AMPA Receptor-Mediated, Calcium-Dependent CREB Phosphorylation in a Subpopulation of Auditory Neurons Surviving Activity Deprivation

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The Journal of Neuroscience, August 15, 2000, 20(16):6267-6275

AMPA Receptor-Mediated, Calcium-Dependent CREB Phosphorylation in a Subpopulation of Auditory Neurons Surviving Activity Deprivation
Lance Zirpel, Mary A. Janowiak, Charles A. Veltri, and Thomas N. Parks
Department of Neurobiology and Anatomy, University of Utah School of Medicine, Salt Lake City, Utah 84132-0001

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Although dependence on afferent synaptic activity has been shown for central neurons in every sensory system, the mechanismsof afferent maintenance of target sensory neurons are not understood.Neurons in the cochlear nucleus (CN) require afferent activityfor maintenance and survival. One of the earliest changes seenafter activity deprivation is an increase in intracellular calciumthat leads to the death of 30% of the neuronal population. Sixtyminutes after deafferentation, the surviving neurons show increasedphosphorylation of the transcription factor calcium/cAMP responseelement-binding protein (CREB). CREB phosphorylation in activity-deprivedCN neurons is dependent on increased intracellular calcium resultingfrom influx through AMPA receptors and is mediated by calcium/calmodulin-dependentkinases and protein kinase A. We conclude that in CN neurons,the deafferentation-induced increase in calcium activates at leasttwo kinase pathways that phosphorylate CREB in surviving neurons.We hypothesize that this phosphorylation results in the transcriptionof genes containing the calcium/cAMP response element within theirpromoter regions, and these genes code for proteins that allowthe neurons to compensate for their hypercalcemic, activity-deprivedstate.

Key words: chick nucleus magnocellularis; activity-dependent; deafferentation; calcium homeostasis; propidium iodide; neuronal survival; cell death; mouse AVCN

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Afferent regulation of target tissues is a common feature of the developing nervous system. Experimental manipulations ofafferent activity have been shown to alter structure, function,and neuronal survival of developing sensory systems (Hubel andWiesel, 1965; Dubin et al., 1986; Stryker and Harris, 1986; Brunjes,1994). In the auditory system, elimination of afferent input altersthe metabolism, morphology, and survival of target neurons (forreview, see Rubel, 1978; Moore, 1992; Friauf and Lohmann, 1999;Parks, 1999). Despite the pervasiveness of these cellular interactions,little is known about the intercellular and intracellular signalsresponsible for theseeffects.

Neurons in the cochlear nucleus [nucleus magnocellularis (NM)] of embryonic and early posthatch chicks require afferent inputfrom the eighth cranial nerve for maintenance and survival. Eliminationof this input results in the death of 20-40% of the NM neurons,whereas the surviving neurons display profound changes in morphology,metabolism, and physiology (for review, see Rubel et al., 1990).Neurons in the neonatal mouse anteroventral cochlear nucleus (AVCN,the mammalian homolog of the avian NM) also show dependence onafferent activity from the eighth nerve (Trune, 1982) (Mostafapouret al., 2000). One of the earliest changes seen in NM after deafferentationis an increase in intracellular calcium concentration ([Ca²⁺]_i) (Zirpel et al., 1995b). This increase in [Ca²⁺]_i can be prevented by activation of metabotropic glutamate receptors(mGluRs) (Zirpel and Rubel, 1996) linked to protein kinase A (PKA)and protein kinase C (PKC) signal transduction pathways (Lachicaet al., 1995; Zirpel et al., 1995a, 1998). Blockade of mGluRsduring eighth nerve activity results in a rapid and large increasein [Ca²⁺]_i (Zirpel and Rubel, 1996) caused, in part, by continued activationof highly Ca²⁺-permeable AMPA receptors (Otis et al., 1995; Ravindranathan etal., 2000). Although this deafferentation-induced increase in[Ca²⁺]_i and the mechanisms preventing it are well characterized, thesource of the Ca²⁺ and its effects on NM neurons areunknown.

Activation of the transcription factor calcium/cAMP response element-binding protein (CREB) is dependent on phosphorylationby PKA, Ca²⁺/calmodulin-dependent kinases (CaMKs), or ribosomal S6 kinases(RSKs) (Walton and Dragunow, 2000). One of the most well characterizedsignals for CREB phosphorylation and activation is an increasein [Ca²⁺]_i (Sheng et al., 1990; Deisseroth et al., 1996; Hardingham etal., 1997; S. C. Hu et al., 1999; Rajadhyaksha et al., 1999).CREB phosphorylation and activation have been shown to be importantfor the survival of neurons in a number of different conditions,including hypercalcemia (Walton et al., 1999; Walton and Dragunow,2000). Thus CREB phosphorylation is a likely candidate for oneof the mechanisms underlying the changes seen in cochlear nucleusneurons after deafferentation. We hypothesize that the [Ca²⁺]_i increase in NM neurons after deafferentation activates kinasepathways that phosphorylate CREB, resulting in the transcriptionof genes that enable the neurons to survive the deafferentation-inducedhypercalcemicstate.

