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The Journal of Neuroscience, August 15, 2002, 22(16):7016-7026

Spatial and Temporal Regulation of Ca²⁺/Calmodulin-Dependent Protein Kinase II Activity in Developing Neurons

Andrea Menegon¹, Claudia Verderio², Chiara Leoni¹, Fabio Benfenati³, Andrew J. Czernik⁴, Paul Greengard⁴, Michela Matteoli², and Flavia Valtorta¹

¹ Department of Neuroscience, S. Raffaele Scientific Institute and "Vita-Salute" University, 20132 Milano, Italy, ² Department of Medical Pharmacology, Consiglio Nazionale delle Ricerche Cellular and Molecular Pharmacology Center, 20129 Milano, Italy, ³ Department of Experimental Medicine, Section of Physiology, University of Genova, 16132 Genova, Italy, and ⁴ Laboratory of Molecular Cellular Neuroscience, The Rockefeller University, New York, New York 10021

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

We have studied Ca²⁺/calmodulin-dependent protein kinase II (CaMKII) isoform distribution and activity in embryonic hippocampal neurons developing in culture. We have found a strong correlation between the expression of the  subunit of the enzyme and the ability to undergo depolarization-dependent phosphorylation, which in young neurons is limited to the somatodendritic pool of the kinase. The lack of responsiveness of the axons of young CaMKII-positive neurons is not caused by a lower Ca²⁺ influx but rather by a differential balance between kinase and phosphatase activities in this compartment. After the establishment of synaptic contacts, the presynaptic pool of the kinase displays an increasing level of activity and acquires the parallel ability to phosphorylate synapsin I, which represents one of the major CaMKII presynaptic targets in mature nerve terminals. In contrast, the activity of the postsynaptic pool of the kinase remains constant throughout synaptogenesis. In the presence of a nearly homogeneous subcellular distribution, this highly regionalized regulation of activity may reflect the multifunctional roles of CaMKII in both developing and mature neurons.

Key words: protein phosphorylation; neuronal differentiation; synapse; phosphospecific antibodies; hippocampal neurons; synapsin

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The multifunctional serine/threonine kinase Ca²⁺/calmodulin-dependent protein kinase II (CaMKII) is highly concentrated in the brain, where it accounts for 1-2% of total protein (Kennedy et al., 1983; Kelly et al., 1984; McGuinness et al., 1985) and phosphorylates several substrates that are involved in the modulation of neuronal excitability and neurotransmission (Soderling, 2000). The elucidation of the biochemical properties of CaMKII has provided evidence that brief [Ca²⁺]_i signals can activate the kinase and stimulate an autophosphorylation reaction, resulting in the generation of long-lasting, Ca²⁺-independent autonomous activity (Lai et al., 1986; Miller et al., 1986). These features support a role for CaMKII as a memory molecule coupled to Ca²⁺ signaling in neurons (Lisman, 1994; Braun and Schulman, 1995; Soderling, 2000).

At the synapse, CaMKII has been localized both presynaptically and postsynaptically and has been implicated in specific functions related to plasticity phenomena (Stevens et al., 1994; Mayford et al., 1995; Lisman et al., 1997). At the postsynaptic level, it has been involved in the stabilization of the dendritic arbor structure (Wu and Cline, 1998), in modulation of dendritic exocytosis (Maletic-Savatic et al., 1998), in Ca²⁺-dependent facilitation of L-type Ca²⁺ channels (Dzhura et al., 2000), and in the regulatory phosphorylation of AMPA- and NMDA-type glutamate receptors (Barria et al., 1997; Gardoni et al., 2001). Furthermore, a functional role of the kinase in this subcellular compartment was suggested by the observation that exogenous CaMKII translocates from the dendritic shaft to the postsynaptic density after NMDA receptor stimulation (Shen and Meyer, 1999).

At the presynaptic level, a fraction of CaMKII was shown to be present on the synaptic vesicle (SV) membrane (Benfenati et al., 1992, 1996), and its activity was proposed to regulate the efficiency of neurotransmitter release, via phosphorylation of the SV-associated protein synapsin I (Greengard et al., 1993).

Much less is known about CaMKII function during neuronal differentiation. Expression of the kinase is developmentally regulated (Hanson and Schulman, 1992), and the enzyme has been implicated in the control of neuronal growth and synaptogenesis (Zou and Cline, 1996). Furthermore, results obtained by expressing constitutively active forms of the kinase indicate that CaMKII plays a role in the developmental program of central glutamatergic synapses, as well as in determining their density (Wu et al., 1996; Rongo and Kaplan, 1999).

The observation that neuronal [Ca²⁺]_i signals can be extremely localized and that CaMKII activation has specific functions in distinct subcellular compartments prompted us to investigate the processes underlying the targeting and activation of CaMKII during the development of hippocampal neurons in culture.

To monitor the topographic activation of CaMKII in developing neurons, we took advantage of phosphorylation state-specific antibodies, recognizing either the autophosphorylated kinase or synapsin I specifically phosphorylated by CaMKII (Czernik et al., 1991; Menegon et al., 2000). Our results show that CaMKII can be subdivided into distinct functional pools that are differentially activated during neuronal development.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Materials. The anti-synapsin I/II (clone 19.11) mouse monoclonal antibody and anti-/CaMKII (RU16), anti-phosphoCaMKII (RU48), and phosphosite-3-specific anti-synapsin I (RU19) rabbit polyclonal antibodies were prepared and characterized at The Rockefeller University (New York, NY) (Czernik et al., 1991; Benfenati et al., 1992, 1996; Vaccaro et al., 1997; Menegon et al., 2000). Conjugation of the RU19 antibody with the fluorescent dye Cy3 and purification of the labeled antibodies were performed with the FluoroLink Cy3 kit and the Hitrap affinity column (Amersham Biosciences, Buckinghamshire, UK) according to the manufacturer's instructions.

