Spike Frequency Decoding and Autonomous Activation of Ca2+-Calmodulin-Dependent Protein Kinase II in Dorsal Root Ganglion Neurons

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (39)

Citing Articles via Google Scholar

Google Scholar

Articles by Eshete, F.

Articles by Fields, R. D.

Search for Related Content

PubMed

PubMed Citation

Articles by Eshete, F.

Articles by Fields, R. D.

Previous Article  |  Next Article

The Journal of Neuroscience, September 1, 2001, 21(17):6694-6705

Spike Frequency Decoding and Autonomous Activation of Ca²⁺-Calmodulin-Dependent Protein Kinase II in Dorsal Root Ganglion Neurons
Feleke Eshete and R. Douglas Fields
National Institutes of Health, National Institute of Child Health and Human Development, Bethesda, Maryland 20892-4480

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Autonomous activation of calcium-calmodulin kinase (CaMKII) has been proposed as a molecular mechanism for decoding Ca²⁺ spike frequencies resulting from action potential firing, butthis has not been investigated in intact neurons. This was studiedin mouse DRG neurons in culture using confocal measurements of[Ca²⁺]_i and biochemical measurements of CaMKII autophosphorylationand autonomous activity. Using electrical stimulation at differentfrequencies, we find that CaMKII autonomous activity reached nearmaximal levels after ~45 impulses, regardless of firing frequency(1-10 Hz), and autonomous activity declined with prolonged stimulation.Frequency-dependent activation of CaMKII was limited to spikefrequencies in the range of 0.1-1 Hz, despite marked increasesin [Ca²⁺]_i at higher frequencies (1-30 Hz). The high levels of autonomousactivity measured before stimulation and the relatively long durationof Ca²⁺ spikes induced by action potentials (~300 msec) are consistentwith the lower frequency range of action potential decoding byCaMKII. The high autonomous activity under basal conditions wasassociated with extracellular [Ca²⁺], independently from changes in [Ca²⁺]_i, and unrelated to synaptic or spontaneous impulse activity.CaMKII autonomous activity in response to brief bursts of actionpotentials correlated better with the frequency of Ca²⁺ transients than with the concentration of [Ca²⁺]_i. In conclusion, CaMKII may decode frequency-modulated responsesbetween 0.1 and 1 Hz in these neurons, but other mechanisms maybe required to decode higher frequencies. Alternatively, CaMKIImay mediate high-frequency responses in subcellular microdomainsin which the enzyme is maintained at a low level of autonomousactivity or the Ca²⁺ transients have fasterkinetics.

Key words: Ca²⁺-calmodulin-dependent protein kinase II; autophosphorylation; Thr-286; frequency decoding; cytoplasmic calcium; extracellular calcium sensor; DRG neurons; CaMKII; LTP

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Action potential firing can regulate many neuronal responses, but it is not understood how the frequency of firing is decodedby intracellular signaling pathways. Theoretical modeling andin vitro simulations provide evidence that calcium-calmodulinkinase (CaMKII) can decode the frequency of Ca²⁺ spikes into graded amounts of kinase activity (Hanson et al.,1994; Dosemeci and Albers, 1996; De Koninck and Schulman, 1998).This results from autophosphorylation at Thr-286, which promotescalmodulin binding to the enzyme (Meyer et al., 1992; Hanson etal., 1994), and converts the enzyme into a Ca²⁺-independent (autonomous) state (Miller and Kennedy, 1986; Thielet al., 1988; Lou and Schulman, 1989; Mukherji and Soderling,1994). Autonomously active CaMKII remains catalytically activeafter [Ca²⁺]_i returns to basal level after stimulation. This property couldenable the enzyme to sustain cellular responses long after a transientstimulus (Lisman and Goldring, 1988). CaMKII has a critical rolein many neuronal responses that exhibit frequency-dependent modulationsuch as hippocampal long-term potentiation (LTP) and long-termdepression (LTD) (Stevens et al., 1994; Lledo et al., 1995; Mayfordet al., 1995), and experiments on transgenic mice indicate thatThr-286 is a critical locus for induction of LTP (Giese et al.,1998).

In vitro simulations indicate that the frequency response of CaMKII can be modulated by factors such as the amplitude of theCa²⁺ spike, the duration of the Ca²⁺ spike, the subunit composition of the enzyme, and the previousactivation state of the kinase (De Koninck and Schulman, 1998).These forms of regulation are thought to contribute specificityto activation of this multifunctional enzyme, to enable phosphorylationof appropriate substrates in response to distinct cellular stimuli.It is important to determine how these factors affect the frequency-decodingproperties of CaMKII in neurons in response to naturally occurringspike-driven Ca²⁺ fluxes. This was investigated using a dorsal root ganglion (DRG)cell culture preparation equipped with stimulating electrodes(Fields et al., 1992).

This preparation offers a number of advantages. DRG neurons do not form synapses in culture, and they are not spontaneouslyactive. This allows good control of the firing frequency and providesa simpler model system than one involving synaptic transmission.DRG neurons have a large spherical cell body, with no dendrites,which allows good correlation between action potential-inducedCa²⁺ dynamics in the cell body with CaMKII activity measured in lysatesof the neurons. Many processes are regulated by action potentialsat 0.1-10 Hz in this preparation. This includes gene expression(Sheng et al., 1993; Itoh et al., 1995, 1997; Fields et al., 1997),neurite outgrowth (Fields et al., 1990, 1993), synaptic plasticity,and elimination (Nelson et al., 1989; Fields et al., 1991), calciumchannel expression (Li et al., 1996), myelination (Stevens etal., 1998), and Schwann cell proliferation and differentiation(Stevens and Fields, 2000).

These studies are the first test of frequency-dependent decoding by CaMKII in intact neurons. The results indicate that thespike frequency decoding of CaMKII is shifted toward low frequenciesof action potential firing, consistent with the high level ofautonomous activity before stimulation and the long duration ofCa²⁺ transients induced by actionpotentials.

Preliminary results have been reported in Eshete and Fields (1999).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Materials. Phosphosite-specific antiserum was a gift from Dr. Y. Yamagata (Laboratory of Neurochemistry, Okazaki, Japan).CaMKII antibodies were purchased from Life Technologies (Gaithersburg,MD), Santa Cruz Biotechnology (San Diego, CA), Transduction Laboratories(Lexington, KY), and Zymed (San Francisco, CA). Horseradish peroxidase-conjugatedanti-rabbit and anti-mouse Ig, ECL, and ECL Plus substrate wereobtained from Amersham Pharmacia Biotech (Piscataway, NJ). Anti-goatIg was from Santa Cruz Biotechnology. The special minimum essentialmedium (Eagle) with Earle's salts used for culturing neurons andphosphocellulose paper were obtained from Life Technologies. [ $gamma$ -³²ATP] (3000 Ci/mmol) was purchased from DuPont-New England Nuclear(Boston, MA). Polyvinylidene difluoride (PVDF) membrane (Immobilon-P)was purchased from Millipore (Bedford, MA). ImageQuant and theStorm image analysis system were from Molecular Dynamics (Sunnyvale,CA). Autocamtide-2, synthide-2, autocamtide-2 related peptides,PKI 6-22 amide, and PKC19-36 were purchased from Bachem (Torrance,CA). Protease inhibitor cocktail (Complete) was from BoehringerMannheim, and indo-1/AM, flu-3, and mag-indo-1 were purchasedfrom Molecular Probes (Eugene, OR). All other chemicals were analyticalgrade and were purchased from Sigma (St. Louis,MO).

