Nerve Growth Factor Rapidly Induces Prolonged Acetylcholine Release from Cultured Basal Forebrain Neurons: Differentiation between Neuromodulatory and Neurotrophic Influences

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The Journal of Neuroscience, May 15, 2001, 21(10):3375-3382

Nerve Growth Factor Rapidly Induces Prolonged Acetylcholine Release from Cultured Basal Forebrain Neurons: Differentiation between Neuromodulatory and Neurotrophic Influences
Daniel S. Auld¹^,², Françoise Mennicken¹, and Rémi Quirion¹^,²^,³
¹ Douglas Hospital Research Center, Montréal, Québec, Canada H4H 1R3, and Departments of ² Neurology and Neurosurgery and ³ Psychiatry, McGill University, Montréal, Québec, Canada H3C 3J7

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Long-term exposure to nerve growth factor (NGF) is well established to have neurotrophic effects on basal forebrain cholinergicneurons, but its potential actions as a fast-acting neuromodulatorare not as well understood. We report that NGF (0.1-100 ng/ml)rapidly (<60 min) and robustly enhanced constitutive acetylcholine(ACh) release (148-384% of control) from basal forebrain cultureswithout immediate persistent increases in choline acetyltransferaseactivity. More ACh was released in response to NGF when exposurewas coupled with a higher depolarization level, suggesting activitydependence. In a long-term potentiation-like manner, brief NGFexposure (10 ng/ml; 60 min) induced robust and prolonged increasesin ACh release, a capacity that was shared with the other neurotrophins.K252a (10-100 nM), BAPTA-AM (25 µM), and Cd²⁺ (200 µM) prevented NGF enhancement of ACh release, suggestingthe involvement of TrkA receptors, Ca²⁺, and voltage-gated Ca²⁺ channels, respectively. Forskolin (10 µM), a cAMP generator,enhanced constitutive ACh release but did not interact synergisticallywith NGF. Tetrodotoxin (1 µM) and cycloheximide (2 µM) did notprevent NGF-induced ACh release, indicative of action at the levelof the cholinergic nerve terminal and that new protein synthesisis not required for this neurotransmitter-like effect, respectively.In contrast, after a 24 hr NGF treatment, distinct protein synthesis-dependentand independent effects on choline acetyltransferase activityand ACh release were observed. These results indicate that neuromodulator/neurotransmitter-like(protein synthesis-independent) and neurotrophic (translation-dependent)actions likely make distinct contributions to the enhancementof cholinergic activity byNGF.

Key words: brain-derived neurotrophic factor; choline acetyltransferase; neurotransmitter release; neuromodulation; cholinergic; neurotrophin

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Basal forebrain cholinergic neurons (BFCNs) innervate cortical and associated structures (Fibiger, 1982), are important forattention (Baxter and Chiba, 1999), and degenerate in Alzheimer'sdisease (Bartus, 2000). Rapid modulation of acetylcholine (ACh)release by physiological and pathological factors [e.g., neurotransmitters(Raiteri et al., 1984; Hersi et al., 1995), certain growth factors(Kar et al., 1997), $beta$ -amyloid (Auld et al., 1998), and interleukins(Hanisch et al., 1993)] is likely critical for the consequencesofinnervation.

Neurotrophins, including nerve growth factor (NGF), are crucial for the survival and function of certain neuronal populations(Levi-Montalcini, 1987). Regions of BFCN innervation (e.g., hippocampus,cortex) are enriched in NGF (Korsching et al., 1985; Large etal., 1986), and NGF is retrogradely transported by BFCNs (DiStefanoet al., 1992), with these neurons expressing TrkA and p75NTR receptors(Koh and Loy, 1989; Holtzman et al., 1992). NGF and TrkA are importantfor BFCN development, maintenance, and function in vivo (Vantiniet al., 1989; Li et al., 1995; Chen et al., 1997; Fagan et al.,1997; Molnar et al., 1998; Debeir et al., 1999; Ruberti et al.,2000), and NGF exposure (days to weeks) enhances cholinergic markersin BF cultures (Hartikka and Hefti, 1988; Takei et al., 1988,1989; Svendsen et al., 1994; Nonner et al., 1996; Pongrac andRylett, 1998; Oosawa et al., 1999; Auld et al., 2001). The neurotrophinsbrain-derived neurotrophic factor (BDNF), neurotrophin-3 (NT-3),and neurotrophin-4 (NT-4) also enhance cholinergic markers (Nonomuraet al., 1995; Nonner et al., 1996; Auld et al., 2001). Interestingly,even a 30 min exposure to NGF, BDNF, NT-3, or NT-4 increases cholineacetyltransferase (ChAT) activity 24 hr later (Nonner et al.,2000).