The following antibodies were purchased from the indicated sources: anti-CaMKII-specific (clone 6G9) mouse monoclonal antibody (Affinity Bioreagents, Golden, CA); anti-CaMKII-specific (clone CB-1) mouse monoclonal antibody (Zymed, San Francisco, CA); anti-tau-1 antibody (Boehringer Mannheim, Mannheim, Germany); peroxidase-conjugated goat anti-rabbit and goat anti-mouse antibodies (Bio-Rad, Hercules, CA); FITC-conjugated goat anti-mouse, tetramethylrhodamine isothiocyanate-conjugated goat anti-rabbit, FITC-conjugated donkey anti-rabbit, 7-amino-4-methylcoumarin-3-acetic acid-conjugated donkey anti-mouse, and pure rabbit IgG antibodies (Jackson ImmunoResearch, West Grove, PA). The enhanced chemiluminescence detection system was from Amersham Biosciences, and the BCA protein assay reagent was from Pierce (Rockford, IL). Ionomycin, norokadaone, okadaic acid (OA), and cyclosporin A were from Calbiochem (La Jolla, CA). All chemicals were of the highest grade available.

Cell cultures. Low-density primary cultures of hippocampal neurons were prepared from embryonic day 18 rat embryos (Charles River, Calco, Italy), essentially as described previously (Banker and Cowan, 1977; Verderio et al., 1999a). Hippocampi were dissociated by a 15 min incubation with 0.25% trypsin at 37°C, and cells were plated at a density of 20,000-30,000/cm² on poly-L-lysine (1 mg/ml)-treated glass coverslips in MEM (Invitrogen, San Giuliano Milanese, Italy), supplemented with 10% horse serum (Hyclone, Logan, UT), 2 mM glutamine (Biowhittaker, Ververs, Belgium), and 3.3 mM glucose. After allowing neurons to adhere to the substrate for 3-4 hr, coverslips were transferred to dishes containing a monolayer of cortical astrocytes (Booher and Sensenbrenner, 1972), without physical contact between neurons and glial cells. Cells were then maintained in serum-free MEM supplemented with 1% N2 supplement (Invitrogen), 2 mM glutamine (Biowhittaker), 0.1% ovalbumin (Sigma, St. Louis, MO), 4 mM glucose, and 1 mM sodium pyruvate.

Primary cultures of cerebellar granule neurons were prepared from postnatal day 5 rats (Charles River) as described previously (Gallo et al., 1987; Menegon et al., 1997). To favor neuronal survival and prevent glial cell proliferation, the medium was supplemented 3 d after plating with 10 mM KCl and 7.5 µM cytosine-1--D-arabinofuranoside (Sigma).

Immunoblot analysis. Cerebellar granule neurons at 12 d in vitro (DIV) or hippocampal pyramidal neurons at 14 DIV were rapidly washed with Krebs-Ringer's solution buffered with HEPES (KRH; in mM: 150 NaCl, 5 KCl, 1.2 MgSO₄, 1.2 KH₂PO₄, 2 CaCl₂, 10 glucose, and 10 HEPES/Na, pH 7.4); supplemented with 2 mM EGTA; solubilized by scraping with solubilization buffer (1% SDS, 2 mM EDTA, and 10 mM HEPES/Na, pH 7.4); and immediately frozen in liquid nitrogen. After thawing, lysates were boiled for 3 min and sonicated. Equal amounts of protein were subjected to SDS-PAGE (Laemmli, 1970) and transferred to nitrocellulose as described previously (Towbin et al., 1979). Filters were blocked for 1 hr at room temperature in TBS (in mM: 150 NaCl and 100 Tris-Na, pH 7.5), supplemented with 5% nonfat dry milk, incubated for 2 hr with either anti-/CaMKII (RU16; 1:10,000) or phosphospecific anti-CaMKII (RU48; 1:5000) antibodies in TBS/milk, washed five times for 5 min with TBS/0.1% Triton X-100, incubated for 1 hr with a peroxidase-conjugated goat anti-rabbit antibody (1:10,000) in TBS/milk, washed five times for 5 min with TBS/0.1% Triton X-100, and finally developed by chemiluminescence. Digital images were obtained with a Speedy II scanner (Umax, Willich, Germany) and processed with the PhotoShop 5.0 program (Adobe Systems, San Jose CA).

Immunofluorescence analysis. Cells were quickly washed with KRH/EGTA and fixed for 30 min at 37°C in 4% formaldehyde (freshly prepared from paraformaldehyde) dissolved in 120 mM sodium phosphate buffer (pH 7.4) supplemented with 4% sucrose and 4 mM EGTA. After washing three times for 10 min in PBS (in mM: 180 NaCl and 10 Na-phosphate buffer, pH 7.4), cells were incubated with antibodies at the appropriate concentrations in goat serum dilution buffer (in mM: 450 NaCl and 20 sodium phosphate buffer, pH 7.4, 15% goat serum, and 0.3% Triton X-100). Between successive incubations with antibodies, cells were washed three times for 10 min in a high salt buffer (in mM: 500 NaCl and 20 mM sodium phosphate buffer, pH 7.4). After the standard double-labeling protocol, in some instances, Cy3-conjugated phosphosite-3-specific anti-synapsin I antibody (RU19) was added. Incubation with the conjugated antibody was performed in the presence of 10 µg/ml rabbit IgG and was preceded by a 20 min blocking reaction in the same solution.

