Pituitary Adenylate Cyclase-Activating Polypeptide (PACAP-38) Protects Cerebellar Granule Neurons from Apoptosis by Activating the Mitogen-Activated Protein Kinase (MAP Kinase) Pathway

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Volume 17, Number 1, Issue of January 1, 1997 pp. 83-90
Copyright ©1997 Society for Neuroscience

Pituitary Adenylate Cyclase-Activating Polypeptide (PACAP-38) Protects Cerebellar Granule Neurons from Apoptosis by Activating the Mitogen-Activated Protein Kinase (MAP Kinase) Pathway

Martin Villalba, Joël Bockaert, and Laurent Journot
Centre National de la Recherche Scientifique (CNRS), Unité Propre de Recherche 9023, Centre CNRS-Institut National de la Santé et de la Recherche Médicale de Pharmacologie-Endocrinologie, F-34094 Montpellier Cedex 05, France

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Pituitary adenylate cyclase-activating polypeptides (PACAP-27 and PACAP-38) are neuropeptides of the vasoactive intestinalpolypeptide (VIP)/secretin/glucagon family. PACAP receptors areexpressed in different brain regions, including cerebellum. Weused primary culture of rat cerebellar granule neurons to studythe effect of PACAP-38 on apoptosis induced by potassium deprivation.We demonstrated that PACAP-38 increased survival of cerebellarneurons in a dose-dependent manner by decreasing the extent ofapoptosis estimated by DNA fragmentation. PACAP-38 induced activationof the extracellular signal-regulated kinase (ERK)-type of mitogen-activatedprotein (MAP) kinase through a cAMP-dependent pathway. PD98059,an inhibitor of MEK (MAP kinase kinase), completely abolishedthe antiapoptotic effect of PACAP-38, suggesting that MAP kinasepathway activation is necessary for PACAP-38 action.
Key words: PACAP; cerebellum; apoptosis; MAP kinase; cAMP; PD 98059

INTRODUCTION

Cerebellar granule cells are among the most abundant neuronal population in the mammalian CNS. During the first few weeksof postnatal life, there is a well documented cell loss in thematuring granule cell layer of the cerebellum (Landis and Sidman,1978). Cerebellar granule cells undergo apoptosis between postnataldays 5 and 9, whereas cell loss between the third and fifth postnatalweeks is not associated with DNA fragmentation (Wood et al., 1993).In vitro culture of newborn rat cerebellar neurons provided agood model to study neuronal apoptosis because of the high degreeof cellular homogeneity (Marini and Paul, 1992). Cerebellar granulecells survive and differentiate in vitro in the presence of depolarizingconcentrations of KCl (25-30 mM) without additional need for neurotrophicfactors (Gallo et al., 1990). The mechanism of action of KCl remainsobscure so far, but, generally, it is believed that an increasein intracellular Ca²⁺ concentration (D'Mello et al., 1993; Yan et al., 1994; Galliet al., 1995) and mitogen-activated protein (MAP) kinase activation(Rosen et al., 1995) induced by depolarization are involved. Inthe presence of a normal concentration of KCl (5-10 mM), cerebellargranule cells undergo apoptosis, which is inhibited by differentcategories of molecules: (1) forskolin (D'Mello et al., 1993)and cholera toxin (Yan et al., 1995a), which raise cAMP levels;(2) IGF-1 (D'Mello et al., 1993), which activates a tyrosine kinasereceptor; and (3) agonists of muscarinic cholinergic receptors(Yan et al., 1995b) and metabotropic glutamate receptors (Copaniet al., 1995), which stimulate phospholipase C. The effect ofcAMP is of particular interest because it was also demonstratedin other neuronal systems, such as sympathetic and sensory neurons(Rydel and Greene, 1988), dopamine neurons (Mena et al., 1995),and developing septal cholinergic neurons (Kew et al., 1996).The mechanism underlying the cAMP antiapoptotic effect is notwell understood; however, it was suggested that the MAP kinasepathway is involved (Kew et al., 1996). Although cAMP inhibitsthe MAP kinase cascade in some cell lines (Burgering et al., 1993;Cook and McCormick, 1993; Graves et al., 1993; Sevetson et al.,1993; Wu et al., 1993) and has no effect in rat sympathetic neurons(Virdee and Tolkovsky, 1995), it stimulates MAP kinase cascadein other cell lines, including PC12 (Faure et al., 1994; Frödinet al., 1994). MAP kinase activation also has been involved inthe protection of PC12 cells from NGF withdrawal-induced apoptosis(Xia et al., 1995).