Neurotrophins rapidly increase intracellular Ca²⁺ in several neuronal phenotypes, including BFCNs (Wildering et al., 1995; Stoopand Poo, 1996; Jiang and Guroff, 1997; Li et al., 1998; Jia etal., 1999; Nonner et al., 2000), and acutely modulate neurotransmission(Lu and Chow, 1999; Schinder and Poo, 2000). BDNF and NT-3 rapidlyand Ca²⁺-dependently enhance neurotransmitter release from Xenopus motorneurons (Lohof et al., 1993; Stoop and Poo, 1996; He et al., 2000).BDNF can enhance hippocampal neurotransmission (Lessmann et al.,1994; Kang and Schuman, 1995; Li et al., 1998), inhibit high-frequencystimulation-associated fatigue (Gottschalk et al., 1998; Pozzo-Milleret al., 1999), and facilitate long-term potentiation (LTP) induction(Korte et al., 1995; Figurov et al., 1996; Patterson et al., 1996;Chen et al., 1999; Xu et al., 2000), with presynaptic TrkB typicallybeing involved. Also, NGF rapidly modulates stimulated ACh releasefrom hippocampal (Knipper et al., 1994) and visual-cortex (Salaet al., 1998) synaptosomes and likely influences visual-cortexLTP by modulating ACh release (Pesavento et al., 2000).

Using embryonic BF cultures, we report that NGF rapidly and potently enhanced ACh release in activity- and Ca²⁺-dependent manners and that increases persisted after NGF removal.Dichotomous actions consisting of protein synthesis-dependent"neurotrophic" effects on ChAT activity and protein synthesis-independent"neuromodulator" increases of ACh release were identified. Thesedistinct capacities may make complementary contributions to NGFenhancement of BFCNfunction.

  MATERIALS AND METHODS

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MATERIALS AND METHODS
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Culture. All experiments followed guidelines of the Canadian Council on Animal Care and McGill University policies. Cultureswere prepared as described previously (Auld et al., 2000a). BFregions (septum, diagonal band of Broca, and substantia innominata)of day 17 rat embryos (Charles River, St. Constant, QC, Canada)were dissected in HBSS (Life Technologies, Burlington, ON, Canada)containing 0.65% D(+)-glucose (Sigma, St. Louis, MO), 15 mM HEPES,10 U/ml penicillin, and 10 mg/ml streptomycin (Life Technologies).These were dissociated at 37°C with 0.08% trypsin (Life Technologies)and 0.1% DNase I (Sigma) for 18 min [terminated with 10% fetalbovine serum (FBS; Immunocorp, Montréal, QC, Canada)]. The dissociationwas completed mechanically with a fire-polished Pasteur pipette.Cultures were plated at 700,000-750,000 cells per well [precoatedwith poly-L-ornithine (0.3 µg/ml); Life Technologies] in 500 µlof growth medium in four-well tissue culture plates (Nunc, Naperville,IL), and cultures were maintained at 37°C and 5% CO₂. The mediumconsisted of DMEM (#11965; Life Technologies) supplemented withKCl [20 mM; total, 25 mM; similar high-K⁺ conditions are associated with improved viability in BF cultures(Nakamura et al., 1994)], sodium pyruvate (1 mM), D(+)-glucose(35 mM), HEPES (15 mM), and FBS (10%). Under similar culture conditions,which were optimized for the study of ACh release, both releaseand ChAT activity steadily increased between plating and 10 dayin vitro (DIV 10) (Auld et al., 2000a).

Acetylcholine release. In most experiments, on DIV 7, the medium was removed, and cells were rinsed with Krebs' buffer [125mM NaCl, 4.8 mM KCl, 1.2 mM KH₂PO₄, 25 mM HEPES, 1.2 mM MgSO₄,2.2 mM CaCl₂, 10 mM glucose, 10 µM choline, and 200 nM neostigmine(all from Sigma), pH adjusted to 7.4] containing 6 mM K⁺. Unless described otherwise in Results, after a 60 min equilibrationperiod at 37°C and 5% CO₂, this buffer was discarded and replacedfor a 45 min period with fresh buffer containing rh $beta$ NGF (R & DSystems, Minneapolis, MN; lots HS178041 or HS189011) or vehicle,from which ACh release was measured. Other compounds were deliveredduring the 60 min equilibration period as well as simultaneouslywith NGF during the ACh release period [BAPTA-AM (RBI, Natick,MA), CdCl₂ (Sigma), cycloheximide (Sigma), forskolin (Sigma),K252a (Calbiochem, La Jolla, CA) Rp-cAMPS (RBI), tetrodotoxin(TTX; Tocris, Ballwin, MO)]. For the rh $beta$ NGF, rhNT-3, rhNT-4, orrhBDNF (R & D Systems; lots NG059091, OU02805, and OD048111) pretreatments(see Figs. 6, 7), medium with FBS was replaced with medium supplementedwith B27 (2%; Life Technologies) containing the neurotrophin.After the indicated exposure period, culture wells were washedfour times with NGF/neurotrophin-free buffer, and constitutiveACh release was then collected for 60 min periods in the bufferdescribed above. In some experiments, p75NTR-IgG fusion protein(R & D Systems) was administered either concurrently with NGFor after NGF removal. All samples were kept at $-$ 80°C until AChor ChAT activity quantification (<2weeks).

