Synaptic Modulation by a Neuropeptide Depends on Temperature and Extracellular Calcium

doi:10.1152/jn.00710.2002

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Synaptic Modulation by a Neuropeptide Depends on Temperature and Extracellular Calcium

Tyler W. Dunn and A. Joffre Mercier

Department of Biological Sciences, Brock University, St. Catharines, Ontario L2S 3A1, Canada

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Dunn, Tyler W. and A. Joffre Mercier. Synaptic Modulation by a Neuropeptide Depends on Temperature and Extracellular Calcium. J. Neurophysiol. 89: 1807-1814, 2003. The crayfish neuropeptide DRNFLRFamide increases transmitter release from synaptic terminals onto muscle cells. As temperaturedecreases from 20 to 8°C, the size of excitatory junctional potentials(EJPs) decreases, and the peptide becomes more effective at increasingEJP amplitude. The goal of the present study was to determinewhether the enhanced effectiveness of the peptide is strictlya temperature-related effect, or whether it is related to thefact that the EJPs are smaller at low temperature, allowing agreater range for EJP amplitude to increase. Decreasing temperaturereduced the number of quanta of transmitter released per nerveimpulse (assessed by recording synaptic currents) and increasedinput resistance in muscle fibers. As in earlier work, the abilityof the peptide to increase EJP amplitude was enhanced by decreasingtemperature. However, the peptide was also more effective at increasingEJP amplitude when transmitter output was lowered by reducingthe ratio of calcium to magnesium ions in the bath. Thus the effectivenessof the peptide may be related to the level of output from thesynapticterminals.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Neuropeptides play important roles in mediating and modulating transmission at chemical synapses. One major "family" of neuropeptidesconsists of those structurally related to FMRFamide (Phe-Met-Arg-Phe-NH₂),a tetrapeptide originally isolated from a mollusk (Price and Greenberg1977). FMRFamide-like peptides are present in every animal phylum(Greenberg and Price 1992) and have a variety of physiologicaleffects, including modulating chemical synapses (e.g., Baux etal. 1992; Cottrell et al. 1992; Jorge-Rivera et al. 1998; Man-Son-Hinget al. 1989).

The FMRFamide-like peptide, DF₂ (DRNFLRFamide), is found in the pericardial organs of crayfish and is thought to be releasedinto the circulation as a neurohormone (Mercier et al. 1993).This peptide increases the amplitude of excitatory junctionalpotentials (EJPs) in crayfish muscles (Mercier et al. 1993; Skerrettet al. 1995). This effect has been studied most extensively indeep extensor muscles (DEMs) of the crayfish abdomen. The neuropeptideincreases the number of quanta of transmitter released per nerveimpulse but does not alter muscle fiber input resistance or responsivenessto iontophoretic application of glutamate (Mercier et al. 2001;Skerrett et al. 1995). Thus the enhancement of EJP amplitude appearsto involve presynaptic rather than postsynaptic mechanisms. Pharmacologicalstudies suggest that the effect requires the activity of calcium/calmodulin-dependentprotein kinase (Noronha and Mercier 1995), protein kinase C (Friedrichet al. 1998), and cyclic nucleotide-dependent protein kinases(Mercier et al. 2001).

One interesting aspect of DF₂'s ability to modulate transmitter release is its apparent temperature-dependence. In the crayfishDEMs, DF₂ is more effective at enhancing EJP amplitude at lowertemperatures (Friedrich et al. 1994). The functional significanceof this temperature dependence and the mechanisms that underlieit are not known. As temperature drops, EJP amplitude decreasesin the DEMs (Friedrich et al. 1994) and in the deep abdominalflexor muscles (Czternasty and Bruner 1980). The enhanced capacityfor DF₂ to increase EJP amplitude might help to compensate forreduced synaptic transmission at lowtemperatures.