Using an antibody that recognizes specifically the phosphorylated form of CREB (Ginty et al., 1993), we examined CREB phosphorylationin cochlear nucleus neurons receiving or after termination ofsynaptic activation via eighth nerve activity. We find that aftercessation of afferent activity, cochlear nucleus neurons showa transient phosphorylation (peaking at 50 min) of CREB in a percentageof neurons equal to the percentage of surviving neurons. Usingdynamic calcium imaging, we show that treatments that block AMPAreceptor activation, or prevent increases in [Ca²⁺]_i, also block the phosphorylation of CREB. CREB phosphorylationis attenuated, but not completely blocked, by inhibition of staurosporine-sensitivekinases (e.g., PKA, PKC, and RSKs), CaMKs (with KN-62), or PKA[with Rp-adenosine 3',5'-cyclic monophosphothioate triethylamine(Rp-cAMPS)], but not by inhibition of mitogen-activated proteinkinase kinase (MAPKK; with PD98059). Inhibition of both staurosporine-sensitiveand CaM kinases eliminates CREB phosphorylation. Constitutiveactivation of PKA (with Sp-cAMPS) increases the number of neuronsshowing CREB phosphorylation. The number of neurons showing CREBphosphorylation is negatively correlated with the number of deador dying neurons. These results suggest that after deafferentation,AMPA receptors are activated by ambient glutamate, causing anincrease in [Ca²⁺]_i that activates more than one calcium-dependent kinase pathway.These kinases then phosphorylate CREB in a subpopulation of neurons,consistent with the hypothesis that CREB-mediated transcriptionallows these neurons to survive in their activity-deprived, hypercalcemicenvironment.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cochlea removals
White Leghorn chicks, 4-7 d posthatch (P4-P7), were anesthetized with halothane. Right cochleae were removed as describedby Born and Rubel (1985). The auricle was removed, and the tympanicmembrane was perforated with fine forceps. The columella was extracted,and forceps were inserted through the oval window. The basilarpapilla was removed and visually examined to ensure complete deafferentation.If the basilar papilla was not 75% intact, or if the lagena wasnot visible, the surgery was deemed a failure, and the animalwas not used for experimentation. After a successful cochlea ablation,the middle ear was packed with Gelfoam. The chick was allowedto survive the appropriate amount of time, anesthetized with ketamineand pentobarbital, and perfused transcardially with 0.9% salinecontaining 1000 IU heparin and 2 mg/ml NaNO₂ followed by 4% paraformaldehydein 0.1 M phosphate buffer, pH 7.2. The brainstem was dissectedfree and placed in 4% paraformaldehyde for 3 hr and then storedin 30% sucrose in 0.1 M phosphate buffer at 4°C overnight. Tissuewas then embedded and frozen in optimal cutting temperature (OCT)compound (VWR Scientific, Salt Lake City, UT). By the use of acryostat, 18-µm-thick coronal sections were cut through the brainstemat the level of the auditory nuclei and placed on microscope slides.Care was taken to acquire sections that were symmetric, thus providinga within-animal control (deafferented vs intact cochlearnuclei).
Mouse pups aged 5 d (P5) were anesthetized with halothane. Right cochleae were removed as described by Mostafapour et al.(2000). The oval window was exposed by dissecting away the pinnaand aspirating the soft tissue filling the middle ear at thisage. The tip of a flame-polished Pasteur pipette was then insertedthrough the oval window, and the cochlea was aspirated with gentlesuction. The middle ear was packed with Gelfoam, and the incisionwas closed with cyanoacrylate adhesive. The pup was allowed tosurvive for 60 min, anesthetized with cooling, and decapitated.The entire cranium was immersed in 4% paraformaldehyde overnight.The brain was dissected free from the cranium, placed in 4% paraformaldehydefor 1 hr, rinsed with PBS (137 mM NaCl, 2.7 mM KCl, 5 mM Na₂HPO₄,and 1.7 mM KH₂PO_4, pH 7.4), rinsed with distilled water, and placedin 70% ethanol overnight. Brains were then dehydrated and embeddedin paraffin. Ten micrometer sections containing the cochlear nucleibilaterally were obtained using a microtome and mounted on microscopeslides. Sections on slides were deparaffinized andrehydrated.

Phospho-CREB immunohistochemistry
Chick tissue. Tissue sections were blocked for 20 min with 1% normal goat serum and 0.4% saponin in PBS. Sections were thenincubated overnight at 4°C with anti-phospho-CREB (rabbit polyclonal;1:1000; Upstate Biotechnology, Lake Placid, NY) or anti-CREB (rabbitpolyclonal; 1:1000; Upstate Biotechnology) diluted in blockingbuffer, pH 7.3-7.4. Primary antibody incubation was continuedfor an additional 1-3 hr at room temperature, followed by three10 min washes in PBS. Alexa 594 secondary antibody (1:800 in 0.4%normal goat serum in PBS; Molecular Probes, Eugene, OR) was appliedfor 90 min at room temperature, followed by three 10 min washeswith PBS. Slides were coverslipped with Fluorsave (Calbiochem,La Jolla, CA) and stored in the dark at 4°C until analyzed. Controlsfor each run were processed identically except instead of a primaryantibody incubation, they were incubated in blockingsolution.
Mouse tissue. Antigen retrieval was performed on the sections of mouse tissue. Slides were placed in a Coplin jar containing10 mM citric acid solution, pH 6, and microwaved on high poweruntil the solution boiled. Evaporated fluid was replaced withdistilled H₂O, and the boiling procedure was repeated two moretimes. After the final boiling, slides were allowed to cool andrinsed in distilled H₂O. Immunohistochemistry was performed identicallyas described above for the chick tissue. No primary controls wereincluded in eachrun.
Image acquisition. By the use of confocal laser-scanning microscopy (Bio-Rad, Hercules, CA), labeled sections were "opticallysectioned." The optical section corresponding to the 50th percentileof the entire section thickness was chosen for analysis. Becausequantitative fluorescence analysis was not performed, acquisitionwas optimized for image quality. Images were acquired via a Fluor40× oil immersion objective (1.3 numerical aperture; Nikon). Imageresolution was set at 1024 × 1024 pixels, and all acquisitionswere Kalman filtered (factor of four). Images were converted toTIFF format using NIH Image (public domain software developedat the United States National Institutes of Health and availableon the internet at http://rsb.info.nih.gov/nih-image).
Data analysis. Cells were counted as either positive or negative on the basis of a clearly identifiable nucleus, labeled ornot labeled, respectively. Cells with ambiguous labeling or anunidentifiable nucleus were excluded from analysis. For each image,all positive- and negative-labeled cells were counted, and thepositive-labeled cells were expressed as the percentage of totalcells. Neurons and glia were counted separately. Multiple sectionswere counted for each animal, averaged, and treated as n = 1.Images were prepared for presentation using Photoshop (Adobe Systems,San Jose, CA). ANOVA and two-tailed t tests were performed usingStatview (SAS Institute, Cary,NC).