The percentage of cholinergic neurons in BF cultures maintained under similar conditions is low (~1%) (Hartikka and Hefti,1988; Svendsen et al., 1994). However, their unique ability tosynthesize ACh makes quantification of supernatant ACh a reliablemeasure of their neurotransmitter release. To our knowledge, noreport concerning an effect of NGF in BF cultures has indicatedan indirect mechanism. BFCNs, but not GABAergic neurons, selectivelyexpress TrkA and p75NTR (Hartikka and Hefti, 1988; Koh and Loy,1989; Holtzman et al., 1992; Svendsen et al., 1994). At a functionallevel, BFCNs, but not GABAergic neurons, respond to NGF and BDNF(Koliatsos et al., 1994). TrkB also appears to be selectivelyexpressed on ChAT-immunoreactive somas in the BF (Molnar et al.,1998). Given that BFCNs selectively release ACh and respond toNGF, these cultures are an excellent model for studying theirinteractions.

Acetylcholine quantification. ACh was assayed by HPLC with electrochemical detection in conjunction with an enzyme reactor.Samples (100 µl) were injected manually via a 100 µl loop on atwo-position valve (Valco, Houston, TX). ACh and choline, separatedon a reverse-phase column (75 × 2.1 mm) pretreated with laurylsulfate, passed through an enzyme reactor (10 × 2.1 mm) containingacetylcholinesterase (EC 3.1.1.7; Sigma, type VI-S) and cholineoxidase (1.1.3.17; Sigma) covalently bound to glutaraldehyde-activatedLichrosorb NH₂ (10 µm; Merck, Darmstadt, Germany). All columnhardware and packing materials were from Chrompack (Raritan, NJ).The resultant hydrogen peroxide was electrochemically detectedat a platinum electrode at a potential of +500 mV versus an Ag/AgClreference electrode (Antec VT-03/Decade, Leiden, The Netherlands).The mobile phase, 0.2 M aqueous potassium phosphate buffer, pH8.0, with 1 mM tetramethylammonium hydroxide (Sigma), was deliveredat 0.4-0.45 ml/min by a dual piston pump (ESA 580, Chelmsford,MA) connected to a degasser (CMA 260, Stockholm, Sweden). ACheluted at ~4min.

Choline acetyltransferase activity. Cultures were homogenized in 200 µl ice-cold buffer (40 mM sodium phosphate buffer, pH7.4, 200 mM NaCl, and 0.5% Triton X-100). Aliquots in duplicatewere assayed for ChAT activity using [¹⁴C]-acetyl-CoA (New England Nuclear/DuPont, Markham, ON, Canada)and choline (Sigma) as substrate. After 60 min at 37°C, the reactionwas stopped with ice-cold 10 mM sodium phosphate buffer, pH 7.4,containing 0.2 mM acetylcholine chloride (Sigma). RadioactiveACh was extracted using butyronitrile (Sigma) containing 15 mg/mlsodium tetraphenylborate(Sigma).

Statistical analysis. Data were statistically analyzed using either Student's t test (unpaired) or one- or two-way ANOVAswith Tukey's post hoc test, where appropriate. In all cases, p< 0.05 was considered statistically significant. The n representsindividual culture wells evaluated in a given experiment, andunless indicated otherwise, data are expressed as mean ± SEM representingpercentage of control wells receiving appropriate vehicletreatments.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

NGF enhancement of ACh release is influenced by depolarization level

Exposure to NGF (100 ng/ml for 60 min in buffer with 6 mM K⁺) resulted in increased ACh release (~192% of control) during animmediately subsequent 10 min period of K⁺ (25 mM) depolarization (control, 168 ± 22 fmol per well per minute;NGF, 322 ± 16; n = 4; p < 0.001). Because some aspects of synapticplasticity are influenced by the level of neuronal electricalactivity, including neurotrophin modulation of neurotransmission(Gottschalk et al., 1998; Boulanger and Poo, 1999a), we examinedwhether NGF-associated increased ACh release could be modifiedby activity level. An identical NGF treatment in sister culturewells was associated with a greater increase in the amount ofACh released when subsequently paired with increased depolarization.Indeed, the same NGF treatment resulted in a ~2.4-fold greaterincrease of ACh release (femtomoles per well per minute) whenfollowed by exposure to 25 mM K⁺ compared with 6 mM K⁺ (the increase in each K⁺ condition was calculated vs ACh release from the same depolarizationconditions in the absence of NGF) (Fig. 1).