The present work represents our first attempt to investigate mechanisms underlying the temperature-dependence of DF₂'s effecton synaptic transmission. Because lowering the temperature reducesEJP amplitude, it seems likely that the number of quanta of transmitterreleased also decreases under these conditions. Such a reductionin transmitter output may simply increase the range through whichthe peptide can increase transmitter release. The present studyconfirms that quantal content, a direct measure of transmitterrelease, decreases with temperature. It also shows that reducingthe Ca²⁺/Mg²⁺ ratio, which would decrease calcium influx, enhances DF₂'s abilityto modulate synaptictransmission.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Crayfish (Procambarus clarkii), approximately 5-8 cm long, were obtained from Atchafalaya Biological Supply (Raceland, LA)and were kept in large holding tanks at 14-16°C. The freshwaterin the tanks was aerated, circulated, and filtered. The crayfishwere fed Tender Vittles dry cat food. Immediately before dissection,the crayfish were cooled in ice and killed by destruction of thecerebral and thoracic ganglia. The dorsal part of the abdomen,containing the DEMs (Parnas and Atwood 1966), was dissected awayand secured in a 1.0-ml recording chamber that was perfused continuouslywith crayfish saline. Temperature was regulated by cooling thesaline and monitored with a digital thermometer (±0.05°C). Thecrayfish saline was modified from that of Van Harreveld (1936).Most experiments were performed in a standard "low calcium, highmagnesium" saline to prevent muscle twitching (Mercier and Atwood1989). This saline had the following constituents (in mM): 200.7NaCl, 5.36 KCl, 6.5 CaCl₂, 12.3 MgCl₂, 5.0 HEPES; pH 7.4. In otherexperiments, the concentration of CaCl₂ was decreased to 4.2 mM,and the MgCl₂ concentration was raised to 14.9 mM to reduce transmitteroutput moredrastically.

EJPs were elicited in muscle L1 of the fourth abdominal segment by stimulating excitatory axon 3 in the third abdominal segment,using methods described elsewhere (Mercier and Atwood 1989; Skerrettet al. 1995). Stimuli were applied at 0.2 Hz using a Grass S88stimulator and a Grass SIU stimulus isolation unit. Postsynapticpotentials were recorded with glass microelectrodes filled with3 M KCl. EJPs were monitored on a digital storage oscilloscopeand were acquired on an IBM-compatible computer using a computerizeddata acquisition system designed and constructed by the ElectronicsDivision at Brock University. The sampling frequency for the acquisitionsystem was 10 kHz. Signals were averaged every 30 s, so that theEJP acquired represented the average of six responses. EJP amplitudeswere measured and compiled using software developed by Mr. TomMacDonald at Brock University. EJPs were corrected for nonlinearsummation (Martin 1955) as in previous experiments (e.g., Mercierand Atwood 1989; Skerrett et al. 1995).

Quantal synaptic currents were recorded using glass macropatch electrodes approximately 10 µm in diameter, as described elsewhere(Dudel 1982; Mercier and Atwood 1989). Electrodes were placedon the surface of the muscle fibers at locations that optimizedthe clarity and size of a single quantal current. Because it wasimpossible to count individual quanta at higher temperatures,quantal content was determined using the "failures method" describedby Del Castillo and Katz (1954). According to this method, quantalcontent (m) can be estimated as

<IT>m</IT><IT>=ln </IT>(<IT>N</IT><IT>/</IT><IT>N</IT><IT>0</IT>)

where N is the number of stimuli, and N₀ is the number of failures. The assumption underlying this method is that the frequencyof quantal releases can be fitted by a Poisson distribution. Thisassumption is valid only when transmitter output is low. Whenquantal content is higher (>1.0), quantal release is fitted betterby a binomial distribution, and the failures method underestimatesquantal content (e.g., (Johnson and Wernig 1971). For these reasons,recording sites were selected based on failure rate. In experimentswhere temperature was raised, sites were selected if the quantalfailure rate was >70% at the low starting temperature; in experimentswhere temperature was lowered, sites were chosen if failure ratewas <30% at the high starting temperature. Thus the temperaturesensitivity of quantal content was assessed from temperatureswhere m < 1. Simultaneous intracellular recording in the musclefiber allowed verification of postsynaptic response to stimuluspulses, so that a failed quantal current represents failed releaseat the monitored bouton and not sub-threshold stimulation of theaxon. The failures method was used in preference to methods thatinvolve comparing averaged responses to spontaneous quanta becausespontaneous releases are infrequent in the DEMs and in at leastsome cases appear to indicate damage to the nerve terminals inthis preparation. To insure that estimates of quantal contentwere accurate, the results from $>=$ 50 stimuli wereused.

