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The Journal of Neuroscience, July 23, 2003, 23(16):6546-6556
Previous Article | Next Article
Experience-Dependent Strengthening of Drosophila Neuromuscular Junctions
Stephan J. Sigrist, * Dierk F. Reiff, * Philippe R. Thiel, Joern R. Steinert, andChristoph M. Schuster Friedrich-Miescher-Laboratorium der Max-Planck-Gesellschaft, 72076 Tübingen, Germany
Abstract
Top
Abstract
Introduction
The genetic analysis of larval neuromuscular junctions (NMJs) of Drosophila has provided detailed insights into molecular mechanisms that control the morphological and physiological development of these glutamatergic synapses. However, because of the chronic defects caused by mutations, a time-resolved analysis of these mechanisms and their functional relationships has been difficult so far. In this study we provide a first temporal map of some of the molecular and cellular key processes, which are triggered in wild-type animals by natural larval locomotor activity and then mediate experience-dependent strengthening of larval NMJs. Larval locomotor activity was increased either by chronically rearing a larval culture at 29°C instead of 18 or 25°C or by acutely transferring larvae from a culture vial onto agar plates. Within 2 hr of enhanced locomotor activity, NMJs showed a significant potentiation of signal transmission that was rapidly reversed by an induced paralysis of the temperature-sensitive mutant parats1. Enhanced locomotor activity was also associated with a significant increase in the number of large subsynaptic translation aggregates. After 4 hr, postsynaptic DGluR-IIA glutamate receptor subunits started to transiently accumulate in ring-shaped areas around synapses, and they condensed later on, after chronic locomotor stimulation at 29°C, into typical postsynaptic patches. These NMJs showed a reduced perisynaptic expression of the cell adhesion molecule Fasciclin II, an increased number of junctional boutons, and significantly more active zones. Such temporal mapping of experience-dependent adaptations at developing wild-type and mutant NMJs will provide detailed insights into the dynamic control of glutamatergic signal transmission.
Key words: larval locomotion; experience-dependent strengthening; time-resolved analysis; synaptic protein synthesis; glutamate receptor; bouton-outgrowth; neuromuscular junction; Drosophila
Introduction
Over the last decade the developing neuromuscular junction (NMJ) of Drosophila larvae has gained much attention as a simple synaptic model system for the genetic analysis of activity-dependent processes at glutamatergic synapses (Budnik et al., 1990; Zhong et al., 1992
In contrast, a time-resolved characterization of the physiological alterations that are involved in different forms of short-term and long-term plasticity has been well established at neuromuscular junctions of crayfish and other crustaceans (Atwood et al., 1975
In the present study, we therefore established an experimental framework to uncover the temporal sequence of events involved in activity-dependent alterations at developing NMJs of Drosophila larvae. Our results show that the locomotor activity of wild-type and mutant larvae can be controlled experimentally in an acute and chronic manner. Increased locomotor activity of wild-type larvae results in a characteristic sequence of physiological and molecular key events that are involved in the long-term strengthening of junctional signal transmission in vivo. Thus, the experimental control of larval locomotor activity now allows a time-resolved dissection of the molecular and genetic mechanisms underlying experience-dependent processes at glutamatergic synapses.
Materials and Methods
Genetics
We used the w- strain CS10 (Yin et al., 1995Larval culture and developmental matching
We have standardized our larval culture to generate consistent and reproducible conditions for larval development with as few as possible individual variances. This was achieved by using a reproducible number of developing larvae (24 hr egg collections from 40 fertilized females at 25°C) and by controlling their rearing conditions in standard 26-mm-diameter fly stock vials [temperature (18, 25, 29°C), humidity (65%), food quality (10 ml of fresh cornmeal food: 6.4% corn meal, 6.4% malt extract, 1.44% dry yeast, 0.8% soy bean meal, 1.76% molasses, 0.64% agar, 0.5% propionic acid)]. Larvae from such 24 hr egg collections rapidly convert the upper few millimeters of the solid cornmeal food into soft slurry, in which the feeding and developmental conditions appear to be very similar for each individual animal.Because the rearing temperature considerably affects the speed of larval development, we could not use the elapsed time after egg deposition to match the developmental status of larvae. However, the rearing temperature did not alter the animal size shortly before pupation [average length ± SD of the mean (SDM) of wandering stage third instar larvae reared at 18°C: 4.1 ± 0.4 mm, n = 25; 25°C: 4.2 ± 0.5 mm, n = 25; 29°C: 4.1 ± 0.2 mm, n = 23]. We therefore used the larval body size as a staging criterion to developmentally match mid third instar male larvae (feeding stage) before processing.
