction. Finally, the movements were
unlikely to be a complication of GFP expression or a result of
culturing conditions because DiI-labeled cells in acutely isolated
retinae displayed similar dynamics (W. B. Gan, J. Grutzendler,
W. T. Wong, R. O. L. Wong, and J. W. Lichtman, unpublished observations).
Calcium imaging. To record spontaneous activity, retinae
were loaded with the calcium indicator dye fura-2 AM (Wong et al., 1998) and imaged using two-photon microscopy (excitation wavelength of
775 nm). Single optical sections were taken every 3 sec, and the
changes in fluorescence with time in selected cells were measured using
MetaFluor (Universal Imaging Corporation, West Chester, PA). Confocal
images of GFP-labeled cells were merged with the fura-2 images to
observe structural motility and spontaneous activity in the same cell.
In pharmacological experiments, time-lapse series were collected
before and during the superfusion of solutions in which the agents
were dissolved. Pharmacological agents were a kainate/AMPA receptor antagonist,
1,2,3,4-tetrahydro-6-nitro-2,3-dioxo-benzo[f]quinoxaline-7-sulfonamide (NBQX; Research Biochemicals, Natick, MA), an NMDA receptor antagonist, (+)-2-amino-5-phosphonopentanoic acid (D-APV; Research
Biochemicals), NMDA (Sigma, St. Louis, MO), tetrodotoxin (TTX; Sigma),
and nickel chloride (Sigma). Inhibitors of actin polymerization,
cytochalasin D, cytochalasin B, and latrunculin A, were obtained from Sigma.
Data analysis. Measurements of dendritic process lengths
were performed on two-dimensional projections in the
z-direction. Although the retinal arbors show a general
horizontal orientation, this approximation may underestimate the
lengths of some of the processes. The analysis of dendritic lengths was
performed using image analysis software (Metamorph; Universal Imaging
Corporation). To follow the length of a process over time, we measured
the distance of the process tip to its base in each image separately.
Processes that extended significantly out of the plane of focus (tips
became fuzzy) were not included in the analysis. The lifetime of an
individual process was estimated to be the total period across a
recording that the process was evident. The rate and extent of
dendritic movements were computed by following the changes in the
length of an individual process across the recording period or, for
nonpersistent processes, the duration over which the process was
evident. Subsequently, to lower the noise inherent in the measurements
(because of exact placement of the cursor at the tip or base, within
1-2 pixels, from measurement to measurement), the length of a process
at a single time point was computed as a moving average over three consecutive time points. We calculated the mean rate of an individual process as:
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where Lt is the calculated process
length at time point t, n is the total number of
time points, and D is the total time for which a process was
monitored. The average rate for multiple processes followed in this
manner was calculated as the average of the mean rates for each
process. The instantaneous rate at time t was calculated
as:
where  t is the interval between time points. The
average or mean rate of movement across a population of processes is
simply the sum of the individual rates divided by the number of
processes. The extent of movement across the recording period (250 sec)
was computed as the difference between the maximum and minimum observed lengths for a particular process. The average extent of movement (averaged across a population of processes) is the sum of the individual "extents" divided by the number of processes.
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RESULTS |
Dendritic remodeling in ganglion cells is extensive and rapid
Our recordings reveal an extensive reorganization of dendritic
structure that is appreciable between consecutive frames
(n = 30 cells examined). At 0.5 hr intervals, for a
total of 10 hr, dendritic changes were comprised of extensions and
retractions of processes, as well as the addition of new processes and
the elimination of existing processes (example shown for two time points in Fig. 1A,B).
These different forms of reorganization occurred simultaneously in all
parts of the dendritic tree and were robust for the duration of the
recording (Fig. 1C). A superposition of the images captured
across the recording period demonstrates that the extent, rate, and
distribution of dendritic movements allow dendritic processes to
traverse in a few hours a much larger volume in space than that
occupied at any single point in time (Fig. 1, compare A,
D). In addition, this figure illustrates how dendritic
motility is primarily restricted to tertiary branches; primary and
secondary branches move little if at all, and the overall shape of the
arbor is not greatly affected by the motility of its terminal
branches.
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Figure 1.
Dendritic remodeling occurs throughout the entire
arbor. A, B, Extended-focus
(z-projection) confocal images of an E12 ganglion cell
taken 3 hr apart are shown. Structural changes include extensions
(ex), retractions (r), addition of
new processes (a), and elimination of previously
existing processes (el). Some processes also
remain stable (s) across this period.
C, Superposition of 21 time-lapse extended-focus images
of the same cell, captured at 0.5 hr intervals, for a total recording
period of 10 hr is shown. The different colors represent
the position occupied by the dendritic tree at different time points,
with the cooler colors corresponding to
earlier time points and the warmer colors
to later ones. A movie (dendrite.avi) of the consecutive frames can be
viewed at http://thalamus.wustl.edu/wonglab/images/dendrite.avi.
D, The sum of all 21 images marks all the positions in
space traversed by dendritic processes during the recording period. The
dendritic volume occupied by the cumulative image in D
is markedly greater than that of the instantaneous image in
A.