After the final incubation, cells were washed three times in high salt buffer, once in PBS, and finally once in 5 mM sodium phosphate buffer, pH 7.4. Coverslips were mounted with 70% glycerol in PBS supplemented with phenylenediamine (1 mg/ml; Sigma) as an anti-bleaching agent and viewed with a Zeiss (Oberkochen, Germany) Axiovert 135 inverted microscope equipped with epifluorescence and differential interference contrast (DIC) optics. Images were taken with a high-resolution Hamamatsu (Shizuoka, Japan) Orca-II digital camera and processed with the Adobe PhotoShop 5.0 program; DIC images were filtered with the Image Pro plus program (Media Cybernetics, Silver Spring, MD).

fura-2 videomicroscopy. Neurons were loaded for 1 hr with 5 µM fura-2 pentacetoxy-methylester in KRH at 37°C, washed three times for 10 min in the same solution without fura-2 to allow de-esterification of the dye, and transferred to the recording chamber of a Zeiss Axiovert 100 inverted microscope equipped with a Ca²⁺ imaging unit using a modified CAM-230 dual-wavelength Jasco (Tokyo, Japan) microfluorimeter as a light source. Experiments were performed at room temperature using the Axon Imaging Workbench 2.2 equipped with a Personal Computer Optics (Computer Optics GmBH, Kelheim, Germany) Super Video Graphics Array SensiCam (Axon Instruments, Foster City, CA). Images were acquired at 0.5-1 340/380 ratios/sec, and ratio values in discrete areas of interest were calculated from sequences of images to obtain temporal analyses. At the end of the experiments, the imaged fields were marked using a diamond-tipped objective, and cells were fixed and processed for immunofluorescence (Pravettoni et al., 2000).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Characterization of the phosphospecific anti-CaMKII antibody

To characterize the phosphospecific anti-CaMKII antibody (RU48), rat cerebellar granule neurons were lysed either under control conditions or after exposure to KCl (55 mM) for 1 min in the absence or presence of EGTA (2 mM). Immunoblot analysis with an anti-/CaMKII (RU16) antibody revealed the presence of two prominent 58-60 kDa bands, corresponding to the /' isoforms of CaMKII and of a minor 50 kDa band corresponding to the  isoform of the kinase (Fig. 1A). These results are consistent with the low levels of CaMKII expression observed in homogenates of rat cerebellum (McGuinness et al., 1985). Both the  and the /' isoforms underwent phosphorylation after depolarization of the cells in the presence of extracellular Ca²⁺, as revealed by labeling with the phosphospecific anti-CaMKII antibody (RU48).

View larger version (31K): [in this window] [in a new window]   Figure 1.   Characterization of the anti-phosphoCaMKII antibody. A, B, Western blot analysis of the specificity of the anti-phosphoCaMKII antibody. Cerebellar granule neurons at 12 DIV (A) or embryonic hippocampal neurons at 14 DIV (B) were lysed under control conditions (KRH) or after exposure to KCl (55 mM) for 1 min either in the absence or in the presence of EGTA (2 mM). Equal amounts of protein were loaded into each lane. Parallel samples were probed with either an anti-/CaMKII (CaMKII) or the phosphospecific anti-CaMKII (P-CaMKII) antibody. C, Immunocytochemical analysis of the specificity of the anti-phosphoCaMKII antibody. Embryonic hippocampal neurons at 21 DIV, treated as in B, were fixed and processed by double immunofluorescence with anti-CaMKII (left) and phosphospecific anti-CaMKII (right) antibody. Note the Ca2+-dependent labeling of phosphorylated CaMKII after depolarization. Scale bar, 20 µm.

In hippocampal neurons at 14 DIV, the  isoform was relatively more abundant, although it represented a minor fraction of the total kinase (Fig. 1B) and appeared to be preferentially phosphorylated after depolarization. Consistent results were obtained by immunofluorescence analysis of rat cerebellar granule (data not shown) or hippocampal (Fig. 1C) neurons after fixation of the cells under the same conditions.

Developmental analysis of CaMKII expression and phosphorylation in embryonic hippocampal neurons in culture

CaMKII is characterized by regional and developmental variations in concentration and isoform ratio in the brain, consistent with a highly regulated role in neuronal function (Hanson and Schulman, 1992). Therefore, we analyzed the cellular distribution of the  and  CaMKII isoforms in rat embryonic hippocampal neurons developing in culture, using isoform-specific antibodies (Fig. 2A,B). Although CaMKII was already present at early stages of development and was ubiquitously and homogeneously distributed in all cells, CaMKII was characterized by a regulated developmental expression. Indeed, it was not expressed by stage I-II cells (i.e., neurons with short, unpolarized processes), starting to be expressed by a fraction (13%) of stage III neurons (i.e., neurons with an identifiable axon). The proportion of CaMKII-positive neurons progressively increased during development (40% of stage IV neurons; i.e., neurons in the phase of dendritic outgrowth) to approach the entire population (97%) of mature, stage V neurons. As observed in the case of CaMKII, in CaMKII-positive stage III neurons, the kinase displayed an apparently homogeneous distribution, with no particular enrichment in any subcellular compartment.