Cell culture. Multicompartment chambers were made of Teflon and attached to collagen-coated 35 mm culture dishes as described(Fields et al., 1992). DRG neurons, dissociated from 13.5 d mousefetuses, were plated at a density of 0.5 × 10⁶ cells into each side compartment in a culture medium containing5% horse serum and 50 ng/ml nerve growth factor as described previously(Sheng et al., 1993). Non-neuronal cells were prevented from multiplyingby adding 13 µg/ml fluoro-2-deoxyuridine 1-2 d after seeding.Cultures were used for experiments 3-4 weeks after plating toallow time for most DRG neurons in the side compartments to extendaxons under the barrier between the side and centralcompartments.

Electrical stimulation of DRG neurons. Axons traversing under the barrier separating the two side compartments from the centralcompartment of the multicompartment insert were stimulated throughplatinum electrodes in contact with the culture medium on oppositesides of the barrier. Stimulation parameters and electrophysiologicalresponses to stimulation have been reported previously for DRGneurons in these multicompartment chambers (Fields et al., 1992).DRG neurons in this preparation respond with a single action potentialto stimulation with a 1-5 V, 200 µsec biphasic pulse. They followstimulation reliably and indefinitely at rates up to 3 Hz andfor several tens of seconds at 30 Hz (Fields et al., 1990, 1992).

Characterization of CaMKII isozymes. CaMKII isozymes were characterized by 8% SDS-PAGE from DRG and brain lysates in samplebuffer (125 mM Tris-HCl, pH 6.8, 4% SDS, 10% $beta$ -mercaptoethanol,20% glycerol, and 0.04% bromphenol blue) and immunoblotting. ThePVDF membranes were blocked in 5% milk in TTBS (10 mM Tris-HCl,pH 7.5, 150 mM NaCl, and 0.1% Tween 20) for 2 hr, washed, andincubated in a manifold (Deca-Probe; Hoefer) with polyclonal antibodiesagainst CaMKII- $alpha$ , - $beta$ , - $gamma$ , and - $delta$ (Santa Cruz Biotechnology), monoclonalantibodies Cb $alpha$ -2 (Life Technologies), and CB $alpha$ -2 (Zymed) at 1:1000for 2 hr at room temperature. The washed membranes were then reactedwith appropriate horseradish peroxidase-conjugated secondary antibodiesfor 1 hr at room temperature and detected byECL.

Autophosphorylation of CaMKII at Thr-286. CaMKII autophosphorylation at Thr-286 was analyzed by immunoblotting using a phosphosite-specificantibody that recognizes CaMKII only when it is autophosphorylatedat Thr-286 ( $alpha$ ) or Thr-287 ( $beta$ , $gamma$ , $delta$ ) (Yamagata and Obata, 1998).Neurons were washed three times and changed to physiological salinesolution containing 50 nM free Ca²⁺ (Scholz and Palfrey, 1998). This was obtained by substituting(in mM): 0.74 CaCl₂, 1.13 MgCl₂, and 2 EGTA in the standard PBSsolution (PSS). After 1 hr of equilibration, the calcium concentrationwas raised to 1.2 mM free Ca²⁺ for 5-45 sec by adding 100 mM CaCl₂ to the same solution. Treatedneurons were lysed in boiling sample buffer for electrophoresisand immunoblotanalysis.

For quantification of Thr-286 autophosphorylation, equal volume of lysates from control and treated neurons were resolvedin parallel by SDS-PAGE in duplicate 10% gels and electroblottedto PVDF membranes. Membranes were blocked in 5% milk in TTBS for2 hr at room temperature, washed, and incubated in antibody thatrecognized total CaMKII at 1:1500 (monoclonal antibody clone 38;Transduction Laboratories) or phosphosite-specific antibody (1:10,000)overnight at 4°C. Incubated membranes were washed and reactedin horseradish peroxidase-conjugated secondary antibody for 1hr at room temperature. The immunocomplexes were visualized withECL Plus substrate and quantified with ImageQuant and Storm imageanalysis system. The linearity of the immunoreactivity measurementwas tested by loading different volumes of lysate from DRG neuronscultured in chambers. The relative immunoreactivity (RFU) againstboth the autophosphorylated and total enzyme was within the dynamicrange. According to the Storm manufacturer (Application note #60), the dynamic range of measurement is 0-3 × 10⁷ RFU, whereas the readings in this study varied between 0.2 and1 × 10⁶ RFU. Relative autophosphorylation at Thr-286 was compared bynormalization of the RFU obtained with the phosphorylated enzymeto that of the total enzyme in the same sample from parallelexperiments.

To determine the [Ca²⁺] needed to autonomously activate CaMKII in vitro, DRG supernatant from unstimulated neurons was autophosphorylatedusing an adaptation of the method of Molloy and Kennedy (1991).Briefly, assay tubes containing different concentration of Ca²⁺ (0.1-1000 µM) and 6 µM CaM were phosphorylated for either 15or 45 sec with 1 mM MgCl₂ and 0.02 mM ATP. After autophosphorylation,autocamtide-2 plus EGTA (2 mM final) was added to each tube, andincubation continued for 5 min. Ca²⁺-dependent and independent activity was also determined in parallelin supernatants that were not autophosphorylated in vitro.

CaMKII activity assay. Ca²⁺-CaM-dependent and -independent activity of CaMKII was measured in neuronal homogenates by phosphorylationof autocamtide-2 (KKALRRQETVDAL), a peptide derived from the autophosphorylationsite of CaMKII. The kinase assay was linear with respect to timeand the amount of lysate used for analysis. Neurons equilibratedin 1.2 mM Ca²⁺-PSS for 1 hr were electrically stimulated at 0.1, 0.3, 0.5, 1,and 10 Hz, delivering 45 pulses at these frequencies for durationsof up to 10 min. At the end of stimulation, neurons were harvestedin 0.20 ml of ice-cold lysis buffer (50 mM HEPES, pH 7.5, 1 mMEDTA, 5 mM EGTA, 2 mM DTT, 0.1% TX-100, 100 mM $beta$ -glycerol phosphate,10 mM sodium pyrophosphate, 50 mM NaF, protease inhibitor cocktail,and 1 µM Microcystein LR). The harvested neurons were sonicatedin an ice bath with a Bronson probe sonicator (two pulses at 40%duty cycle and output of 2) and centrifuged at 15,000 × g, for15 min at 4°C. Kinase assays were performed on 8.5 µl aliquotsof the supernatant using 20 µM autocamtide-2 in the presence of1 mM Ca²⁺ and 6 µM CaM (total activity), and in parallel samples the reactionwas performed in the absence of Ca²⁺ with 1 mM EGTA (Ca²⁺-independent activity). Background activity was determined fromsupernatant reacted without the substrate. The reaction tubesalso contained 5 µM of the protein kinase A inhibitor PKI 6-22amide and 2 µM of the protein kinase C inhibitor (PKC19-36). Enzymereactions, in a final volume of 50 µl, were initiated by the additionof Mg²⁺-ATP cocktail [5 mM magnesium acetate and 0.1 mM ATP (2000-3000cpm/pmol)]. The reaction was stopped after 5 min with saturatedsolution of EDTA-EGTA, and 40 µl was spotted onto phosphocellulosepaper. The phosphocellulose paper was washed once in water andthree times in 75 mM phosphoric acid. The membranes were air-driedand used for radioactivity measurement by liquid scintillationcounting. For each sample, the radioactive phosphorous countsfrom assay tubes in which the reaction mix contained cell lysatein the presence of 1 mM EGTA and no Ca²⁺ were compared with counts from tubes in which an equal amountof the cell lysate was reacted in the presence of 1 mM Ca²⁺ and 6 µM CaM. The autonomous activity of CaMKII in these celllysates was determined by the ratio of the calcium-independentand calcium-dependentactivities.