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Subsequently we obtained images of the dendrites at more frequent time
intervals to determine whether the structural changes we observed
across the arbor actually occurred more rapidly. To follow the changes
in structure completely, we captured confocal images of individual
dendritic processes at high magnification, every 3-5 sec over a period
of 4-16 min. In these recordings, the confocal aperture was fully
opened, so that processes leaving the plane of focus could be
distinguished from those that remained within the focal plane during
the period of recording. Over 100 such recordings were obtained. Figure
2A, left,
shows a portion of a dendritic arbor followed in this way. These fast
time-lapse recordings revealed that most processes changed markedly in
length and shape over seconds. Neighboring processes on a dendritic
branch exhibited varied behaviors; addition, extension, elimination, and retraction of processes were observed (Fig.
2A, right). A minority (~6%) of
processes, however, remained relatively stationary (rate < 0.5 µm/min) throughout the period of observation. In addition, individual
processes were moved at different rates and directions during the
course of the recording. Also, although some processes persisted
throughout the recording period, others were transient. Figure
2B illustrates the behavior of eight processes from a
single dendritic arbor during a 1000 sec recording period. In all
recordings, individual processes appeared to behave independently
irrespective of their neighbors.
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Figure 2.
Movements of individual dendritic processes are
highly rapid and diverse. A, Left,
Confocal image of a dendritic branch of an E12 ganglion cell captured
at high magnification. Right, Time-lapse images of
processes on the same primary dendrite, indicated by
arrows in the left panel. The interval
between frames is 10 sec. Process 1 is relatively
stable. Adjacent processes show motility of different kinds, with
process 2 exhibiting small changes in its length in the
same time that process 3 appears de novo
and then retracts completely. Process 4 is an example of
a continuous and progressive extension. A movie (filopodia. avi) of
the consecutive frames can seen at
http://thalamus.wustl.edu/wonglab/images/filipodia.avi.
B, Length-versus-time plots for eight other
representative processes from different parts of the cell shown in
A (left), illustrating the diversity and rate of dynamic
movements.
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Having observed continuous movements in each process, we used two
parameters to quantify their dynamics. First, we calculated the
rate of movement, which is the sum of the length changes
exhibited by a process across the recording period divided by the time
that the process was present (defined mathematically in Materials and Methods). This parameter gives an indication of how quickly a particular process moves. Second, we measured the extent of
movement, which is defined as the difference between the maximum and
minimum lengths exhibited by a process across the recording period of 250 sec. This parameter reflects the "reach" achieved by a process over a few minutes.
The rate of movement averaged across 188 processes from 14 cells was
1.33 ± 0.89 µm/min (mean ± SD). Mean rates for individual processes ranged up to 5 µm/min, and maximum instantaneous rates (see
Materials and Methods) reached 10 µm/min. The average extent of
movement by a process over this period was 1.88 ± 1.53 µm, which is ~50% of the average process length (3.91 ± 3.30 µm;
n = 100). Moreover, if we estimate a process to have a
cross-sectional area of 0.5 µm2, then
the tip of an average process would traverse in 250 sec a volume of
0.94 µm3 (0.5 µm2 × 1.88 µm), 50% of the volume of
an average process (0.5 µm2 × 3.91 µm = 1.96 µm3). By moving at the
average rate of 1.33 µm/min, the dendrite would sample each portion
of that volume approximately three times in 250 sec (1.33/1.88 × 250/60 = 2.95). Although imprecise, these calculations show that
dendritic movements enable processes to cover an expanded volume around
themselves (illustrated also in Fig. 1D), potentially
increasing the probability of contact with nearby afferents.
Restructuring events are balanced across the dendritic arbor
How do the rapid dendritic movements that occur over seconds to
minutes relate to the change in the overall size and complexity of the
dendritic arbor over hours? To address this issue, we monitored changes
in entire arbors by capturing images every 20 min for 3 hr
(n = 4 cells). We observed that the number and the size
of additions to the arbor in each interval were closely matched to the
number and the size of the losses (example shown in Fig.
3A-C). To test the
possibility that an apparent balance actually reflects separate large
areas of addition and elimination of processes, we calculated the
number of branch points of the arbor separately for the central and
peripheral halves of each cell. Although many branch points were added
and eliminated between consecutive time points, the net change in the
overall number of branch points in both the central and peripheral
halves of the arbor was close to zero (Fig. 3D,E). This
trend is also present in the total dendritic length of the arbor (Fig.
3F; n = 4 cells); the net change in dendritic length between the time points was small compared with the
total dendritic length of the tree (averaging 3.25 ± 0.95% for
four cells over the periods of recording). Thus, despite considerable local change over seconds, the total dendritic length remained surprisingly constant over the time scale of a few hours. Taken together, our results indicate that the rapid restructuring is balanced
across the arbor to maintain relatively constant not only the size but
also the complexity of the tree over the time scale of a few hours.
Although dendritic trees appeared immature at this stage (E12-E13) in
comparison with those in the posthatchling (Thanos et al., 1992), we
estimate that the overall growth and elaboration of the ganglion cell
dendritic arbor proceed at a much slower rate (many hours to days) than
the rate of dendritic remodeling (seconds to minutes). Therefore, the
rapid movements observed on a short time scale do not result in a rapid
net growth and elaboration of the dendritic tree but rather serve to
distribute dendritic processes rapidly throughout the space around the
arbor.
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Figure 3.
Rapid dendritic motility results in extensive
remodeling while maintaining the overall size and complexity of the
dendritic arbor. A, The z-projection of
the confocal image stack capturing the entire arbor of an E12 ganglion
cell at the start of a time-lapse recording. This image thus represents
the three-dimensional reconstruction of the arbor at one time point.