Johnson and Wernig (1971) showed that at crayfish neuromuscular junctions, the Poisson calculation overestimates m by 4-39%when estimated values of p, the release probability, are between0.1 and 0.5. Although we sought conditions where p < 0.1, we couldnot estimate p reliably in the present experiments. One can approximatep from the relation

<IT>m</IT><IT>=</IT><IT>np</IT>

where m is the number of quanta released per nerve impulse, and n is the number of active zones. Morphological studies indicatethat crustacean synapses can have 20-100 active zones in the vicinityof a macropatch electrode of the size we used (Atwood and Tse1988; Msghina et al. 1998). Using these estimates, a quantal contentof 0.36 [which corresponds to ln (N/N₀) with a 70% failure rate],would yield p values in the range of 0.004 to 0.02. A 70% failurerate, therefore, was considered sufficient to satisfy the criterionthat p is sufficiently low to estimate m from the Poisson relation.Lower failure rates (as occurred at 17.5°C in the present study)overestimate m (see DISCUSSION).

Another way to address the question of whether the synaptic changes occur presynaptically or postsynaptically involves calculatingthe coefficient of variation (CV) associated with EJP fluctuations.This method does not assume that the data fit a Poisson distribution.CV is calculated from the relation

CV=<IT>s</IT><IT>EJP</IT><IT>/mean EJP</IT>

where s_EJP is the SD associated with EJP fluctuations. As m increases, CV decreases (Martin 1966). Factors that increaseEJPs through presynaptic mechanisms decrease CV. Presynaptic andpostsynaptic effects of an experimental treatment can be distinguishedby comparing two ratios

<IT>r</IT><IT>=CV</IT><IT>2</IT><IT>before</IT><IT>/CV</IT><IT>2</IT><IT>after</IT>

and

&pgr;=<IT>M</IT><IT>after</IT><IT>/</IT><IT>M</IT><IT>before</IT>

where CV and CV are, respectively, the squares of the coefficients ofvariation before and after treatment, and M_after and M_before are,respectively, the mean EJP amplitudes after and before treatment(Faber and Korn 1991). A plot of r versus $pi$ will yield a positiveslope if the treatment increases EJPs through presynaptic mechanisms.The same plot, however, will produce a horizontal line where r= 1 if EJPs increase only through postsynaptic changes (Faberand Korn 1991).

Input resistance in the muscle fibers was measured using two microelectrodes inserted approximately 50 µm apart into the samefiber. One electrode was used to inject electrical current, whilethe other was used to recordvoltage.

The temperature sensitivity of EJP amplitude, quantal content, and muscle fiber input resistance was assessed by calculatinga Q₁₀ value for each of these variables. Q₁₀, the temperaturecoefficient, was calculated using the van't Hoff equation

<IT>Q</IT><IT>10</IT><IT>=</IT>(<IT>k</IT><IT>2/</IT><IT>k</IT><IT>1</IT>)<IT>10/</IT>(<IT>T</IT><IT>2−</IT><IT>T</IT><IT>1</IT>)

where k1 and k2 are mean values for a given variable at temperatures T1 and T2. Thus a Q₁₀ of 1 represents no temperaturesensitivity in variable X, and a Q₁₀ of 3 indicates a threefoldincrease in k with an increase in 10°C.

All values represent means ± SE, and statistical comparisons were made using a Mann-Whitney U test unless otherwisenoted.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

EJP amplitude and quantal content (measured at a stimulus frequency of 0.2 Hz) were both affected by changes in the bath temperaturebetween 8 and 20°C. Figure 1A displays a representative trialin which the temperature was reduced from 20 to 8.5°C while EJPamplitude and the quantal synaptic currents were monitored simultaneously.Quantal content (determined from the percentage of failures) andEJP amplitude both decreased as temperature decreased. The effecton quantal content was more pronounced than the effect on EJPamplitude in this example. This experiment was performed witha total of six preparations. Temperature was lowered in half thepreparations and raised in the other half to ensure that the reductionin quantal content with decreased temperature was not the resultof changes in muscle tonus that might move the macropatch fromthe original recording site. Mean EJP amplitudes, the percentageof failures, and mean values for quantal content for all six preparationsare shown in Fig. 2, A-C, respectively. As temperature decreasedfrom 17.5 to 10°C, mean EJP amplitude decreased significantly(P < 0.05), the mean percentage of failures decreased significantly(P < 0.005), and mean quantal content decreased significantly(P < 0.005). The mean Q₁₀ value associated with changes in EJPamplitude (averaged from individual trials) was 3.46 ± 0.52, andthe mean Q₁₀ for changes in quantal content was 7.62 ± 1.49.