Intracellular calcium measurements. Electrically or chemically evoked calcium transients in DRG neurons were measured usinga Bio-Rad (Hercules, CA) 1024 visible/UV confocal microscope anda Nikon 40× 1.3 numerical aperture oil immersion objective ona Nikon inverted microscope. Quantitative calcium measurementswere made using ratiometric measurements of fluorescence intensityat 460 and 405 nm emission from DRG neurons loaded by incubationin 7.5 µM indo-1/AM or mag indo-1/AM and excited by an argon-ionlaser at 350 nm (Fields and O'Donovan, 1997). Measurements wereperformed at room temperature in HEPES-buffered balanced saltsolution, pH 7.2. In-cell calibration, as described in Fieldset al. (1993), was used to provide an estimate of the [Ca²⁺]_i associated with the fluorescence ratios. Briefly, R_min andR_max were determined in neurons permeabilized by 10 µM ionomycin,in solutions containing 1.8 mM Ca²⁺ and 0 mM Ca²⁺/10 mM EGTA, under the same intensifier gains and pinhole settingsthat were used during the experiments. Measurements of [Ca²⁺]_i were made within an optical plane passing through the centerof the nucleus in the area of the cytoplasm midway between cellmembrane and the nucleus. The area of measurement comprised ~1/8of the area of cytoplasm in the plane of section. The measuredresponses were uniform within different regions of the cell onthe time scale reported in these experiments. An electromagneticvalve-controlled perfusion device (Warner Instruments, Hamlin,CT) was used to rapidly change the concentration of extracellularcalcium in the bathingsolution.

Single line-scan mode confocal microscopy was used for high-speed acquisition of changes in [Ca²⁺]_i in response to action potentials of 0.1-30 Hz using the ratiometriccalcium indicator indo-1 and the fluorescent intensity indicatorfluo-3. Data were acquired at a rate of 8 msec/line scan for 2sec (250 line scans) for both ratiometric and nonratiometric indicators.In individual neurons, quantitative measurements were taken atfour points along a line bisecting the neuron within an opticalsection passing through the center of the nucleus: (1) in thesubmembrane region, (2) in the cytoplasm midway between the membraneand the nucleus, (3) in the center of the nucleus, and (4) atthe midpoint in the cytoplasm on the opposite side of thenucleus.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cytoplasmic Ca²⁺ transients induced by different frequencies of action potentials

Intracellular calcium imaging was used to determine the spatial and temporal characteristics of intracellular calcium responsesto action potentials delivered at different frequencies in DRGneurons. Changes in [Ca²⁺]_i were measured in the cell body using confocal microscopy insingle line-scan and x-y scanning modes with fluo-3, indo-1, andmag-indo fluorescent calcium indicators. Several calcium indicatorswere used to explore possible effects of the calcium dissociationconstant of the indicator on the measurements and to evaluatepotential differences caused by ratiometric and nonratiometricmeasurementmethods.

Responses to individual action potentials could be resolved with high-speed calcium imaging. In Figure 1A, an optical sectionof a single mouse DRG neuron is shown loaded with the calciumindicator fluo-3. The nucleus can be discerned by differentialfluorescence of the calcium indicator in the nucleus and cytoplasm;this is not caused by differences in free calcium concentrationbetween the nucleus and the cytosol in the resting state (Gillotand Whitaker, 1993, 1994; O'Malley 1994; Meyer et al., 1995).To obtain high-speed measurements, the excitation laser was scannedrepeatedly through the center of the cell, and data were acquiredat a rate of 8 msec/scan. Fluorescence intensity changes shownin Figure 1B are from a DRG neuron filled with the calcium indicatorindo-1, which exhibits a decrease in fluorescence intensity at460 nm emission with increasing calcium concentration. A singleaction potential induced an increase in intracellular calciumwith a magnitude of ~20 nM and a duration of ~300 msec (Fig. 1B).The calcium increase was much faster than the kinetics of recoveryto resting calcium concentration.

View larger version (67K):
[in this window]
[in a new window]
Figure 1. High-speed measurements of action potential-induced changes in intracellular calcium in DRG neurons using confocal microscopy in single line-scan mode. A, An optical section of a single mouse DRG neuron is shown loaded with the calcium indicator fluo-3 (black and white image). The excitation laser was scanned repeatedly through the center of the cell, and data were acquired at a rate of 8 msec/scan and displayed as a stack of sequential scans. Changes in intracellular calcium induced by action potential stimulation are shown for 250 sequential samples (2 sec total). Thus, the vertical dimension displays changes in calcium concentration with time, and the horizontal dimension displays one-dimensional spatial information on the calcium concentration along a transect across the center of the neuronal cell body. Measurements were taken in response to 0.1-30 Hz stimulation; the response to 20 Hz stimulation is shown here. Electrical stimulation caused an influx of calcium from the cell membrane and the increase in intracellular calcium propagated to the nucleus within ~200 msec. Intracellular calcium concentration reached similar peak levels in the cytoplasm and nucleus. The three vertical magenta lines indicate the regions used for quantitative comparisons (black arrows). B, The increase in intracellular calcium concentration induced by single action potentials could be resolved with single line-scan measurements. Fluorescence intensity at 460 nm emission is shown from a DRG neuron filled with the calcium indicator indo-1. This indicator exhibits a decrease in fluorescence intensity with increasing calcium concentration at this emission wavelength. The ratio of such images at 460 and 405 nm emission wavelengths was used for quantitative analysis, as shown in Figure 2G. The increase in intracellular calcium induced by an action potential lasted ~300 msec after each action potential, and the kinetics of increase were much faster than the recovery to resting calcium levels. Scale bar, 10 µm.

After delivering trains of action potentials, a rapid increase in intracellular calcium could be resolved with single line-scancalcium imaging spreading from the membrane to the nucleus within~200 msec (Fig. 1A) (see also Hernandez-Cruz et al., 1990). Thepeak concentration of calcium was quantified adjacent to the plasmamembrane, in the cytoplasm midway between the cell membrane andnucleus, and in the center of the nucleus (Fig. 1A, three verticalmagenta lines). Intracellular calcium concentration quickly reachedsimilar peak levels in all three regions of the cell after electricalstimulation, with a phase lag of ~300 msec from the cell membraneto the center of thenucleus.

The relation between action potential firing frequency and cytoplasmic calcium dynamics in DRG neurons was determined in responseto stimulus trains of 15-30 sec, using confocal calcium imagingin x-y scanning mode at acquisition rates of 3 images/sec. Duringlow-frequency stimulus trains (0.1-1 Hz), individual spikes in[Ca²⁺]_i could be resolved in response to individual action potentials(Fig. 2B, D-F). Trains of stimulation at and above frequenciesof 0.3 Hz resulted in temporal summation of calcium spikes andcalcium accumulation (Fig. 2A-D). In response to high-frequencystimulation (20 Hz), individual calcium spikes could only be resolvedwith high-speed single line-scan confocal microscopy (Fig. 2G).At these higher frequencies, temporal summation of calcium spikesresulted in a rapid and large increase in intracellular calciumthat was maintained for the duration of the stimulus burst (Fig.2G). As with the single-line scan measurements, and as previouslyreported by O'Malley (1994) and Fields et al. (1997), peak calciumresponses were similar in the submembrane region, central cytoplasm,and nucleus.

View larger version (28K):
[in this window]
[in a new window]
Figure 2. Intracellular calcium transients induced by action potential stimulation of different frequencies were measured in the cell body of DRG neurons with confocal microscopy and the ratiometric calcium indicator indo-1. Individual cytoplasmic calcium spikes (B, D-F) can be seen in response to individual action potentials (arrows) elicited by electrical stimulation at different frequencies. Stimulation at higher frequencies resulted in temporal summation and an elevation in intracellular calcium level that was positively correlated with the stimulus frequency and sustained for the period of the stimulus train (A-D). In response to higher frequency stimulation, individual calcium spikes (arrows) could be resolved using single line-scan mode confocal microscopy on top of a large increase in intracellular calcium concentration (G). Note the difference in axis scaling for each graph.