B, C, Difference images generated by digitally
subtracting the image in A from the
z-projection of an image stack captured 1 hr later. The
black areas in B indicate
dendritic structures that have been added or have undergone extension
in the intervening hour, whereas the black
areas in C indicate structures that have
been eliminated or have undergone retraction. The white
areas in both B and C
indicate dendritic structures that were unchanged. Note that the
relative amount and distribution of the structures added
(B) and taken away (C) are
approximately balanced. D, Plot of the total number of
branch points and the number of branch points in the central and
peripheral halves of the dendritic tree. Central and periphery halves
of the tree are separated by the line bisecting the midpoints of radii
extending from the soma to the perimeter of the arbor.
E, Histogram representing the change in the number of
branch points with time. White bars
(addition) indicate the number of novel branch points
added at that time point (i.e., those not observed at the preceding
time point), whereas hatched bars
(elimination) indicate those eliminated since the
preceding time point. Dark bars
(net) indicate the difference between additions and
eliminations. F, Percent change in the total dendritic
length (TDL) of four cells (each cell represented by a
different symbol) as a function of
time, illustrating the relative constancy in the total length despite
extensive dendritic movements occurring across this period.
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Dendritic motility is developmentally regulated
To determine whether the rapid dendritic movements observed
in E12-E13 retinal ganglion cells are a feature of immature cells undergoing synaptogenesis, we compared the motility of the dendrites in
this early age group with that in older retina at a stage when synaptogenesis in the inner plexiform layer is relatively more advanced (E15-E16) (Hughes and LaVelle, 1974; Hering and
Kröger, 1996). It is evident from Figure
4 that, although many processes at
E12-E13 moved at rates >2.0 µm/min, at E15-E16, the processes moved at rates below this value. Processes from E12 to E13 cells moved
at an average rate of 1.54 ± 0.11 µm/min (± SE), whereas at
E15-E16, the average rate was 0.84 ± 0.04 µm/min. The
difference in the average rate of movement between these two age groups
was also statistically significant (Mann-Whitney U test,
p < 0.0001). Thus, the dendritic motility appears to
be developmentally regulated, being prominent during the time of active
synaptogenesis, but becomes downregulated as synapses form and
mature.
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Figure 4.
Developmental regulation of dendritic motility.
Frequency histograms showing the distribution of the rates of movements
of dendritic processes of cells from two periods of development
[E12-E13 (top); E15-E16 (bottom)].
The number of cells = 9 for E12-E13 and 8 for E15-E16; the
number of processes = 83 for E12-E13 and 50 for E15-E16.
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Dendritic remodeling occurs in spontaneously active cells
In previous studies, we showed that retinal ganglion cells at the
ages studied here exhibit spontaneous rhythmic-bursting activity that
propagates horizontally across the retina in the form of waves (Wong et
al., 1998). To confirm that rapid dendritic change occurs in cells that
are physiologically intact and that neurotransmission continues in the
retinae after biolistic delivery of the particles, we used two-photon
calcium imaging to examine the activity of cells in the GFP-transfected
retinae. We found that GFP-labeled ganglion cells fired in synchrony
with their untransfected neighbors (Fig.
5). Thus the restructuring events we
observed are likely to be representative of those occurring in intact
circuits. In addition, it raises the possibility that the structural
changes we observed may be regulated by neurotransmission between
retinal interneurons and the ganglion cells.
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Figure 5.
Dendritic remodeling occurs in intact,
endogenously active retinal circuits. A, The field of
cells in the ganglion cell layer of a transfected E13 retina that was
loaded with the calcium-sensitive dye fura-2 AM is shown. Fura-2 AM
labeling was visualized using two-photon microscopy
(left), whereas GFP expression in the same field was
visualized using confocal microscopy (right). Alignment
of the two fields was confirmed by using a sample that can be detected
by both recording modes. Arrows indicate a GFP-labeled
cell (Cell 1) and a neighboring untransfected cell
(Cell 2). Cell 1 exhibited dendritic
changes as confirmed by time-lapse confocal imaging. B,
GFP-labeled cells (Cell 1) retained their endogenous
pattern of spontaneous bursting activity, as indicated by patterns of
rhythmic [Ca2+]i elevations
that were similar to those in the untransfected cells (Cell
2). dF/F indicates percent change in fluorescence
intensity.
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Afferent glutamatergic signaling regulates
dendritic remodeling
Retinal ganglion cells at the ages studied (E12-E13) receive
excitatory glutamatergic inputs from bipolar cells. These excitatory inputs drive the endogenous rhythmic-bursting activity exhibited by
ganglion cells (Wong et al., 1998; Wong, 1999; Sernagor et al., 2000).
Antagonists of ionotropic glutamate receptors (10 µM NBQX
and 100 µM D-APV, selective antagonists of
non-NMDA and NMDA glutamate receptors, respectively) suppress this
bursting activity (Fig.
6A).
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Figure 6.
Dynamic dendritic remodeling is regulated by
endogenous ionotropic glutamatergic transmission. A,
Calcium recording showing rhythmic spontaneous activity in an E12
retinal ganglion cell and a suppression of this activity in the
presence of the ionotropic glutamate antagonists NBQX (10 µM) and D-APV (100 µM).
B, z-projection of the confocal image of
an E12 ganglion cell before (left) and 1.5 hr after
(right) the application of NBQX (10 µM)
and D-APV (100 µM). C, Changes
in the number of terminal processes undergoing growth versus retraction
before (left) and during (right)
glutamatergic blockade. For the cell shown in B, the
total number of growing processes (comprising existing processes that
elongate or are formed de novo; black
bars) was compared with the total number of retracting
processes (comprising existing processes that shorten or are
eliminated; white bars) in a 1 hr period.