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Fig. 1. Reducing temperature decreased excitatory junctional potential (EJP) amplitude and quantal content, while increasing muscle fiber input resistance. A: in this representative trial, EJP amplitude (corrected for nonlinear summation) and quantal content (calculated using the failures method) increased as temperature increased. The large jump in quantal content above 17°C is a result of the overestimation of the failures method when m > 1 (for explanation of this, see Johnson and Wernig 1971

). The inset box shows representative traces of single EJPs at 2 temperatures, 20°C (top trace) and 10°C (bottom trace). As observed in earlier work, reducing temperature increased the latency and slowed the time course of the EJP (Friedrich et al. 1994

). Bars: 20 mV, 5 ms. B: muscle fiber input resistance decreased as temperature was increased. This representative trial shows the gradual decrease in input resistance to a 100-nA hyperpolarizing current pulse as temperature is increased by 12°C.

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Fig. 2. Evidence that changes in temperature alter transmitter release presynaptically. A: EJP amplitude was significantly decreased (P < 0.05) by a reduction in temperature from 17.5 to 10°C. The average EJP amplitude at 17.5 and 10°C was measured in 6 preparations. B: average percentage of failures at 2 temperatures in the 6 preparations used to determine quantal content. The percentage of failures was significantly lower (P < 0.005) at 10°C than at 17.5°C. C: quantal content, estimated from $>=$ 50 stimuli using the failures method, was significantly reduced (P < 0.005) between 17.5 and 10°C (n = 6 preparations). These 2 temperatures were chosen because quantal currents were measured at these 2 temperatures in all preparations and m < 1. D: relationship of the ratio of the coefficients of variation squared for EJP amplitude at 2 different temperatures is plotted against the modification factor, which is the ratio of the mean EJP amplitudes at the 2 temperatures. Notice the points follow a positive slope and in all cases r > P.

The decrease in estimated quantal content suggests that the effects of temperature on EJP amplitude are mainly presynaptic,attributable to changes in transmitter output from the synapticterminals. To obtain corroborative evidence for a presynapticeffect, the CV associated with EJP amplitudes was calculated foreach of the six trials in which temperature was altered (Table1). In each trial, CV was lower at 17.5°C than at 10°C, suggestingenhancement of transmitter output at the higher temperature. Wealso plotted r (the ratio of CV² values) versus $pi$ (the ratio of mean EJP amplitudes) for eachof the temperature trials (see METHODS). The data from our sixtemperature trials (Fig. 2D) fell within an area where the slopeis >1 (i.e., r > $pi$ ). This result is predicted when EJP amplitudeis enhanced by presynaptic mechanisms and not by postsynapticmechanisms (Faber and Korn 1991).

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Table 1. The coefficient of variation for EJP amplitude is shown for each trial at the two temperatures

In another set of trials (6 preparations), muscle fibers were penetrated with two microelectrodes, and input resistance wasmeasured as temperature was changed. Data from a representativetrial are illustrated in Fig. 1B. As with EJP amplitude and quantalcontent measurements, temperature was changed in both directions,from 20 to 8°C and from 8 to 20°C. The Q₁₀ value associated withchanges in input resistance was $-$ 1.82 ± 0.25; the negative valueindicates that input resistance increased with decreasing temperature.Czternasty and Bruner (1980) also reported that input resistanceof crayfish muscle fibers increased when temperature was loweredfrom 19 to 9°C, and they obtained a Q₁₀ value equivalent to $-$ 2.1.The increase in input resistance with decreasing temperature probablyhelps to compensate somewhat for the reduction in quantal contentand explains why the Q₁₀ value for the effect on EJP amplitudeis lower than that for quantalcontent.