Analysis of larval locomotion
Size-matched mid third instar larvae (feeding stage) were video taped directly either from the wall of culture vials (average larval length ± SDM: 3.6 ± 0.6 mm, n = 40) or from the surface of agar plates (average larval length: 3.7 ± 0.2 mm, n = 13), onto which they have been transferred after a short rinse in water. The temperature of agar plates was controlled with a custom-made water bath, in which the bottom of the agar plate dipped into circulating water of 18, 25, or 29°C. Video sessions started 20-60 min after the transfer of larvae onto agar plates, and they typically lasted 10-15 min; in a few experiments, they lasted up to 90 min. These recordings were used for off-line analysis of (1) larval locomotor parameters during stretches of fast-forward locomotion and (2) the total crawling distance over time.Locomotor parameters. From each recorded animal we first selected two stretches of fast-forward locomotion, which is characterized by a straight and uninterrupted crawling path. We measured the larval length (ll), the moved distance (d1 and d2), the time spent (t1 and t2), and the number of performed contractions (c1 and c2). From these measurements we calculated the stride length [(d1/c1 + d2/c2)/2ll], i.e., the moved distance per contraction wave, the stride frequency [(c1/t1 + c2/t2)/2], and the speed [(d1/t1 + d2/t2)/2ll].
Crawling distance. This is a measurement of the length of the entire crawling path covered within 45 min (see Fig. 2a,b) or 10 min (see Fig. 2c-e) after an equilibration period of 20-60 min.
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Figure 2. Temperature dependence of larval locomotor activity. Larvae were reared at the indicated temperatures and video taped as mid third instar larvae (feeding stage) either from the wall of culture vials (a) or from the surface of isothermal agar plates (b-e). Shown are the following locomotor parameters during stretches of fast-forward locomotion (see Materials and Methods) of size-matched animals: moved distance per contraction wave (stride-length), frequency of contraction waves (stride-frequency), and the average speed of locomotion. To estimate the overall locomotor activity of larvae, we monitored the crawling distances (see Materials and Methods) of size-matched animals over 45 min (a, b) or 10 min (c-e). a, b, At a given temperature, wild-type animals showed similar locomotor parameters during stretches of fast-forward locomotion on both culture vials and agar plates. However, because of the strong differences of larval behavior within the food slurry of culture vials and on agar plates, the overall larval crawling distance was significantly larger on 25°C agar plates than in 25°C food vials. At 29°C the measured parameters of fast-forward locomotion were significantly higher than at 18°C, resulting in a significantly larger larval crawling distance per 10 min interval on 29°C agar plates versus 18°C agar plates (c). d, In dglurIIA-ko mutants the stride length remained unaltered at 18 and 29°C, whereas stride frequency and speed of locomotion showed significant temperature-dependent changes. However, these temperature-dependent differences did not significantly alter the crawling distance. e, pabpP970/+ mutants showed enhanced locomotor parameters during fast-forward locomotion at 18°C; however, the crawling distance over 10 min remained similar to wild type. Rearing at 29°C further increased the locomotor parameters and resulted in similarly larger crawling distances as in wild-type larvae. The number of animals was as follows: locomotor parameters: a, 21, 40, 42; b, 11, 13, 25; d, 5, 6; e, 11, 18; crawling distance: a, 4; b, 20, c,: 9, 8; d, 9, 19; e, 16, 11. Data represent means ± SEM.
NMJ size
Size-matched mid third instar male larvae (feeding stage) were filleted and processed for immunofluorescence with antibodies recognizing the cell adhesion molecule Fasciclin II (Fas II) [monoclonal antibody (mAb) 1D4] or the anti-HRP-epitope (Sigma, St. Louis, MO) as described previously (Schuster et al., 1996). The number of type I boutons was counted from muscles 6/7 of abdominal segment 2 or 3, the dimensions (length x width of the exposed muscle surface) of which were comparable as measured with an eyepiece micrometer (average inner muscle 6/7 surface area ± SDM: 43.9 ± 5.9 eyepiece units2, n = 200; 1 U21400 µm2). To obtain a value that expresses the size of a given NMJ per muscle surface area (see Fig. 1, "# of boutons/muscle surface area"), we divided the counted number of boutons by the measured muscle surface area of that muscle.