View larger version (19K): [in this window] [in a new window]   Figure 2.   Morphological analysis of CaMKII isoform expression and phosphorylation in stage III embryonic hippocampal neurons in culture. A, Hippocampal slices were lysed under control conditions and probed by immunoblotting with either anti-/ (RU16) or - or -specific anti-CaMKII antibodies. B, B', Stage III embryonic hippocampal neurons were fixed under control conditions and processed by double immunofluorescence with anti-/CaMKII antibody (red) and either anti-CaMKII (B) or anti-CaMKII (B') antibodies (green). C, Stage III embryonic hippocampal neurons were exposed for 1 min to KCl (55 mM), fixed, and processed for double immunofluorescence with anti-CaMKII (green) and anti-phosphoCaMKII (red) antibodies. D, Neurons treated as in C were processed for double immunofluorescence with anti-tau-1 (green) and anti-phosphoCaMKII (red) antibodies. The arrowheads in C and D point to the axon, which is virtually devoid of labeling for phosphoCaMKII. Scale bar, 20 µm.

After exposure to depolarizing agents, a prominent phosphorylation of the kinase was apparent in the fraction of cells that corresponded at all stages exactly to the CaMKII-positive neurons. Phosphorylation of the kinase was confined to the somatodendritic compartment, whereas the axon (identified by staining with antibodies to the axonal protein tau-1) was negative, despite the presence of the protein (Fig. 2C,D).

View larger version (23K): [in this window] [in a new window]   Figure 5.   Analysis of CaMKII and synapsin I phosphorylation in stage III neurons treated with ionomycin in either physiological or high [Ca2+]o. A, Stage III neurons were exposed to ionomycin (1 µM) in either physiological (2 mM) or high (10 mM) [Ca2+]o for 2 min, fixed, and either double-labeled with anti-CaMKII (top panels) and phosphospecific anti-CaMKII (P-CaMKII; middle panels) antibodies or labeled with a phosphospecific anti-synapsin I antibody (P-Syn; bottom panels). The phosphosynapsin staining is superimposed to the corresponding DIC image to visualize the axonal compartment. Note the prominent CaMKII phosphorylation in the high [Ca2+]o protocol, where phosphorylation of the kinase can be seen also in the axonal compartment (arrows) and in CaMKII-negative cells (arrowheads). Under this condition, the CaMKII presynaptic substrate synapsin I also undergoes phosphorylation. Scale bar, 20 µm. B, Temporal analysis of fura-2 F340:380 ratio values measured in the cell body, dendrite, and axon of representative cells exposed sequentially to KCl (55 mM) in 2 mM [Ca2+]o and then to ionomycin (IONO; 1 µM) in either physiological (2 mM, left) or high (10 mM, right) [Ca2+]o. C, Analysis of peak fura-2 F340:380 ratio values (difference from basal ratio values, F340:380) measured in cell bodies of neurons after exposure to the following stimulating protocols: ionomycin (1 µM) in physiological (2 mM) [Ca2+]o for 2 min, KCl (55 mM) for 1 min, and ionomycin (1 µM) in high (10 mM) [Ca2+]o for 2 min. Bars represent means ± SD with n = 10 cells/condition. For the KCl-treated sample, the mean value is calculated on -positive, responsive neurons, whereas the average value calculated on the entire population is 0.51 ± 0.22 (n = 46 cells).

Analysis of the role of Ca²⁺ in CaMKII activation

Depolarization-induced Ca²⁺ influx and CaMKII activation in stage III hippocampal neurons were monitored by fura-2 Ca²⁺ imaging, followed by retrospective double immunofluorescence with anti-CaMKII and phosphospecific anti-CaMKII antibodies. Figure 3 shows an example of these experiments. The temporal analysis of depolarization-induced [Ca²⁺]_i variations in the neuronal cell bodies showed similar kinetics but different peak levels in the various cells. CaMKII phosphorylation was apparent only in those cells expressing the  isoform of CaMKII, regardless of the [Ca²⁺]_i levels reached.

View larger version (35K): [in this window] [in a new window]   Figure 3.   Analysis of Ca2+ influx in phosphoCaMKII-positive and -negative stage III neurons. A, B, Time-resolved (A) and space-resolved (B) analysis of [Ca2+]i dynamics in stage III embryonic hippocampal neurons loaded with fura-2 and treated with KCl (55 mM) for 1 min. The image shown in B corresponds to the peak of [Ca2+]i in A. C, Retrospective double immunofluorescence with anti-CaMKII (green) and phosphospecific anti-CaMKII (red) antibodies of the cells in the field shown in B. Scale bar, 10 µm. Note that the [Ca2+]i levels in one of the phosphoCaMKII-negative cells (1) are higher than those reached in the phosphoCaMKII-positive, CaMKII-expressing cell (2).

The lack of CaMKII phosphorylation in the axons of CaMKII-positive neurons was not caused by lower [Ca²⁺] levels reached after depolarization in this compartment. Figure 4 shows a time-resolved analysis of [Ca²⁺]_i variations in single neurons. The [Ca²⁺]_i levels reached in the axon after exposure to KCl were similar to those reached in the dendritic compartment of the same cell, whereas phosphorylation of the kinase was apparent only in the cell body and proximal dendrites.