The increase in peak [Ca²⁺]_i and the rise time were positively correlated with the frequency of stimulation (Fig. 3A). Afterstopping stimulus trains, calcium levels recovered at a slowerrate; with higher frequency stimulation causing more sustainedelevations in calcium concentration than lower frequency stimulation(Fig. 3A, insets). Similar calcium dynamics were seen using thecalcium indicator indo-1, a ratiometric indicator that is notsubject to artifacts associated with fluorescence intensity calciumindicators (e.g., fura-2 and fluo-3), and using the very low-affinitycalcium indicator, mag-indo-1 (K_d = 35,000 nM as compared with230 nM for indo-1) (Fig. 3B).

View larger version (34K):
[in this window]
[in a new window]
Figure 3. The concentration dynamics of electrically evoked intracellular Ca²⁺ concentration varied directly with the stimulus frequency. A, Changes in cytoplasmic calcium were measured by confocal microscopy using the ratiometric fluorescent calcium indicator indo-1/AM. The rate of rise, peak, concentration, and duration of Ca²⁺ increase were positively correlated with stimulus frequency between 1 and 30 Hz. Data for 1 and 10 Hz are shown as insets on an expanded time scale. Results shown are mean ± SEM (n = 12 neurons). Scale bar, 30 sec stimulation. B, Similar responses are observed using the low-affinity indicator mag-indo-1, which is less sensitive to small changes in intracellular calcium.

The results of these calcium imaging studies show that action potentials induced by electrical stimulation of different frequenciesare effective in causing large changes in [Ca²⁺]_i that are positively correlated with the frequency of stimulation.However, the action potential-induced intracellular Ca²⁺ fluxes are much slower and more persistent than the spikes usedin some theoretical models (Hanson et al., 1994; Okamoto and Ishikawa2000) and in vitro simulations giving sensitive frequency decoding(De Koninck and Schulman, 1998).

Within the temporal and spatial limits defined by these measurements, microdomains of [Ca²⁺]_i were not apparent in response to membrane depolarization fromtrains of action potentials lasting several seconds. This allowsa reasonably good correlation between action potential-inducedcalcium dynamics measured in the cell body after several secondsof action potential stimulation, with CaMKII autonomous activitymeasured from lysates of neurons in the side compartments of culturechambers that contained the cell bodies of DRGneurons.

Autonomous activity is the ratio of catalytic activity of CaMKII in the absence of Ca²⁺ to the activity in the presence of Ca²⁺. This is of interest because autonomous activity of CaMKII allowsthe enzyme to sustain a response long after the neuron experiencesa burst of action potentials and intracellular calcium returnsto basal levels. Autonomous activity derives from phosphorylationof Thr-286, which we assessed by an immunoblot using a phosphosite-specificantibody (Yamagata and Obata, 1998).

In vitro measurements using CaMKII- $alpha$ immobilized in PVC tubing indicate that varying the duration of individual calcium pulsesshifted the frequency response of CaMKII autonomous activationand changed its steepness (De Koninck and Schulman, 1998). Thefrequency response of CaMKII to calcium pulses with a durationof 300 msec or longer would be relatively shallow and limitedto frequencies of less than ~1 Hz (De Koninck and Schulman, 1998).Therefore, we tested the autonomous activation of CaMKII in responseto different frequencies of action potential stimulation in DRGneurons. Before measuring the basal and stimulus-induced autophosphorylationof CaMKII at Thr-286, we examined the subunit composition of CaMKIIin DRGneurons.

Characterization of CaMKII in DRG neurons

Immunohistochemical staining shows a ubiquitous distribution of CaMKII throughout the neuron, and the enzyme represented ~70-80%of the total Ca²⁺-CaM-dependent kinase activity in cultured DRG neurons as determinedby inhibition of phosphorylation of the glycogen synthase peptide(syntide-2) with a specific inhibitory peptide related to autocamtide-2(F. Eshete and R. D. Fields, unpublished data). Immunoblottingstudies revealed that the $gamma$ (~58-60 kDa) and $delta$ (~60, 58, 56 kDa)isozymes are the predominant CaMKII isozymes in DRG neurons, whereasthe $alpha$ and $beta$ isozymes are either expressed in very low amountsor absent from these neurons (Fig. 4A,B). These observations areconsistent with the recent report on the developmental expressionof CaMKII isozymes in the mouse nervous system (Bayer et al.,1999).

View larger version (75K):
[in this window]
[in a new window]
Figure 4. $delta$ and $gamma$ are the two major CaMKII isozymes expressed in cultured DRG neurons. A, Lysate from cultured neurons was resolved in 8% single well gel and immunoblotted in a manifold with polyclonal antibodies that reacted with the $alpha$ , $beta$ , $gamma$ , and $delta$ isozymes (Santa Cruz Biotechnology) and a monoclonal antibody specific to CaMKII- $alpha$ (Life Technologies). The anti-CaMKII- $gamma$ antibody reacted with bands (58-60 kDa) representing the $gamma$ isoforms, whereas the antibody against CaMKII- $delta$ recognized bands with apparent molecular mass of ~56, 58, and 60 kDa. B, Lysates from DRG neurons, mouse hippocampus, cortex, and cerebellum were immunoblotted with antibody specific to CaMKII phosphorylated at Thr-286. In DRG lysate the phospho-specific antibody mainly reacted with bands of ~56, 58, 59, and 60 kDa. Note the relative absence of the CaMKII- $alpha$ band in both DRG neurons and mouse cerebellum.

The CaMKII enzymes present in DRG neurons would be expected to exhibit similar frequency responses to the isotypes examinedin vitro (De Koninck and Schulman, 1998). The CaM affinity ofthe $gamma$ and $delta$ isoforms of CaMKII is similar to that of CaMKII- $alpha$ isozymes (Edman and Schulman, 1994). All CaMKII isozymes containa MHRQETV motif that is responsible for autonomous activationof the enzyme through phosphorylation of Thr 286. These isoformsdiffer in the variable domain of the protein (Brocke et al., 1999).CaMKII measured in brain homogenates and the $delta$ isozymes (Edmanand Schulman, 1994) both exhibit Ca²⁺-independent activation after autophosphorylation of Thr-286 (Kwiatkowskiand McGill, 2000).

CaMKII autophosphorylated at Thr-286 was detected by immunoblotting with a phosphosite-specific CaMKII antibody (Fig. 4B).All isoforms of CaMKII in DRG neurons, freshly dissected hippocampus,cortex, and cerebellum showed immunoreactivity to CaMKII phosphorylatedat Thr-286 (Fig. 4B). Note the low levels of the $alpha$ -CaMKII isoformin DRG neurons and cerebellum with the phosphosite-specificantibody.

Action potential frequency dependence of CaMKII autonomous activity

CaMKII autonomous activity was found to vary as a function of action potential firing frequency and the duration of actionpotential firing (p < 0.0001, ANOVA) (Fig. 5A, Table 1). Theobserved response to constant frequency action potential stimulationwas biphasic, with a rapid increase to peak CaMKII autonomousactivation followed by a subsequent decline in autonomous activitywith more prolonged stimulation. The frequency of action potentialsin the stimulus train affected both the rising and declining phaseof CaMKII autonomy with respect to stimulus time. Higher frequencystimulation promoted both the rate of increase and the rate ofdecline in the autonomous activity of the enzyme. CaMKII autonomousactivity was increased significantly (p < 0.01) after stimulationat 1, 3, and 10 Hz stimulation for 15 sec, but the differencesamong these stimulus frequencies were not statistically significantat 15 and 45 sec.