Modulation of granule cell loss by physiological agents has not been described carefully. Evidence for the presence of pituitaryadenylate cyclase-activating polypeptides (PACAP) and PACAP receptorin the cerebellum is compelling and suggests a physiological rolefor PACAP in cerebellum development (Lam et al., 1990; Cauvinet al., 1991; Basille et al., 1993, 1995; Hashimoto et al., 1993;Spengler et al., 1993; Favit et al., 1995). PACAPs are neuropeptidesof the vasoactive intestinal polypeptide (VIP)/secretin/glucagonfamily, which are named according to their amino acid number:PACAP-27 and PACAP-38. PACAP-27 corresponds to the 27 N-terminalamino acids of PACAP-38 and displays 68% homology with VIP. Twoclasses of PACAP receptors have been described with respect totheir pharmacological properties: type I PACAP receptors bindPACAP-27 and -38 two orders of magnitude more potently than VIP,whereas type II PACAP receptors do not discriminate between PACAP-27,-38, and VIP. At present three genes encoding PACAP/VIP receptorshave been cloned. PACAP₁-R corresponds to type I binding sites,whereas PACAP/VIP₁-R and PACAP/VIP₂-R correspond to type II PACAPreceptors. No VIP-specific receptor has been cloned yet. PACAP-38modulates the release of several pituitary hormones (Miyata etal., 1989) and of catecholamines from the adrenal gland (Watanabeet al., 1992; Isokobe et al., 1993). In addition, PACAP-38 promotesneurite outgrowth in PC12 cells (Deutsch and Sun, 1992; Hernandezet al., 1995) and NB-OK neuroblastoma (Deutsch et al., 1993),stimulates neuritogenesis and survival of cultured rat sympatheticneuroblasts (Pincus et al., 1990; DiCicco-Bloom and Deutsch, 1992),and prevents natural neuronal cell death in chick embryo and HIVgp120-induced cell death in hippocampal cultures (Arimura et al.,1994). Because of the demonstrated presence of PACAP-38 in thecerebellum and the neurotrophic and neuroprotective activity ofPACAP-38 in other systems and because PACAP-38 stimulates cAMPproduction, we tested PACAP-38 as a modulator of apoptosis inprimary culture of cerebellar granule cells.

MATERIALS AND METHODS
Materials. PACAP was obtained from Neosystem (Strasbourg, France), [ $gamma$ -³²P]ATP and [2-³H]adenine from Isotopchim, Biotrak MAP Kinase Enzyme assay kitfrom Amersham (Arlington Heights, IL), IGF-1 from Bachem AG (Torrence,CA), Rp-cAMP and Sp-cAMP from RBI, antibody against phospho-ERKfrom New England Biolabs (Beverly, MA), H89 from Calbiochem (Lucerne,Switzerland), BMEM and BMEM-Glutamax-I from Life Technologies(Gaithersburg, MD), and Taq DNA polymerase from Eurobio. PD98059was a generous gift from Dr. Alan R. Saltiel (Parke-Davis PharmaceuticalResearch). All other reagents, unless otherwise indicated, werefrom Sigma (St. Louis, MO).

Culture of cerebellar granule cells. Rat cerebellar granule neurons were prepared from 8-d-old Wistar rat pups, as previouslydescribed (Levi et al., 1984). Briefly, freshly dissected cerebellawere incubated with 0.25 mg/ml trypsin for 10 min at 37°C. Trypsininhibitor (0.5 mg/ml) and 0.08 mg/ml DNase were added to stopthe reaction. Digested cerebella were centrifuged and disruptedmechanically with a Pasteur pipette in the presence of DNase andtrypsin inhibitor. Cells were seeded at a density of 0.25 × 10⁶ cells/cm² in Falcon dishes coated with poly-L-lysine in BMEM supplementedwith 10% fetal calf serum (FCS), 10 U of penicillin, 10 µg ofstreptomycin, 30 mM KCl, 10 mM HEPES, pH 7.4, 17 mM glucose, and2 mM glutamine. After 24 hr, 10 µM cytosine arabinoside was addedto the culture medium. Cultures were used after 7 d in vitro (DIV).

Neuronal viability. Viable granule neurons were quantified as previously described (Didier et al., 1990). Briefly, 7 DIV cultureswere washed twice with HK medium (BMEM-glutamax-I supplementedwith 30 mM KCl, 10 mM HEPES, pH 7.4, and 17 mM glucose) and cultivatedfor 48 hr in HK or LK medium (BMEM-glutamax-I supplemented with10 mM KCl, 10 mM HEPES, pH 7.4, and 17 mM glucose) with or withoutthe different drugs. For control cultures in serum-containingmedium, the cells were washed twice with HK medium and refed withculture medium used throughout the culture to avoid the neurotoxiceffect of fresh serum-containing medium (Yan et al., 1994). Cultureswere exposed to 15 µg/ml fluorescein diacetate (FDA) for 10 minat 37°C. The medium was aspirated, and lysis buffer (15 mM Tris-HCl,pH 7.4, and 1% SDS) was added. After 15 min, the supernatant wascollected, and the amount of fluorescein was determined with aspectrofluorometer.