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Figure 1. Activity-dependent enhancement of ACh release by NGF. Cultures were preexposed to NGF (10 ng/ml) for 60 min in low K⁺ (6 mM) buffer. ACh release was then evaluated from low-activity (6 mM K⁺) or high-depolarization (25 mM K⁺) conditions for a 15 min period. Columns represent increased ACh (femtomoles per well per minute ± SEM; n = 8) associated with NGF preexposure versus the same depolarizing conditions without NGF preexposure. Significance was determined using Student's t test (*p < 0.001 vs 6 mM K⁺).

We chose to further examine NGF enhancement of ACh release under conditions of constitutive ACh release associated with endogenousactivity levels (in 6 mM K⁺ buffer) because interpretation of mechanistic aspects of theNGF-associated increases would be complicated by the facts thatK⁺ (25 mM) depolarization was associated with a large Ca²⁺-dependent induction of ACh release by itself, as well as thesynergistic interaction between increased activity level and NGFaction on ACh release. That most of the constitutive release wasnot sensitive to intracellular Ca²⁺ chelation (see below) enabled us to focus subsequent mechanisticstudies directly on NGF-induced ACh release. It should be pointedout that although there was a large relative effect of NGF comparedwith this spontaneous release (possibly representing nonspecificleakage), NGF actually induced more ACh release when coupled witha depolarizing stimulation (seeabove).

NGF enhances constitutive ACh release: contribution of TrkA and calcium

NGF (0.1-100 ng/ml) robustly enhanced constitutive ACh release from embryonic BF cultures during a 45 min exposure periodwithout inducing an immediate, persistent increase in ChAT activity(Fig. 2). Furthermore, under these conditions, neither cultureprotein levels (control, 100 ± 1%, n = 21; NGF, 100 ng/ml, 103± 2%, n = 8) nor metabolic activity, indicated by MTT reduction(control, 100 ± 2%, n = 7; NGF 100 ng/ml, 99 ± 5%, n = 4), werealtered; given the low percentage of cholinergic neurons in BFcultures, this was not unexpected (Hartikka and Hefti, 1988; Svendsenet al., 1994). The relative magnitude of NGF enhancement of AChrelease was time dependent and during 15, 30, and 60 min exposure/releaseperiods, NGF (1 ng/ml) enhanced constitutive ACh release to 127± 9% (n = 4; p < 0.05 vs control), 182 ± 11% (n = 6; p < 0.001),and 238 ± 25% (n = 6; p < 0.001) of control level, respectively.In the presence of TTX (1 µM), a 45 min exposure to NGF (1 ng/ml)still elicited robust ACh release (control, 100 ± 2%; TTX, 80± 6%; NGF, 287 ± 17%; NGF/TTX, 258 ± 27%; n = 6), suggesting anaction at the level of the cholinergic nerve terminal.

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Figure 2. NGF acutely enhances constitutive ACh release from embryonic basal forebrain neurons in a concentration-dependent manner during a short-term exposure but does not induce persistent ChAT activity changes. Data are expressed as a percentage of release or ChAT activity in the absence of NGF [mean ± SEM; 0 ng/ml (n = 59), 0.1 ng/ml (14), 0.5 ng/ml (14), 1 ng/ml (37), 10 ng/ml (27), and 100 ng/ml (19); control ACh release was ~630 fmol/well for the 45 min exposure period, representing ~14 fmol per well per minute]. Significance was determined using a one-way ANOVA with Tukey's post-test (*p < 0.001 vs control).

The tyrosine kinase inhibitor K252a blocked NGF (10 ng/ml)-induced increases in constitutive ACh release, suggesting the involvementof TrkA receptor signaling (Fig. 3). In the presence of 100 nMK252a, NGF did not increase ACh release beyond the control treatedwith K252a alone. Because cAMP signaling has been shown to enhancethe effects of neurotrophins (Meyer-Franke et al., 1998; Boulangerand Poo, 1999b), we examined its actions on NGF-induced ACh release(Fig. 4). Forskolin, at a much higher concentration (10 µM), increasedACh release to a magnitude similar to NGF (1 ng/ml). The coapplicationof NGF and forskolin, at these same concentrations, had only anadditive effect without evidence of synergistic interaction. Furthermore,Rp-cAMPS (100 µM), a protein kinase A (PKA) antagonist, did notsignificantly decrease NGF (1 ng/ml)-induced increases in constitutiveACh release associated with a 45 min exposure (control, 100 ±4%; Rp-cAMPS, 104 ± 1%; NGF, 329 ± 12%; NGF/Rp-cAMPS, 312 ± 12%;n = 4-9). Thus, the NGF increase of ACh release appears to notinvolve cAMP or PKA, at least under these low-K⁺ conditions.