Gray bars indicate the difference between
the growing and retracting processes. D, The percent
change in total dendritic length for six cells before and 30 min after
application of NBQX (10 µM) and D-APV (100 µM). E, Blockade of ionotropic
glutamatergic transmission decreases the motility of individual
terminal processes. Histograms indicate the rate and extent of movement
of individual processes as a percentage of control values after 30 min
of drug application in six E12-E13 retinal ganglion cells (number of
processes = 100 in control and 59 in drug). Statistical analyses
[SAS/STAT (SAS, 1996)] for the entire population showed a significant
reduction for both extent (p = 0.0177) and
rate (p = 0.0017). F, Summary
of the effect of different antagonists on the motility of individual
processes. Histograms indicate the percentage change in the extents and
rates of movement 15-30 min after the application of the compound.
Applications of NBQX (10 µM) and D-APV (100 µM) together (100 processes in control; 59 processes in
drug; 6 cells), D-APV alone (100 µM; 85 processes in control; 55 processes in drug; 3 cells), NBQX alone (10 µM; 84 processes in control; 63 processes in drug; 3 cells), and Ni2+ (5 mM; 74 processes in
control; 43 processes in drug; 3 cells) all significantly reduced the
extent and rate of movement (p < 0.01, Mann-Whitney U test). Application of TTX (1 µM; 102 processes in control; 79 processes in drug; 5 cells) had no significant effect on either the extent or rate
(p > 0.25, Mann-Whitney U
test).
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|
This blockade resulted in a decrease in the number of branch points
(60 ± 12% of controls; n = 6 cells) and in the
total dendritic length in ganglion cells (Fig. 6B,D).
Remodeling events in the absence of glutamatergic transmission are not
completely arrested; however, the numbers of dendritic additions
(scored as the number of processes that elongate or are added de
novo) and reductions (the number of processes that shorten or are
eliminated) are both decreased (Fig. 6C). Moreover, the
balance between processes added and taken away is no longer maintained;
reductions outnumber additions (Fig. 6C), resulting in a net
decrease in the amount of dendritic material with time (Fig.
6D; Mann-Whitney U analysis for the
effect of antagonist on the total dendritic length, p < 0.0001). The decrease in total dendritic length occurs progressively
across the period of blockade (up to 50 min) and recovers partially
after a prolonged washout of an hour (data not shown) (see also Rajan and Cline, 1998; Rajan et al., 1999).
We found that the dynamics of individual dendritic processes were also
regulated by glutamatergic transmission. The dynamics were unchanged
immediately after the application of the antagonists NBQX and
D-APV, but after 15-30 min in glutamatergic blockade, both
the extent and the rate of movement were reduced compared with control
(Fig. 6E). This effect is likely to be mediated via both NMDA and non-NMDA glutamate receptors because separate
applications of D-APV (100 µM) and NBQX (10 µM)
each significantly reduced both the extent and the rate of movement
(Fig. 6F). The influx of extracellular calcium via
voltage-gated calcium channels may also be important in potentiating
the dynamics of processes because blockade of voltage-sensitive calcium
channels with Ni2+ (5 mM) (Yuste and Denk, 1995) suppressed motility
(Fig. 6F). Interestingly, the elimination of sodium
action potentials by the application of TTX (1 µM) did not change either the rate or the
extent of dendritic movements. Because bipolar cells have graded
membrane potentials and do not depend on axonal action potentials for
neurotransmitter release (Rodieck, 1998), TTX is unlikely to affect
afferent glutamatergic signaling from bipolar cells to ganglion cells.
However, TTX inhibits voltage-gated sodium channels, blocking
spontaneous bursting activity in retinal ganglion cells (Wong et al.,
1995) and the propagation of dendritic action potentials in other
neurons (Yuste and Tank, 1996). Dendritic motility is therefore not
regulated as a function of spiking activity on the level of the cell
body, nor is it dependent on the spread of sodium action potentials
into dendritic processes.
Together, our results indicate that glutamatergic signaling onto
dendrites is important in regulating the motility in individual dendrites, as well as in maintaining the overall size and complexity of
the dendritic arbor by controlling the balance between the addition and
removal of dendritic processes. This effect is mediated via both NMDA
and non-NMDA receptors and is dependent on calcium influx but not on
sodium channel-mediated action potentials.
Dendritic remodeling is an actin-dependent process
Terminal dendritic processes are devoid of microtubules but
contain a dense actin matrix (Matus et al., 1982; Markham and Fifkova,
1986; Fiala et al., 1998), and rapid alterations in the shape of mature
dendritic spines depend on actin polymerization (Fischer et al., 1998).
As a first step in elucidating the intracellular mechanisms that
regulate dendritic remodeling, we asked whether the actin cytoskeleton
is also required for dendritic motility. We thus applied drugs that
interfere with actin polymerization. Figure
7A shows the degree of
dendritic remodeling in a branch before (left) and after
(right) the addition of cytochalasin D (500 nM), a drug that binds to the fast-growing end of
actin filaments and inhibits their growth and disassembly (Cooper,
1987). Application of this drug results in a rapid arrest in motility
of dendritic processes (one example is shown in Fig. 7B).
This effect was reversible after washout (data not shown). All
filopodia investigated in this way behaved similarly regardless of
their initial motility before drug application (Fig. 7C).