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Figure 1. Increased outgrowth of NMJs at 29°C rearing temperature. a,b, Confocal images of anti-HRP-labeled NMJs (muscle 6/7, abdominal segment 2) of wild-type larvae reared at 18°C (a) or 29°C (b). Scale bar, 20 µm. c-e, Quantification of NMJ size on muscle 6/7 of abdominal segment 2 (see Materials and Methods) in wild-type larvae (c), dglur-IIA-ko animals (dglurIIAAD9/df(2L)clh4) (d), and pabpP970/+ larvae (e) that have been reared at the indicated temperatures. Larvae reared at 29°C developed significantly larger NMJs than animals raised at 25 or 18°C (*p < 0.001). This effect was particularly prominent in pabpP970/+ larvae but significantly suppressed in dglur-IIA-ko animals (p << 0.001). Note that pabpP970/+ larvae showed a strong increase in bouton outgrowth at 25°C, whereas NMJs of wild-type and dglur-IIA-ko animals developed simple NMJs at this rearing temperature. Data represent means ± SEM.
Electrophysiology
Experiments were performed on size-matched mid third instar male larvae at 22°C. All recordings of evoked excitatory junctional currents (eEJCs) and miniature EJCs (mEJCs) were performed in two-electrode voltage clamp mode as described previously (Reiff et al., 2002microelectrodes filled with 2 M KCl. Cells with a resting potential more negative than -60 mV and an input resistance Rin of
5 M
U) caused by injection of
Antibodies
We used the following antibodies: Fasciclin II: mAb 1D4 (gift of Corey S. Goodman, University of California Berkeley, Berkeley, CA); DGluR-IIA: DM2 (gift from Yoshiaki Kidokoro, Gunma University, Gunma, Japan); eukaryotic initiation factor 4e (eIF4e) (gift of Paul Lasko, University of Montreal, Montreal, Canada); anti-HRP (Sigma).Quantification of immunofluorescence signals
Size-matched mid third instar male larvae (feeding stage) of 18 and 29°C reared wild-type Drosophila were filleted and processed in the same vial for immunofluorescence with antibodies recognizing DGluR-IIA (DM2) and Fas II (mAb 1D4) as described previously (Schuster et al., 1996). Three isolated type Ib boutons (muscle 6/7, abdominal segment 2) were randomly selected in the anti-Fas II channel from a recorded confocal image stack, and the average fluorescence signal of this selection was determined in both channels. From these mean pixel values we subtracted the mean background pixel value obtained similarly from a nearby muscle region of the same shape. This quantification of the mean pixel values was performed at six nonoverlapping areas of a given NMJ and subsequently averaged. We analyzed six animals per experimental condition.Electron microscopy
Ultrastructural examinations were performed as described previously (Sigrist et al., 2002
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Figure 6. Ultrastructural effects of elevated locomotor activity. a, Representative transmission electron microscopy image of a type Ib bouton of a wild-type larva (muscle 6/7, abdominal segment 2). Marked are synapses (dense areas between arrowheads), the subsynaptic reticulum (ssr), and a presynaptic dense body (T-bar, arrow). Large sequential series of such images were used to reconstruct junctional branches and analyze ultrastructural changes in larvae reared at 18 or 29°C (Table 1; see Materials and Methods). b, Rearing at 18 and 29°C resulted in a similar density of synapses with T-bars (i.e., active zones; gray bars) and without T-bars (white bars). Because 29°C larvae develop more synapse-harboring boutons, this lead to a significant increase in the total number of active zones per NMJ compared with 18°C reared larvae (black bars; p < 0.001). Data are taken from Table 1 and given as means ± SEM.