In vitro experiments
Slice preparation. Live in vitro tissue slices (300 µm) were acquired as described previously (Zirpel et al., 1995a,b, 1998;Zirpel and Rubel, 1996) and maintained in oxygenated artificialCSF (ACSF; 130 mM NaCl, 3 mM KCl, 2 mM CaCl₂, 2 mM MgCl₂, 26 mMNaHCO₃, 1.25 mM NaH₂PO₄, and 10 mM D-glucose, pH 7.4). For pharmacologyexperiments, a drug was added to ACSF and was present throughoutthe dissection and slicing procedure. At the end of each experiment,slices were immersed in 4% paraformaldehyde for 1 hr, cryoprotected,rinsed, embedded in OCT, and sectioned for immunohistochemistryas describedabove.
Electrophysiology. Methods for stimulating and recording from in vitro chick brainstem slices have been described previously(Jackson et al., 1985; Hyson and Rubel, 1989; Zirpel and Rubel,1996; Zirpel et al., 1998). A concentric bipolar-stimulating electrode(FHC, Bowdoinham, ME) was placed on the eighth nerve dorsal andlateral to NM. Stimulation pulses (50-100 µsec duration; 60-80V) were delivered at a rate of 0.1-1.0 Hz. Responses were recordedwith an ACSF-filled microelectrode (~1 M $Omega$ ) attached to an intracellularamplifier and monitored on anoscilloscope.
Calcium imaging. Tissue slices were incubated in oxygenated ACSF containing 8 µM fura-2 AM, 1.7% anhydrous dimethylsulfoxide,and 0.03% pluronic for 30 min at room temperature. Slices wereplaced in the imaging chamber and bathed in normal, oxygenatedACSF for ~5 min before data acquisition. The ratiometric fluorescence-imagingtechniques used in this study were similar to those describedpreviously (Zirpel et al., 1995a,b, 1998, 2000; Zirpel and Rubel,1996). Paired 350/380 excitation images were acquired approximatelyevery 3-5 sec or at 1 min intervals, and ratios were determinedon a pixel-by-pixel basis. Intracellular calcium concentrationwas estimated according to the method of Grynkiewicz et al. (1985)using NIH Image. Five-point external calibrations were performedon the imaging system routinely, and the Kd for fura was calculatedwith each calibration. The range of Kd values was 75-172 nM. Upto 10 neurons were analyzed for any given experiment. However,each slice was considered n = 1, and the data from all neuronsin an experiment were averaged. Cells were not included in theanalysis if the baseline [Ca²⁺]_i was >250 nM, because this concentration is indicative of adying cell (Zirpel et al., 1998). Cells were neither added tonor subtracted from the analysis of an experiment except whena complete loss of fluorescence was observed, indicating celldeath (Johnson et al., 1994).
Values of [Ca²⁺]_i were plotted as a function of time using EXCEL (Microsoft, Redmond, WA) and Cricket Graph (Cricket Software,Malvern, PA). Data are presented as the means ± 1 SEM unless otherwiseindicated.
Propidium iodide labeling. For selected experiments, 1.5 µM propidium iodide (PI) was added to the superfusate at the 30 mintime point. Thirty minutes later, an image was captured, in situ,through a 600 nm long-pass filter using 510 nm excitation. PI-labeledneurons were counted and expressed as a percentage of the sumof PI-labeled and fura-2-labeledneurons.

Western immunoblots
Westerns were performed as described previously (Zirpel et al., 2000). Brainstem areas containing the nucleus magnocellularisfrom P2 to P7 chicks were dissected out in ACSF or in ACSF containinga selected drug at room temperature for a 60 min total deafferentationtime. Nuclei magnocellularis were then dissected from the brainstemand homogenized in lysis buffer [50 mM Tris, pH 7.4, 1 mM EDTA,1% Triton X-100, and protease inhibitors (7 µg/ml chymostatin,7 µg/ml leupeptin, 7 µg/ml antipain, 7 µg/ml pepstatin, 5 µg/mlaprotinin, and 350 µg/ml PMSF)]. One brainstem was dissected inACSF and homogenized immediately in lysis buffer. The sampleswere sonicated (3-5 sec) and centrifuged at 14000 rpm for 40 minat 4°C. The protein concentration of the samples was determinedusing a BCA assay (Bio-Rad). Twenty-five and fifty microgramsof protein were resolved via 10% SDS-PAGE (100 V for 2.5 hr atroom temperature) for blots to be probed with anti-CREB and anti-phospho-CREB,respectively. Gels were transferred onto Immobilon-P membranes(Millipore, Bedford, MA) at 30 V overnight at 4°C. Blots wereprobed with anti-CREB or anti-phospho-CREB polyclonal antibodiesdiluted 1:1000. Blots were rinsed in buffer B (0.5 M NaCl, 0.02M Tris base, and 0.1% Tween 20, pH 7.5) and incubated with donkeyanti-rabbit Ig, horseradish peroxidase-linked whole antibody (Amersham),diluted 1:5000 at room temperature for 1.5 hr. Blots were rinsedin buffer B followed by buffer A (0.5 M NaCl and 0.02 M Tris base,pH 7.5). Bound secondary antibodies were developed by enhancedchemiluminescence using ECL Western Blotting Detection Reagents(Pharmacia, Piscataway, NJ). Blots were scanned into a computer,and the relative levels of CREB or phosphorylated-CREB (p-CREB)were determined by densitometry using NIH Image. To insure consistentmeasurements, a box of defined size was used to measure the opticaldensity of each band in a given lane at the same position in they dimension on eachblot.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activity deprivation results in CREB phosphorylation