View larger version (27K):
[in this window]
[in a new window]
Figure 5. The effect of action potential frequency and stimulus duration on autonomous activation of CaMKII. CaMKII autonomy ratio is the ratio of Ca²⁺-independent activity/total activity. Autonomous activity of CaMKII was measured by in vitro phosphorylation assay in homogenates of neurons electrically stimulated for 5, 15, 45, and 600 sec at 0.1, 1, 3, and 10 Hz. A, Stimulation at 1, 3, and 10 Hz for 15 sec induced statistically significant Ca²⁺-independent activation of CaMKII compared with unstimulated controls (p < 0.01; t test; n = 24 dishes), but the differences among responses to 1, 3, and 10 Hz were not statistically significant at 15 and 45 sec. The results shown (mean ± SEM) are from five independent experiments (ANOVA; p = 0.02; n = 150 dishes). Inactivation of the enzyme was promoted by long-duration high-frequency stimulation. The duration of stimulation required to reach maximal levels of CaMKII autonomy varied inversely with the frequency of stimulation. Stimulation at very low frequency (0.1 Hz) failed to increase CaMKII autonomous activity significantly. B, Maximal autonomous activation of CaMKII correlated with the number of action potentials delivered at these different frequencies. Within the range of 1-10 Hz, near-maximal autonomous activity was reached after ~45 action potentials, regardless of stimulus frequency. Statistical analysis by ANOVA (p < 0.0001; n = 178), followed by Fisher's LSD multiple comparison procedure (Table 1) indicates significant increases in CaMKII autonomous activation after 45 action potentials are delivered at all frequencies tested within the range of 0.5-10 Hz, despite large differences in the stimulus duration required to reach 45 action potentials at these different frequencies (i.e., 4.5-90 sec).


View this table:
[in this window]
[in a new window]
Table 1. Pairwise multiple comparison test using Fisher's LSD procedure for differences in CaMKII autonomous activation after electrical stimulation, varying action potential frequency, number, and stimulus duration

Similar peak levels of CaMKII autonomous activity were reached with stimulus trains of 1-10 Hz, but the optimal duration ofconstant-frequency action potential firing was different for eachstimulus frequency and varied inversely with the action potentialfiring frequency. Near maximal levels were reached after only4.5 sec stimulation at 10 Hz, in contrast to 15-150 sec for stimulationat 1 Hz. The slope of the function after 15 sec stimulation at1 Hz was positive (p < 0.0001), but after 45 action potentials,the slope could not be distinguished statistically from zero,indicating a near maximal response had been reached. Low-frequencystimulation (0.1 Hz) did not alter CaMKII autonomous activitysignificantly, even after prolonged stimulation (7.5min).

The optimal duration of stimulation and inverse relation to the stimulus frequency implies that maximal CaMKII autonomousactivity may be dependent on the number of action potentials deliveredover this range of stimulus frequencies. Replotting the data inFigure 5A as a function of action potential number, rather thanstimulus duration shows that near maximal CaMKII autonomous activationwas attained by stimulation with 45 action potentials at 1 Hz,and by 45 action potentials (the shortest duration assayed) at3 and 10 Hz (Fig. 5B). Analysis by one-way ANOVA, followed byFisher's LSD multiple comparison test showed statistically significantincreases in autonomous activation after 45 action potentialsdelivered at 0.5-10 Hz, despite marked differences in the durationof stimulation required to deliver 45 action potentials at thesedifferent frequencies (Table 1).

The ratio of calcium-independent to calcium-dependent CaMKII activity was high in DRG neurons under basal conditions (0.28± 0.068; n = 36 dishes). Previous studies have also shown highautonomous CaMKII activity in freshly dissociated brain tissueand unstimulated hippocampal slice in the range of 0.15-0.20 (Molloyand Kennedy, 1991; Ocorr and Schulman, 1991).

A frequency response curve for CaMKII autonomous activation was derived by delivering equal numbers of action potentials (45)at different frequencies within the range of 0.1-10 Hz (Fig. 6).CaMKII exhibited frequency-dependent activation in DRG neuronsin response to action potentials between 0.1 and 1 Hz (p < 0.001;slope of linear regression = +30.2 ± 9.01; n = 84), but the responseplateaued at higher frequencies (1-10 Hz) (slope not significantlydifferent from 0; p = 0.89; n = 46), despite marked differencesin [Ca²⁺]_i in response to these frequencies of stimulation (Fig. 3). Spikefrequency decoding by CaMKII has not been demonstrated in intactneurons, but the behavior of CaMKII- $alpha$ in vitro would predict thatthe high level of CaMKII autophosphorylation in unstimulated DRGneurons and the persistence of [Ca²⁺]_i after action potentials should shift the spike frequency decodingto lower frequencies of calcium pulses, which is consistent withthe present results.

View larger version (17K):
[in this window]
[in a new window]
Figure 6. Spike frequency decoding by CaMKII in DRG neurons. The frequency response curve was derived by delivering 45 action potentials at frequencies of 0.1, 0.3, 1, 3, and 10 Hz. Results are plotted as percentage of maximum stimulus-induced increase in CaMKII autonomy ratio (mean ± SEM; n = 111 dishes). CaMKII in DRG neurons showed sensitivity to low frequencies of action potentials <1 Hz, but higher frequency stimulation produced similar levels of CaMKII autonomous activation, despite marked differences in intracellular Ca²⁺ (compare Fig. 3). The mean ratio of Ca²⁺-independent activity/total activity in unstimulated neurons (0 Hz) was 0.28 ± 0.068 (n = 36 dishes).

Relation between CaMKII autonomy and intracellular calcium dynamics

A useful simplifying assumption in mathematical modeling and in vitro simulations of CaMKII activity has been to model actionpotential-induced calcium transients as fixed-amplitude rectangularpulses of defined pulse width that returned to baseline duringthe interpulse interval (Hanson et al., 1994; DeKoninck and Schulman1998; Okamoto and Ishikawa, 2000.) The actual [Ca²⁺] dynamics induced by action potentials are somewhat more complicated.Notably, higher frequency stimulation leads to temporal summationof intracellular calcium concentration because the rate of restoringintracellular Ca²⁺ to basal levels, via pumps and exchangers, is much slower thanthe rate of Ca²⁺ accumulation in the cytoplasm via influx through Ca²⁺ channels in the plasma membrane and intracellular organelles.The accumulation of "residual" Ca²⁺ accompanying higher frequency action potential stimulation hasimportant physiological implications, for example in paired-pulsefacilitation, and this behavior is shown clearly by Ca²⁺ imaging in DRG neurons (Fig. 1A-D). Changes in calcium bufferingmechanisms after trains of stimulation may also increase calciumaccumulation and raise the steady-state calcium set-point (Colegroveet al., 2000). These Ca²⁺ measurements show that accumulation of residual Ca²⁺ and peak Ca²⁺ levels are positively correlated with action potential frequency(Fig. 3A). Thus, it is necessary to examine the extent to whichthe action potential decoding of CaMKII is dependent on the temporaldynamics of intracellular Ca²⁺ spikes or the associated concentration of cytoplasmic Ca²⁺.

Several lines of evidence suggest that the Ca²⁺ spike frequency can be more important than the [Ca²⁺]_i in autonomous activation of CaMKII. Over the range of actionpotential frequencies in which CaMKII decodes action potentialfrequency (0.1-1 Hz), the increase in residual Ca²⁺ is comparatively small (100-300 nM) (Fig. 1), relative to theconcentration of Ca²⁺ necessary for autophosphorylation of the enzyme in vitro. Consistentwith studies from several laboratories (Katoh and Fujisawa, 1991;Rich and Schulman, 1998), our measurements of CaMKII autophosphorylationin lysates of DRG neurons in vitro show a dependence on steady-stateCa²⁺ concentration >1 µM, which is much greater than the residual[Ca²⁺]_i induced by 0.1-1 Hz stimulation. Ca²⁺-independent activity (autonomy ratio) was measured in lysatesof unstimulated neurons after autophosphorylation for 15 and 45sec in the presence of 0.1, 0.2, 0.3, and 1 µM and 1 mM Ca²⁺ in vitro. The autonomy ratios after autophosphorylation at 0.1-1µM Ca²⁺ were not significantly different from controls, but increasedsignificantly to 0.72 ± 0.09 after 15 sec autophosphorylationwith 1 mM Ca²⁺ (ANOVA with Fisher's multiple comparison test; n =21).