View larger version (34K): [in this window] [in a new window]   Figure 4.   Analysis of Ca2+ influx in the axonal and dendritic compartments of CaMKII-expressing stage III neurons. A, B, Time-resolved (A) and space-resolved (B) analysis of [Ca2+]i dynamics in the processes of a neuron treated and analyzed as described in the legend to Figure 3. Traces in A refer to the color-coded spots marked in B. C, Retrospective immunofluorescence with phosphospecific anti-CaMKII antibody of the cell shown in B. Note the similar [Ca2+]i levels reached after depolarization in the phosphoCaMKII-positive dendrites and in the phosphoCaMKII-negative axon. Scale bar, 10 µm.

To determine whether the observed pattern of CaMKII activation was specifically coupled to Ca²⁺ influx through voltage-gated channels, stage III neurons were exposed to ionomycin (1 µM) for 2 min in the presence of either physiological (2 mM) or high (10 mM) [Ca²⁺]_o. Although virtually no CaMKII phosphorylation could be observed in the presence of 2 mM [Ca²⁺]_o, regardless of the expression of the  isoform, a prominent and diffuse phosphorylation of CaMKII was apparent in the presence of 10 mM [Ca²⁺]_o, in both CaMKII-positive and -negative cells. Furthermore, using the high [Ca²⁺]_o protocol, the kinase also underwent phosphorylation in the axonal compartment (Fig. 5A, top and middle panels).

This observation prompted us to analyze phosphorylation of the CaMKII substrate synapsin I in the axon, using a previously characterized phosphosite-3-specific antibody directed against Ser⁶⁰³ of synapsin I, phosphorylated by CaMKII (Menegon et al., 2000). Exposure of neurons to ionomycin (1 µM) for 2 min in the presence of 10 mM [Ca²⁺]_o caused a strong and specific phosphorylation of synapsin I (Fig. 5A, bottom panels). In contrast, labeling for phosphosynapsin I was not observed after exposure to ionomycin in the presence of 2 mM [Ca²⁺]_o or after exposure to depolarizing agents (data not shown), as expected by the lack of axonal CaMKII activation.

The distinct responses in terms of CaMKII phosphorylation to the various experimental protocols (depolarizing agents, ionomycin in the presence of physiological or high [Ca²⁺]_o) were related to the different peak levels of [Ca²⁺]_i, as shown by measuring the mean difference between basal and peak ratio values (F340/380) of the fura-2 signal in the cell bodies. The results showed that the cells treated with ionomycin in high [Ca²⁺]_o reached a peak [Ca²⁺]_i, which was approximately threefold higher than that reached in physiological [Ca²⁺]_o. Intermediate levels of [Ca²⁺]_i were reached in the case of neurons treated with KCl, with higher levels in the case of the responsive -positive cells (Fig. 5C).

Single-cell temporal analyses were performed to compare the relative [Ca²⁺]_i levels reached after depolarization in the various subcellular compartments (soma, axon, and dendrites) with those reached after exposure to ionomycin in either physiological or high [Ca²⁺]_o. The traces indicated that, in the case of the high [Ca²⁺]_o protocol, the axonal compartment reached higher [Ca²⁺]_i levels than under the other experimental conditions both in terms of peak levels (Fig. 5B) and in terms of the of total amount of Ca²⁺ influx, as evaluated by comparison of the integrals under the curves (data not shown).

Effect of phosphatase inhibitors on the state of phosphorylation of axonal CaMKII

In principle, the failure to reveal a depolarization-dependent increase in the state of phosphorylation of CaMKII in the axons of stage III neurons might be attributable either to a lack of activation of the kinase or to a high level of phosphatase activity in this compartment. To distinguish between these possibilities, neurons were treated with serine/threonine phosphatase inhibitors.

Virtually no immunolabeling for phosphoCaMKII could be detected in the axons of neurons stimulated with KCl after exposure to cyclosporin, a selective inhibitor of calcineurin (Fig. 6). In contrast, in the axons of neurons stimulated after exposure to OA, an inhibitor of protein phosphatase 2A (PP2A) and PP1, an intense labeling for phosphoCaMKII was evident. Under these conditions, in the same compartment, site 3 phosphorylation of synapsin I could also be detected. In neurons exposed to the OA-related, inactive compound norokadaone, depolarization failed to induce labeling for either phosphoCaMKII or site 3-phosphorylated synapsin I. 

View larger version (42K): [in this window] [in a new window]   Figure 6.   Effect of phosphatase inhibitors on the KCl-induced activation of CaMKII in stage III hippocampal neurons. Neurons were incubated for 10 min with KRH in the presence or absence of either OA (500 nM) or cyclosporin (10 nM) and successively stimulated for 2 min with 55 mM KCl. Double immunofluorescence was performed with either phosphospecific anti-CaMKII (P-CaMKII) and anti-CaMKII (top panels) or site 3 phosphospecific anti-synapsin I (P-Syn I) and anti-total synapsin (bottom panels). Arrowheads point to axons negative for phosphoCaMKII or phosphosynapsin I in cells stimulated with KCl in the presence or absence of cyclosporin; arrows point to axons positive for phosphoCaMKII or phosphosynapsin I in cells stimulated in the presence of OA. The inset in the top panel shows an CaMKII-negative cell in which labeling for phosphoCaMKII was undetectable after KCl stimulation in the presence of OA. Scale bar, 20 µm.

