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Previous Article | Next Article
The Journal of Neuroscience, August 15, 2000, 20(16):6039-6047
Cysteine-String Protein Increases the Calcium Sensitivity of Neurotransmitter Exocytosis in Drosophila
Ken Dawson-Scully2, Peter Bronk1, Harold L. Atwood2, and Konrad E. Zinsmaier1 1 Department of Neuroscience, University of Pennsylvania School of Medicine, Philadelphia, Pennsylvania 19104-6974, and 2 Department of Physiology, University of Toronto, Toronto, Ontario M5S 1A8, Canada
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Previous studies suggest that the vesicular cysteine-string protein (CSP) may modulate presynaptic Ca2+ channel activity in fast neurotransmitter release. To test this hypothesis, we analyzed the dynamics of presynaptic Ca2+ ion influx with the Ca2+ indicator fluo-4 AM at csp mutant neuromuscular junctions of Drosophila. From 24 to 30°C, stimulus-evoked, relative presynaptic Ca2+ signals were increasingly larger in csp mutant boutons than in controls. Above 30°C, Ca2+ signals declined and were similar to controls at 34°C. A prolonged decay of Ca2+ signals in mutant boutons at high temperatures indicated abnormally slow Ca2+ clearance. Cytosolic Ca2+ at rest was determined with the ratiometric Ca2+ indicator fura-2 AM and was similar in mutant and control boutons at 24°C but higher in mutant boutons at 34°C. Despite larger Ca2+ signals in mutant boutons, evoked neurotransmitter release was always reduced in csp mutants and exhibited pronounced facilitation. Thus, a lack of Ca2+ entry cannot explain the reduction of neurotransmitter release in csp mutants. At all temperatures tested, raising extracellular Ca2+ increased transmitter release elicited by single stimuli in csp mutants. Collectively, these data suggest multiple functions for CSP at synaptic terminals. Increased Ca2+ signals coupled with reduced release suggest a direct function of CSP in exocytosis downstream from Ca2+ entry. Because the reduction of evoked release in csp mutants is counteracted by increased Ca2+ levels, we suggest that CSP primarily increases the Ca2+ sensitivity of the exocytotic machinery.
Key words: cysteine-string protein; Ca2+ channel; syntaxin; neurotransmitter release; exocytosis; synaptic transmission; Ca2+ clearance; Drosophila; neuromuscular junction; Ca2+ measurement
INTRODUCTION
Cysteine-string protein (CSP), originally identified as a synapse-associated antigen in the nervous system of Drosophila (Zinsmaier et al., 1990
), is associated with secretory vesicles and is conserved from invertebrates to man (for review, see Umbach et al., 1995
Coexpression of Torpedo CSP RNA in frog oocytes altered the activity of ectopically expressed N-type Ca2+ channels (Gundersen and Umbach, 1992
Regulation of Ca2+ channels, however, is unlikely to be the only function of CSP. An increase or decrease of CSP levels in PC12 and insulin-secreting cells severely reduced exocytosis without affecting transmembrane Ca2+ fluxes, suggesting that CSP may mediate a direct step of exocytosis (Brown et al., 1998
The ability of CSP to interact with syntaxin (Nie et al., 1999
MATERIALS AND METHODS
Fly stocks
Flies were raised on standard molasses food at 25°C. The homozygous semi-lethal cspU1 allele is a molecular null mutation deleting the entire csp gene and was generated by heat-shock-enhanced recombination between two P elements flanking the csp gene (Eberle et al., 1998Electrophysiology
Both voltage-clamp and current-clamp recordings were made at the indicated temperatures from muscle 6 in the anterior ventral abdomen (primarily abdominal segment A3) of control and mutant climbing third instar larvae raised at 18°C. Dissections and recordings were made in HL3 medium (Stewart et al., 1994. Voltage signals were amplified with an Axopatch 1D amplifier (Axon Instruments, Foster City, CA), filtered at 1 kHz, and digitized at 5 kHz directly to disk with a DigiData 1200 interface and pClamp 6.0 software (Axon Instruments). To evoke an excitatory junction potential (EJP), we stimulated the segmental nerve (0.1 msec pulse duration) at 2.5-3 times the stimulus amplitude required for a threshold response with a fire-polished glass suction electrode (10 µm diameter tip opening) filled with extracellular saline. The whole-cell EJPs were the combined responses of the two axons innervating muscles 6 and 7 (Kurdyak et al., 1994