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Table 1. Summary of ultrastructural analysis
Results
Rearing temperature can alter the morphological outgrowth of developing Drosophila NMJs
The morphological analysis of larval NMJs of Drosophila has revealed that the number of synaptic boutons varies even within an isogenic population of animals of comparable age and size (unpublished observations). This variability in NMJ size can be reduced by controlling the culture conditions of the animals to be examined (Schuster et al., 1996aWe first tested whether the rearing temperature affects the development of NMJs. Although the NMJ morphologies of mid third instar wild-type larvae reared at 18 or 25°C were relatively simple (Fig. 1a), size-matched animals reared at 29°C showed consistently larger and apparently more complex NMJs on similarly sized larval muscles (Fig. 1b). In fact, quantification of muscle 6/7 NMJ size by counting the number of synaptic boutons and measuring exposed muscle surface in the filet preparations area of the muscle 6/7 pair revealed a significant increase in the normalized NMJ size in 29°C reared animals compared with larvae raised at 18 or 25°C (Fig. 1c). These temperature treatments of developing Drosophila larvae affected neither the size of larval body wall muscles nor the viability and fertility of emerging adult flies, suggesting that 29°C rearing of Drosophila larvae triggers cellular signals that can accumulate in an over-proportional outgrowth of junctional boutons on larval muscles of similar sizes.
Temperature-induced bouton outgrowth requires intact synaptic signal transmission
The temperature-induced bouton outgrowth at developing NMJs of wild-type larvae was similar in shape and dimension to that described previously for model genotypes of activity-dependent junctional plasticity, such as the hyperactive potassium channel mutant eag1, Sh102 (Budnik et al., 1990Rearing of dglurIIA-ko mutants at 18 or 25°C revealed no difference in the morphological development of NMJs compared with wild-type controls (Fig. 1c,d). Rearing of dglurIIA-ko mutants at 29°C resulted in a small but significant (p < 0.01) increase in the number of presynaptic boutons relative to 18 or 25°C reared mutants (Fig. 1d, right bar). However, compared with similarly raised wild-type animals (Fig. 1c, right bar), the stimulation of bouton outgrowth at 29°C was significantly suppressed in this mutant (p << 0.001). These results show that the temperature-induced outgrowth of wild-type NMJs depends primarily on an intact synaptic expression of the DGluR-IIA subunit.
On the basis of the specific defects in synaptic signal transmission described for this postsynaptic glutamate receptor mutant (Petersen et al., 1997
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Figure 3. Experience-dependent strengthening of Drosophila NMJs. Two-electrode voltage-clamp recording of eEJCs and mEJCs from muscle 6 of abdominal segment 2. a, Shown are representative traces of mEJC recordings (top panels) and average traces of 10 consecutively recorded eEJCs of animals raised at either 18 or 29°C. b, All locomotor-stimulated animals showed a significantly larger junctional quantal content and thus enhanced junctional signal transmission compared with controls. This effect was already maximal after 2 hr of enhanced locomotor activity. Larval locomotor activity was acutely enhanced by transferring 18°C reared mid third instar larvae (feeding stage) onto agar plates (29°C) for 2 and 4 hr; chronic locomotor enhancement was achieved by continuously rearing larvae at 29°C (Fig. 2). From these animals we measured the muscle 6 input resistances Rin as an estimate of the relative muscle sizes (bottom panel, gray bars) and the amplitudes of spontaneous mEJCs and stimulation evoked eEJCs (top panel, gray and black bars). The derived junctional quantal content (mean eEJC amplitude/mean mEJC amplitude) (bottom panel, black bars) gives an estimate of the number of presynaptic vesicles released per action potential and thus represents a measure of the efficacy of evoked junctional signal transmission. Note that the slight but significant reduction of mEJCs in 4 hr stimulated animals is likely caused by the somewhat smaller muscle cells (larger Rin) of this animal population. Because the eEJC amplitudes are reduced proportionally in these cells, the quantal content is restored. The number of analyzed cells per experimental condition is given in b, below the top