The effect of OA was specific for the axons of CaMKII-positive cells: after KCl stimulation in the presence of OA, CaMKII-negative cells remained negative for phosphoCaMKII in all neuronal compartments.

Developmental organization of the presynaptic CaMKII/synapsin I complex

A preformed complex between CaMKII and synapsin I on the SV membrane has been proposed to participate in the regulation of neurotransmitter release from mature nerve terminals (Benfenati et al., 1992; Greengard et al., 1993).

In our model system, when neurons start to establish intercellular contacts (stage IV), the presynaptic pool of CaMKII and its phosphorylation were generally undetectable, because of the abundance of the adjacent postsynaptic pool. The low percentage of stage IV neurons responsive to K⁺ depolarization allowed us to directly assess phosphorylation of the presynaptic pool of the kinase, which could be visualized in neurons making synapses on CaMKII-negative cells. In those cases, presynaptic CaMKII appeared to be concentrated in varicosities and undergo phosphorylation (Fig. 7A). In the same synaptic boutons, phosphorylation of synapsin I, which becomes progressively enriched in the terminals undergoing maturation, could also be detected. Although synapsin I underwent phosphorylation in virtually all of the terminals after exposure of the cells to ionomycin in the presence of high [Ca²⁺]_o, only a fraction of the terminals appeared to be labeled with either ionomycin applied in physiological [Ca²⁺]_o or after K⁺ depolarization, suggesting heterogeneity in the state of maturation of the boutons (Fig. 7B). Interestingly, synapsin I phosphorylation could be detected only in presynaptic terminals possessing a postsynaptic counterpart, as assessed by DIC microscopy. Quantitative analysis performed on KCl-treated neurons demonstrated that the percentage of phosphosynapsin I-positive terminals, initially low, steadily increased over development, with the recruitment of virtually the entire population of mature synaptic boutons at 21 DIV (Fig. 8). However, the apparent stoichiometry of synapsin I phosphorylation varied markedly in the various synaptic terminals.

View larger version (90K): [in this window] [in a new window]   Figure 7.   Distribution and phosphorylation of presynaptic CaMKII and synapsin I in stage IV neurons. A, Stage IV embryonic hippocampal neurons were exposed for 1 min to KCl (55 mM) in the presence of 2 mM [Ca2+]o. Cells were then fixed and processed for triple immunofluorescence with phosphospecific anti-CaMKII (P-CaMKII; green), site 3 phosphospecific anti-synapsin (P-Syn I; red), and anti-vesicle-associated membrane protein-2 (VAMP-2; blue) antibodies. The presynaptic pool of the kinase can be visualized in axons of CaMKII-positive cells making contacts on CaMKII-negative neurons (asterisks). Note the white spots (arrowheads), corresponding to structures that stain positively for the three antibodies, identifying them as synaptic boutons in which phosphorylation of both CaMKII and synapsin I has occurred. B, Stage IV embryonic hippocampal neurons were exposed to either KCl (55 mM) for 1 min or ionomycin (1 µM) for 2 min in the presence of either physiological (2 mM) or high (10 mM) [Ca2+]o. Cells were then fixed and processed for double immunofluorescence with anti-synapsin (green, top panels) and phosphospecific anti-synapsin I (P-Syn I; red, bottom panels) antibodies. At this stage, synapsin labeling starts to be concentrated in varicosities. Although only a fraction of the synapsin pool appears to be phosphorylated after depolarization or exposure to ionomycin in physiological [Ca2+]o, the entire synapsin pool undergoes phosphorylation with the high [Ca2+]o protocol. The fluorescence labeling in B is superimposed to the corresponding DIC image. Scale bars: A, left panel, 20 µm; right panel, 1 µm; B, 12 µm.

View larger version (30K): [in this window] [in a new window]   Figure 8.   CaMKII-dependent synapsin I phosphorylation in stage V neurons. A, Stage V embryonic hippocampal neurons at 7, 14, or 21 DIV were exposed to KCl (55 mM) for 1 min, fixed, and processed for double immunofluorescence with anti-synapsin and site 3 phosphospecific anti-synapsin I (P-syn) antibodies. The histograms show the percentage of phosphosynapsin I-positive boutons (mean ± SD) at each stage. The number of phosphosynapsin I-positive boutons was normalized for the number of synapsin-positive presynaptic terminals present in each field. B, Representative immunofluorescence image of a 21 DIV neuron double-stained with anti-synapsin (green) and site 3 phosphospecific anti-synapsin I (red) antibodies. Scale bars: B, 10 µm; inset in B, 2 µm.

Exposure of the neurons to OA (but not to the related inactive compound norokadaone) before the depolarizing pulse strongly increased synapsin I phosphorylation at immature presynaptic terminals. Indeed, under these conditions, >80% of the synaptic boutons were labeled by phosphospecific antibodies to synapsin I already at 7 DIV (Fig. 9). In addition, in the phosphosynapsin I-positive boutons, the apparent stoichiometry of synapsin I phosphorylation was increased.