Second, there was not a good correlation between residual or peak calcium levels and CaMKII autonomous activity. Similar levelsof CaMKII autonomous activity were reached in response to trainsof action potentials of 1-10 Hz (Fig. 5A), but the residual orpeak increase in [Ca²⁺]_i were markedly different (Fig. 3A). A 10 Hz stimulus raisedaverage [Ca²⁺]_i to a peak level of 780 nM after 15 sec of stimulation comparedwith 370 nM peak response to 1 Hz stimulation. Stimulation of~2 sec was required to achieve 50% of the maximum cytoplasmiccalcium amplitude with 10 Hz stimulus frequency (Fig. 3C) comparedwith 10 sec for 1 Hz stimulation (Fig. 3B). The increase in [Ca²⁺]_i was larger and remained elevated for a longer time after stimulationregardless of whether a high [Ca²⁺] affinity (indo-1) or low Ca²⁺ affinity (mag-indo-1) Ca²⁺ indicator was used. The sustained large increase in [Ca²⁺]_i argues against ineffective stimulation as an explanation forthe similar stimulus-induced increase in CaMKII autonomy in responseto action potential firing at 1-10Hz.

To further explore this issue, bursts of action potentials were used to vary the duration of cytoplasmic calcium transients,their amplitude, and the level of cytoplasmic calcium accumulationunderlying the transients. The change in [Ca²⁺]_i in response to a single action potential was resolved in theseexperiments (Fig. 2F) and in previous studies (Fields et al.,1997) and was estimated to reach a peak of ~20 nM above restinglevels. To distinguish whether the enzyme failed to respond to0.1 Hz stimulation because of Ca²⁺ pulse frequency decoding of the enzyme or its sensitivity toCa²⁺ concentration, short bursts of 18 action potentials (at 10 Hz)were delivered repeatedly at intervals of 10 sec (a frequencyof 0.1 Hz). Intracellular calcium measurements in these neuronsshow that a single burst of this type produces a peak concentrationof ~500 nM (Fields et al., 1997), and trains of such bursts repeatedat 0.1 Hz result in a large increase in [Ca²⁺]_i (Fig. 7Aa). When 45 bursts of this type were repeated at afrequency of 0.1 Hz, CaMKII autonomous activity was not significantlydifferent from unstimulated neurons (Fig. 7B, bar a). Althoughthis pulsed stimulus delivered a total of 810 individual actionpotentials and raised [Ca²⁺]_i to high levels, the low-frequency pulse-train of action potentialbursts was not effective in increasing the autonomous activityof the enzyme, whereas only 15 individual action potentials at1 Hz was highly effective (Fig. 5A).

View larger version (22K):
[in this window]
[in a new window]
Figure 7. CaMKII autonomous activity in response to periodic bursts of action potentials correlates with the frequency of calcium pulses rather than concentration of intracellular calcium. A, Intracellular calcium transients were measured by confocal microscopy in neurons stimulated in three patterns: 18 action potential bursts (at 10 Hz) repeated at 10 sec intervals (0.1 Hz) (a); three action potential bursts (at 10 Hz) repeated at 3 sec intervals (0.3 Hz) (b); and single action potentials delivered at 3 sec intervals (0.3 Hz) (c). The net increase in [Ca²⁺]_i during the entire stimulus period with each stimulus pattern is given in brackets in the top right of each plot (calcium concentration time integral, nanomolar con- centration). The average calcium response of the same five neurons is plotted in response to each stimulus. B, Comparing CaMKII autonomous activity in response to single action potentials and repetitive bursts of action potentials at different frequencies. Stimulation at low frequency failed to increase CaMKII autonomous activity regardless of whether single action potentials or bursts of 18 action potentials were delivered. The increase in [Ca²⁺]_i produced by these different stimuli (A, a-c) did not correlate with CaMKII autonomous activation, suggesting that the frequency of calcium transients was more critical than the calcium levels. CaMKII autonomy is plotted as the percentage of maximal stimulus-induced increase in ratio of calcium-independent-calcium-dependent activity, which averages 0.28 ± 0.068 in unstimulated neurons; p < 0.01; ANOVA; n = 96; *values outside the indicated range are significantly different by Fisher's LSD multiple comparison test.

In addition to peak and residual [Ca²⁺]_i, the time-integrated increases in [Ca²⁺]_i produced during the stimuli were not well correlated with theautonomous activity of CaMKII (Fig. 7B vs the net increase inCa²⁺ shown in brackets in Fig. 7A). In contrast to the long-durationbursts of 18 action potentials, shorter bursts (3 action potentialsat 10 Hz) that were repeated at more frequent intervals of 3 sec(0.3 Hz) did increase CaMKII autonomous activity to near maximallevels (Fig. 7B, bar b). The long-duration pulses of 18 actionpotentials repeated at 0.1 Hz (Fig. 7Aa), caused ~11.4 times greatertime-integrated [Ca²⁺]_i increase than the short-duration pulses (3 action potentialsrepeated at 0.3 Hz) (Fig. 7Ab), and ~137 times more than constant-frequencystimulation at 0.3 Hz (Fig. 7Ac), yet this stimulus pattern wasless effective than either pulsed or single action potential stimulationat 0.3 Hz in increasing autonomous activity of CaMKII (Fig. 7B,bars b,c). As with constant frequency stimulation, the best correlationwith CaMKII autonomous activity after bursts of action potentialswas with the frequency of Ca²⁺ transients rather than with the [Ca²⁺]_i.

Extracellular calcium affects CaMKII autophosphorylation and autonomy

The high levels of autonomously active CaMKII in unstimulated neurons has significant functional effects on the frequencyresponse of the enzyme, making it important to better understandthe mechanisms regulating the level of CaMKII autonomy in unstimulatedconditions. Previous studies in hippocampal slice (Molloy andKennedy, 1991) and hippocampal neurons in culture (Scholz andPalfrey, 1998) also report high levels of CaMKII autonomous activityunder basal conditions. Interestingly, those studies reportedthat the level of CaMKII autonomy could be reduced by loweringthe concentration of extracellular calcium ([Ca²⁺]_o) (Molloy and Kennedy, 1991; Scholz and Palfrey, 1998). It hasbeen hypothesized that the high levels of autophosphorylationof CaMKII in unstimulated neurons is a result of sustained kinaseactivity associated with spontaneous synaptic activity in thecultures or brain slice, which is suppressed by lowering the [Ca²⁺]_o. De Koninck and Schulman (1998) suggest that this relativelyhigh level of autonomously active CaMKII in unstimulated conditionscould allow CaMKII to act as a tag of the history of activityat a synapse, because partial autophosphorylation of CaMKII underbasal conditions would shift the frequency response curve towardlower frequencies of Ca²⁺ spikes. This property of the enzyme would permit low-frequency,subthreshold activation to maintain the phosphorylated state ofthe enzyme at the taggedsynapse.

Alternatively, changes in [Ca²⁺]_i secondary to changes in [Ca²⁺]_o could affect autophosphorylation and autonomy of CaMKII (Scholzand Palfrey, 1998). It has also been proposed that the high levelsof CaMKII autonomy under basal conditions and the reduction afterlowering [Ca²⁺]_o, could result from phosphorylation of the enzyme that is dependenton a specialized synaptic extracellular Ca²⁺ sensor (Scholz and Palfrey, 1998).

