A Novel Particulate Form of Ca2+/CaMKII-Dependent Protein Kinase II in Neurons

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The Journal of Neuroscience, May 1, 2000, 20(9):3076-3084

A Novel Particulate Form of Ca²⁺/CaMKII-Dependent Protein Kinase II in Neurons
Ayse Dosemeci, Thomas S. Reese, Jennifer Petersen, and Jung-Hwa Tao-Cheng
Laboratory of Neurobiology, National Institute of Neurological Disorders and Stroke, National Institutes of Health, Bethesda, Maryland 20892

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cytoskeletal and postsynaptic density (PSD) fractions from forebrain contain discrete spherical structures that are immunopositivefor Ca²⁺/calmodulin-dependent protein kinase II (CaMKII). Spherical structuresviewed by rotary shadow electron microscopy have an average diameterof ~100 nm and, in distinction to postsynaptic densities, do notimmunolabel for PSD-95. These structures were purified to nearhomogeneity by extraction with the detergent N-lauryl sarcosinate.Biochemical analysis revealed that CaMKII accounts for virtuallyall of the protein in the purified preparation, suggesting thatspherical structures are clusters of self-associated CaMKII. Exposureof cultured hippocampal neurons to a mitochondrial uncoupler inglucose-free medium promotes the formation of numerous CaMKII-immunopositivestructures identical in size and shape to the CaMKII clustersobserved in subcellular fractions. Clustering of CaMKII wouldreduce its kinase function by preventing its access to fixed substrates.On the other hand, clustering would not affect the ability ofthe large cellular pool of CaMKII to act as a calmodulin sink,as demonstrated by the Ca²⁺-dependent binding of gold-conjugated calmodulin to CaMKII clusters.We propose that the observed clustering of CaMKII into sphericalstructures is a protective mechanism preventing excessive proteinphosphorylation upon loss of Ca²⁺ homeostasis, without compromising calmodulinregulation.

Key words: Ca²⁺/calmodulin-dependent protein kinase II; CaMKII; hippocampal cultures; postsynaptic density; energy depletion; translocation

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ca²⁺/calmodulin-dependent protein kinase II (CaMKII) is present in very high quantities in neurons, making up 1-2% of the totalprotein in certain regions of the brain (Erondu and Kennedy, 1985).Two isoforms, $alpha$ - and $beta$ -CaMKII, are neuron-specific and are foundin both cytosolic and particulate forms. CaMKII translocates fromthe cytosolic to the particulate pool under a variety of physiologicaland pathological conditions. Treatment of hippocampal neuronswith NMDA causes the translocation of green fluorescent protein(GFP)-linked CaMKII to "punctate structures" along the dendritesvia a Ca²⁺-mediated mechanism (Shen and Meyer, 1999). Also, the proportionof CaMKII in the particulate fraction increases after brain ischemia(Aronowski et al., 1992; Hu and Wieloch, 1995; Shackelford etal., 1995). Numerous studies suggested that the postsynaptic density(PSD) may be the site to which the cytosolic CaMKII translocates.Indeed, purified CaMKII is observed to associate with a PSD fractionupon Ca²⁺-dependent autophosphorylation (Strack et al., 1997), and theCaMKII content of the PSD fraction increases after ischemic episodes(Hu et al., 1998).

In the present study, we set out to analyze the precise distribution of CaMKII in a PSD fraction by structural techniquesthat allow examination of individual PSDs. We thought that suchanalysis would help understand the functional consequence of translocationand also would confirm that CaMKII is truly associated with thePSD and not with other structures present in the PSD fraction.To our surprise, immunogold labeling of the PSD fraction revealedthat a significant portion of the CaMKII is associated with discretespherical structures, ~100 nm in diameter, which are not partof the PSDs. The same structures were also observed in a cytoskeletalfraction that is not derived from synaptosomes. These sphericalstructures, purified by extraction with a strong detergent, werefound to contain no other protein but CaMKII and, therefore, areclusters of CaMKII. Exposure of cultured hippocampal cells toconditions that cause mitochondrial dysfunction and energy depletionwas observed to promote the formation of CaMKIIclusters.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Antibodies
Polyclonal antibody to CaMKII was custom made by Multiple Peptide Systems (San Diego, CA); rabbit antiserum to a 14 aminoacid peptide corresponding to the calmodulin binding domain ofCaMKII (residues 296-309 of $alpha$ -CaMKII) was obtained and affinity-purifiedusing the same peptide. Monoclonal antibodies to $alpha$ -CaMKII (clone6G9-2; Boehringer Mannheim, Indianapolis, IN) and to PSD-95 (MA1-046;Affinity BioReagents, Golden, CO) were obtainedcommercially.