View larger version (34K): [in this window] [in a new window]   Figure 9.   Effect of phosphatase inhibitors on synapsin I phosphorylation in stage V neurons. A, Embryonic hippocampal neurons at 7 DIV were exposed for 10 min to KRH in the absence or presence of either OA (O.A.; 500 nM) or norokadaone (Nok; 500 nM). In the stimulated samples (KCl), 55 mM KCl was present during the last minute of the incubation. The samples were then fixed and processed for double immunofluorescence with anti-synapsin (Syn; left panels) and phosphospecific anti-synapsin I (P-syn I; right panels) antibodies. Scale bar, 10 µM. B, The percentage of phosphosynapsin I-positive boutons (mean ± SD) was calculated for all of the samples in A (n = 260-280, gray bars). In phosphosynapsin I-positive boutons, the average fluorescence intensity ratio between the signals for phosphosynapsin I and for total synapsins was also calculated (white bars).

Spatially heterogeneous activation of CaMKII in the somatodendritic compartment of mature neurons

Depolarization-induced phosphorylation of CaMKII in the somatodendritic compartment was apparently homogeneous in younger neurons. In contrast, in stage V neurons, two distinct and physically separated domains of activation of the kinase became apparent: a domain strongly and uniformly activated by depolarizing agents, represented by the neuronal cell body and proximal dendrites, and a distal domain (>20-30 µm from the cell body) characterized by the absence of activation in the dendritic shaft and by the presence of isolated spots of activation (Fig. 10). These spots were identified as postsynaptic spines, because they appeared to be always juxtaposed to synapsin-positive presynaptic terminals and were negative for MAP2 immunostaining.

View larger version (21K): [in this window] [in a new window]   Figure 10.   Postsynaptic CaMKII phosphorylation in stage V neurons. A, Stage V embryonic hippocampal neurons at 21 DIV were exposed to KCl (55 mM) for 1 min, fixed, and processed for double immunofluorescence with anti-synapsin (green) and phosphospecific anti-CaMKII (red) antibodies. B, C, High-magnification images of distal dendrites treated as in A and processed for double immunofluorescence with phosphospecific anti-CaMKII (red) and either anti-synapsin (B) or anti-MAP2 (C) antibodies (green). Note the absence of labeling for phosphoCaMKII in the dendritic shaft. The phosphoCaMKII-positive spots are always juxtaposed to synapsin-positive, presynaptic terminals and confined to MAP2-negative areas, defining them as spines. D, Size distribution of the phosphoCaMKII-positive areas in distal dendrites. The continuous red line represents the Gaussian fitting of the curve. E, Stage V embryonic hippocampal neurons at 7, 14, and 21 DIV were processed as in A. The histograms show the percentage of phosphoCaMKII-positive spines (mean ± SD) at each stage. The number of activated spines was normalized for the number of synapsin-positive presynaptic boutons present in each field. Scale bars: A, 6 µm; B, C, 2 µm.

Quantitative analysis of the surface area of the spots labeled in the distal region demonstrated that CaMKII activation remained confined to spines. Indeed, the histogram representing the classes of phosphoCaMKII-labeled areas was consistent with the reported size distribution of dendritic spines (Harris, 1999; Kennedy, 2000). The percentage of activated spines remained constant during development in culture, once normalized for the number of presynaptic boutons present in the field.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

CaMKII is a multifunctional protein kinase that represents a central element in neuronal signaling and a likely candidate as a Ca²⁺-sensing memory molecule. Several functions of the kinase are associated with specific subcellular compartments in mature neurons.

We investigated the expression and activity of the different functional pools of the kinase during neuronal development, taking advantage of phosphorylation state- and isoform-specific antibodies directed toward CaMKII or its major presynaptic target, synapsin I.

Four distinct CaMKII isoforms (, , , and ) encoded by distinct genes are known. The  and  isoforms are restricted to the nervous tissue, whereas the  and  isoforms are expressed in a variety of tissues, including the brain (Braun and Schulman, 1995). The various isoforms can coassemble to form multisubunit holoenzymes whose composition varies in different brain regions (Hanson and Schulman, 1992). We have found that in embryonic hippocampal neurons in culture, the  and  isoforms display differential regulation during development. CaMKII is expressed by all cells as early as 12 hr after plating (corresponding to stage I neurons), and its level of expression remains constant throughout differentiation. In contrast, CaMKII is not present at early developmental stages, starts to be expressed by a fraction of stage III neurons, and becomes expressed by the entire population of stage V neurons. An increase in the expression of this isoform has also been observed during brain development (Hanson and Schulman, 1992).

In our model system, we have detected a strict correlation between CaMKII expression and depolarization-induced activation of CaMKII, which, before synaptogenesis, is confined to the somatodendritic pool of the kinase. The apparent requirement for CaMKII expression is consistent with the reported low levels of Ca²⁺/calmodulin-stimulated protein phosphorylation in 2 DIV cultures of hippocampal neurons (Scholz et al., 1988).

Although the [Ca²⁺]_i levels reached after depolarization are generally higher in CaMKII-expressing stage III neurons than in neurons of the same developmental stage negative for this isoform of the kinase, the unresponsiveness of CaMKII-negative neurons is not strictly linked to a lower Ca²⁺ influx, as demonstrated by fura-2 videomicroscopy.

In CaMKII-expressing young neurons, this isoform of the kinase is present also in the axon, although in this compartment, it does not undergo depolarization-dependent phosphorylation. The lack of activation of the kinase in the axons of the CaMKII-expressing neurons is not attributable to a reduced Ca²⁺ influx, because the [Ca²⁺]_i levels reached in this compartment after depolarization are generally comparable with those reached in the dendritic tree of the same cell. However, the selectivity of activation of the kinase in the somatodendritic region of the CaMKII-expressing neurons is lost using stimulating protocols that induce supraphysiological increases in [Ca²⁺]_i levels (i.e., ionomycin in the presence of 10 mM [Ca²⁺]_o), indicating that both CaMKII in CaMKII-negative cells and the axonal pool of the kinase in the CaMKII-expressing cells are not completely refractory to phosphorylation. In addition, this observation indicates that Ca²⁺ influx through voltage-gated channels is not strictly required.