80 mV. The voltage-sensing electrode had a resistance of 18-30 M
Calcium imaging procedures
Loading of nerve terminal boutons with the calcium indicator fluo-4 AM for Ca2+ imaging was performed using a modified version of the protocol described by Karunanithi et al (1997)F/Frest), was expressed as the change in fluorescence (Fstim
bx + ce
RESULTS
Ca2+ signals persist in csp mutants at temperatures above 30°C
In previous reports on Drosophila csp mutants, both evoked neurotransmitter release elicited by single stimuli (Umbach et al., 1994
Surprisingly, both control and csp null mutant boutons loaded with fluo-4 AM showed robust increases in presynaptic Ca2+ signals when stimulated at temperatures above 30°C (Fig. 1A), even after prolonged thermal equilibration. Mutant boutons exhibited a much slower time course of decay for the Ca2+ signal, especially at the higher temperatures (Fig. 1A). Sometimes boutons of csp mutants failed to regain their resting fluorescence values, unlike control boutons. For example, when the original "standard" Drosophila solution (Jan and Jan, 1976
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Figure 1. Ca2+ imaging of csp mutant and control neuromuscular junctions with fluo-4 AM. A, At 34°C, control and cspU1 null mutant terminals were stimulated at 40 Hz for 5 sec in HL3 solution. Both terminals exhibit a large Ca2+ signal; the csp mutant terminal recovers more slowly than the control terminal. B, Images of boutons in cspU1 mutants stimulated for 2 min (0-120 sec) at 10 Hz in standard solution at 22 and 34°C. Signals are observed at both temperatures, but recovery was incomplete at 34°C. C, Spontaneous Ca2+ flash phenomenon observed in cspU1 boutons in HL3 solution containing 3 mM external Ca2+ when the temperature is increased at a rate of 1°/min. At 28°C, the cspU1 boutons exhibited a large spontaneous Ca2+ signal; high Ca2+ persisted in the terminals at higher temperatures. Scale bars, 2 µm.
Because the results obtained with fluo-4 AM differed from those reported by Umbach et al. (1998)
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Figure 2. Ca2+ imaging of csp mutant neuromuscular junctions with calcium crimson AM in 2 mM extracellular calcium. A, Images of cspU1 mutant boutons stimulated for 2 min at 10 Hz in standard solution at 21 and 34°C. Signals are observed in the same preparation at both temperatures. Note higher resting fluorescence at 34°C. B, Mean peak Ca2+ signals at the two temperatures 21 and 34°C after 2 min of stimulation at 10 Hz. A larger signal is observed at 34°C, as shown with the Ca2+ indicator fluo-4 AM.
Although Ca2+ entry persisted at nonpermissive temperatures, csp mutant boutons were more readily incapacitated. The occasional occurrence of spontaneous Ca2+ "flashes" at high external Ca2+ (>2 mM) suggested greater susceptibility of mutant boutons to increased temperature (Fig. 1C). In the example shown, the temperature was slowly raised. At 28°C, a sudden large increase in Ca2+ occurred, affecting all boutons in one branch of the nerve terminal. Once the spontaneous flash had occurred, elevated Ca2+ persisted in the boutons, and they became unresponsive to stimulation of their parent motor axon. Sometimes, an apparently irreversible change (manifested as persistent elevation in [Ca2+]i) occurred spontaneously in csp mutant boutons in HL3 solution, provided that 3 or 4 mM Ca2+ was present; however, such events were not observed in control boutons and rarely in mutant boutons in solutions containing 1 mM [Ca2+]e. The observations indicate that csp mutant boutons are adversely affected by high temperature and sometimes irreversibly altered because unregulated Ca2+ accumulation. Nevertheless, changes in Ca2+ can almost always be detected in mutant boutons at high temperatures in HL3 solution containing 1 mM Ca2+, which preserves responsiveness of the boutons to stimulation of the motor axon.