panel. c, Intracellular recordings of mEJPs and eEJPs in wild-type larvae and the temperature-sensitive paralytic mutant parats1 revealed that 2 hr of enhanced larval locomotor activity at permissive temperature (22°C agar plates) results in a consistent and significant strengthening of junctional signal transmission in both genotypes (wild type, n = 7; parats1, n = 6) compared with their 18°C reared siblings (wild type, n = 11; parats1, n = 9). These larvae were then treated with a temperature-shift protocol (20 min at 34°C followed by maintained 29°C on agar plates) that results in immediate paralysis of parats1 mutants, whereas wild-type larvae continue vigorous locomotion. Within 2 hr of paralysis the eEJP amplitudes of parats1 mutants dropped to the control value (n = 5), whereas signal transmission at wild-type NMJs was enhanced further (n = 6). The mEJP amplitudes of all three experimental conditions were similar (wild type 18°C:1.17 ± 0.07 mV; 2 hr 22°C plate:1.06 ± 0.08 mV; +2 hr paralysis protocol: 1.06 ± 0.05 mV; parats1 18°C: 1.02 ± 0.12 mV; 22°C plate: 0.91 ± 0.06 mV; +2 hr paralysis protocol: 1.14 ± 0.11 mV). d, The quantal content (expressed as percentage of control genotypes) is plotted as a function of the normalized NMJ size. Wild-type larvae that have been chronically reared at either 18 or 29°C develop NMJs with a typical relationship between NMJ size and transmission strength (black and white pentagons). A similar relationship has been described previously in several model genotypes of junctional plasticity, such as the transgenic overexpression of the glutamate receptor subunit DGluR-IIA (black and white circles) and the pabpP970/+ mutant (black square and white triangle) (Sigrist et al., 2002
We similarly analyzed larvae that were heterozygous mutant for the poly(A)-binding-protein locus (pabpP970/+) (Sigrist et al., 2000
Experimental control of larval locomotor activity
Our above results suggest that the observed morphological phenotypes require intact synaptic signal transmission at NMJs. NMJs couple neuronal excitation to muscle contractions, which in the case of the single-fibered body wall muscles of Drosophila larvae drive body movements and ultimately larval crawling. It is therefore likely that the neuronal activity, which is transmitted by NMJs, is reflected in the crawling behavior of larvae. Crawling of Drosophila larvae is a simple locomotor behavior that has been analyzed extensively to detect alterations in the locomotor pattern in wild-type and mutant animals (Sokolowski, 1980At a given rearing temperature, wild-type animals showed similar stride lengths, frequencies of contraction waves, and crawling speeds during stretches of fast-forward locomotion either on walls of culture vials or on agar plates (Fig. 2a,b). These findings suggest that fast-forward locomotion is a rather stereotypic locomotor behavior that appears to be used by larvae on relatively clean surfaces. It is important to note, however, that feeding-stage third instar larvae, which are kept in the soft food slurry of culture vials, stay feeding within the food most of the time and only occasionally leave the food for short stretches of fast-forward locomotion on the vial wall. In contrast, larvae transferred onto isothermal agar plates show an almost continuous locomotor performance with only short resting phases, presumably for reorientation. These obvious behavioral differences of feeding stage third instar larvae in food vials and on agar plates are well reflected in the crawling distances measured over 45 min (Fig. 2a,b, white bars) (see Materials and Methods), which are significantly longer on agar plates (160.8 ± 10.6 cm; n = 20) than in food slurry (39.8 ± 13.8 cm; n = 4). We therefore conclude that larvae that have been transferred onto isothermal agar plates have a significantly enhanced locomotor activity compared with their siblings in culture vials.
We found further that increased larval rearing temperatures are associated with significant increases of all analyzed locomotor parameters in vials and on plates (Fig. 2a,b). These changes are well reflected in the crawling distances measured over 10 min on agar plates (Fig. 2c, white bars), with a significantly enhanced locomotor activity of larvae on 29°C agar plates compared with those at 18°C. These results demonstrate that the locomotor activity of size-matched third instar larvae is subject to temperature-dependent and environmental changes, which can be controlled experimentally.