Okadaic acid, which has been shown previously to increase the state of phosphorylation of CaMKII in rat hippocampal neurons (Kasahara et al., 1999), is able to determine a marked increase in the state of phosphorylation of axonal CaMKII, suggesting that a differential balance between kinase and phosphatase activities plays a role in selectively silencing CaMKII activity in the axonal compartment of stage III neurons. Okadaic acid is known to inhibit PP2A and PP1. However, the phosphatase involved in silencing axonal CaMKII is likely to be PP2A, because the experimental conditions that we have used conform to established protocols for the selective inhibition of PP2A in intact cells (Favre et al., 1997).

PP2A activity is known to be modulated by various regulatory subunits, which determine the catalytic activity, substrate specificity, and subcellular localization of the enzyme (Janssens and Goris, 2001). Interestingly, one of these subunits, ', is selectively localized in the soma and proximal dendrites, thus providing a possible explanation for our observations. The actual involvement of this or other subunits in the observed differential behavior between axons and somatodendrites in terms of PP2A activity, as well as the mechanisms of their targeting to selected neuronal compartments, will be an interesting subject for future investigations.

Interestingly, OA was not able to rescue CaMKII phosphorylation in neurons not expressing the  subunit of the kinase, suggesting that the absence of detectable CaMKII phosphorylation cannot be ascribed to the activity of PP2A in these neurons.

In neurons that have already established synaptic contacts, treatment with OA increased the percentage of synapses in which CaMKII-mediated synapsin phosphorylation can be detected after depolarization, indicating that the kinase-silencing mechanism is active also within the immature presynaptic compartment. In contrast, at the postsynaptic level, the percentage of phosphoCaMKII-positive spines was not altered by OA, consistent with the notion that in this compartment, CaMKII is dephosphorylated by PP1 and not by PP2A (Strack et al., 1997).

In mature nerve terminals, a complex of synapsin I and CaMKII on the SV membrane has been implicated in the regulation of SV availability for neurotransmitter release (Benfenati et al., 1992, 1996; Greengard et al., 1993). Although both synapsin I and CaMKII are expressed starting from early developmental stages, with an overlapping pattern of expression in the axonal compartment, their functional coupling can be seen only in mature terminals. Thus, activation of the presynaptic pool of CaMKII, coupled to synapsin I phosphorylation, increases with development in culture in parallel with synaptogenesis and synaptic maturation. Together, our data support the hypothesis that, during development, dephosphorylated synapsin I plays a role in the interaction of SVs with the cytomatrix of nascent synapses, thus acting as a molecular switch that operates to assemble SV clusters before and during synapse formation and that dynamically modulates SV availability for exocytosis in mature nerve terminals (Greengard et al., 1993; Valtorta et al., 1995).

Activation of the somatodendritic pool of the kinase, which appears to be homogeneous in stage III neurons, becomes regionalized in mature, stage V neurons. At this stage, it is possible to identify a proximal compartment of CaMKII activation, composed by the soma and proximal dendrites, and a distal compartment, localized in isolated spines. The absence of labeling in the distal dendritic shaft suggests partially independent generative mechanisms for distal and proximal CaMKII activation.

In the distal domain, where CaMKII activation can be analyzed without an interfering signal from the dendrite, KCl depolarization activates only 40% of the total number of spines. In contrast, the same stimulation appears to elicit activation of the kinase in >90% of the presynaptic terminals, as assayed by CaMKII-dependent synapsin I phosphorylation. The latter figure is in agreement with the percentage of presynaptic terminals in these cultures that respond to depolarization with Ca²⁺-dependent neurotransmitter release, as assayed by labeling with antibodies against the intravesicular lumen of the SV protein synaptotagmin, an indicator of SV recycling (Verderio et al., 1999b). The observation that the fraction of spines in which CaMKII is activated remains relatively constant during synaptogenesis, in contrast to the progressively increasing activation of the presynaptic pool, indicates that the maturation of the presynaptic and postsynaptic compartments is independently regulated and suggests that the postsynaptic receptive apparatus is tuned to a submaximal level, allowing synaptic efficiency to be effectively modulated in both directions by CaMKII activation.

	FOOTNOTES

Received Feb. 8, 2002; revised May 16, 2002; accepted May 31, 2002.

This work was supported by Telethon Grants 1000 (F.V.), 1042 (M.M.), and 1131 (F.B.), by the Harvard-Armenise Foundation, by the Italian Ministry of Education (University Excellence Center on Physiopathology of Cell Differentiation and National Interest Research Program 2001), by European Community Grant QLGR3-CT-2000-01343 (M.M.), by Human Frontier Science Program Grant RGY0022/01 (M.M.), and by United States Public Health Service Grants MH39327 and AG15072 (P.G.).

Correspondence should be addressed to Flavia Valtorta, Unit of Experimental Neuropharmacology, San Raffaele Scientific Institute, Via Olgettina, 58, 20132 Milano, Italy. E-mail: valtorta.flavia{at}hsr.it.

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