Two other drugs, cytochalasin B (1 µM), which
acts similarly to cytochalasin D (Cooper, 1987), and latrunculin A (100 ng/ml), which inhibits actin polymerization by sequestering actin
monomers (Spector et al., 1989), were also effective in arresting
dendritic motility (data not shown). These results suggest that rapid
dendritic dynamics are driven by changes in the polymerization of
actin.
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Figure 7.
Rapid dendritic remodeling is dependent on actin
polymerization. A, Left, Difference image
of a dendritic branch of an E12 ganglion cell generated by subtracting
two confocal images taken 5 min apart under control conditions.
Black areas (indicated by
arrows) indicate regions of structural change (dendrites
that have been either added or eliminated in the intervening 5 min
period). Right, Difference image of the same dendritic
branch generated by similarly subtracting two confocal images taken 5 min apart after the application of cytochalasin D (500 nM).
Note the absence of black profiles, indicating a
reduction in the amount of dendritic restructuring in the same time
period when actin polymerization is arrested. Scale bar, 5 µm.
B, Length-versus-time plots for the process indicated by
the asterisk in A before
(top) and after (bottom) the application
of cytochalasin D. The actively extending and retracting process
becomes relatively stationary after drug application. C,
Average rates of individual processes in three separate recordings at
E12-E13 before (left) and after (right)
the introduction of cytochalasin D. The wide range of motilities
exhibited by individual processes under control conditions is replaced
by uniform stability after the arrest of actin polymerization (number
of processes, control = 41; cytochalasin D = 26).
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Dendritic remodeling is regulated by Rho and Rac
Members of the Rho family of small GTPases are components of
intracellular pathways via which extracellular influences organize the
actin cytoskeleton (Tapon and Hall, 1997; Van Aelst and
D'Souza-Schorey, 1997; Hall, 1998). These molecules are expressed by
many parts of the nervous system, including the developing chick retina
(Malosio et al., 1997). We therefore evaluated the role of two
subfamilies within the family, the Rho and Rac proteins, in regulating
actin-dependent dendritic remodeling. We transfected retinal ganglion
cells with expression plasmids encoding mutant proteins that increase
or decrease Rho or Rac activity. Endogenous forms of Rho and Rac cycle
between a GDP-bound inactive form and a GTP-bound active form.
Constitutively active mutants of Rac1 and RhoA (ca-V12 Rac1 and ca-V14
RhoA; abbreviated in this manuscript Rac+ and Rho+) are unresponsive to
regulatory proteins that trigger the hydrolysis of GTP to GDP and thus
are permanently in the activated state (Ridley et al., 1992).
Dominant-negative mutants (dn-N17 Rac1 and dn-N19 RhoA; abbreviated
Rac and Rho) bind irreversibly to the specific intracellular
factors mediating the exchange of GDP for GTP, thus preventing the
activation of endogenous forms of Rac or Rho (Diekmann et al., 1991).
Mutant RhoA and Rac1 proteins might affect multiple Rho and Rac
isoforms, respectively, so we ascribe their effects to Rho and Rac
generally, and not specifically. In each case, the Rho or Rac mutant
was cotransfected with DNA encoding GFP in a 2.3/1 (GTPase/GFP) ratio.
The constructs were tagged with the myc-epitope, and reliable
contransfection was confirmed by post hoc
immunohistochemistry in GFP-labeled cells (data not shown). Transfected
ganglion cells were evaluated 18-24 hr after biolistic delivery.
We were first concerned that the upregulation or downregulation of
these key regulatory proteins might have deleterious effects on the
physiology or morphology of transfected cells. We therefore evaluated
the endogenous activity of transfected cells using calcium imaging with
fura-2 AM. Retinal waves persisted in the transfected retinae, and
transfected cells exhibited the same pattern of spontaneous rhythmic
bursting seen in neighboring untransfected cells (data not shown;
records were qualitatively similar to those shown in Fig. 5). This
indicated that the transfected cells were physiologically active and
remained in communication with neighboring cells. Moreover, transfected
ganglion cells maintained an elaborate arbor and did not show
indications of deleterious effects such as swollen cell bodies,
dendritic varicosities, and pyknosis (Fig.
8). There were, however, some
morphological differences between transfected ganglion cells and their
controls. Rac+-expressing ganglion cells tended to have fewer secondary
and tertiary branches but an increased number of short terminal
processes. Conversely, Rac and Rho+ cells had arbors that exhibited
secondary and tertiary branching but had fewer small terminal
processes. These structural effects resembled those observed by
Ruchhoeft et al. (1999). Cells expressing Rho were qualitatively more
similar to those in controls. In any event, terminal dendritic
processes remained motile, thus allowing us to assess the role of these
GTPases in regulating the dynamics of their remodeling behavior.
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Figure 8.
Rac and Rho regulate the dendritic architecture of
retinal ganglion cells. Representative dendritic arbors
(left column) and higher magnification
views of the dendritic structure (right
column) of E12-E13 ganglion cells expressing GFP alone
(control) or expressing both GFP and constitutively active (Rac+, Rho+)
or dominant-negative (Rac, Rho) forms of Rac or Rho. Expression of
Rac+ increases the density of fine terminal processes, whereas
expression of Rac reduces it. Expression of Rho+ results in a
morphology similar to that in Rac, whereas dendritic arbors
expressing Rho are similar to that in the
control.