To determine the state of CREB phosphorylation in neurons receiving, and neurons deprived of, normal synaptic activity, weexamined p-CREB labeling in the cochlear nuclei of chicks thathad undergone unilateral cochlea ablation. Removal of the cochleaeliminates all excitatory input to the ipsilateral cochlear nucleuswhile leaving intact the normal afferent activity in the contralateralcochlear nucleus. Figure 1A shows an example of p-CREB labelingin NM 60 min after cochlea removal. Glial nuclei (arrowheads)are easily distinguished from neuronal nuclei, and it is readilyapparent that the labeling is localized to the nuclei of bothglia and neurons. Cells were counted as either labeled or not;no attempt was made to quantify varying degrees of p-CREB labeling.p-CREB labeling was never seen in glia or neurons contralateralto deafferentation (i.e., on the side receiving normal eighthnerve input; Fig. 1B). p-CREB labeling was first seen 30 min aftercochlea ablation when 72 ± 12% of the glia labeled positive forp-CREB (Fig. 1C, $open circle$ ). The percentage of p-CREB-labeled (p-CREB+)glia remained elevated at 50 min (70 ± 11%), fell to 20 ± 8% at70 min, and was absent at 90 min. Neuronal p-CREB labeling wasfirst observed 50 min after cochlea ablation when 74 ± 14% ofthe neurons were p-CREB+ (Fig. 1C, $black-square$ ). The percentage of p-CREB+neurons remained high at 60 min (70 ± 10%), fell to 43 ± 8% at70 min, and was absent by 90 min. To facilitate pharmacologicalmanipulation, activity deprivation-induced CREB phosphorylationwas also demonstrated using in vitro slice preparations. The eighthnerve was unilaterally stimulated (field potentials were recordedto ensure synaptic activation; data not shown) for defined periodsof time after which the slices were processed for anti-p-CREBimmunohistochemistry. As with the in vivo cochlea removal, thisallows for a within-slice control in which one NM receives normalinput from the ipsilateral eighth nerve and the contralateralNM is activity deprived. The timing and pattern of CREB phosphorylationin neurons from in vitro slices mirrored that seen with in vivocochlea removal; p-CREB+ neurons were first seen at 50 min andwere absent at 90 min (Fig. 1C, $triangle$ ). The percentage of p-CREB+neurons observed in the in vitro slice preparations was slightlylower than that seen with cochlea ablation (53 ± 11% vs 74 ± 14%at 50 min and 52 ± 12% vs 70 ± 10% at 60 min) perhaps because,in part, of damage caused by the dissection and slicing procedure.p-CREB labeling was never observed in glia or neurons in the NMipsilateral to nerve stimulation. The remainder of the experimentsin this report were conducted using in vitro slice preparations,and thus, control or no stimulation refers to the 60 min in vitropercentage of p-CREB+ neurons shown in Figure 1C. All chick cochlearnucleus neurons show diffuse nuclear and cytoplasmic labelingfor CREB (data not shown).

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Figure 1. CREB phosphorylation after deafferentation in a subset of neurons. A, Chick cochlear nucleus immunostained for p-CREB 60 min after an in vivo, unilateral cochlea removal. Note that both neuronal and glial (arrowheads) nuclei show staining. B, Chick cochlear nucleus contralateral to cochlea removal (i.e., intact) immunostained for p-CREB. C, Percentage of p-CREB+ cells in chick cochlear nucleus neurons and glia as a function of time after an in vivo cochlea ablation and in vitro slice preparations. Error bars represent the SEM. For in vivo cochlea ablation, n = a minimum of 3 animals per data point. For in vitro data, n = a minimum of 5 slices per data point. D, Mouse (P5) AVCN immunostained for p-CREB 60 min after unilateral cochlea ablation. a, AVCN ipsilateral to cochlea ablation. b, AVCN contralateral to cochlea ablation (i.e., intact). Scale bar: A, B, D, 30 µm.

To determine whether CREB phosphorylation occurred in mice as well as chicks after deafferentation, four mouse pups underwentunilateral cochlea ablation. Sixty minutes after cochlea ablation,a subpopulation of AVCN neurons showed p-CREB labeling (Fig. 1Da).No p-CREB+ cells were observed in the AVCN contralateral to cochlearemoval (Fig. 1Db). The percentage of p-CREB+ AVCN neurons ipsilateralto cochlea ablation (53 ± 13%) is similar to the mean number ofAVCN neurons reported by Trune (1982) (66%) and by Mostafapouret al. (2000) (40%) to survive cochlea ablation. Similarly, thepercentage of chick NM neurons that show CREB phosphorylation60 min after cochlea ablation (70 ± 10%) is equivalent to thepercentage of neurons that survive deafferentation (70%) (Bornand Rubel, 1985). All mouse cochlear nucleus neurons show diffusenuclear and cytoplasmic labeling for CREB (data notshown).

Activity deprivation-induced CREB phosphorylation is calcium dependent

After cessation of eighth nerve input, NM neurons show a gradual [Ca²⁺]_i increase from a resting level of 100 ± 13 nM to 242 ± 18 nMat 90 min (Fig. 2Aa, $black-square$ ) (see also Zirpel and Rubel, 1996). Adding5 µM ionomycin, a Ca²⁺ ionophore, to the superfusate of in vitro slices containing NMcauses the [Ca²⁺]_i increase to occur sooner (Fig. 2Aa, $open circle$ ) but does not alter thelevel reached (267 ± 25 nM) at 90 min. In parallel with this morerapid ionomycin-induced [Ca²⁺]_i increase is a temporal phase advance of peak p-CREB labelingin NM neurons (Fig. 2Ab). Thirty minutes after deafferentation55 ± 12% of the ionomycin-treated neurons are p-CREB+ (comparedwith 0% of the control neurons in normal ACSF), and at 60 minthis percentage has dropped to 11 ± 12% versus 52 ± 12% of thecontrol neurons. These results suggest that CREB phosphorylationis mediated by increased [Ca²⁺]_i.

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Figure 2. Deafferentation-induced CREB phosphorylation is Ca²⁺ dependent. A, Effects of ionomycin on [Ca²⁺]_i and CREB phosphorylation. a, Fura-2-measured mean [Ca²⁺]_i increase in chick NM neurons in the absence of activity in normal ACSF ( $black-square$ ; 38 neurons; n = 4 slices) and in ACSF containing 5 µM ionomycin ( $open circle$ ; 47 neurons; n = 5 slices). Error bars represent the SEM and are <20 nM where not visible. b, Percentage of p-CREB+ NM neurons in the presence ( $black-diamond$ ) and absence ( $triangle$ ) of 5 µM ionomycin as a function of time in the absence of activity in vitro. Error bars represent the SEM (n = 4 for the 30 min ionomycin data point, 5 for the 60 min data point, and 3 for all others). The No Stimulation data are the same as those presented in Figure 1C. B, Effects of [Ca²⁺]_i on CREB phosphorylation. a, Fura-2-measured mean [Ca²⁺]_i of NM neurons in the absence of activity in normal ACSF ( $black-square$ ; 38 neurons; n = 4 slices; same data shown in Aa), in ACSF containing 1 mM ACPD ( $triangle$ ; 39 neurons; n = 4 slices), in ACSF containing 1 µM nifedipine ( $open circle$ ; 37 neurons; n = 4 slices), and in normal ACSF after incubation in 5 µM BAPTA AM (Kd = 160 nM; $diamond$ ; 29 neurons; n = 3 slices). Error bars represent the SEM and are <20 nM where not visible. b, Percentage of p-CREB+ NM neurons after 60 min in the four conditions shown in Ba. Error bars represent the SEM. Control, n = 19; BAPTA, n = 3; ACPD, n = 3; and nifedipine, n = 3. *, p < 0.05