As reported in Friedrich et al. (1994), DF₂ is more effective at increasing EJP amplitude at lower temperatures. Figure 3Ashows the effect of 200 nM DF₂ on deep abdominal extensor muscleL1 at two different temperatures, 12 and 20°C. (In this experiment,the Ca²⁺ and Mg²⁺ concentrations of the saline were 4.2 and 14.9 mM, respectively.)EJP amplitude increased by approximately 80% at 12°C and by approximately30% at 20°C. Actual EJP amplitudes increased from 2.6 ± 0.5 to4.2 ± 0.7 mV at 12°C and from 9.6 ± 3.5 to 15.5 ± 6.3 mV at 20°C.The EJP amplitudes observed in the presence of DF₂ at 12°C weresignificantly lower (P < 0.05) than the EJP amplitudes prior topeptide application at 20°C. The initial rate of increase in EJPamplitude appeared to be similar at both temperatures, which issurprising because decreasing temperature generally slows therate of biochemical and physiological processes. However, themaximal increase in EJP amplitude occurred slightly earlier at20°C (7.5 min) than at 12°C (9.5 min), and the effect of the peptideappeared to decline slightly at 20°C but not at 12°C. A declinein the effect of DF₂ on EJPs has been observed previously at 12°C,but only after approximately 15 min (Noronha and Mercier 1995).The mechanisms underlying this decline are not known, but thedata suggest that raising the temperature from 12 to 20°C speedsup some of the subcellular processes activated by DF₂.

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Fig. 3. Increasing temperature and/or extracellular calcium levels reduced the percentage increase in EJP amplitude caused by 200 nM DF₂. A: effect of temperature. EJP amplitude is expressed as the percentage change from the average EJP amplitude prior to peptide application. The Ca²⁺/Mg²⁺ concentrations are 4.2 and 14.9 mM, respectively (n = 7 for both 20 and 12°C; error bars are SE). B: effect of extracellular calcium. These trials were conducted at 12°C and as in Fig. 3A, EJP amplitude is expressed as the percentage change from the average amplitude during the prepeptide period (n = 7 for 4.2 mM Ca²⁺ saline and 6 for 6.5 mM Ca²⁺ saline).

To further examine the possibility that the enhanced effect of the peptide at low temperatures is directly related to reducedtransmitter output, EJPs were raised slightly by increasing theratio of Ca²⁺ to Mg²⁺ ions in the saline. A saline containing 6.5 mM Ca²⁺ and 12.3 mM Mg²⁺ was used in these experiments (which were performed at 12°C).Raising the Ca²⁺/Mg²⁺ ratio in this manner increased the initial EJP amplitude andreduced the effectiveness of the peptide (expressed as the percentagechange in EJP amplitude). The mean EJP amplitude during the 8-minperiod immediately prior to peptide application was 6.3 ± 1.5mV in 6.5 mM Ca²⁺/12.3 mM Mg²⁺. This was significantly larger than the mean EJP amplitude overthe same time period in 4.2 mM Ca²⁺/14.9 mM Mg²⁺ (2.6 ± 0.5 mV; P < 0.05). Following application of DF₂ in thehigher Ca²⁺ saline, EJPs increased by approximately 30% (Fig. 3B) to an averagevalue of 8.1 ± 2.0 mV. A comparison of data from the two salinesolutions indicates that increasing the extracellular Ca²⁺/Mg²⁺ ratio increases the initial EJP amplitude and reduces the responseto thepeptide.

The effects of DF₂ at the two different temperatures and Ca²⁺/Mg²⁺ ratios are summarized in Fig. 4A. The percentage increase inEJP amplitude was calculated by comparing EJPs 5-8 min after applyingDF₂ with EJP amplitudes averaged over the 3-min period immediatelybefore peptide application. Reducing temperature and reducingthe Ca²⁺/Mg²⁺ ratio have similar effects on the ability of DF₂ to enhance transmitteroutput. Decreasing temperature and decreasing the Ca²⁺/Mg²⁺ ratio both significantly (P < 0.05) enhance the percentage increasein EJP amplitude elicited by DF₂. DF₂ elicited the largest percentageincrease in EJP amplitude in the lower calcium saline at the lowertemperature, when the two factors were combined.