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Fast time-lapse imaging revealed significant effects of Rac and Rho
activity on the rapid remodeling of dendritic processes. In general,
dominant-negative and constitutively active mutants of each of the
GTPases had opposite effects on dendritic motility. Moreover, the
effects of Rac and Rho perturbations were also opposite in nature. We
used the parameters of rate and extent, defined above, to quantitate
the dynamics of each process. Figure
9A shows the frequency
distribution of average rates and extents for individual processes in
the background of upregulated and downregulated Rac and Rho function;
the net effects are summarized in Figure 9B. Expression of
Rho+ decreased both the rate and the extent of movements, whereas
expression of Rho increased both the rate and the extent. Modulation
of Rac function produced opposite results. Rac decreased both the
rate and the extent of motility, whereas Rac+ increased both parameters
slightly. Although the effects of Rac+ were not statistically
significant, the effects of Rac, Rho+, and Rho were all highly
significant (p < 0.001, Mann-Whitney
U test). Evaluated together, the opposite effects of Rho and
Rac activity and, in particular, the similarity in the effects of the
downregulation of Rac and the upregulation of Rho suggest that Rac and
Rho act reciprocally to regulate rapid dendritic remodeling.
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Figure 9.
Rac and Rho regulate the rate, extent, and process
turnover in dynamic processes in ganglion cells. A,
Distributions of process rates (left) and extents
(right) for cells with upregulated and downregulated
levels of Rac or Rho activity. B, Percentage change in
rates (left) and extents (right) for
cells with upregulated and downregulated levels of Rac or Rho activity
relative to that of control (Asterisks,
p < 0.001, Mann-Whitney U
test). C, Histograms showing the distributions of
process lifetimes for cells with upregulated and downregulated levels
of Rac or Rho activity. Numbers within
the horizontal segments indicate the
percent of the processes with the indicated lifetime range. Number of
processes analyzed, Control = 165; Rac+ = 147; Rac = 54; Rho+ = 71; Rho = 89. Number of cells analyzed, Control = 14; Rac+ = 9;
Rac = 5; Rho+ = 7; Rho = 7.
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For a third measure of dendritic dynamics, we measured how Rho and Rac
regulate the turnover of processes (Fig. 9C). Upregulating Rac function resulted in an increased turnover of processes; in cells
expressing Rac+, the proportion of processes persisting across the
recording period (lifetime > 250 sec) decreased (48% compared
with 75% in the control), whereas the proportion of short-lived processes (0-125 sec) doubled (23 vs 10%). Conversely, attenuation of
Rac function by expression of Rac increased the proportion of
persistent processes (87 vs 75%) and decreased that of short-lived processes (6 vs 10%). Modulation of Rho function had effects opposite to those of Rac; constitutively active Rho increased the fraction of
persistent processes, whereas dominant-negative Rho decreased the
fraction slightly. These results suggest that as in the case for the
rate and extent of process movements, endogenous Rac and Rho exert
reciprocal effects on the rate at which processes are eliminated and
replaced by new ones (Fig. 10).
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Figure 10.
Model for the regulation of rapid dendritic
modeling. Signals originating from presynaptic terminals and other
extracellular sources are received at the cell membrane of dendritic
processes. These signals are then transduced via intracellular pathways
to affect the cycling of Rac and Rho between their GTP-bound (active)
and GDP-bound (inactive) forms, thus controlling the intracellular
levels of endogenous Rac and Rho activity. These levels of activity
jointly control the organization and polymerization of the actin
cytoskeleton that subsequently determine the rate at which dendritic
processes move and are turned over. Rac and Rho exert opposite effects
on dynamic remodeling, with Rac activity promoting greater motility and
Rho suppressing it. The reciprocal control of dynamic dendritic
behavior may be achieved by Rac and Rho exerting separate convergent
effects on the actin cytoskeleton; it is also possible that they may
exert antagonistic effects on each other directly. The potentiation of
dendritic motility by glutamatergic transmission may be affected via
these intracellular pathways, either via the upregulation of Rac
activity, the downregulation of Rho activity, or both. Other
extracellular cues, acting as stop signals, can also stabilize
dendrites by regulating GTPase activity appropriately.
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DISCUSSION |
Rapid dendritic motility in developing dendrites
Our observations revealed a surprisingly high degree of endogenous
motility in developing dendrites, with rates that exceed those recorded
in other systems (Dailey and Smith, 1996; Ziv and Smith, 1996). This
may reflect intrinsic differences between systems; alternatively, the
motility in retinal ganglion cell dendrites may be potentiated by the
prominent spontaneous activity preserved in our whole-mount retinal
preparations. Dendritic movements lacked synchrony with each other and
were collectively balanced across the arbor to maintain the overall
arbor size and complexity. Structural changes were primarily confined
to terminal dendritic processes; primary and secondary dendritic trunks
were comparatively stable in structure and position. Taken together,
the characteristics of these movements suggest that they are unlikely
to underlie a general growth program but may instead play roles in
synapse formation.
Intercellular regulation of dendritic motility
In the developing retina, bipolar cells drive synchronous activity
in ganglion cells via glutamatergic neurotransmission (Wong et al.,
2000). Because patterned activity is retained for >24 hr in explants,
we were able to ask whether afferent signaling affects dendritic
motility. We found that the blockade of endogenous ionotropic
glutamatergic transmission significantly decreased dendritic motility.