Quantification of DNA fragmentation. Cultures (7 DIV) were washed twice with HK medium. HK or LK medium with or without thedifferent drugs was added for 24 hr. In experiments in which antagonistswere tested, neurons were preincubated for 1 hr with the antagonistsin serum-containing medium to allow loading of the cells. Neurons(5 × 10⁶) were trypsinized, scraped, and collected by centrifugation.Three hundred microliters of lysis buffer (0.5% Triton X-100,20 mM EDTA, and 5 mM Tris-HCl, pH 7.4) were added, and incubationwas continued for 20 min at 4°C. Cells were centrifuged at 27,000× g for 15 min. Pellets (nuclei plus intact chromatin) were incubatedwith 300 µl of lysis buffer plus 100 µg of proteinase K. ProteinaseK (60 µg) was added to the supernatant (soluble DNA). Sampleswere incubated for 2 hr at 60°C and then overnight at 37°C withgentle shaking. The DNA was extracted with phenol-chloroform.Soluble DNA (200 µl) or nonsoluble DNA (50 µl) was incubated inTNE buffer (10 mM Tris-HCl, pH 7.4, 200 mM NaCl, and 1 mM EDTA)with 0.5 µg/ml of Hoechst 33258. Fluorescence was measured witha spectrofluorometer (excitation 356 nm; emission 492 nm). Similarresults were obtained with the Cell Death Detection ELISA kitfrom Boehringer Mannheim (Cat. No. 1544 675; Mannheim, Germany).

DNA laddering. DNA extraction was performed as described above. After phenol-chloroform extraction, the DNA was precipitatedwith ethanol, resuspended in TE buffer (10 mM Tris-HCl, pH 8.0,and 1 mM EDTA) supplemented with 2 µg/ml RNase A, and incubatedovernight at 37°C. Samples were electrophoresed through a 1.2%agarose gel. DNA was visualized by ethidium bromide staining.

Photomicrographs. Cultures (7 DIV) were incubated for 48 hr as indicated above with the different drugs. Cells were incubatedwith FDA as indicated above and photographed with a phase-contrastmicroscope or with a fluorescence microscope using the fluoresceinfilter after three washes with PBS. For propidium iodide staining,7 DIV cultures were incubated for 48 hr as indicated above withthe different drugs. At the end of the incubation period, cellswere fixed with 3% paraformaldehyde in PBS and then permeabilizedwith 0.2% Triton X-100 in PBS for 15 min at room temperature.Cells were incubated overnight with 50 µg/ml propidium iodideat 4°C. After three washes with PBS, coverslips were mounted withMowiol and examined by fluorescence microscopy using a rhodaminefilter.

Extracellular signal-regulated kinase (ERK) activity. ERK activity was determined by the Biotrak p42/p44 MAP kinase enzymeassay kit as recommended by the manufacturer (Amersham). Briefly,7 DIV cultures were washed twice with HK medium. HK or LK mediumwith or without the different drugs was added for 10 min at 37°C.In experiments in which antagonists were tested, neurons werepreincubated for 1 hr with the antagonists in serum-containingmedium to allow loading of the cells. The incubations were terminatedby aspiration, and the cells were lysed immediately in lysis buffercontaining (in mM): Tris-HCl 10, pH 7.4, NaCl 150, EGTA 2, DTT2, orthovanadate 1, and PMSF 1 with 10 µg/ml leupeptin, 10 µg/mlaprotinin, and 0.2% Triton X-100. Cell extract (15 µl) was mixedwith 10 µl of substrate buffer containing an ERK-specific peptidesubstrate, and the reaction was started by adding 5 µl of [ $gamma$ ³²P]-ATP. After 30 min at 30°C, the reaction was terminated by adding10 µl of stop reagent containing orthophosphoric acid. Then 30µl was pipetted onto the center of paper disks, followed by washingtwice in 75 mM orthophosphoric acid for 2 min and twice in waterfor 2 min. Disks containing phosphorylated peptide were countedon a scintillation counter.

Detection of phospho-ERKs. After incubation for 10 min at 37°C as described above for determination of ERK activity, 7 DIVcultures were lysed in Laemmli buffer. Samples were electrophoresedthrough a 10% acrylamide gel and blotted on a nitrocellulose membrane.Membranes were treated with a phospho-specific MAPK antibody (1:1000;New England Biolabs) and developed with the Phototope-Star WesternBlot Detection kit (New England Biolabs). Then membranes werestripped with stripping solution (100 mM Tris-HCl, pH 6.7, 2%SDS, and 100 mM $beta$ -mercaptoethanol), incubated with anti-ERK1 andanti-ERK2 antibodies (1:400 each; Santa Cruz Biotechnology, Tebu,France), and developed with the Renaissance Western detectionkit (Dupont NEN, Boston, MA).