Enhanced facilitation of neurotransmitter release in csp mutants
Having established that nerve-evoked Ca2+ signals can be detected in both control and csp null mutant boutons over a wide range of temperatures, we investigated the dynamic features of neurotransmitter release during repetitive stimulation to study the relationship between depolarization-dependent Ca2+ entry and neurotransmitter release in csp mutants. Neurotransmitter release was assayed at larval neuromuscular junctions of muscle 6 by TEVC recordings of nerve-evoked EJCs in [Ca2+]e ranging from 1 to 8 mM at 23°C. In 1 mM [Ca2+]e, 30 Hz stimulation rapidly depressed control EJC amplitudes (77 ± 3%, mean ± SEM) but facilitated EJCs of cspX1 mutants by 258 ± 42% (Fig. 3A). Similar results were obtained with other csp null alleles, such as cspU1 (data not shown). Facilitation of EJCs at mutant NMJs decreased progressively as [Ca2+]e was increased (Fig. 3B-D). Specifically, mutant preparations showed much less facilitation in 4 (159 ± 20%), 6 (130 ± 18%), and 8 (116 ± 18%) mM than at 1 mM [Ca2+]e; in fact, facilitation was negligible in [Ca2+]e of 8 mM (Fig. 3D). Control responses, however, showed a further relative depression of neurotransmitter release in elevated [Ca2+]e; EJCs declined to 53% of the initial amplitude during repetitive stimulation in 8 mM [Ca2+]e.
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Figure 3. Facilitation of transmission at csp mutant neuromuscular junctions. Postsynaptic responses at 23°C in csp null mutants show facilitation of evoked neurotransmitter release under conditions in which control responses show a depression. EJCs at Drosophila larval NMJs were recorded under two-electrode voltage clamp at different [Ca2+]e while stimulating the motor nerve at 30 Hz. Symbols represent mean EJC amplitudes normalized to the first response. Error bars indicate SEM. A, In 1 mM, pronounced facilitation occurs in the cspX1 null mutant. Normalized mutant amplitudes measured for pulses 2-10 are significantly different from control (p < 0.02, Student's t test). B, At 4 mM Ca2+, facilitation of mutant responses is reduced compared with the results obtained in 1 mM Ca2+, and all responses are significantly different from control (p < 0.02, Student's t test). C, Facilitation of csp mutant responses is further reduced in 6 mM Ca2+ (p < 0.02, Student's t test). D, In 8 mM Ca2+, facilitation of csp mutant responses becomes negligible, because none of the subsequent mutant responses (2-10) is significantly different from controls (p > 0.06, Student's t test). E, Absolute EJC amplitudes in 1 mM Ca2+ normalized for muscle size by dividing the current amplitude by the cell capacitance. All mutant EJC amplitudes in 1 mM Ca2+ are significantly different from control (p < 0.04, Student's t test). F, Absolute EJC amplitudes in 8 mM Ca2+. None of the mutant EJC amplitudes are significantly different from control (p > 0.1, Student's t test).