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Figure 3. K252a (10-100 nM) prevents NGF (10 ng/ml) enhancement of ACh release during a short-term exposure. Data are expressed as a percentage of release in the absence of NGF and K252a (mean ± SEM; n = 6-8). Statistical analysis was performed using a two-way ANOVA with Tukey's post-test (*p < 0.001 vs K252a only, at the same concentration; p = 0.0627 vs cultures receiving neither K252a nor NGF).

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Figure 4. Forskolin (10 µM) alone increases ACh release but does not synergistically enhance NGF (1 ng/ml)-induced ACh release during a short-term exposure in low K⁺ (6 mM) conditions. Data are expressed as a percentage of release in the absence of forskolin and NGF (mean ± SEM; n = 6). Significance was determined using a one-way ANOVA with Tukey's post-test (*p < 0.001 vs control; p < 0.001 vs both NGF and forskolin).

To determine whether Ca²⁺ was involved in the NGF-induced increases in constitutive ACh release, intracellular Ca²⁺ was chelated using BAPTA-AM (25 µM), and under these conditionsNGF (1 ng/ml)-associated ACh release was prevented (Fig. 5A).We next investigated the involvement of voltage-gated Ca²⁺ channels (VGCC) using Cd²⁺, a nonspecific antagonist. Cd²⁺ (200 µM) blocked NGF (1 ng/ml)-induced increases in ACh release,suggesting that voltage-gated Ca²⁺ channels were involved (Fig. 5B). Together with inhibiting AChrelease increases caused by K⁺ stimulation (25 mM; 10 min), Cd²⁺ blocked NGF enhancement of release under these conditions aswell (data not shown).

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Figure 5. NGF (1 ng/ml)-enhanced ACh release involves Ca²⁺. A, The intracellular Ca²⁺ chelator BAPTA-AM (25 µM) inhibits NGF-induced ACh release during a short-term exposure. Data are expressed as a percentage of release in the absence of BAPTA-AM and NGF (mean ± SEM). Significance was determined using a one-way ANOVA with Tukey's post-test (*p < 0.001 vs control; p < 0.001 vs NGF/BAPTA-AM). B, NGF-induced ACh release is inhibited by the voltage-gated Ca²⁺ channel antagonist Cd²⁺ (200 µM). Data are expressed as a percentage of release in the absence of Cd²⁺ and NGF (mean ± SEM; n = 6). Significance was determined using a one-way ANOVA with Tukey's post-test (*p < 0.001 vs control; p < 0.001 vs NGF/Cd²⁺).

Brief exposure to neurotrophins induces prolonged ACh release

Treatment with NGF (10 ng/ml) for 60 min (followed by four rinses of culture plates) resulted in a robust increase of constitutiveACh release for at least the next 4 hr (Fig. 6A). Interestingly,comparable to the 60 min treatment, a 5 min exposure to NGF (10ng/ml) also resulted in increased ACh release during the hour-longperiod subsequent to NGF removal (289 ± 31% of control; n = 2;p < 0.05). Thus, it is likely that increased time after initialNGF exposure, rather than the duration of NGF exposure, was importantfor the time-dependent effect noted previously. The specificityof the prolonged influence of NGF on ACh release for the definedexposure period, as opposed to a possible influence of potentialresidual NGF left after rinse with NGF-free buffer, was indicatedby the capacity of a p75NTR-IgG (5 µg/ml) fusion protein to blockincreases when coadministered with NGF (10 ng/ml), but not ifgiven during the period of release determination immediately afterNGF washout (Fig. 6B).

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Figure 6. Brief exposure to NGF induces prolonged increase in ACh release. A, NGF (10 ng/ml for 60 min) treatment is associated with increased ACh release for at least 4 hr. Data are normalized according to release from control wells at the same hour and are expressed as mean ± SEM (n = 17-23). Statistical analysis was performed using repeated measure one-way ANOVA with Tukey's post-test; *p < 0.001 vs control. B, Treatment with NGF (10 ng/ml for 60 min) was associated with enhanced ACh release during the subsequent 60 min and was specific to availability during the defined exposure period, because a p75NTR-IgG fusion protein (5 µg/ml) only blocked the effect when coadministered with NGF. Data are normalized according to control wells and are expressed as mean ± SEM (n = 4-8). Statistical analysis was performed using a one-way ANOVA with Tukey's post-test: *p < 0.001 vs control, p < 0.001 vs NGF/co-p75NTR-IgG fusion protein.