Determination of cAMP levels. Cultures (7 DIV) were washed twice with HK medium and incubated for 2 hr in the presence of[2-³H]adenine in HK medium. Cells were incubated in the same mediumsupplemented with 0.5 mM 3-isobutyl-1-methylxanthine (IBMX) for15 min at 37°C. Various concentrations of PACAP or VIP were addedfor 15 min. The medium was aspirated, and the reaction was stoppedby the addition of 1 ml of 5% trichloroacetic acid (TCA) at 4°C.Cells then were scraped and centrifuged. cAMP levels in the supernatantwere measured as previously described (Salomon et al., 1974).

RT-PCR experiments. Total RNA was prepared from 7 DIV cultures using standard techniques (Chomczynski and Sacchi, 1987). RT-PCRreaction was performed as described (Rawlings et al., 1995). Single-strandedcDNA was synthesized from total RNA with the following protocol.One microliter of total RNA (3 µg/µl) was preincubated with 3µl of a hexamer random primer mixture (100 µM) and 22.5 µl ofH₂O at 70°C for 10 min and then rapidly chilled on ice. To thisreaction were added 1 µl of RNasin (40 U/µl), 10 µl of 5× RT buffer,5 µl of dithiothreitol (100 mM), and 2.5 µl of deoxyribonucleotides(dNTP; 10 mM of each), and the mixture was incubated at 45°C for2 min. Finally, 5 µl of Moloney murine leukemia virus reversetranscriptase (MoMuLVRT; 200 U/µl) was added to give a final volumeof 50 µl; the reaction was incubated at 45°C for 60 min and thenterminated by placing it on ice. The template produced from theRT reaction was amplified using one of three sets of primers,dependent on the PACAP/VIP receptor we wished to identify. Forall three receptors we used primers that flank the putative thirdintracellular loop of the receptor. For PACAP₁-R, the two primersused were PAC1-FL (5 $'$ -TTTCATCGGCATCATCATCATCATCCTT-3 $'$ ) and PAC1-VK(5 $'$ -CCTTCCAGCTCCTC-CATTTCCTCTT-3 $'$ ), which would be expected toproduce PCR product sizes of 280 base pairs (bp) for the "short"variant, 361 bp for the "hop2" variant, 364 bp for the "hip" or"hop1" variants, 445 for the "hip-hop2" variant and 448 bp forthe "hip-hop1" variant (Spengler et al., 1993). For PACAP/VIP₁-R,the primers used were VIP1-AI (5 $'$ -GCCCCCATCCTCCTCTCCATC-3 $'$ ) andVIP1-EL (5 $'$ -TCCGCCTGCACCTCACCATTG-3 $'$ ), which should give a PCRproduct of 299 bp (Ishihara et al., 1992). The PACAP/VIP₂-R primersused were VIP2-AE (5 $'$ -ATGGATAGCAACTCGCCTTTCTTTAG-3 $'$ ) and VIP2-QL(5 $'$ -GGAAGGAACCAACACATAACTCAAACAG-3 $'$ ), yielding a predicted PCRproduct 325 bp in length (Lutz et al., 1993). For the PCR reaction,29 µl of H₂O, 5 µl of 10× PCR buffer, 4 µl of MgCl₂ (25 mM), 1µl of dNTP (10 mM of each), 0.5 µl of Taq DNA polymerase (5 U/µl),0.25 µl of both the relevant oligonucleotide primers (50 µM),and 5 µl of the relevant RT products (or, for the controls, 5µl of the RT reaction in which reverse transcriptase had beenomitted) were added to each tube to give a final volume of 50µl. The PCR reaction was run on a GeneAmp PCR system 9600 (Perkin-Elmer/Cetus,Norwalk, CT) at 94°C for 1 min, followed by 35 cycles of 94°Cfor 30 sec, 58°C for 30 sec, 72°C for 45 sec, and then a finalcycle of 72°C for 420 sec. Because the same primer pair is usedto amplify all variants of the PACAP₁-R, the relative abundanceof the PCR products is a qualitative index of the abundance ofthe corresponding transcripts. This point was verified by mixingvarious proportions of different plasmids containing, each, adifferent insert encoding a different variant (data not shown).