A comparison of absolute EJC amplitudes of csp and control NMJs showed that, despite greater facilitation (Fig 3A), neurotransmitter release in csp mutants was nevertheless significantly reduced compared with controls after repetitive stimulation in 1 mM [Ca2+]e (Fig. 3E). During the 30 Hz stimulus, the initial EJC amplitude in csp mutants in 1 mM [Ca2+]e was reduced by 84 ± 2% compared with controls, whereas the amplitude of the 10th EJC was reduced by 44 ± 4% (Fig. 3E). The convergence of absolute EJC amplitudes from control and csp mutants was attributable to depression of control and facilitation of mutant responses. Consistently, in 8 mM [Ca2+]e, this convergence led to similar absolute EJC amplitudes in mutants and controls (p > 0.1, Student's t test) (Fig. 3F), because facilitation of mutant responses was negligible, whereas control responses were further depressed (Fig. 3D).
The "rescue" of the mutant defect in neurotransmitter release was not dependent on the combination of high [Ca2+]e and high-frequency stimulation. High [Ca2+]e was sufficient to rescue csp mutant responses elicited by single stimuli at 0.2 Hz (Fig. 4). In controls, EJC amplitudes did not significantly increase beyond 4 mM [Ca2+]e. Mutant EJC amplitudes, however, increased gradually with increasing [Ca2+]e and were significantly different from controls up to 6 mM [Ca2+]e (p < 0.007, Student's t test). At 8 mM [Ca2+]e, csp mutant EJC amplitudes became statistically similar to controls (p > 0.1, Student's t test).
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Figure 4. Ca2+ dependence of evoked release elicited by single stimuli at 23°C in csp mutants. High [Ca2+]e restores the loss of evoked release at cspX1 mutant NMJs. A, Typical two-electrode voltage-clamp recordings of EJCs elicited at 0.2 Hz from larval NMJs in 1 and 8 mM [Ca2+]e. Each EJC represents an average of 20 trials. B, Recorded EJC amplitudes at the indicated [Ca2+]e were normalized for muscle size by dividing the current amplitude by the cell capacitance. Twenty trials were averaged for n larvae. Each point represents the mean EJC amplitude of at least four larvae. Error bars indicate SEM. In 1, 4, and 6 mM [Ca2+]e, cspX1 amplitudes are significantly different from control (p < 0.007, Student's t test). In 8 mM [Ca2+]e, cspX1 mutant amplitudes are no longer significantly different from control (p = 0.15, Student's t test). Mean EJC amplitudes were 15.6 ± 2.1 nA/nF (mean ± SEM) for control and 3.4 ± 0.7 nA/nF for cspX1 mutants in 1 mM [Ca2+]e, and 49.1 ± 8.8 nA/nF for control and 31.1 ± 6.4 nA/nF for cspX1 mutants in 8 mM [Ca2+]e.
By Ca2+ imaging, we established that depolarization-dependent Ca2+ entry into boutons of both csp mutants and controls gradually increased with higher [Ca2+]e (Fig. 5). Thus, the facilitated EJC amplitudes were correlated with more Ca2+ entry at higher [Ca2+]e, as would be expected from entry of Ca2+ through voltage-activated Ca2+ channels. However, in the present experiments, we did not simultaneously measure Ca2+ signals and transmitter release from the same bouton.
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Figure 5. Ca2+ signals in boutons at different external Ca2+ levels at 21°C. As [Ca2+]e was increased, a larger Ca2+ signal was observed for both controls and cspU1 mutants. A, B, Ca2+ changes in type Ib boutons of controls (A, n = 12) and cspU1 mutants (B, n = 5) with increased [Ca2+]e: 0.5, 1, and 3 mM. Symbols indicate mean ± SEM values at each time point. Preparations were stimulated in HL3 solution at 5 Hz for 5 sec (solid horizontal bar). Large error bars shown at 3 mM [Ca2+]e during stimulation resulted from contraction of the muscle. C, Peak values for intracellular Ca2+ signal with different extracellular Ca2+ concentrations.