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Fig. 4. Reducing temperature and extracellular calcium levels both lead to greater modulation by DF₂. A: mean values of the increase in EJP amplitude measured between 5 and 8 min after peptide application. Amplitudes in this period are expressed as the percentage change from the average EJP amplitude during the prepeptide period. The trials at low temperature and in the low calcium saline are significantly different from all the other trials. (Error bars depict SE; n = 8, 7, 6, 7 from left to right.) B: initial EJP amplitude is inversely related to the effectiveness of DF₂ to increase transmitter release. The initial EJP amplitude of each trial was plotted with the percentage change (increase) in EJP amplitude to 200 nM DF₂ as compared with the prepeptide period. This trend is significant (r = $-$ 0.417; n = 32; P < 0.05), and the data are fit best by the complex function, y = $-$ 0.1393 ln (x) + 0.5984.

The similarity between the effects of changing temperature and Ca²⁺/Mg²⁺ levels suggests that the effectiveness of DF₂ is inversely relatedto initial EJP amplitude. To test this idea, data from both experimentswere combined and plotted in Fig. 4B. There was a significant,negative correlation between the percentage increase in EJP amplitudeelicited by DF₂ and the initial EJP amplitude (r = $-$ 0.417; n =32; P < 0.05). The data suggest that the effectiveness of thepeptide is inversely related to the log of the initial EJPamplitude.

An alternative method for reducing the initial EJP amplitude was explored. In some crustacean muscles, stimulating the axonrepeatedly at low frequencies (e.g., 0.2 Hz or lower) causes areduction in EJP amplitude, referred to as low-frequency depression(Bruner and Kennedy 1970; Bryan and Atwood 1981; Zucker and Bruner1977). Such low-frequency depression is thought to be presynapticin origin, resulting from a gradual reduction in transmitter output.Two sets of trials were conducted at room temperature to determinewhether this method of reducing transmitter release would alsoenhance the ability of DF₂ to increase transmitter output. Inone set of preparations, the nerve was stimulated for approximately30 min before DF₂ was applied. This decreased EJP amplitude from11.1 ± 1.7 to 5.9 ± 0.9 mV before peptide application. In a separateset of preparations, the nerve was stimulated for only 8 min beforeapplying the peptide, causing very little low-frequency depression.(In this case, the EJPs decreased from 9.8 ± 2.0 to 9.1 ± 0.4mV.) The initial EJP amplitudes (at the beginning of each trial)were not significantly different between the two sets of trials(P > 0.05). Representative examples of both types of trial areshown in Fig. 5, A and B. Figure 5A shows actual changes in EJPamplitude (in mV), and Fig. 5B shows the effectiveness of DF₂,expressed as the percentage change in EJP compared with the averageamplitude recorded 3 min before peptide application. In the exampleshown in Fig. 5A, the peptide increased EJP amplitude from approximately17 mV to approximately 24 mV when there was little or no low-frequencydepression and from approximately 8 mV to approximately 12 mVafter substantial low-frequency depression. The percentage increasein EJP amplitude between the two trials was comparable (Fig. 5B).Data from six trials in each group were combined (Fig. 5C). Thepercentage increase in EJP amplitude 5-8 min after peptide applicationwas not significantly different between the two groups (P > 0.05).

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Fig. 5. Tonic stimulation gradually reduces EJP amplitude but does not alter the percentage increase in EJP amplitude caused by DF₂. A: in this figure the y-axis intersects at the point of peptide application in both trials; this is done to compare the effect of the peptide between the 2 trials. Both of these representative trials begin at similar EJP amplitudes and both are clearly modulated by DF₂. One trial exhibits a 9-mV reduction in EJP amplitude prior to DF₂ application. B: when the same trials as in Fig. 5A are compared by expressing EJP amplitude as a percentage change of the average EJP amplitude between 0 and 3 min before peptide application, there is no apparent difference in the peptide's effects. C: 2 groups have no significant difference (P > 0.05) in the percentage increase in EJP amplitude 5-8 min after DF₂ application as compared with the 3-min control period (n = 6 for each group and the bath temperature was 22°C for all trials).