RESULTS
Cultures (7 DIV) were washed and incubated with HK medium or LK medium with or without the different drugs, as indicated inMaterials and Methods. Viable cells were visualized by stainingwith FDA (Fig. 1A). As previously reported (D'Mello et al., 1993),decreasing potassium concentration induced a large decrease inthe number of cells stained by FDA, and this effect was abrogatedby IGF-1 and partially abolished by compounds raising cAMP levels,such as forskolin (Fig. 1A). Interestingly, the effect of forskolinwas reproduced fully by PACAP-38 (Fig. 1A). For more quantitativeresults, we measured cell survival via the FDA conversion technique(Fig. 1B). The decrease in potassium concentration induced a largedecrease in FDA conversion, which was protected partially by forskolinor PACAP-38. Interestingly, protection by PACAP-38 was dose-dependentwith a maximal effect at 100 nM and an EC₅₀ of 5 nM (Fig. 1C).
Fig. 1. PACAP-38 increases survival of cerebellar granule neurons. A, Seven-day-old neurons were deprived of serum and maintainedfor 48 hr in serum-containing medium (FCS), HK medium (HK), LKmedium (LK), or LK medium supplemented with 25 ng/ml IGF-1 (IGF),100 nM PACAP38 (P38), or 10 µM forskolin (FK). Then cultures wereincubated with FDA and photographed by phase-contrast and fluorescencemicroscopy. Magnification bar, 50 µm. B, Survival was determinedby the FDA method (see Materials and Methods). Results were expressedas the percentage of total fluorescein production in sister culturestreated with HK medium. Data are the mean ± SEM of three independentexperiments performed in triplicate. *p < 0.0005 with Student'st test, as compared with (a) HK and (b) LK. C, Dose-response curveof PACAP-38-induced increase in FDA conversion. Data are the mean± SEM of three independent experiments performed in triplicate.
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A decrease in potassium concentration was reported previously to induce apoptosis in cerebellar granule cells (D'Mello etal., 1993; Yan et al., 1994). Therefore, staining with propidiumiodide was performed after permeabilization of the cells. Changingfrom serum-containing medium to HK medium did not induce apoptosis(Fig. 2A). In contrast, the presence of numerous nuclei displayingfragmented or condensed chromatin, a characteristic feature ofapoptotic nuclei (Earnshaw, 1995), revealed apoptosis in LK medium(Fig. 2A). Interestingly, PACAP-38 (100 nM) and forskolin (10µM) efficiently protected neurons from apoptosis, because thenumber of apoptotic nuclei was reduced (Fig. 2A). The biochemicalhallmark of apoptosis is nuclear DNA fragmentation into oligonucleosomalfragments, which can be visualized as a DNA ladder by agarosegel electrophoresis of soluble DNA (Wyllie, 1980; Hockenberryet al., 1990). Using this method, we confirmed that potassiumdeprivation induced apoptosis in cerebellar granule cell culturesand showed that PACAP-38 (100 nM) or forskolin (10 µM) decreasedthe intensity of DNA laddering. High KCl concentration completelyblocked laddering (Fig. 2B). By comparing the amount of fragmentedDNA in the presence of PACAP-38 with different amounts of fragmentedDNA from LK condition, we estimated the protective effect of PACAP-38to 60% (Fig. 2B). To have a more quantitative assessment of DNAladdering, we developed a protocol to quantify the proportionof fragmented DNA, as described in Materials and Methods. PACAP-38protected cerebellar granule neurons from apoptosis in a dose-dependentmanner, with a maximal effect ~100 nM (Fig. 2C).
Fig. 2. PACAP-38 protects cerebellar granule neurons from apoptosis. A, Changes in nuclear morphology. Seven-day-old neurons weredeprived of serum and maintained for 24 hr in HK medium (HK),LK medium (LK), or LK medium supplemented with either 100 nM PACAP-38(P38) or 10 µM forskolin (FK). Control cultures were kept in serum-containingmedium (FCS). Magnification bar, 10 µm. B, PACAP decreased fragmentationof DNA from cerebellar granule cells induced by LK medium. Cultureswere incubated as in A. Soluble DNA was extracted, electrophoresed,and visualized with ethidium bromide staining. To illustrate quantitativelythe extent of protection from DNA laddering by PACAP or forskolin,we loaded a different amount of soluble DNA obtained from oneplate incubated in LK medium alone (100-20%). Data are representativeof three independent experiments. C, Dose-response curve of PACAP-38-induceddecrease in DNA fragmentation. Seven-day-old neurons were deprivedof serum and maintained for 24 hr in LK medium supplemented withdifferent PACAP-38 concentrations. Soluble and nonsoluble DNAwas isolated and quantified as described in Materials and Methods.Data are the mean ± SEM of three independent experiments.
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It is noteworthy that the switch from serum-containing medium used throughout the culture to HK medium also induced some celldeath (data not shown). However, this death was essentially necrotic,because no DNA laddering and no chromatin condensation were shownin HK medium (Fig. 2B). Furthermore, neither forskolin nor PACAP-38had any protective effect in HK medium, as compared with HK mediumalone, when FDA conversion was measured (data not shown). Thisindicates that the cells protected by forskolin or PACAP-38 werethose dying by apoptosis because of potassium deprivation andnot those dying by necrosis because of serum withdrawal.