Studies in DRG neurons could be helpful in distinguishing between these alternatives, because DRG neurons in culture lacksynapses and spontaneous impulse activity. The results showedthat incubating DRG neurons in low Ca²⁺ solution (50 nM) for 1 hr induced a dramatic reduction in theautophosphorylation (Fig. 8A,B) and the autonomous activity ofCaMKII (Fig. 8C). When neurons preincubated in low [Ca²⁺]_o (50 nM Ca²⁺-PSS for 60 min) were switched to physiological calcium concentrationof 1.2 mM, a large and significant increase (p = 0.0004; t test;n = 8 dishes) in autophosphorylation of CaMKII at Thr-286 wasobserved (Fig. 8B). Lowering [Ca²⁺]_o also induced a decline in CaMKII autonomous activity measuredin the in vitro kinase assay. This decline in enzyme activitycaused by preincubation in low [Ca²⁺]_o (50 nM Ca²⁺-PSS) was reversed significantly within 5 sec of switching to1.2 mM Ca²⁺ (p < 0.001; ANOVA; n = 36 dishes) (Fig. 8C). Moreover, the enzymemaintained a prolonged autonomous activity at 1.2 mM [Ca²⁺]_o for up to 30 min. This is consistent with the high level ofautonomous activity observed in unstimulated neurons in culture.

View larger version (28K):
[in this window]
[in a new window]
Figure 8. Autophosphorylation of CaMKII at Thr-286 was reduced in DRG neurons in low extracellular concentration of Ca²⁺. A, DRG neurons were changed to low calcium (50 nM Ca²⁺-PSS) for 1 hr before switching to normal calcium concentration (1.2 mM Ca²⁺-PSS) for 45 sec. Lysates were analyzed by immunoblotting with an antibody recognizing the phospho-Thr-286 CaMKII. Each lane represents data from a single neuronal culture. Two replicate experiments of three cultures per treatment (12 cultures total) are shown, in which neurons were either incubated in 50 nM Ca²⁺ for 1 hr (Low Ca²⁺) or switched from this low-Ca²⁺ solution to 1.2 mM Ca²⁺ (Normal Ca²⁺) for 45 sec. The same volume of lysate was analyzed for both phospho- and total-CaMKII immunoreactivity. B shows the normalized relative immunoreactivity of Thr-286 CaMKII in low and normal [Ca²⁺]. Data are mean ± SEM (n = 8 dishes). *Significantly different from neurons equilibrated at low [Ca²⁺]_o (p = 0.0004; t test). C, The autonomous activation of CaMKII is rapid and persistent in DRG neurons equilibrated in low [Ca²⁺]_o and switched into 1.2 mM Ca²⁺. Cultured neurons exposed to 50 nM Ca²⁺ for 1 hr were switched to 1.2 mM Ca²⁺-PSS for 5, 15, and 45 sec and 10 and 30 min before lysis. Data are mean ± SEM from two separate experiments of equal sample size. Autonomous activity ratio (Ca²⁺-independent/total) was calculated for each dish. *The level of activation is significantly different from neurons equilibrated in 50 nM Ca²⁺-PSS (p = 0.001; ANOVA; n = 36 dishes). Note that changes in extracellular calcium concentration did not alter intracellular calcium levels measurably (Fig. 9).

Calcium imaging was used to determine if these changes in [Ca²⁺]_o altered the level of free calcium in the cell body. No measurablealterations in [Ca²⁺]_i were detected when the [Ca²⁺]_o was either lowered to 50 nM from 1.2 mM or raised to 1.2 mMfrom 50 nM (Fig. 9). In contrast, brief electrical stimulationat 10 Hz, depolarization with 90 mM KCl, or calcium ionophorecaused large increases in [Ca²⁺]_i in these same neurons, validating the measurement method (Fig.9). This would be consistent with minimal transmembrane Ca²⁺ leak currents in unstimulated DRG neurons and a lack of spontaneoussynaptic activity.

View larger version (28K):
[in this window]
[in a new window]
Figure 9. Changes in concentration of extracellular Ca²⁺ that affect CaMKII autophosphorylation produced no detectable change in intracellular concentration in DRG neurons. A, Action potentials induced by brief electrical stimulation (10 Hz) caused a large increase in intracellular calcium as measured with fluo-3 fluorescence in time-lapse confocal microscopy. After intracellular calcium concentration recovered to basal levels, the extracellular calcium concentration was lowered from 1.2 mM Ca²⁺ to 50 nM Ca²⁺ using a rapid bath perfusion system (Low Ca²⁺). The intracellular calcium concentration was not altered significantly (a), and remained constant over the next 25 min (b). Electrical stimulation produced no change in intracellular calcium in low calcium conditions (b, inset, 10 Hz), indicating that the change to low extracellular calcium concentration by perfusion of 50 nM Ca²⁺ solution had been effective. After then returning extracellular calcium concentration to 1.2 mM (Ca²⁺ stim), intracellular calcium concentration remained constant for the next 40 min (b, inset). Calcium ionophore A23187 applied at the end of the experiment (*) caused a large increase in intracellular calcium, demonstrating the efficacy of the measurement technique. B, Similar results were obtained using the ratiometric calcium indicator indo-1, to correct for decreasing fluorescence caused by photobleaching in prolonged recordings and to obtain a quantitative estimate of changes in intracellular calcium. Brief 10 Hz stimulation or depolarization with 90 mM KCl caused large increases in intracellular Ca²⁺ concentration, but intracellular Ca²⁺ levels remained constant after lowering extracellular Ca²⁺ concentration from 1.2 mM to 50 nM or increasing extracellular Ca²⁺ from 50 nM to 1.2 mM (Ca²⁺ stim). Results shown are mean ± SEM; n = 8 neurons in A and 13 neurons in B. Although extracellular Ca²⁺ stimulation did not alter intracellular calcium measurably, the changes in extracellular calcium caused large changes in autonomous activity of CaMKII (Fig. 8).

The results indicate that mechanisms linked to the [Ca²⁺]_o in nonsynaptic regions of the neuron are responsible for the highlevel of CaMKII autonomy and autophosphorylation under basal conditions,rather than effects dependent on synaptic activity or changesin [Ca²⁺]_i. This is further supported by experiments showing that CaMKIIautonomous activity was not different in cultures exposed to 1µM TTX for 1 hr (0.26 ± 0.013; n = 8 dishes; mean ± SD) versusunstimulated cultures (0.28 ± 0.068; n = 36dishes).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

These are the first measurements of the frequency response of CaMKII decoding in neurons. The autonomous activity of the enzymehas been tested in response to a natural stimulus generating intracellularcalcium fluxes. This approach allows examination of the enzymeunder conditions that simulate the natural environment, a necessarystep in understanding the frequency decoding properties of CaMKII.The results indicate that the spike frequency decoding by CaMKIIautonomous activation is limited to action potential frequenciesof <1 Hz and >0.1 Hz. These findings are consistent with the behaviorof the enzyme in vitro to Ca²⁺ pulses of different frequencies (De Koninck and Schulman, 1998).The in vitro studies indicated that a sharper threshold for frequencydecoding by CaMKII is promoted by shorter duration Ca²⁺ pulses, lower free CaM concentration, and isozymes with higheraffinity for CaM (De Koninck and Schulman, 1998). The physiologicalconditions in DRG neurons would modulate the frequency responseof CaMKII toward higher levels of activation in response to low-frequencystimulation. Frequency decoding of CaMKII- $alpha$ is reported to be<1-3Hz for Ca²⁺ pulses >300 msec in duration (approximately the duration of acalcium transient induced by an action potential in DRG neurons);and partial autophosphorylation of the kinase shifts the levelof autonomy to near maximal levels in response to low-frequencystimulation. CaMKII was highly autophosphorylated in unstimulatedDRGneurons.