If increased calcium is indeed the signal for CREB phosphorylation, preventing the [Ca²⁺]_i increase should prevent CREB phosphorylation. Adding 5 µM BAPTAAM, a Ca²⁺ chelator, to the fura-2 loading solution not only prevents thedeafferentation-induced increase in [Ca²⁺]_i (Fig. 2Ba, $diamond$ ) but also causes a lower resting [Ca²⁺]_i in NM neurons (63 ± 25% vs 100 ± 13%). Sixty minutes afterdeafferentation, only 4.8 ± 4.8% of the BAPTA-treated NM neuronsshow p-CREB labeling (Fig. 2Bb). A one-factor ANOVA revealed avery highly significant effect of experimental treatment on thepercentage of p-CREB+ neurons [F_(13,65) = 12.64; p < 0.0001].Post hoc comparisons with Scheffe's method showed several significantdifferences between groups, including a lower percentage of p-CREB+neurons in the BAPTA treatment group than in controls (p = 0.03).

Reducing [Ca²⁺]_i by a second, independent mechanism shows a similar effect on CREB phosphorylation. 1-Amino-1,3-cyclopentanedicarboxylicacid (ACPD) prevents the increase in [Ca²⁺]_i in NM neurons after deafferentation by activating metabotropicglutamate receptors, which play a pivotal role in NM neuron [Ca²⁺]_i homeostasis (Zirpel and Rubel, 1996; Zirpel et al., 1998).ACPD (1 mM) added to the superfusate of slices prevented the [Ca²⁺]_i increase (Fig. 2Ba, $triangle$ ) and reduced the percentage of p-CREB+neurons at 60 min to 6.2 ± 2.9% (Fig. 2Bb; p = 0.04).

The L-type voltage-gated calcium channel antagonist nifedipine (1 µM) had no effect on the increase in [Ca²⁺]_i in the absence of activity (Fig. 2Ba, $open circle$ ) or on the percentageof p-CREB+ NM neurons (44 ± 4%; p = 0.043) 60 min after activitydeprivation (Fig. 2Bb).

Altering the temporal characteristics of the [Ca²⁺]_i increase in NM neurons after deafferentation also alters the temporal characteristicsof p-CREB labeling. Furthermore, preventing the [Ca²⁺]_i increase via two different mechanisms virtually eliminatesp-CREB labeling. Therefore, we conclude that the phosphorylationof CREB in NM neurons after deafferentation is a calcium-dependentprocess.

AMPA receptors mediate the increase in [Ca²⁺]_i and CREB phosphorylation

AMPA receptors expressed by NM neurons show extremely rapid kinetics (Raman and Trussell, 1992; Raman et al., 1994) that allowsthese neurons to encode faithfully temporal aspects of acousticstimuli (Trussell, 1999). The AMPA receptor subunit compositionthat allows rapid kinetics also imparts Ca²⁺ permeability to the receptor complex (Geiger et al., 1995). ThusNM neurons express AMPA receptors that are highly permeable toCa²⁺ (Otis et al., 1995; Ravindranathan et al., 2000).

Residual neurotransmitter in the synaptic cleft in the absence of activity is a well established phenomenon (Barbour et al.,1994; Timmerman and Westerink, 1997), and whole-cell patch-clampedNM neurons in an in vitro slice show miniature EPSCs in the absenceof eighth nerve stimulation (L. Zirpel, unpublished observations).It is therefore plausible that after an in ovo cochlea removaland in vitro, there is spontaneous leak of glutamate from theeighth nerve terminals that activates AMPA receptors enough tocause the gradual increase in [Ca²⁺]_i seen in NMneurons.

To test this hypothesis of AMPA receptor-mediated Ca²⁺ influx, 30 µM CNQX, a AMPA/kainate receptor antagonist, or 50 µM GYKI52466, a more specific AMPA receptor antagonist (Donevan and Rogawski,1993), was added to the superfusate of slices while [Ca²⁺]_i was monitored. Figure 3A shows that both CNQX ( $triangle$ ) and GYKI52466 () prevented the [Ca²⁺]_i increase in NM neurons in the absence of activity. Cyclothiazide(CTZ) is a benzothiadiazide that inhibits the rapid desensitizationof AMPA receptors (Partin et al., 1993; Wong and Mayer, 1993).Addition of 100 µM CTZ to the superfusate of slices had no effecton the [Ca²⁺]_i increase in NM neurons (Fig. 3A, $diamond$ ). NMDA receptors have beenshown to contribute little to synaptic transmission (Zhang andTrussell, 1994) or calcium regulation (Zirpel et al., 1995a) inNM neurons in late embryonic or early posthatch chicks. In agreementwith this idea, application of the NMDA receptor antagonist (±)-2-amino-5-phosphonopentanoicacid (APV; 200 µM) had no effect on the increase in [Ca²⁺]_i in the absence of activity (data not shown).

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Figure 3. The [Ca²⁺]_i increase and CREB phosphorylation depend on AMPA receptor activation. A, Fura-2-measured mean [Ca²⁺]_i of NM neurons in the absence of activity in normal ACSF ( $black-square$ ; 38 neurons; n = 4 slices; same data shown in Fig. 2Aa) and in ACSF containing 30 µM CNQX ( $triangle$ ; 37 neurons; n = 5 slices), 50 µM GYKI 52466 (GYKI; ; 33 neurons; n = 4 slices), or 100 µM CTZ ( $diamond$ ; 37 neurons; n = 5 slices) is shown. Error bars represent the SEM. B, AMPA receptor blockade inhibits CREB phosphorylation. The percentage of p-CREB+ NM neurons 60 min after deafferentation in the conditions described in A and after incubation in ACSF containing 200 µM APV is shown. Error bars represent the SEM. CNQX, n = 13; GYKI 52466, n = 4; CTZ, n = 4; APV, n = 3. *, p < 0.05. No stim, No stimulation.

CNQX and GYKI 52466 both significantly reduced the number of p-CREB+ NM neurons 60 min after deafferentation (Fig. 3B; p <0.0001 and p = 0.012, respectively). CTZ showed a trend of increasingthe number of p-CREB+ NM neurons (Fig. 3B), but this effect wasnot statistically significant (p = 0.16). APV had no effect onthe percentage of p-CREB+ NM neurons (Fig. 3B; p = 0.71). Theresults of these experiments indicate that the deafferentation-induced[Ca²⁺]_i increase in NM neurons and the underlying CREB phosphorylationrequire activation of AMPAreceptors.