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

These experiments confirm earlier observations that DF₂ increases EJP amplitude more effectively (when expressed as percentagechange) at low temperature (Friedrich et al. 1994). These experimentsalso confirm that decreasing temperature reduces EJP amplitude,and they provide direct evidence that this is caused by a presynapticreduction in transmitter release. An increase in input resistancecompensates somewhat for reduced quantal content at low temperatures,but EJP amplitude remains highly temperature dependent (Fig. 1).This suggests that one of the physiological roles of the neuropeptideDF₂ may be to compensate for reduced transmitter output when temperatureis reduced. This idea is supported by observations that the pericardialorgans of spiny lobsters, which contain and release peptides homologousto DF₂, fire impulses when temperature is reduced from 20 to 14°C(Kuramoto and Tani 1994).

The reduction in quantal content with temperature is probably the result of reduced calcium influx through voltage-gated calciumchannels in the synaptic terminals. The temperature coefficientquantifies the sensitivity of an event to a change in temperatureof 10°C. Biochemical events involving changes in covalent bondinghave Q₁₀s generally between 2 and 3, as do many physiologicalprocesses (Purves et al. 1995). The method used for estimatingm may contribute somewhat to the high mean value (Q₁₀ > 7.0) andlarge variance in the Q₁₀ for quantal content. The failures methodtends to overestimate quantal content when release levels arehigh and the data do not fit a Poisson distribution. This wouldtend to make estimated values of m excessively high only at thehigher temperatures (e.g., at temperatures above 17°C in Fig.1A). Such an effect would exaggerate the changes caused by temperatureand probably contributes to the high Q₁₀ values for m and forthe high variance associated with them. However, even at 17.5°C,values of m approached 1.0 but did not exceed it. Using data fromstudies where m was estimated by directly counting quanta (Johnsonand Wernig 1971; Mercier and Atwood 1989; Zucker 1973), ln (N/N₀)overestimates m by 5-25% when ln (N/N₀) is between 0.7 and 1.0.Even a 25% overestimate of m cannot account for the 200% increasein m that we observe when temperature increases from 10 to 17.5°C(Fig. 2C). Thus it is unlikely that the high Q₁₀ values are whollythe result of overestimating m. In fact, since input resistanceincreased with a drop in temperature, the effect of temperatureon m should be more pronounced than for EJPamplitude.

Calcium passage through the pore-forming region of an open calcium channel has little temperature sensitivity (Q₁₀ of roughly1.5; Klockner et al. 1990), as would be expected for diffusionthrough an aqueous medium (Hille 1991). However, Charlton andAtwood (1979) reported a large reduction in excitatory postsynapticpotential (EPSP) amplitude at the squid giant synapse that correspondedto a reduction in the presynaptic calcium current. The temperature-sensitivityof the calcium currents appears to be due to temperature-dependentchanges in the calcium channels. The major temperature-sensitivecomponents are not yet fully understood, but probably involveinteraction between channel subunits, interaction between calciumchannels and SNARE proteins, and phosphorylation state of thecalcium channels (Allen 1996; Allen and Mikala 1998; Bunemannet al. 1999; Wiser et al. 1996, 1997). Some of the kinetic parametersof calcium channels have large Q₁₀s, well above 3 (Allen 1996;McAllister-Williams and Kelly 1995; McNaughton et al. 1998), suggestingthat the high temperature-sensitivity of calcium channels resultsfrom the coupling of multiple metabolic events (Morris and Clarke1981). Thus the high Q₁₀ values for quantal content in the presentstudy probably reflect high temperature-sensitivity of the calciumchannels to someextent.

Quantal content (m) is determined by two variables (Del Castillo and Katz 1954): n, the average number of synaptic vesiclesready for release; and p, the average probability of a singlequantum being released (m = np). Thus DF₂ could potentially increasetransmitter release either by increasing p or by increasing n.An increase in p would be brought about by increasing calciuminflux into the synaptic terminals, by releasing calcium fromintracellular stores, or by increasing the sensitivity of thesecretory apparatus to intracellular calcium. An increase in nwould be brought about by increasing the number of vesicles thatare docked at activezones.