The high levels of autonomous activity of CaMKII in DRG neurons in the basal state are consistent with previous studies onother preparations (Molloy and Kennedy, 1991). This was attributedto low-frequency spontaneous synaptic activity, but the presentstudies show that synaptic activity is not essential for maintainingthe highly autophosphorylated state of CaMKII in basal conditions,because this preparation lacks synapses. Spontaneous action potentialactivity also does not appear to be responsible for the high autophosphorylatedstate in unstimulated conditions, because the DRG neurons arenot spontaneously active in vitro, and treatment with TTX didnot lower the CaMKII autonomous activity. However, the [Ca²⁺]_o strongly modulated this critical property of theenzyme.

The mechanism for the link between extracellular calcium and high levels of CaMKII autophosphorylation is unknown, but [Ca²⁺]_i imaging shows that it is not associated with measurable changesin [Ca²⁺]_i. Regulation of phosphatases, calmodulin-binding proteins, andkinase activity linked to the [Ca²⁺]_o are reasonable mechanisms. These studies indicate that theprocesses responsible for the effect of extracellular Ca²⁺ on CaMKII autonomy are not limited to specialized subsynapticcompartments, as had been assumed, because this preparation lackssynapses.

Conditions may exist in specialized cellular compartments to maintain the enzyme at a lower level of autophosphorylation,which would permit the enzyme to decode higher frequencies ofstimulation. It is possible that the kinetics of Ca²⁺ transients are more rapid in microdomains beyond the resolutionof confocal measurements. Shorter duration Ca²⁺ pulses would permit the kinase to exhibit a sharper frequency-dependentactivation in association with activity-dependent functions, suchas synaptic plasticity. Greater spatial heterogeneity and compartmentalizationwould be provided by neurons that are morphologically more complexthan DRG neurons, which lack dendrites and dendritic spines. Inthis regard, local phosphatase activity could have a significantinfluence on the frequency-response ofCaMKII.

CaMKII autonomous activity declined to near baseline with longer stimulation (>1 min) at higher frequencies. This could resultfrom stimulus failure, loss of total CaMKII activity, phosphorylationof an inhibitory site, e.g., Thr-305/306 (Patton et al., 1990;Dosemeci and Albers, 1993; Coomber, 1998), or increased phosphataseactivity. There is no evidence of stimulus failure, because [Ca²⁺]_i remained elevated throughout the stimulus period, and anotherkinase (extracellular signal regulated kinase) exhibited increasedphosphorylation under these conditions (Eshete and Fields, unpublisheddata). No decrease in total CaMKII activity was observed on immunoblotsor activity assays in lysates from neurons stimulated 10 min at10 Hz or (data not shown). This suggests that phosphatases maybe activated by prolonged stimulation. Previous studies have shownthat electroconvulsive treatment causes dephosphorylation of CaMKIIat Thr-286 in rat hippocampus and cortex (Yamagata and Obata 1998).The spike frequency decoding by CaMKII could be modulated by regulationof phosphatases in response to longer duration action potentialfiring. The effects of phosphatase activity on spike frequencydecoding by CaMKII autonomous activity has been incorporated insome mathematical models (Dupont and Goldbetter, 1992; Matsushitaet al., 1995, Coomber, 1998; Holmes, 2000).

An important finding of the present study is that the kinetics of Ca²⁺ transients in these neurons induced by trains of action potentialswere markedly different from the Ca²⁺ pulses that exhibited strong frequency decoding in experimentsusing pulsed perfusion of calcium solutions in vitro (De Koninckand Schulman, 1988). The cytoplasmic Ca²⁺ transient in these neurons lasts ~300 msec or longer after singleaction potentials. This makes the amplitude and duration of thecalcium response highly dependent on action potential firing frequency.The Ca²⁺ transient measured in the cell body of DRG neurons evoked byelectrically elicited action potentials persisted well beyondthe stimulus period; ~1 min after 15 sec of 1 Hz stimulation and4 min after 15 sec of 10 Hz stimulation (Fig. 3B,C). These sustainedincreases in intracellular calcium may influence other calcium-dependentprocesses, possibly including phosphatase activity, that mightinteract with phosphorylation of certain CaMKII substrates. Ifthere are substrates of CaMKII that are selectively regulatedby higher frequencies of action potentials, the present findingssuggest that this would occur only in local submembrane regionssurrounding Ca²⁺-permeable channels or in specialized compartments, such as dendriticspines, because the Ca²⁺ transients induced by action potentials may only have temporaldynamics that are appropriate for high frequency-dependent decodingby CaMKII autonomy in microscopic domains beyond the limits ofcurrentmeasurements.

The correlation with Ca²⁺ pulse frequency, not simply the [Ca²⁺]_i suggests that time-dependent processes, such as the kineticsof CaM dissociation, phosphorylation of regulatory and inhibitorysites on the enzyme, and activation of phosphatases cooperatein regulating the level of autonomous activation induced by actionpotential firing patterns. Such time-dependent effects on CaMKIIregulation would appear to allow more robust responses to dynamicstimulation than would be afforded by simple dependence on calciumconcentration in equilibrium reactions. In combination with concentration-dependentforms of regulation, these time-dependent regulatory effects maybe essential in transducing the information contained in the temporalpattern of neuronal membrane depolarization into intracellularsignaling reactions that control the appropriate neuronalresponse.

Thus, CaMKII could participate in decoding action potentials at a frequency <1 and >0.1 Hz in these neurons. This may be importantduring development when neurons generate low-frequency burstsof action potentials spontaneously (Fields, 1998). This is nota favorable mechanism for regulating activity-dependent responsesin these neurons in the range of 1-10 Hz. The specific activationof genes and other functional responses of DRG neurons that havebeen observed in response to appropriate frequencies of actionpotentials at frequencies >1 Hz are either dependent on localizedresponses of CaMKII beyond the limits of the present measurementtechniques or they may involve other frequency-decoding intracellularsignaling mechanisms, such as temporal integration within intracellularsignaling networks (Fields, 1996; Fields et al., 1997, 2001).

  FOOTNOTES

Received Dec. 13, 2000; revised May 31, 2001; accepted June 8, 2001.

This work was supported by the National Institute of Child Health and Human Development. We thank B. Stevens for providingthe cultures of DRG neurons and Dr. Yoko Yamagata for the phosphosite-specificantibodies used in thestudy.
Correspondence should be addressed to Dr. R. Douglas Fields, Head, Neurocytology and Physiology Unit, National Institutesof Health, National Institute of Child Health and Human Development,Laboratory of Cellular and Synaptic Neurophysiology, 49 ConventDrive, Building 49, Room 5A78, Bethesda, MD 20892-4480. E-mail:fields{at}helix.nih.gov.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Bayer K-U, Lohler J, Schulman H, Harbers K (1999) Developmental expression of the CaM kinase II isoforms: ubiquitous $gamma$ - and $delta$ -CaM kinase II are the early isoforms and most abundant in the developing nervous system. Mol Brain Res 70:147-154[Medline].
Brocke L, Chiang LW, Wagner PD, Schulman H (1999) Functional implications of the subunit composition of neuronal CaM Kinase II. J Biol Chem 274:22713-22722[Abstract/Free Full Text].
Colegrove SL, Albrecth MA, Friel DD (2000) Quantitative analysis of mitochondrial C12+ uptake and release pathways in sympathetic neurons. Reconstruction of the recovery after depolarization-evoked [Ca²⁺]_i elevations. J Gen Physiol 115:347-350[Free Full Text].
Coomber CJ (1998) Site-selective autophosphorylation of Ca²⁺/calmodulin-dependence protein kinase II as a synaptic encoding mechanism. Neura