To confirm the specificity of the antibodies on chick tissue, Western immunoblots were performed using antibodies againstCREB and phospho-CREB. Figure 4A shows that the anti-CREB antibodyrecognizes an appropriately sized protein (43 kDa) in both ratcerebellum (positive control) and chick tissue. Chick tissue consistedof isolated NM from the following three conditions: normal stimulation(no p-CREB via immunohistochemistry), no stimulation for 60 min(high p-CREB levels via immunohistochemistry), and no stimulationin the presence of 30 µM CNQX for 60 min (very low p-CREB levelsvia immunohistochemistry). This antibody recognizes a 30 kDa protein,which may be a CRE-modulating protein, as well as CREB in differentstates of phosphorylation (Ginty et al., 1993). Thus, only thelower of the three bands near 43 kDa was quantified using NIHImage. The results of the CREB Western show that there are nosignificant differences in CREB levels among the chick groups.It can also be seen that CNQX treatment decreases the intensityof the upper bands that represent phosphorylated-CREB. For thep-CREB Western the stimulation, no stimulation, and CNQX groupswere identical to those used for the CREB Western. NM tissue treatedwith BAPTA for 60 min in the absence of activity was also included.Consistent with our immunohistochemistry results, the p-CREB Westernshows significant bands at the appropriate size for the no stimulationor control tissue, and p-CREB levels are attenuated by BAPTA andCNQX treatment. The p-CREB antibody also recognizes a 38 kDa proteinthat may be phosphorylated activating transcription factor-1 (Gintyet al., 1993).

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Figure 4. Western immunoblots confirm immunohistochemistry. A, Immunoblot analysis of CREB levels using 25 µg of protein from isolated NM receiving normal stimulation (Stim), in ACSF for 60 min with no stimulation (No stim), and in ACSF containing 30 µM CNQX for 60 min (CNQX). Rat cerebellum (Rat cb.; 25 µg) was used as a positive control. B, Immunoblot analysis of phosphorylated-CREB levels using 50 µg of isolated NM tissue from the identical stimulation, no stimulation, and CNQX groups described for the CREB Western immunoblot in A. NM tissue in ACSF containing BAPTA AM for 60 min (BAPTA) was also included. Rat cerebellum (25 µg) was included as a positive control.

Inhibition of CaM kinases and staurosporine-sensitive kinases prevents CREB phosphorylation

CREB can be phosphorylated by a number of kinases, including PKA, PKC, CaM kinases, and RSKs (Walton and Dragunow, 2000).To determine whether these particular kinases were involved inCREB phosphorylation in NM neurons after deafferentation, we pharmacologicallyinhibited kinases in slices and assayed for CREB phosphorylationafter 60 min of deafferentation. At micromolar concentrations,staurosporine is a nonspecific kinase inhibitor (Shapiro et al.,1996) that inhibits, among others, PKA, PKC, and RSKs but notCaM kinases (Hidaka and Kobayashi, 1992). Application of 1 µMstaurosporine to slices for 60 min of deafferentation reducedthe percentage of p-CREB+ NM neurons by 51% (Fig. 5; from 52 ±6% of total neurons to 25 ± 2%). Similarly, inhibition of CaMkinases with 1 µM KN-62 resulted in a 65% reduction in the percentageof p-CREB+ NM neurons (Fig. 5; from 52 to 18 ± 3%). Inhibitionof PKA with 100 µM Rp-cAMPS reduced the number of p-CREB+ neuronsby 61% (Fig. 5; from 52 to 20%; p = 0.0007). The combination of1 µM staurosporine and 1 µM KN-62 eliminated p-CREB labeling inNM neurons (Fig. 5; 8 ± 3%). This value is significantly differentfrom the control (p = 0.036) but not from 0 (one-sample t test,t = 1.76; p = 0.22). MAPKK inhibition eliminates downstream activationof RSKs and thus CREB phosphorylation (Impey et al., 1998a). Applicationof the MAPKK inhibitor PD98059 (Alessi et al., 1995) at 1, 10,or 50 µM (n = 3 for each concentration) had no effect on the numberof p-CREB+ NM neurons after 60 min of activity deprivation (Fig.5; p = 0.1339 on nine slices from all three concentrations). Activationof PKA (with 100 µM Sp-cAMPS) in the absence of activity attenuatesthe increase in [Ca²⁺]_i (Zirpel et al., 1998) but increases the percentage of p-CREB+NM neurons (Fig. 5; p = 0.0466). None of the kinase inhibitorsused had any effect on the increase in [Ca²⁺]_i (data not shown) (but see Zirpel et al., 1998).

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Figure 5. Kinase activity affects CREB phosphorylation. Percentage of p-CREB+ NM neurons after 60 min of deafferentation in normal ACSF (n = 19; same control data shown in Figs. 2Bb, 3B) and in ACSF containing 1 µM staurosporine (n = 5), 1 µM KN-62 (n = 3), the combination of 1 µM KN-62 and 1 µM staurosporine (KN-62 + Stauro; n = 3), 100 µM Rp-cAMPS (n = 4), PD98059 (n = 9; pooled data from 1, 10, and 50 µM; see Results), and 100 µM Sp-cAMPS (n = 3). *, p < 0.05.

Preliminary experiments (n = 3 for each treatment; data not shown) further support the involvement of PKA in the deafferentation-inducedCREB phosphorylation. Stimulating PKA directly with 1 mM 8-bromo-cAMPor indirectly with the adenylate cyclase activator forskolin (50µM) for 30 min [when CREB phosphorylation is not normally observed(Fig. 1C)] results in p-CREB+ labeling in 30-50% of the NM neurons.Conversely, stimulating PKC with phorbol 12-myristate 13-acetate(PMA; 100 nM) or application of the inactive dideoxyforskolin(50 µM) or 4 $alpha$ -PMA did not result in any p-CREB+ NM neurons 30min after activitydeprivation.