This result indicated that dendritic remodeling can be regulated by
intercellular communication from presynaptic cells. Recent studies have
demonstrated that tetanic stimulation of glutamatergic afferents to a
local region of a dendritic arbor can elicit rapid increases in the
length and number of terminal processes (Engert and Bonhoeffer, 1999;
Maletic-Savatic et al., 1999) and the formation of multiple
spine synapses (Toni et al., 1999). Our results extend those
observations in an important way by demonstrating that
neurotransmission in spontaneously active, developing circuits does
indeed play a prominent endogenous role in regulating dendritic
remodeling. In addition, we show here that glutamatergic signaling in
developing circuits not only regulates how rapidly and extensively
individual processes remodel but also maintains the overall size and
complexity of the tree, by balancing the number of dendritic additions
with an equal number of reductions. At the particular developmental
stage examined, the effect is primarily mediated via ionotropic
glutamatergic transmission, involving both NMDA and non-NMDA channels,
as well as the influx of extracellular calcium.
Chronic in vivo application of
D,L-2-amino-4-phosphonobutyric acid, which
suppresses glutamatergic transmission from ON bipolar cells in the
mature retina, reduces the specificity of stratification patterns of ON
and OFF ganglion cell dendritic arbors (Bodnarenko and Chalupa, 1993;
Bodnarenko et al., 1995; Bisti et al., 1998). Our time-lapse
observations suggest that glutamatergic signaling might contribute to
this stratification process of ganglion cells by promoting the growth
or maintenance of dendrites only within the appropriate sublamina. But,
our current observations do not distinguish between the effects of
local versus global influences on dendritic dynamics and structure by
neurotransmission. This would be an interesting avenue to pursue in
future studies.
Dendritic remodeling is unperturbed by the blockade of sodium
channel-mediated action potentials by TTX, corroborating previous in vivo studies on ganglion cells (Wong et al., 1991). This
result also indicates that the regulation of process outgrowth in
dendrites, unlike that in axons, occurs independently of sodium action
potential activity (Sretavan et al., 1988; Dalva et al., 1994;
O'Rourke et al., 1994). Our findings here contrast with those of
Dunaevsky et al. (1999) that indicate that rapid changes in
spines and filopodia in brain slices are not regulated by neuronal activity.
Intracellular regulation of rapid dendritic motility
In a wide variety of cell types, small GTPases in the Rho
subfamily link extracellular signals to actin-dependent motility (for
review, see Tapon and Hall, 1997; Van Aelst and D'Souza-Schorey, 1997;
Hall, 1998). Three subfamilies within this family, Rho, Rac, and cdc42,
have been well characterized. These factors are able to interact with
each other but also can be activated by different extracellular cues
acting on independent effectors to organize distinct cytoskeletal
structures (Ridley and Hall, 1992; Ridley et al., 1992; Nobes and Hall,
1995). Recent studies have shown that members of this family regulate
neuronal morphology, as well as the response of outgrowing neurites to
intercellular signals (Luo et al., 1994, 1996; Jin and Strittmatter,
1997; Kozma et al., 1997; Lamoureux et al., 1997; Threadgill et al.,
1997; Zipkin et al., 1997; Albertinazzi et al., 1998; Daniels et al., 1998; Kuhn et al., 1998, 1999).
In this study, we demonstrate a role for two GTPases, Rho and Rac, in
the regulation of dendritic motility in developing neurons. Although
levels of Rho and Rac activity influence the shape of dendritic trees
(see Threadgill et al., 1997; Ruchhoeft et al., 1999), we have focused
our analysis on their effects on the dynamism of terminal dendritic
processes. Inhibition of Rac activity by the expression of
dominant-negative Rac in ganglion cells decreased the process turnover
rate and reduced both the rate and the extent of dendritic movements.
Terminal dendritic processes persisted for a longer time than did those
in control neurons, changing their lengths less markedly and at slower
speeds. Conversely, upregulation of Rac function by expression of
constitutively active Rac increased process turnover rate. Rac+ did
not, however, increase the rate and extent of process motility
significantly, perhaps because basal motility is already close to its
maximum level in the range modulated by Rac function.
In contrast to Rac, the downregulation of Rho activity by the
expression of the dominant-negative mutant of Rho increased the rate
and extent of process motility and also increased process turnover.
Conversely, the upregulation of Rho activity by expression of a
constitutively active mutant of Rho had the opposite effect on these
motility parameters, indicating that, like Rac, Rho may also modulate
the dynamics of remodeling by changing its level of activation. Thus,
Rho activity acts to limit the speed and the range of remodeling events
and promotes the stability of terminal processes.
Effects of Rho and Rac on dendritic motility are generally consistent
with those on neurite outgrowth documented previously in dissociated
cells. The inhibition of Rac function decreased process outgrowth
elicited by cues such as nerve growth factor (Lamoureux et al., 1997;
Daniels et al., 1998),  1-integrin (Kuhn et al., 1998), and
acetylcholine (Kozma et al., 1997). Conversely, inhibition of Rho
activity prevented the retraction of neurites normally induced by
exogenously applied lysophospholipid acid or thrombin (Jalink et al.,
1994; Tigyi et al., 1996; Gebbink et al., 1997).
The reciprocal effects of Rac and Rho activity indicate a mutual
antagonism in their regulation of dendritic motility. The situation is
complex, in that Rac may activate Rho in some circumstances and
antagonize it in others (for review, see Mackay and Hall, 1998).