Rescue of neurotransmitter release in csp mutants at temperatures above 30°C
Previous reports have described a temperature-sensitive block of neurotransmitter release elicited by single stimuli at temperatures above 29°C in csp mutants (Umbach et al., 1994
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Figure 6. Rescue of the temperature-sensitive block of evoked release at 30°C in csp mutants. When single stimuli (0.2 Hz) failed to evoke neurotransmission in csp null mutants at 30°C, it was possible to partially rescue the temperature-sensitive defect with high-frequency stimulation or high [Ca2+]e. Traces represent typical recordings under current clamp at 30°C. A, Evoked EJPs were blocked in cspU1 null mutants with 0.2 Hz stimulation and 1 mM [Ca2+]e. B, After neurotransmission was blocked, the preparation was stimulated at 10 Hz. The mean amplitude of the first 40 rescued responses was 4.6 ± 1.7 mV (n = 6, ±SEM). C, After neurotransmission at 0.2 Hz was blocked in 1 mM [Ca2+]e, the bath solution was switched to 4 mM [Ca2+]e. Subsequently, stimulation at 0.2 Hz evoked EJPs; the mean amplitude of 12 responses was 19.1 ± 6.1 mV (n = 4).
Temperature-dependence of evoked neurotransmitter release and Ca2+ entry
To correlate defects of cytosolic Ca2+ entry and neurotransmitter release in csp mutants over the same temperature range, we used the same stimulation to measure both Ca2+ entry and neurotransmitter release. In contrast with a previous report showing that Ca2+ signals do not increase in csp mutant boutons after 10 Hz stimulation for 2 min at restrictive temperatures (Umbach et al., 1998
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Figure 7. Temperature dependence of evoked release and cytosolic Ca2+ levels in csp mutants and controls. A-C, Comparison of Ca2+ signals in type Ib boutons of cspU1 mutants and controls at different temperatures. Preparations were stimulated in HL3 solution containing 1 mM Ca2+ at 5 Hz for 5 sec (solid horizontal bar). Symbols indicate mean ±SEM values for each time. A, Ca2+ signals in control boutons at temperatures between 24 and 34°C, showing a small increase with little change at higher temperatures. B, Ca2+ signals in cspU1 boutons at temperatures between 24 and 34°C. Larger Ca2+ signals and increased variability compared with controls are apparent at all temperatures. C, Maximum relative Ca2+ changes in Ib boutons. cspU1 mutants show a significantly larger change in Ca2+ than controls at all temperatures except 34°C. D, Temperature dependence of mean EJP responses evoked by repetitive stimulation. EJP recordings were made after 30 min at each temperature in 1 mM Ca2+ HL3 solution. For each specimen, the mean of 25 responses was obtained; the mean values for all specimens were then averaged for each point on the graph.
Together, these experiments show that the relative increase of intraterminal Ca2+ is generally larger in csp mutants than in controls, that recovery (clearance) of intraterminal Ca2+ at high temperatures is much slower, and that the reduction of neurotransmitter release cannot be entirely explained by a loss of Ca2+ entry into the nerve terminal.
Comparison of resting [Ca2+]i in csp and control boutons
Relative changes in fluorescence were often larger in csp mutant boutons than in controls, even at nonpermissive temperatures, whereas transmitter release was markedly reduced under the same conditions. This result could suggest that a primary defect of Ca2+-triggered exocytosis may be partially compensated by increased Ca2+ entry in csp mutants. Alternatively, it could be that resting [Ca2+]i is actually lower in csp mutants than in controls. If this were the case, the observed relative changes in fluorescence would not necessarily indicate a larger Ca2+ accumulation in csp mutant boutons, because peak fluorescence values are normalized to the initial (resting) values. Thus, a normal [Ca2+]i at rest in combination with higher normalized peak fluorescence values during stimulation would signify higher stimulus-evoked cytosolic Ca2+ levels.