Thus, at least two different kinases, a minimum of one CaM kinase and PKA but not PKC or MAPKK/RSK, converge to phosphorylateCREB in response to the AMPA receptor-mediated, deafferentation-inducedincrease in [Ca²⁺]_i.

p-CREB labeling is correlated with neuronal survival

To determine whether p-CREB labeling occurs in a random subpopulation of NM neurons or in the subpopulation of NM neuronsthat survive deafferentation, slices in various treatment groupswere labeled with PI 30 min before fixation for p-CREB immunohistochemistryas described by Zirpel et al. (1998). PI is a fluorescent dyethat binds to DNA and, when used in live tissue, functions asan exclusion dye that labels dead or dying cells (Jiang et al.,1993; Wilde et al., 1994; Behl et al., 1995; Kuroda et al., 1995).However PI is not fixable when used in live tissue, and this precludesdouble-label experiments with immunohistochemistry. Figure 6 showsthat treatments that prevent CREB phosphorylation in activity-deprivedNM neurons without preventing the [Ca²⁺]_i increase result in a higher number of PI-labeled neurons. However,activation of PKA with Sp-cAMPS attenuates the increase in [Ca²⁺]_i (Zirpel et al., 1998), increases the number of p-CREB+ NM neurons(Fig. 5), and decreases the number of PI-labeled neurons (Fig.6, top, bottom). There is a strong and significant negative correlationbetween the proportions of PI+ and p-CREB+ NM neurons across thefive experimental treatments (r² = 0.943; p < 0.01). These results indicate that CREB phosphorylationoccurs in the NM neurons that will survive the deafferentation-inducedhypercalcemia.

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Figure 6. CREB phosphorylation is inversely correlated with propidium iodide labeling. Top, PI labeling in NM after 60 min of activity deprivation in the presence of the PKA activator Sp-cAMPS. Middle, PI labeling after 60 min of activity deprivation in the presence of the nonspecific kinase inhibitor staurosporine. NM neurons show clearly labeled nuclei and diffusely labeled cytoplasm. Smaller, punctate labeling is glial nuclei. Scale bar: A, B, 30 µm. Bottom, Percentage of p-CREB+ NM neurons as a function of the percentage of propidium iodide-labeled neurons after 60 min of deafferentation in (from left to right on x-axis) ACSF containing 100 µM Sp-cAMPS, normal ACSF, and ACSF containing 1 µM staurosporine, 1 µM KN-62, or the combination of 1 µM staurosporine and 1 µM KN-62. Error bars represent the SEM (n = 6 for all PI-labeling points and 19 for control p-CREB, 5 for staurosporine p-CREB, and 3 for the KN-62, staurosporine + KN-62, and Sp-cAMPS p-CREB groups).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Afferent regulation of target neurons is a well established phenomenon in the developing nervous system. Although this hasbeen demonstrated in all sensory systems, little is known aboutthe mechanisms underlying this regulation or the converse of neuronaldegeneration, or survival, in the absence of afferent activity.In this study we have shown that a subpopulation of auditory neuronsthat survive deafferentation shows CREB phosphorylation in responseto the AMPA receptor-mediated increase in [Ca²⁺]_i. This CREB phosphorylation is the result of the activity ofat least two Ca²⁺-dependent kinase pathways. This study suggests that in conditionsof activity deprivation, neurons are able to implement activemechanisms that allow them to cope with and survive in their newenvironment.

This study and others have shown that CREB phosphorylation is Ca²⁺ dependent (Sheng et al., 1990; Deisseroth et al., 1996; Hardinghamet al., 1997; S. C. Hu et al., 1999). Whereas other studies havedemonstrated CREB phosphorylation in response to increased levelsof synaptic activity (Deisseroth et al., 1996; Impey et al., 1998b;Lin et al., 1998; Sgambato et al., 1998; Moon et al., 1999; Sakaguchiet al., 1999), we show here an increase in CREB phosphorylationin response to activity deprivation. However, even in the absenceof eighth nerve synaptic activity, AMPA receptor activity is requiredfor the increase in [Ca²⁺]_i that drives CREB phosphorylation in cochlear nucleus neurons.Some studies have suggested that Ca²⁺ influx through L-type calcium channels and/or NMDA receptor channelsis required for CREB phosphorylation (Hardingham et al., 1999;Rajadhyaksha et al., 1999; Mermelstein et al., 2000). This doesnot seem to be the case in cochlear nucleus neurons because specificinhibition of AMPA receptors, which leaves available NMDA receptorsfor neuron depolarization and Ca²⁺ influx, completely prevents the [Ca²⁺]_i increase and subsequent CREB phosphorylation. In addition,inhibiting L-type Ca²⁺ channels or NMDA receptors with nifedipine or APV, respectively,has no effect on the deafferentation-induced increase in [Ca²⁺]_i in NM neurons or the number of p-CREB+ neurons. Perkinton etal. (1999) report that in primary cultures of mouse striatal neurons,Ca²⁺-permeable AMPA receptors cause an increase in [Ca²⁺]_i, with no contribution from voltage-gated Ca²⁺ channels or NMDA receptors. This [Ca²⁺]_i increase stimulates a mitogen-activated protein kinase cascaderesulting in CREBphosphorylation.

Residual glutamate in synaptic clefts has been reported to be in the low micromolar range (Sarantis et al., 1993; Jay et al.,1999). This concentration of glutamate has also been reportedto stimulate NMDA receptors but not AMPA/kainate receptors (Sarantiset al., 1993). Because of the unique morphological characteristicsof the eighth nerve calycine synapses (Parks, 1981; Carr and Boudreau,1991), which cover two-thirds of the NM neuron's surface, it isplausible to hypothesize that glutamate may reach higher concentrations $---$ highenough to activate the Ca²⁺-permeable AMPA receptors on these neurons. The NM neuron AMPAreceptors have an EC₅₀ of glutamate (Raman and Trussell, 1992;Raman et al., 1994) that is an order of magnitude lower than thatof the mGluRs in NM (Zirpel et al., 1994, 1995a). Thus, in theabsence of activity, the residual glutamate within the eighthnerve synaptic cleft may activate the AMPA receptors, but notthe mGluRs. Because the mGluRs mediate the calcium-clearing andhomeostatic mechanisms of NM neurons (Zirpel and Rubel, 1996;Zirpel et al., 1998, 2000; Kato and Rubel, 1999), after deafferentationan important Ca²⁺ regulatory mechanism is disabled, and the Ca²⁺ influx through AMPA receptors becomes cumulative and causes agradual [Ca²⁺]_i increase. Also consistent with AMPA receptor involvement isthe report by Solum et al. (1997) showing that AMPA receptor antagonistsprevent both normal developmental neuronal death and deafferentation-induceddeath in the auditory nuclei of chickembryos.