Considering that these neurons respond to NT-3, NT-4, and BDNF with increased ChAT activity (Nonomura et al., 1995; Nonneret al., 1996, 2000), as well as retrogradely transport them fromtarget regions (DiStefano et al., 1992), we sought to determinewhether they acutely induced a persistent increase in ACh release.Under the same conditions as with NGF, a 60 min pretreatment withthe other neurotrophins (10 ng/ml) also enhanced ACh release inthe hour subsequent to their removal: NT-3, 153 ± 6% of control(n = 4; p < 0.001 vs control); NT-4, 161 ± 16% (n = 4; p < 0.01);and BDNF, 177 ± 19% (n = 4; p < 0.001). Furthermore, NGF was alsoassociated with increased K⁺-stimulated ACh release that persisted after its removal (datanotshown).

Differentiation between neurotrophic and neuromodulatory effects of NGF

Exposure to the protein synthesis inhibitor cycloheximide (2 µM) did not reduce NGF (1 ng/ml) enhancement of ACh release duringa 45 min exposure period (control, 100 ± 3%; cycloheximide, 97± 5%; NGF, 329 ± 35%; NGF/cycloheximide, 362 ± 57%; n = 6-8),suggesting that new protein synthesis was not required for therapid effect of NGF on ACh release. We next examined changes inChAT activity and ACh release after 6-24 hr NGF (100 ng/ml) exposureand the contribution of protein synthesis to these effects (Fig.7). After 6 and 12 hr of NGF exposure, ChAT activity was not significantlyincreased versus vehicle-treated control. Regardless of treatmentwith cycloheximide (2 µM), there was increased release of AChfrom NGF-treated groups. After 24 hr, ChAT activity was significantlyincreased in the NGF condition but was not increased in the NGF/cycloheximide-exposedcondition. Remarkably, the enhancement of ACh release associatedwith NGF/cycloheximide treatment was slightly larger than thatassociated with the NGF-alone condition, despite the markedlylower level of ChAT activity in the NGF/cycloheximide-treatedcultures after 24 hr exposures (Fig. 7). Our preliminary datasuggest that after a 24-hr treatment, enhanced ACh release associatedwith the NGF/cycloheximide treatment decays faster on removalof NGF compared with conditions in which protein synthesis isnot prevented, which are associated with increased ChAT activity(Auld et al., 2000b).

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Figure 7. Evidence for protein synthesis-dependent and -independent effects of NGF on ChAT activity and ACh release, respectively. ChAT activity (A) and constitutive ACh release (B) were compared after 6, 12, and 24 hr exposures to NGF (100 ng/ml) and/or cycloheximide (CY; 2 µM). Data are normalized according to controls and are expressed as mean ± SEM (6 hr, n = 4; 12 hr, n = 4-8; 24 hr, n = 20-24). Statistical analysis was performed using two-way ANOVAs with Tukey's post-test: *p <0.05 vs vehicle-treated control and p <0.05 vs NGF/CY (within ChAT and ACh, same hour); p < 0.05 vs NGF at 6 and 12 hr (within ChAT and ACh); ^§p < 0.05 vs NGF/CY at 6 and 12 hr (within ACh). Furthermore, at 6, 12, and 24 hr, the percentage changes in ACh release and ChAT activity were different within NGF and NGF/CY groups (p < 0.05).

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We report that NGF influences BFCNs in a manner encompassing acute enhancement of ACh release in a neurotransmitter/neuromodulator-likemanner. The concentrations of NGF enhancing ACh release indicatethat it as one of the most potent ACh secretagogues ever recognized.More NGF-enhanced ACh release was associated with a greater depolarization,suggesting that this interaction could underlie some aspects ofactivity-dependent sculpting of BFCN synapses. Even brief exposuresto NGF potentiated release for several hours after its removal,and this capacity was shared with BDNF, NT-4, and NT-3. Aftera 24 hr NGF treatment, distinct protein synthesis-dependent and-independent effects on ChAT activity and ACh release were observed.These findings imply that acute neurotransmitter-like as wellas classical neurotrophic influences contribute to the effectsof NGF on BFCN. These capabilities may make complementary contributionsto the formation, maintenance, and activity of BFCNsynapses.

The effective concentrations of NGF on ACh release suggest the involvement of TrkA receptors, which autophosphorylate at similarlylow ligand concentrations (Kaplan et al., 1991). Inhibition ofTrkA signaling with K252a prevented NGF-enhanced ACh release,consistent with K252a prevention of BDNF-enhanced neurotransmissionin hippocampal cultures (Li et al., 1998). Considering that K252a(100 nM) increased ACh release to some extent in our model, itwas not possible to reduce NGF-associated ACh release to vehicle-treatedlevels. Accordingly, a direct or modulatory role for p75NTR remainspossible.