To identify the PACAP receptor(s) involved, we performed RT-PCR with primers specific for the different PACAP/VIP receptorsubtypes and splice variants. We demonstrated the expression ofPACAP₁-R and PACAP/VIP₁-R (Fig. 3A). The products obtained withprimers specific for the PACAP₁-R indicated that variants withone cassette (hip or hop) were expressed preferentially and thatthe short variant was expressed at much lower levels. Using restrictionenzymes that are specific for the hip (AvaII) or hop (Bpu1102I) variants (Rawlings et al., 1995), we identified the one cassetteband as PACAP₁-R hop (data not shown). Conclusively, cerebellargranule cells mainly express PACAP₁-R hop mRNA. In addition, weperformed pharmacological characterization of the expressed PACAP/VIPreceptor(s) (Fig. 3B). Stimulation of cAMP production by PACAPand VIP indicated the presence of type I PACAP receptor, whichis compatible with RT-PCR experiments. On the other hand, thepotency of VIP to stimulate cAMP production was low, indicatingthat no type II PACAP receptor (PACAP/VIP₁-R or PACAP/VIP₂-R)was expressed significantly in contrast to what was anticipatedfrom RT-PCR experiments.
Fig. 3. A, Cerebellar granule neurons express predominantly PACAP₁-R with one cassette. Seven-day-old neurons were washed twice withHK medium, and total RNA was isolated. After reverse transcription(RT+) and PCR amplification, DNA was electrophoresed and visualizedwith ethidium bromide. Reverse transcriptase was omitted in controlexperiments (RT $-$ ). The predicted fragment size was 280 bp forPACAP₁-R s (short variant), 361 bp (hop2) or 364 bp (hip or hop1)for a single cassette insert, and 445 bp (hip-hop2) or 448 bp(hip-hop1) for double insert, 299 bp for PACAP/VIP₁-R, and 325bp for PACAP/VIP₂-R. Data are representative of two independentexperiments. B, PACAP- or VIP-stimulated cAMP production in cerebellargranule cells. Neurons were incubated for 15 min at 37°C in LKmedium containing the indicated concentrations of PACAP-38 (opencircles), PACAP-27 (open squares), or VIP (filled triangles).Data are expressed as the percentage of cAMP production inducedby 20 µM forskolin. Data are the mean ± SEM of three independentexperiments performed in triplicate.
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Because activation of the MAP kinase pathway has been involved in protection from apoptosis and because cAMP has been shownto stimulate MAP kinase activity in some experimental systems,we measured PACAP-stimulated ERK activity. PACAP-38 stimulatedERK activity in a dose-dependent manner with a maximal effectat 100 nM (Fig. 4A). We demonstrated that tetrodotoxin (TTX) didnot block PACAP-induced stimulation of MAP kinase activity (Fig.4B), suggesting that the effect of PACAP was not mediated by therelease of neurotransmitters or neurotrophic factors. Rp-cAMPand H89, two inhibitors of PKA, and PD98059, an inhibitor of MEK,blocked stimulation of ERK activity by PACAP-38 and forskolin(Fig. 4C). We extended our analysis by performing Western blotswith anti-phospho-ERK antibodies. We demonstrated that ERK2 wasmore abundant than ERK1 and that PACAP-38 induced phosphorylationof both kinases (Fig. 4D). Modulation of the phosphorylation stateof ERK1 and ERK2 by the different treatments was in agreementwith results obtained by the measurement of ERK activity.
Fig. 4. A, PACAP-38 stimulated MAP kinase activity. Neurons were incubated with the indicated concentrations of PACAP-38 for 10 minat 37°C. MAPK activity was determined as described in Materialsand Methods. Data are expressed as the percentage of MAP kinaseactivity in LK medium alone. Data are the mean ± SEM of threeindependent experiments performed in triplicate. B, PACAP-38 andforskolin induced MAPK activation independently of neuronal activity.Neurons were incubated for 1 hr in the presence of 1 µM tetrodotoxin(TTX) and then stimulated with HK medium, 100 nM PACAP-38, or10 µM forskolin for 10 min. Data are the mean ± SEM of three independentexperiments performed in triplicate. *p < 0.005; **p < 0.0005with Student's t test. Values were compared with the correspondingcontrol (LK alone or LK + TTX). C, PACAP stimulates MAP kinaseactivity via a PKA- and MEK-dependent mechanism. Neurons wereincubated for 1 hr in the presence or absence of different inhibitors(25 µM PD98059; 20 µM H89; 200 µM Rp-cAMP), washed twice, andincubated at 37°C for 10 min with 100 nM PACAP-38 and 10 µM forskolinin the presence or absence of the inhibitors. Data are the mean± SEM of three independent experiments performed in triplicate.*p < 0.0005 with Student's t test, as compared with (a) LK, (b)PACAP-38 (P38), and (c) forskolin (FK). D, PACAP-38 and forskolin-inducedphosphorylation of ERK1 and ERK2. Western blotting with an antibodyspecific for phosphorylated ERKs was performed as described inMaterials and Methods. Western blotting with an antibody againsttotal ERKs is shown to document equal loading.
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To test whether PACAP-induced ERK activation was involved in the anti-apoptotic effect of PACAP-38, we measured DNA fragmentationin the presence of PD98059 and Rp-cAMP. Both compounds did notaffect the protection induced by high KCl concentrations, excludingtoxic or nonspecific effect (Fig. 5). Interestingly, both PD98059and Rp-cAMP blocked the effect of PACAP-38 on DNA fragmentation(Fig. 5).
Fig. 5. PACAP-38 decreased DNA fragmentation via a PKA- and MEK-dependent mechanism. Neurons were incubated with 25 µM PD98059 or200 µM Rp-cAMP for 1 hr before the addition of 100 nM PACAP-38or 2 µg/ml actinomycin D. Cells were washed twice with HK mediumand incubated with different drugs and inhibitors for 24 hr. Solubleand nonsoluble DNA were isolated and quantified, as indicatedin Materials and Methods. Data are the mean ± SEM of at leastthree independent experiments. *p < 0.005 with Student's t test,as compared with PACAP-38 alone.
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DISCUSSION
It was reported recently that forskolin, a direct activator of adenylyl cyclase, and cholera toxin (CTX), an activator ofG_s, protected cerebellar granule cells from cell death (D'Melloet al., 1993; Galli et al., 1995; Yan et al., 1995a). However,no physiological activator of the cAMP pathway displaying thesame protective effect was characterized. In the present work,we demonstrated that PACAP-38 was as efficient as forskolin inprotecting cerebellar granule cells from KCl deprivation-inducedapoptosis. Arimura and coworkers reported a neurotrophic biphasiceffect of low PACAP-38 concentrations on gp120-induced apoptosisin hippocampal cultures (Arimura et al., 1994). At concentrationsabove 1 nM, PACAP-38 was not effective in that system. In contrast,the effect of PACAP-38 on cerebellar granule neurons was monophasic,with a maximum at 100 nM. The effect of PACAP-38 on cerebellargranule neurons is, therefore, likely to involve mechanisms differentfrom those recruited in hippocampal cultures.