It is well established that decreasing the extracellular Ca²⁺ level reduces quantal content and EJP amplitude by reducing calciuminflux (e.g., Augustine and Charlton 1986; Dodge and Rahamimoff1967; Dudel 1981). The similarities between the effects of reducingtemperature and reducing extracellular calcium suggest that thesetwo treatments enhance the ability of DF₂ to increase transmitterrelease via a common mechanism. Since both these treatments arelikely to reduce quantal content by lowering calcium influx, itseems likely that the enhanced effectiveness of the peptide isrelated to a reduction in calcium influx and, thus, to a reductionin binomial variable p. Reducing the extracellular Ca²⁺ level has been shown to reduce p without affecting n at crayfishneuromuscular junctions (Dudel 1981). The ability of DF₂ to enhancetransmitter output from the fast closer excitor axon of crabsrequires N-type calcium channels (Rathmayer et al. 2002). Thissuggests that DF₂ acts by increasing calcium influx, which wouldincrease binomial variable p. The present data suggest that ifp is reduced at low-temperature or low-extracellular Ca²⁺ levels, the scope for modulation by the neuropeptide may be enhanced.Experiments involving calcium imaging in nerve terminals wouldhelp to determine whether or not DF₂ acts on calciuminflux.

In this and a previous report (Friedrich et al. 1994), the effectiveness of DF₂ in modulating chemical synapses has been expressedas the percentage change in EJP values, rather than in the actualchange in millivolts. This was done primarily to minimize theeffect of variation in EJP amplitudes between different preparations.However, it is worth noting that actual EJP amplitudes after peptideapplication at 12°C were still lower than those recorded at 20°Cbefore peptide application. Thus although the percentage changein EJP amplitude induced by the peptide is greater at the lowertemperature, the actual EJP amplitudes do not even approach thoseat the higher temperature with no peptide. Thus it seems unlikelythat reducing temperature simply leaves a greater supply of transmitterquanta and that the peptide is less effective at the higher temperaturebecause there are smaller reserves of quanta available forrelease.

To further investigate the effect of lowering transmitter release on effectiveness of the peptide, the EJP amplitude was loweredthrough low-frequency depression. Tonic low-frequency stimulation(0.2 Hz) of crustacean phasic excitors often leads to a reductionin EJP amplitude over time (Bruner and Kennedy 1970; Lnenickaand Atwood 1985; Pahapill et al. 1986; Zucker and Bruner 1977).Although initial EJP amplitude was significantly reduced by lowfrequency depression, the magnitude of the modulation by DF₂ wasunaffected. Thus the mechanisms through which low-frequency depressionreduces transmitter output may differ from those underlying theeffects of reducing temperature and reducing extracellular calcium.The mechanisms underlying low-frequency depression are not wellunderstood, but appear to involve the generation of nitric oxide(Aonuma et al. 2000). Treatments that reduce calcium influx, suchas lowering extracellular Ca²⁺ (Czternasty and Bruner 1980), raising extracellular Mg²⁺ (Bruner and Kennedy 1970), and adding Mn²⁺ to the bath (Bryan and Atwood 1981), drastically reduce transmitterrelease without affecting low-frequency depression. Such observationssuggest that this form of depression does not result from a reductionin calciuminflux.

In summary, reducing extracellular calcium level and reducing the temperature both enhance the ability of neuropeptide DF₂to increase transmitter release. The similarity of the effectsof these two experimental treatments suggests common underlyingmechanisms related to changes in calcium influx. The results alsosuggest that the mechanisms through which low-frequency depressionreduces transmitter output differ from those underlying reductionsin temperature or extracellular calcium. Taken together, the presentdata and those of Rathmayer et al. (2002) suggest that presynapticcalcium channels are involved in the modulatory effect of DF₂.The functional significance of the sensitivity and calcium sensitivityof the peptide's effects are still to bedetermined.

	ACKNOWLEDGMENTS

We thank Dr. Mary Kate Worden for helpful discussions during the course of this work. We are also grateful to P. Orth andDr. Milton Charlton for helpful comments on themanuscript.

This work was supported by a grant to A. J. Mercier from the Natural Sciences and Engineering Research Council ofCanada.

	FOOTNOTES

Address reprint requests to: T. W. Dunn (E-mail: appollyon{at}hotmail.com).

REFERENCES

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
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Synaptic Modulation by a Neuropeptide Depends on Temperature and Extracellular Calcium

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