We addressed this question by measuring resting values of [Ca2+]i using the ratiometric indicator fura-2 AM. This indicator was much more difficult to use than the selected non-ratiometric indicators because of less efficient loading of the terminals and a higher background signal in the muscle. Nevertheless, resting values for [Ca2+]i were obtained in several experiments (Fig. 8). Estimates of [Ca2+]i were made in 1 mM [Ca2+]e. No significant differences in resting [Ca2+]i were found between control (170 ± 6.1 nM) and csp mutant boutons (195 ± 15.0 nM) at room temperature (24°C) (Fig. 8A). However, at 34°C, csp mutant terminals had a significantly higher resting level of [Ca2+]i (361.4 ± 35.72 nM) than control terminals (230 ± 6.7 nM; p = 0.01, df = 5, Student's t test).
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Figure 8. Estimated [Ca2+]i for Drosophila type Ib boutons in 1 mM [Ca2+]e. Values of resting [Ca2+]i estimated with ratiometric imaging using fura-2 AM are shown for control and cspU1 boutons (4 animals, 14 boutons). No difference was found between control and csp boutons at room temperature (23°C). However, at 34°C, [Ca2+]i was significantly higher in csp boutons than in controls (p = 0.01, Student's t test).
Our results suggest that, at room temperature, cytosolic Ca2+ attains significantly higher values in csp mutant than in control boutons during nerve stimulation. This is indicated by normal resting levels of [Ca2+]i and increased evoked fluo-4 signals (
Frequency dependence of presynaptic Ca2+ entry and Ca2+ clearance
An additional set of experiments was performed to examine the effect of stimulation frequency on peak Ca2+ signals and their recovery after stimulation at high temperatures (34°C). In controls, Ca2+ signals increased progressively with frequency, as found previously (Karunanithi et al., 1997
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Figure 9. Ca2+ clearance in csp mutant and control boutons at 34°C. A-C, Preparations were stimulated in HL3 solution for 5 sec (horizontal bar). Symbols indicate mean ± SEM values at each time. A, Control preparations show abrupt increases in Ca2+ signals with a plateau for all frequencies. B, cspX1 mutants exhibit an exaggerated slowing of Ca2+ decay after stimulation and relative small increases in peak Ca2+ signals when the stimulus frequency is increased. C, cspU1 preparations show an increase in Ca2+ signals with increased stimulus frequency and prolonged recovery, especially at high frequencies. A significant difference was found between cspU1 and control preparations at 15, 20, and 40 Hz (ANOVA, df = 5, p < 0.05). D, Relative changes of cytosolic Ca2+ in type Ib boutons of cspU1 Drosophila larvae before, during, and after a 120 sec stimulus at 10 Hz (horizontal bar) at two different temperatures, 20 and 34°C. Symbols indicate mean ± SEM values, and asterisks indicate significant differences. Experiments were performed in standard Drosophila (Jan and Jan, 1976
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Table 1. Decay kinetics of Ca2+ signals in cspU1 mutants and controls The slower decay of Ca2+ signals after stimulation indicates a possible defect of Ca2+ extrusion in csp mutants at elevated temperatures. A final set of experiments was conducted to ascertain the temperature dependence of this phenotype. Relative changes of Ca2+ in type Ib boutons of cspU1 Drosophila larvae were recorded before, during, and after a 120 sec stimulus at 10 Hz at two different temperatures, 20 and 34°C (Fig. 9D). The relatively prolonged stimulation in the standard Drosophila solution duplicates the conditions used for calcium imaging by Umbach et al. (1998)
These observations indicate a deficit in Ca2+ clearance in both mutant alleles, with a more extreme impairment of Ca2+ extrusion in the cspX1 allele. The effect is exacerbated at high temperatures (Fig. 9D). The slower clearance of Ca2+ probably contributes to the build-up of Ca2+ in the boutons and to the distinctive properties of the Ca2+ signals generally observed in the mutants (slower time course, and greater variability in amplitude and time course).