Elevated locomotor activity induces NMJ outgrowth
A similar behavioral analysis of dglurIIA-ko mutants revealed an unaltered stride length at 29 and 18°C but significant changes in the frequency of contraction waves and the speed of locomotion (Fig. 2d, gray and hatched bars). However, these significant changes did not translate into a similarly large increase of the measured crawling distance over 10 min as seen in wild-type animals at 29°C (Fig. 2c,d, white bars). This observation may be explained by the obviously altered locomotor pattern of dglurIIA-ko mutants, which shows only short stretches of uninterrupted locomotion and longer and more frequent resting phases. dglurIIA-ko mutants still developed slightly larger NMJs at 29°C than at 18°C (Fig. 1d); however, this additional bouton outgrowth at 29°C was significantly suppressed compared with that observed in wild-type animals (Fig. 1c). These data suggest that the specific defects in synaptic signal transmission at NMJs are responsible for both the failure of dglurIIA-ko mutants to significantly enhance the overall locomotor activity at 29°C and the strong suppression of induced bouton outgrowth. They also suggest that the temperature-dependent changes of some of the locomotor parameters are sufficient to induce NMJ growth at a low rate. We therefore conclude that it is not the increased rearing temperature itself that causes the observed large-scale overgrowth of NMJs in wild-type larvae; rather, it appears that elevated temperature results in enhanced overall locomotor activity, which then seems to trigger the outgrowth of additional boutons.To test this idea, we morphologically analyzed NMJs of mid third instar wild-type larvae that were raised at 25°C and experienced increased locomotor activity on 25°C agar plates for 12-18 hr (see Materials and Methods) or that were kept for the same time in 25°C culture vials. As mentioned above, the crawling distance covered by larvae on agar plates is approximately fourfold at 25°C compared with that of their siblings within the food slurry. Larvae that experienced such enhanced locomotor activity for 12-18 hr developed slightly but significantly more boutons per muscle surface area than animals with lower locomotor activity over the entire period (normalized NMJ size in vials: 2.25 ± 0.09; 100 ± 4%, n = 23; on plates: 2.49 ± 0.06; 111 ± 3%, n = 50; p = 0.04). These on average slightly larger NMJs in animals with acutely increased locomotor activity show that bouton outgrowth can indeed be induced in the absence of temperature shifts. However, compared with chronic treatments of larvae, e.g., by continuous 29°C rearing or mutant backgrounds (e.g., pabpP970/+ or eag, Sh, or transgenic DGluR-IIA overexpression), which typically result in >50% larger and more complex NMJs (Fig. 1c,e) (Sigrist et al., 2002
We finally analyzed the locomotor behavior of the abovementioned mutant of the pabp gene, pabpP970/+, which enhances growth stimuli and results in larger NMJs than wild-type animals (Fig. 1c) at all tested rearing temperatures (Fig. 1e) presumably because of its sensitized subsynaptic protein synthesis machinery (Sigrist et al., 2000
Experience-dependent strengthening of junctional signal transmission is rapid and reversible
Several recent reports have suggested that the morphological development of larval NMJs is tightly correlated with the strength of junctional signal transmission (Budnik et al., 1990To exclude any potential temperature effects on the development of the junctional transmission strength, we included an analysis of the temperature-sensitive paralytic mutant parats1 (Ganetzky, 1984
22°C. At restrictive temperatures, however, such as 29°C or higher, the voltage-gated sodium channel encoded by the gene para fails to operate and eliminates action potential propagation and larval locomotion. We found that 2 hr of surface locomotion on agar plates at permissive 22°C resulted in a consistent strengthening of junctional signal transmission in both genotypes, as indicated by their significantly larger eEJPs compared with animals that remained in the food slurry at 18°C (Fig. 3c). After 3 hr of locomotor stimulation on 22°C agar plates, we transferred the larvae onto agar plates at 34°C for 20 min and then maintained them at 29°C. This protocol resulted in an immediate and persisting paralysis of parats1 mutants, whereas wild-type animals continued vigorous surface locomotion. Within 2 hr of paralysis the eEJP amplitudes of parats1 mutants dropped significantly to a value close to the one before the experiment, whereas signal transmission at wild-type NMJs remained enhanced. These results demonstrate that experience-dependent strengthening of junctional signal transmission does not rely on a temperature shift to 29°C. They instead suggest that enhanced locomotor activity on agar plates can trigger a rapid and reversible strengthening of junctional signal transmission. Moreover, within the up to 6 hr time window of these experiments, we did not observe obvious morphological changes at NMJs, demonstrating that the rapid physiological changes occur in the absence of large-scale morphological growth (Fig. 3d). This finding is consistent with our morphological results, which suggested that the acute induction or execution of additional bouton outgrowth is a rather slow process.