Using RT-PCR, we demonstrated the presence of PACAP₁-R and PACAP/VIP₁-R mRNAs. In addition, the PACAP₁-R gene is spliced alternativelyand generates different variants with possible insertion of twocassettes named "hip" and "hop" in the third intracellular loopof the receptor (Spengler et al., 1993). RT-PCR experiments revealedthe presence of two variants: (1) PACAP₁-R s (short), which doesnot contain any insert, and (2) PACAP₁-R hop, a variant with oneinsertion. These results are in agreement with recently publishedexperiments by D'Agata and coworkers (1996), who showed a majorPCR product corresponding to the hop variant at postnatal day4 (P4) and P8. Interestingly, at P25 the major PCR product correspondedto the short variant, suggesting a possible role for alternativesplicing of the PACAP₁-R during postnatal development of the cerebellum.We confirmed expression of the PACAP₁-R protein by measuring PACAP-and VIP-stimulated cAMP production. Although expression of PACAP/VIP₁-RmRNA was demonstrated with RT-PCR, pharmacological characterizationindicated that PACAP/VIP₁-R protein was expressed at very lowlevel, because VIP did not stimulate cAMP formation potently.The effect of PACAP-38 on cerebellar granule cells was, therefore,mediated mainly by PACAP₁-R activation. Basille and coworkersdocumented the presence of PACAP receptors on cells of the proliferatingexternal granule cell layer (EGL) at P8 (Basille et al., 1993).At that time, granule cells undergo both maximal proliferationand massive DNA fragmentation, indicating that apoptosis occursin the EGL very soon after neurogenesis, before maximal migrationto the internal granule cell layer (IGL), and synaptogenesis withPurkinje cells occurs ~P10. This indicates that factors otherthan synaptogenesis must regulate the number of granule cellsthat survive (Wood et al., 1993). The present work suggests thatPACAP-38 might be one of these factors.