Although the steps linking TrkA to ACh release remain to be fully established, in our model, TTX-sensitive Na⁺ channels were not critical. However, NGF-enhanced ACh releasewas prevented by BAPTA-AM and Cd²⁺, suggesting that Ca²⁺ action after entry via VGCC was critical. In accord with thesefindings, NGF rapidly increases voltage-sensitive Ca²⁺ currents in molluscan neurons and PC12 cells (Wildering et al.,1995; Jia et al., 1999), as well as increasing intracellular Ca²⁺ in primary BF cultures (Nonner et al., 2000).

Depolarization augmented the quantity of ACh release associated with NGF exposure, implying a mechanism for preferentiallymaintaining more release at active synapses. This is in agreementwith other reports of activity-dependent neurotrophin action onsynaptic efficacy (Gottschalk et al., 1998; Boulanger and Poo,1999a). Considering that synaptic fatigue may contribute to establishingACh release levels during the high-K⁺ exposure period, it is interesting that fatigue accompanyinghigh-frequency stimulation is prevented by BDNF (Gottschalk etal., 1998).

Our protocol involved a brief period of low activity (during and immediately before NGF exposure; 6 mM K⁺) after sustained high-activity levels (growth conditions; 25mM K⁺). It is possible that depolarization during the maturation ofBF cultures influenced NGF-associated signal transduction pathwaysand/or interacted with other BFCN characteristics to alter orfacilitate NGF-induced ACh release. Indeed, short-term or multi-dayK⁺ depolarization has been shown to modulate features of neurotrophinsignaling pathways in central (Meyer-Franke et al., 1998) or peripheralneurons (Vaillant et al., 1999), respectively. Moreover, in Xenopusmotor neurons, K⁺ depolarization rapidly increases the sensitivity of neurotransmissionto enhancement by BDNF (Boulanger and Poo, 1999a). Nevertheless,our preliminary observations suggest that BF cultures grown underlow-K⁺ conditions also respond acutely to NGF (10 ng/ml) with increasedACh release (data not shown). Thus, NGF-induced ACh release isnot unique to cultures grown under high-K⁺ conditions, although more subtle differences couldexist.

Activity upregulates synthesis and release of neurotrophins (Thoenen, 1995), with hippocampal expression and secretion ofNGF being elevated by muscarinic and nicotinic receptor signaling(da Penha Berzaghi et al., 1993; Knipper et al., 1994; Blochland Thoenen, 1995; French et al., 1999). The capacity of NGF toenhance ACh release and of ACh to increase NGF has been hypothesizedto contribute to synaptic efficiency (Knipper et al., 1994). Thesecharacteristics suggest potential mechanisms for immediate (i.e.,translation-independent secretagogue effects at the terminal level)and long-term (i.e., transcription/translation-dependent neurotrophiceffects) strengthening of synaptic connectivity resulting fromincreased NGF availability. Moreover, the activity-dependent natureof NGF-enhanced ACh release implies that this feedback could beamplified at more activesynapses.

TTX exposure did not prevent NGF-enhanced ACh release, and this is consistent with the selective expression of NGF receptorson BFCNs (Hartikka and Hefti, 1988; Koh and Loy, 1989; Holtzmanet al., 1992; Svendsen et al., 1994). Because NGF is highly expressedin regions of BF innervation (Korsching et al., 1985; Large etal., 1986), action at the terminal agrees with the potential physiologicalmodulation of ACh release by target-derived NGF. The TTX dataalso suggest that although increased depolarization is associatedwith greater NGF enhancement of ACh release, high levels of concurrentactivity are not required. This may be significant for developingBFCNs first encountering target-derived NGF, which may increaseACh release from innervating fibers with low intrinsic activity,resulting in feedback between ACh release and NGF secretion andthereby increasing NGF available for retrograde transport. Thetranslation-dependent actions of NGF likely include direct andindirect enhancement of action-potential generation probability.In an indirect neurotrophic manner, NGF increases BFCN excitabilityby altering properties of Ca²⁺ currents at the soma level (Levine et al., 1995) and increasesexcitability in other developing neurons by inducing expressionof Na⁺, K⁺, and Ca²⁺ channels (Lesser and Lo, 1995; Toledo-Aral et al., 1995; Hilbornet al., 1998). At the soma level, NGF increases BFCN firing undersome conditions, indicating that it can directly induce actionpotentials (Palmer et al., 1993; Albeck et al., 1999). Thus, target-derived,retrogradely transported NGF is likely to facilitate generationof action potentials, and this would be amplified by the synapse-strengtheningfeedback between ACh release and NGF secretion at the terminallevel. This could subsequently interact with the activity-dependentnature of the NGF secretagogue action to further promote synapseconsolidation.