DISCUSSION
Our observations suggest that the loss of neurotransmitter release in csp mutants is primarily caused by a defect in a direct step of Ca2+-regulated exocytosis and not by inactivation of presynaptic Ca2+ channels as suggested previously (Umbach et al., 1998
Our results support the hypothesis that CSP may regulate a direct step in exocytosis (Brown et al., 1998
The regulatory or protective effects of CSP on cellular mechanisms are apparently more widespread than previously thought. CSP may act on multiple synaptic mechanisms as indicated by the variety of defects observed at csp mutant boutons. Mutant terminals exhibit relatively slow Ca2+ clearance after repetitive stimulation, in particular at high temperatures. Consistently, cytosolic Ca2+ at rest is elevated in mutant boutons at high but not at low temperatures. Although a slower Ca2+ clearance would increase the build-up of cytosolic Ca2+ in the terminal (Tank et al., 1995
In addition to altered Ca2+ homeostasis, presynaptic Ca2+ entry appears to be less firmly regulated in csp mutants than in controls, although it is not the primary cause for the loss of neurotransmitter release. Evidence for abnormal Ca2+ entry was apparent in the unusual temperature dependence of stimulus-evoked intraterminal Ca2+ signals and in spontaneous flashes of cytosolic Ca2+. In principle, these could be caused by a variety of defects, including accumulation of cytosolic Ca2+, increased numbers of Ca2+ channels, prolonged Ca2+ channel opening times, and/or a defect in Ca2+-activated K+ conductance.
Ca2+ entry can be compromised at high temperatures in csp mutants, particularly under adverse or stressful physiological conditions. For example, use of the standard recording solution (Jan and Jan, 1976
CSP appears to protect cellular mechanisms controlling intracellular Ca2+ signaling and homeostasis. These functions may involve known interactions with heat-shock proteins and heat-shock cognate proteins (Braun et al., 1996
A direct role of CSP in exocytosis was suggested by several studies using slow secretion systems. Although overexpression of bovine CSP in neuroendocrine PC12 cells had no effect on Ca2+ entry, it enhanced Ca2+-dependent dopamine release in permeabilized PC12 cells and GTP
S-induced release in the absence of Ca2+ (Chamberlain and Burgoyne, 1998
-cell lines (Zhang et al., 1998
The original hypothesis of CSP function at nerve terminals proposed that CSP may promote neurotransmitter release by increasing Ca2+ channel activity (Mastrogiacomo et al., 1994
The present study suggests similar functions of CSP in evoked neurotransmitter and peptidergic exocytosis. We suggest multiple synaptic functions for CSP in nerve terminals. The most significant one for neurotransmitter release appears to increase the Ca2+ sensitivity of a direct step in exocytosis, as proposed for slow peptidergic exocytosis. This regulatory action may include steps of Ca2+ signaling located between the postulated Ca2+ sensor of vesicle fusion and the fusion machinery itself. In addition, CSP appears to stabilize Ca2+ entry and Ca2+ clearance, although these functions may only be significant for evoked release at high temperatures. The recently demonstrated in vitro and in vivo interaction of CSP with syntaxin (Nie et al., 1999
FOOTNOTES Received April 28, 2000; revised June 2, 2000; accepted June 2, 2000.
This work was supported in part by grants from the National Science Foundation and the National Institute of Neurological Disorders and Stroke to K.E.Z., a National Research Service award to P.B., and grants from the Medical Research Council of Canada to H.L.A. We thank Gowan Tervo (National Sciences and Engineering Research Council of Canada summer student) for his contributions to initial trials of fura-2 AM in Drosophila boutons and Andrew Millar for helping with the measurements of resting Ca2+ reported here.
K.D.-S and P.B. contributed equally to this work.
Correspondence should be addressed to Konrad E. Zinsmaier, Department of Neuroscience, 234d Stemmler Hall, University of Pennsylvania School of Medicine, Philadelphia, PA 19104-6974. E-mail: zinsmaie{at}mail.med.upenn.edu.
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