Antagonism has been noted previously in other neuronal culture systems
in which structural changes induced by the activation of one GTPase can
be antagonized or potentiated depending on whether the other GTPase is
activated or inactivated, respectively (Kozma et al., 1997; Van Leeuwen
et al., 1997; Hirose et al., 1998). This antagonism between Rac and Rho
on dendritic remodeling posits a mechanism in which the dynamics of
remodeling can be controlled precisely according to the balance of the
two regulating GTPases (Fig. 8). Importantly, dendritic remodeling
appears to be modulated by, rather than being absolutely dependent on,
Rho and Rac activity because dendritic movements persist even when
their activities are perturbed. These results are consistent with those
of Lamoureux et al. (1997) and Zipkin et al. (1997).
Roles of rapid dendritic motility
Why do dendrites remodel rapidly? We initially considered the
possibility that the rapid movements observed over tens of seconds contribute to the overall growth of the dendritic arbor, which also
takes place during the embryonic period studied. Surprisingly, however,
this seems not to be the case; as noted above, the rapid movements are
balanced across the arbor and therefore contribute little to net
growth. Instead, several observations support an alternative
possibility, that the rapid movements promote synaptogenesis. First,
the movements are primarily restricted to tertiary branches, which are
the portions of the arbor on which most synapses form. Differentiated
synapses first appear on the chick retinal ganglion cell dendrites at
E12-E13, at the time that we examine their motility (Hughes and
LaVelle, 1974; Hering and Kroger, 1996). In neonatal cat retinal
ganglion cells, filopodia have been observed by electron microscopy to
be associated with presynaptic specializations, even though the
majority of differentiated synapses are on dendritic shafts (Wong et
al., 1992). Similarly, dendritic filopodia in the developing
hippocampus have also been associated with differentiated synapses
(Fiala et al., 1998). Second, motility is high at E12-E13, when
synaptogenesis is at its peak, and then declines by E15-E16, when
synaptogenesis is more advanced. In this respect, our results are
consistent with those of Dailey and Smith (1996), Ziv and Smith (1996),
and Fischer et al. (1998), all of which report lower levels of
endogenous dendritic motility in more mature systems. Third, the
balanced movements allow dendritic branches to over time sample a
severalfold larger volume than that physically occupied at any single
point in time. As Ziv and Smith (1996) noted, this expanded volume
increases the probability that an afferent would contact its
appropriate postsynaptic partner. Fourth, intracellular modulators of
motility include the Rho family of GTPases, which are well established
as intracellular regulators of axonal motility and dendritic morphology
and have been implicated in synaptogenesis in invertebrates (Sone et
al., 1997). Finally, dendritic motility is modulated by excitatory
neurotransmission. Throughout the nervous system, patterns of synaptic
connectivity are modulated by synaptic activity (Goodman and Shatz,
1993; Lichtman et al., 1998).
How might synaptic enhancement of motility promote synaptogenesis?
Motor axons can release their neurotransmitter (acetylcholine) even
before forming close contacts with myotubes (Hume et al., 1983; Young
and Poo, 1983). If the same is true for excitatory inputs to retinal
ganglion cells, released neurotransmitter would stimulate dendritic
exploration as afferents approach, increasing the probability of close
contact. On the other hand, unchecked enhancement of motility by
glutamate receptor activation might be counterproductive, because
activity presumably increases as synaptogenesis proceeds yet the
desired outcome is a stable synapse. However, numerous extracellular
factors are known that can arrest axonal advance by causing growth
cones to collapse, and it is reasonable to imagine that some of them
might also arrest dendritic motility. For example, molecular cues such
as ephrins or semaphorins might act as stop signals, arresting
dendritic motility after contact is established and thereby overcoming
the motility-promoting effects of activity.
In this regard, the reciprocal effects of Rho and Rac on dendritic
motility may be especially pertinent. The similar effects of glutamate,
Rac activation, and Rho inhibition on dendritic dynamics (Figs. 8, 10)
invite the speculation that synaptic activity promotes motility by
activating Rac and/or inhibiting Rho. Conversely, effects of at least
one collapsing factor, lysophosphatidic acid, appear to be mediated by
activation of Rho (Jalink et al., 1994; Tigyi et al., 1996; Gebbink et
al., 1997; Kozma et al., 1997). We suggest that the Rho family of
GTPases provides a means by which the dendrite integrates multiple
extracellular factors to optimize the extent, and perhaps even the
direction, of its movement. In this way, afferents could use a
combination of diffusible and contact-mediated cues first to maximize
the probability of synaptic contact and subsequently to transform that
contact into a functional synapse.
| |
FOOTNOTES |
Received Jan. 27, 2000; revised April 4, 2000; accepted April 11, 2000.
This work was supported by grants from the Human Frontiers Science
Program and the McDonnell Foundation (R.O.L.W.), a grant from the
National Health and Medical Research Council (Australia) (B.E.F.-J.), a
grant from the National Institutes of Health (NIH) (J.R.S.), and an
instrumentation grant from NIH. We are grateful to Dr. A. Hall for
providing GTPase cDNA constructs, Drs. J. W. Lichtman, S. Eglen,
W.-B. Gan, B. Nadarajah, K. Myhr, and C. Lohman for their critical
reading of this manuscript, R. Stacy for her help in data analysis, and
Drs. J. Beiser and M. Gordon for help in statistical analysis.
Correspondence should be addressed to Dr. Rachel O. L Wong, Department
of Anatomy and Neurobiology, Washington University School of Medicine,
660 South Euclid, St. Louis, MO 63110. E-mail: wongr{at}thalamus.wustl.edu.
| |
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TOP
ABSTRACT
INTRODUCTION