A 60 min NGF exposure increased ACh release for at least 4 hr after its removal. This was not observed when ACh release wasstimulated with high K⁺ (without NGF), despite the ~10-fold increase (Auld et al., 2000a).The long-term enhancement of ACh release was dependent on NGFavailability only during the exposure period, suggesting thatcritical signal transduction/effector processes were initiatedquickly and remained activated for several hours. Even a 5 minexposure was associated with prolonged enhancement of release.These time frames are similar to NGF-induced increases in Ca²⁺, TrkA phosphorylation, and downstream pathways in primary BFcultures (Knusel et al., 1992; Downen et al., 1993; Nonner etal., 2000). Thus, transitory target-derived NGF secretion maysubsequently augment ACh release for several hours, greatly strengtheningthe synapse, although potential in vivo interactions with establishedcircuitry could modify this response. Considering that NT-3, NT-4,and BDNF also induced prolonged ACh release, they could play asimilar role during synaptic development andmaintenance.

Complementary to our observations, a 30 min neurotrophin exposure increased ChAT activity measured 24 hr later in BFCNs (Nonneret al., 2000), and a 1 min exposure to NGF induced Na⁺ channel expression in PC12 cells (Toledo-Aral et al., 1995).Thus, even short exposures to neurotrophins can cause lastingeffects via both neurotrophic and secretagogue mechanisms. Regardingprolonged responses of BFCNs to brief neurotrophin exposures,it seems likely that increases in ChAT activity (Nonner et al.,2000) and translation-independent ACh release (this report) dependon common (e.g., TrkA, Ca²⁺) and disparate (e.g., translation) mechanisms. Because Ca²⁺ is involved in NGF-induced ACh release, the mechanism(s) sustainingprolonged release likely involves Ca²⁺-dependent elements. Ca²⁺ activates kinases that regulate neurotransmission and vesicletrafficking, such as Ca²⁺/calmodulin-dependent kinase II (Llinas et al., 1985; Greengardet al., 1993). Interestingly, this kinase has been implicatedin NT-3-induced neurotransmitter release from Xenopus motor neurons(He et al., 2000).

Rapid NGF enhancement of ACh release was not reduced by cycloheximide, suggesting that protein translation is not involved.In agreement with previous observations (Pongrac and Rylett, 1998),increased ChAT activity after 24 hr NGF exposure was dependenton new protein synthesis. Interestingly, even after 24 hr, andregardless of the lack of increase in ChAT activity, there wasa large protein synthesis-independent enhancement of ACh releaseassociated with the NGF/cycloheximide condition. Thus, NGF canenhance ACh release in a secretagogue manner after prolonged exposure,and this may have relevance for maintenance of ACh release levelsat BFCN synapses that are exposed to target-derived NGF. It isalso apparent that under some conditions, increased ChAT activityis not associated with $---$ or required for $---$ enhancement of ACh releaseafter prolonged NGF exposure. Together, these data suggest thatthe translation-independent secretagogue action of NGF may contributeto a portion of increased ACh release, even after prolonged NGFexposures sufficient to induce transcription and translation-dependentincreases in ACh synthesiscapacity.

In summary, NGF rapidly enhanced ACh release from embryonic BF cultures. The NGF-associated increase was activity dependentand, unlike classical neurotransmitter modulation, persisted forseveral hours after NGF removal in a manner akin to LTP. The NGF-inducedincrease was dependent on TrkA signaling, Ca²⁺, and VGCCs, but not dependent on new protein synthesis. Aftera 24 hr treatment with NGF, distinct protein synthesis-dependentand -independent effects on ChAT activity and ACh release, respectively,were observed. Together, these data suggest that in addition totranslation-dependent neurotrophic actions, NGF has strong influenceson BFCN function via both rapid and prolonged modulation of AChrelease in a neurotransmitter/neuromodulator-likemanner.

  FOOTNOTES

Received Dec. 5, 2000; revised March 8, 2001; accepted March 9, 2001.

This work was supported by the Medical Research Council of Canada (MRCC)/Canadian Institutes of Health Research (CIHR). D.S.A.holds a Doctoral Award from MRCC/CIHR. We thank Dr. Brian Collierand Dr. Freda Miller for critically reading this manuscript, andDr. Joseph Rochford for advice concerning statisticalanalyses.
Correspondence should be addressed to Dr. Rémi Quirion, Scientific Director, Douglas Hospital Research Center, 6875 BoulevardLasalle, Montréal, Québec, Canada H4H 1R3. E-mail: quirem{at}douglas.mcgill.ca.

D. S. Auld's present address: Centre de Recherche en Sciences Neurologiques, Département de Physiologie, Université de Montréal,P.O. Box 6128, Station Centre-ville, Montreal, Québec, CanadaH3C3J7.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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