CREB can be phosphorylated on Ser133 by PKA, PKC, CaM kinases, and RSKs (Walton and Dragunow, 2000). There is considerableinteraction among these kinase pathways and the MAPK pathway,resulting in complex phosphorylation mechanisms that convergeon CREB (Roberson et al., 1999). In murine F9 cells, basic FGFinduced CREB phosphorylation via stimulation of the PKA and MAPKpathways (Hansen et al., 1999). Similarly, Impey et al. (1998a)demonstrated in pheochromocytoma-12 (PC-12) cells and hippocampalneurons that RSK phosphorylation of CREB depends on PKA activationand that CaMKIV is not essential for CREB phosphorylation. Itis not surprising, then, that our results indicate that at leasttwo different kinase pathways are capable of phosphorylating CREBin NM neurons after deafferentation. The protein kinase A andC pathways play a significant role in NM neuron calcium homeostasisduring normal eighth nerve stimulation (Zirpel et al., 1998) andare therefore prime candidates for involvement in Ca²⁺-dependent CREB phosphorylation. However, our results indicatethat CaM kinases and PKA are the primary CREB-phosphorylatingkinases active in NM neurons after activity deprivation. ThatPD98059 had no effect on the number of p-CREB+ neurons suggeststhat RSKs are not involved and hints that PKC also may not bedirectly involved because it is thought that PKC mediates CREBphosphorylation via the MAPK/RSKpathway.

CREB phosphorylation has been shown to be critical for neuronal survival in a variety of cell types and conditions. CREB phosphorylationprotects PC-12 cells from okadaic acid-induced apoptosis (Waltonet al., 1999) and seems to protect hippocampal dentate gyrus neuronsfrom ischemia (B. R. Hu et al., 1999; Walton and Dragunow, 2000).Some of the survival-promoting effects of NGF also seem to bemediated by CREB phosphorylation (Finkbeiner et al., 1997; Riccioet al., 1999; for review, see Finkbeiner, 2000). After deafferentation,30% of chick cochlear nucleus neurons die (Born and Rubel, 1985).Our results suggest that CREB phosphorylation occurs in the remaining70% of the activity-deprived neurons and promotes their survivalin their new hypercalcemic environment. All chick cochlear nucleusneurons express CREB, and all show increased [Ca²⁺]_i after deafferentation. Why, then, do only 70% show CREB phosphorylationand survive? It seems that the deafferentation-induced rise in[Ca²⁺]_i serves as a general signal to which 30% of the neurons respondby dying (perhaps via Ca²⁺-mediated apoptosis) and 70% respond by phosphorylating CREB andimplementing compensatory mechanisms. In agreement with this hypothesis,there appears to be an [Ca²⁺]_i threshold above which NM neurons begin to die (Zirpel et al.,1998); manipulations that prevent the [Ca²⁺]_i increase also prevent increased neuronal death. In the presentstudy, we show that manipulations (namely, kinase inhibition)that prevent CREB phosphorylation in the presence of the [Ca²⁺]_i increase result in increased neuronal death. Hence, in theabsence of activity, increased [Ca²⁺]_i serves as a signal for neuronal death or CREB phosphorylation:those neurons unable to phosphorylate or prevented from phosphorylatingCREBdie.

Our working hypothesis, based on the current study and consistent with the existing data, follows. Ambient glutamate in theeighth nerve synaptic cleft activates Ca²⁺-permeable AMPA receptors on the postsynaptic NM neurons. Thisallows an influx of Ca²⁺ that causes a gradual increase in [Ca²⁺]_i because of the absence of mGluR-mediated mechanisms for clearingCa²⁺. This increased [Ca²⁺]_i activates Ca²⁺-sensitive adenylate cyclases (AC). The cAMP generated by AC activatesPKA. PKA then directly phosphorylates CREB. Increased Ca²⁺ would also interact with CaM, translocate to the nucleus, andactivate a CaMK, most likely CaMKIV (Deisseroth et al., 1996;Chawla et al., 1998). CaMK would then phosphorylate CREB. In thisscenario, staurosporine would inhibit PKA, leaving CaMK activeto phosphorylate CREB. Our results showed a 51% decrease in CREBphosphorylation with staurosporine (Fig. 5). Alternatively, inthis scenario, inhibition of CaM kinase with KN-62 would leaveactive PKA to phosphorylate CREB. Our results showed a 65% decreasein CREB phosphorylation with KN-62 and a complete eliminationof CREB phosphorylation in the presence of both KN-62 and staurosporine.Inhibition of PKA with Rp-cAMPS showed a reduction in CREB phosphorylationsimilar in magnitude to that seen with staurosporine, suggestingthat the majority of staurosporine effects are mediated by inhibitionof PKA. After being phosphorylated by these pathways, CREB interactswith CREB binding protein and initiates the transcription of genescontaining the Ca²⁺/cAMP response element within their promoter region. These geneproducts may be proteins that allow the neuron to compensate forthe deafferentation-induced hypercalcemia and absence of synapticactivity. One gene of particular interest, which is known to beregulated by CREB transcription, is Bcl-2 (Wilson et al., 1996).BCL-2 is well known to serve an antiapoptotic role, and recentstudies have shown that BCL-2 message expression is upregulatedwithin hours of NM deafferentation (Wilkinson and Hyson, 2000).Future experiments using the genetics of a mouse model of deafferentation-inducedCREB phosphorylation will help elucidate which genes are transcribedand the mechanisms that allow neurons to survive activitydeprivation.

  FOOTNOTES

Received April 7, 2000; revised May 23, 2000; accepted June 1, 2000.

This work was supported by National Institutes of Health Grants HD 07491 and DC 00144. We are grateful to Dr. S. B. Katerfor allowing us to use his imaging facilities and to Alan C. Petersonand Dwan A. Taylor for technical assistance. We also thank MaeDel Puerto and Drs. Edwin W Rubel, Sara Cochran, and Sam Mostafapour,of the Virginia Merrill Bloedel Hearing Research Center, for theirinvaluable assistance with the mouse experiments and Dr. NikiHack for intellectualcamaraderie.
Correspondence should be addressed to Dr. Lance Zirpel at the above address. E-mail: zlance{at}mailman.med.utah.edu.

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