Taken together, our results show that enhanced larval locomotor activity can trigger a rapid and reversible strengthening of junctional signal transmission even in the absence of large-scale morphological alterations. Bouton outgrowth appears to start with a considerable delay relative to the acutely induced physiological changes, so that chronic locomotor stimulation results in NMJs with a typical relationship between transmission strength and NMJ size (Fig. 3d). It therefore appears that the tight correlation between NMJ size and transmission strength that has been described for several genetic backgrounds (Budnik et al., 1990
Experience-dependent regulation of subsynaptic protein synthesis
Because of the presumed major importance of local subsynaptic protein synthesis in the spatial organization of synaptic and morphological changes of neuronal connectivity (Martin et al., 2000
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Figure 4. Experience-dependent regulation of subsynaptic protein synthesis. a, Large eIF4e aggregates (Sigrist et al., 2000
To control for potential temperature effects on general protein synthesis that are not triggered by locomotion, we included the temperature-sensitive paralytic mutant parats-1 (Ganetzky, 1984
We performed a similar analysis with pabpP970/+ mutants, which showed a very large increase in the number of subsynaptic eIF4e aggregates after 5 hr of sustained surface locomotion on 29°C agar plates (Fig. 4e). This finding is consistent with the idea that the subsynaptic translation machinery in pabpP970/+ mutants is genetically sensitized (Sigrist et al., 2000
Experience-dependent upregulation of postsynaptic DGluRIIA expression precedes the downregulation of perisynaptic Fasciclin II
We recently showed that the strengthening of junctional signal transmission that can be observed in animals with genetically enhanced subsynaptic protein synthesis (Sigrist et al., 2000
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Figure 5. Experience-dependent upregulation of postsynaptic DGluR-IIA expression precedes the downregulation of Fasciclin II (Fas II). Shown are confocal images of boutons double labeled with antibodies recognizing the cell adhesion molecule Fasciclin II (left panels and green channel) and the postsynaptic glutamate receptor subunit DGluR-IIA (middle panels with enlarged insets and red channel). a, Control animals, which have been reared at constant 18°C in standardized larval cultures, show strong perisynaptic Fas II expression (arrowhead) and few DGluR-IIA positive synapses. b, After 4 hr of vigorous locomotor activity on 29°C agar plates, the perisynaptic Fas II expression was essentially unaltered (compare green channels), whereas DGluR-IIA showed an increased, ring-shaped immunoreactivity (arrows) at preexisting synapses (holes in Fas II expression, arrows). c, Larval rearing at 29°C, which is associated with chronically enhanced locomotor activity, leads to an enhanced overall DGluR-IIA immunoreactivity at an increased number of postsynaptic patches. The perisynaptic Fas II immunoreactivity is significantly downregulated (arrowhead, compare green channels). Scale bar, 5 µm. d, Quantification of immunofluorescence signals at NMJs (see Materials and Methods) revealed a significantly enhanced immunoreactivity of postsynaptic DGluR-IIA and a reduced immunoreactivity of Fas II in animals reared at 29°C compared with their 18°C reared sibling. Note that the enhanced DGluR-IIA immunoreactivity is caused by an increased number of DGluR-IIA patches and obviously stronger fluorescence signals per DGluR-IIA patch.
A time-resolved analysis of these events revealed that the DGluR-IIA immunoreactivity at NMJs increases visibly already after 4 hr of surface locomotion on 29°C agar plates (Fig. 5b, red channel). At this time point of acute locomotor stimulation, the DGluR-IIA immunoreactivity often showed a ring-shaped appearance at the outer edge of presumably preexisting synapses (Fig. 5b, inset). This has been rarely or never observed in control larvae (Fig. 5a), chronically stimulated animals (Fig. 5c), or mutants (Sigrist et al., 2002
Interestingly, 4 hr after acute locomotor stimulation the perisynaptic Fas II immunoreactivity remained unaltered (Fig. 5b, green channel). A visible downregulation of perisynaptic Fas II was detectable only after chronic locomotor stimulation at 29°C (Fig. 5c,d, green channel). This suggests that Fas II-mediated morphological changes are induced with a significant delay after alterations to postsynaptic glutamate receptors. Taken together, our results demonstrate that the experimental control of larval locomotor activity allows insights into the dynamics of molecular and physiological changes that are involved in the execution of experience-dependent plasticity at larval NMJs.