Most neurotrophic factors concurrently participate in neuronal differentiation and protection from apoptosis. It is, therefore,not surprising that these two processes involve common mechanisms,and studies on neuronal differentiation help to elucidate mechanismsunderlying protection from apoptosis. PACAP-38 was shown to displayneurotrophic properties in several systems, namely PC12 (Deutschand Sun, 1992), sympathetic neurons (Pincus et al., 1990; DiCicco-Bloomand Deutsch, 1992), and chick embryo and hippocampal cultures(Arimura et al., 1994). In PC12 cells, it was demonstrated thatMAP kinase activation is necessary and sufficient for differentiation(Cowley et al., 1994) and that blockade of the MAP kinase pathwayby PD98059, a specific MEK inhibitor (Alessi et al., 1995; Dudleyet al., 1995), prevented differentiation of PC12 cells by NGF(Pang et al., 1995). Interestingly, it also was shown that cAMP-induceddifferentiation was accompanied by activation of the MAP kinasepathway (Frödin et al., 1994; Young et al., 1994) and that PACAP-38stimulates ERK1 activity (Frödin et al., 1994). These resultssuggested a possible mechanism for PACAP-38 action on cerebellargranule cells. Conversely, Edwards et al. (1991) demonstratedthat cAMP protected sympathetic neurons from NGF withdrawal-inducedapoptosis without activating ERK (Virdee and Tolkovsky, 1995).In cerebellar granule cells we demonstrated that PACAP-38 stimulatedERK1 and ERK2 activity and phosphorylation. Interestingly, Rp-cAMPand H89, two inhibitors of PKA, totally blocked ERK stimulationby PACAP-38, indicating that activation of PKA is necessary forPACAP-induced ERK activation (Fig. 4C). In addition, we showedthat blockade of the cAMP pathway with Rp-cAMP or of the MAP kinasepathway with PD98059 abrogated the antiapoptotic effect of PACAP-38.Conclusively, protection of cerebellar granule cells by PACAP-38likely involves the same mechanism as the one suggested in PC12cells for cAMP-induced differentiation, namely activation of PKA,which stimulates MEK activity, resulting in activation of ERK.The precise pathway linking PKA activation to stimulation of MEKactivity remains elusive at present (Frödin et al., 1994; Younget al., 1994).

Interestingly, we also demonstrated that activation of the MAP kinase pathway is not the exclusive way to protect cerebellargranule neurons from KCl deprivation-induced cell death. For instanceIGF-1 or high KCl concentration protected neurons (Fig. 1) butweakly stimulated ERK activity (Fig. 4B) (data not shown). Furthermore,the protective effect of KCl was not affected by PD98059 (Fig.5). This suggests that other pathways, which work independentlyof ERK activation, possibly are involved in protection from apoptosis.Xia and coworkers (1995) recently proposed that NGF withdrawal-inducedapoptosis of PC12 cells requires concurrent activation of thestress kinases [C-Jun N-terminal protein kinase (JNK) and p38]and inhibition of ERK kinases. Hence, either stimulation of ERKactivity or inhibition of the JNK/p38 pathway could result inthe same protection from apoptosis.

In the present work, we investigated the effect of activation of adenylyl cyclase and ERKs by PACAP-38 during cerebellar granulecells apoptosis and demonstrated that it is necessary to the antiapoptoticeffect of PACAP-38. PACAP₁-R also stimulates phospholipase C athigh PACAP-38 concentrations. Further work will be necessary toevaluate the relevance of possible crosstalk between AC and PLCpathways. Finally, generation of a mouse strain deficient forPACAP₁-R gene will be a helpful tool to assess the effect of PACAP-38on cerebellum development in vivo.

FOOTNOTES

Received Aug. 12, 1996; revised Sept. 30, 1996; accepted Oct. 8, 1996.

M.V. was supported by Centre National de la Recherche Scientifique, La Fondation pour la Recherche Médicale (FRM). This workwas supported by Grant ACC-SV4/9504087 from the Ministère del'Education Nationale et de la Recherche, La Ligue pour la Recherchecontre le Cancer, and Boehringer-Ingelheim. We gratefully acknowledgethe help of Dr. Mireille Lafon for cerebellar granule cell cultureand the generous gift of PD98059 by Dr. Alan R. Saltiel (Parke-DavisPharmaceutical Research).

Correspondence should be addressed to Dr. Laurent Journot, Centre National de la Recherche Scientifique, UPR 9023, CCIPE,141 Rue de la Cardonille, F-34094 Montpellier Cedex 05, France.

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Volume 17, Number 1, Issue of January 1, 1997 pp. 83-90 Copyright ©1997 Society for Neuroscience

Pituitary Adenylate Cyclase-Activating Polypeptide (PACAP-38) Protects Cerebellar Granule Neurons from Apoptosis by Activating the Mitogen-Activated Protein Kinase (MAP Kinase) Pathway

Copyright ©1997 Society for Neuroscience 0270-6474/1997/1783-08$05.00/0

Volume 17, Number 1, Issue of January 1, 1997 pp. 83-90
Copyright ©1997 Society for Neuroscience