Experience-dependent strengthening of NMJs involves an increase in the number of active zones per NMJ
On the basis of extensive ultrastructural analyses in several mutations that enhance junctional signal transmission and morphological growth, it has been suggested recently that the number and density of active zones within NMJs are tightly regulated throughout development (Meinertzhagen et al., 1998
Discussion
So far, activity-dependent changes at Drosophila NMJs have been analyzed almost exclusively in mutants. Such mutant animals were affected in their neural excitability or in one of the potential downstream mechanisms that sense, signal, or execute alterations at NMJs. These studies have provided detailed insights into the functional relevance of individual genes for NMJ plasticity. However, because of the mostly chronic defects of mutations, the temporal sequence of the identified mechanisms remained elusive. This study therefore aimed at providing an experimental framework to uncover the temporal sequence of events involved in activity-dependent alterations at developing larval NMJs. We show that locomotor activity of larvae can be controlled experimentally and that enhanced locomotor activity triggers a cascade of, in part, reversible events that result in the long-term strengthening of larval NMJs.Temperature, locomotor activity, and experience-dependent adaptations at larval NMJs
One of the prerequisites for a time-resolved analysis of experience-dependent adaptations at Drosophila NMJs was the tight control of larval locomotor activity. Acute enhancement of larval locomotor activity was achieved by transferring larvae from food vials onto agar plates (Fig. 2c,d), a procedure that has been used extensively before as a locomotor reference in the genetic analysis of larval foraging behavior (Shaver et al., 2000Three independent lines of evidence suggest that the morphological and physiological changes at NMJs described here are triggered by enhanced larval locomotor activity and not caused by temperature treatment or plate transfer itself. First, the considerable bouton outgrowth seen in wild-type larvae reared at 29°C was significantly suppressed in 29°C reared dglurIIA-ko mutants (Fig. 1), which show defective postsynaptic signal transmission (Petersen et al., 1997
Experience-dependent strengthening of Drosophila NMJs
One of the first obvious consequences of enhanced locomotor activity was the fast enhancement of evoked junctional signal transmission, which was already maximal after 2-4 hr of locomotor stimulation on agar plates and was rapidly reversed by paralysis (Fig. 3d). The observation that the quantal sizes remained unaltered at the indicated time points of locomotor stimulation, whereas evoked junctional responses increased significantly, strongly suggests that the phases of experience-dependent strengthening of Drosophila NMJs are based primarily on an enhanced release of presynaptic vesicles per NMJ (Fig. 3b).Mechanisms that can result in a fast increase in the number of released vesicles include an enhanced presynaptic Ca2+ influx (Mallart, 1993
The number of released presynaptic vesicles can also increase at NMJs with a larger number of active release sites (Reiff et al., 2002
It is intriguing to note that the scored electrophysiological parameters were indistinguishable among most locomotor-stimulated animals (Fig. 3). This included larvae, which experienced 2-6 hr of locomotor stimulation. NMJs of these larvae showed no detectable bouton outgrowth compared with their controls (Fig. 3d, white squares), suggesting that this early phase of junctional strengthening does not rely on large-scale morphological alterations. We have shown recently that dglurIIA-ko mutants are unable to greatly enlarge their NMJs by bouton addition (Reiff et al., 2002
A temporal map of experience-dependent alterations at Drosophila NMJs
Our results show that enhanced locomotor activity results within 2 hr in a rapid and reversible enhancement of evoked junctional signal transmission and in a similarly fast stimulation of local subsynaptic protein synthesis (Fig. 4). Although it remains to be investigated whether localized subsynaptic protein synthesis could play an instructive role during these early physiological events, we have found recently that the mRNA encoding the glutamate receptor subunit DGluR-IIA (Schuster et al., 1991
Footnotes
Received Jan. 24, 2003; revised May. 21, 2003; accepted May. 23, 2003.This work was funded by the Max-Planck-Society. We thank C. S. Goodman (University of California Berkeley, Berkeley, CA) and J. Kidokoro (Gunma University, Gunma, Japan) for kindly providing reagents, E. Illgen and M. Langegger for excellent technical assistance, and S. Marella for critical comments on this manuscript.
Correspondence should be addressed to C. M. Schuster, Friedrich-Miescher-Laboratorium der Max-Planck-Gesellschaft, Spemannstrasse 39, 72076 Tübingen, Germany. E-mail: christoph.schuster{at}tuebingen.mpg.de.
S. J. Sigrist's current address: European Neuroscience Institute Göttingen, Max-Planck-Institute for Biophysical Chemistry, Waldweg 33, 37073 Göttingen, Germany.
D. F. Reiff's current address: Max-Planck-Institute of Neurobiology, Neur