Subcellular fractionation
Preparation of the PSD fraction. PSD fraction was prepared using the method of Carlin et al. (1980), with some modifications.Frozen brains from adult Sprague Dawley rats were obtained fromPel-Freez Biologicals (Rogers, AR). Custom collection of brainswas as follows: animals were decapitated after ~1 min exposureto a CO₂-rich atmosphere above dry ice. The brains were then quicklyremoved, placed in liquid nitrogen, and shipped on dry ice. Eachbrain was thawed individually for 1 min at 37°C in isotonic sucrose,and white matter was removed from the forebrain leaving mainlycerebral cortex. Whenever indicated, fresh brains were obtainedfrom 12-week-old Sprague Dawley rats that were killed by decapitation.The brains were then quickly removed, and cerebral cortices weredissected as above within 2 min. The tissue was homogenized immediatelyin 0.32 M sucrose, 1 mM MgCl₂, and 1 µg/ml leupeptin in 1 mM HEPES,pH 7. Homogenates were centrifuged at 1400 × g for 10 min. Supernatantswere saved, and pellets were resuspended in the same solutionand centrifuged at 710 × g for 10 min. Supernatants from the abovetwo steps were combined and were recentrifuged at 710 × g for10 min. The pellets were again discarded. Pellet (P2) and supernatant(S2) fractions were obtained by centrifugation of the supernatantat 13,800 × g for 10 min. P2 were fractionated by sucrose densitycentrifugation. Synaptosomes were collected from the 1/1.25 Msucrose interface and treated with 0.5% Triton X-100. Detergent-insolublepellets from synaptosomes were further fractionated by sucrosedensity gradient centrifugation (200,000 × g for 2 hr). Materialfrom the 1.5/2.1 M sucrose interface was treated with 0.5% TritonX-100 and 75 mM KCl and collected on a 2.1 M sucrose cushion bycentrifugation at 200,000 × g for 40 min. The samples were resuspendedin 20 mM HEPES, pH 7.4, and again collected on 2.1 M sucrose bycentrifugation at 200,000 × g for 30min.
Preparation of the heavy microsomal cytoskeleton. The procedures were identical to those described above up to the 13,000× g for 10 min centrifugation step that yields the P2 and S2 fractions.S2 from this step was fractionated further to obtain the heavymicrosomal cytoskeleton, whereas, as explained above, P2 was usedto prepare the PSD fraction. S2 fraction was layered on 0.8 Msucrose and was centrifuged 85,000 × g for 120 min. The materialsedimented through 0.8 M sucrose was treated with 0.5% TritonX-100. Detergent-insoluble pellets were recovered by centrifugation,resuspended into 0.32 M sucrose, and layered on a 1/1.5/2.1 Msucrose gradient. After centrifugation (200,000 × g for 2 hr),material from the 1.5/2.1 M sucrose interface wascollected.
Protein concentrations were estimated by the method of Peterson (1977). Fractions were stored at $-$ 20^°C in 40%glycerol.

Identification of electrophoretic bands
Proteins were separated on 7.5% SDS-PAGE and were either stained with Coomassie blue or transferred to nitrocellulose. Forimmunoblotting, the polyclonal antibody to CaMKII (1:500 dilution),monoclonal antibodies to $alpha$ -CaMKII (5 µg/ml) and to PSD-95 (1:1000dilution), and alkaline phosphatase conjugated anti-mouse (Sigma,St. Louis, MO) and anti-rabbit (Pierce, Rockford, IL) secondaryantibodies wereused.
Coomassie blue-stained gel bands were excised and subjected to in-gel proteolytic digestion with trypsin essentially accordingto the method of Moritz et al. (1995). Methanol was used insteadof acetonitrile in the washing steps. Digests were subjected toliquid-chromatography tandem mass spectrometry (LC-MS/MS) analysison a previously described Michrom Bioresources Magic 2002 Modelmicrobore HPLC coupled to a Finnigan (San Jose, CA) Model LCQion trap mass spectrometer (Jaffe et al., 1998). The mass spectrometerwas operated in the "Top 5" mode in which the instrument was setup to automatically acquire (1) a full-scan between m/z 300 andm/z 1300 and (2) tandem MS/MS spectra (relative collision energyof 35%) of the five most intense ions in the full scan. MS/MSspectra were analyzed using the BioExplore software package (Finnigan).Individual uninterpreted MS/MS spectra were searched in batchmode against the Genpept database using the SEQUESTprogram.

Kinase assay
Fractions (1 µg of protein/100 µl of final volume) were incubated at room temperature in media containing 50 µM Syntide (Sigma),10 mM MgCl₂, 0.2 mM [ $gamma$ -³²P]ATP, and 0.8 mg/ml bovine serum albumin (BSA) in 50 mM HEPES,pH 7.4, with either 2 mM CaCl₂ and 20 µg/ml calmodulin or 1 mMEGTA. Reactions were stopped by spotting 20 µl aliquots on phosphocellulosepaper. ³²P-labeling was measured by scintillation counting after extensivewashing of excess [³²P]ATP with 75 mM phosphoricacid.

Immunocytochemistry of neuronal cell fractions for rotary-shadowing electron microscopy
Subcellular fractions were adhered to 5 mm² nitric acid-cleaned coverslips by submerging them in 15 µl drops of the fraction(1 mg/ml protein in 20 mM HEPES, pH 7.3) for 5 min. Coverslipswere then rinsed in 5 mM HEPES for 15 min and blocked in 1% BSAin TBS for 60 min, followed by 2% fish gelatin (Ted Pella, Redding,CA) in TBS for 30 min. Coverslips were subsequently incubatedin 15 µl drops of primary antibody (monoclonal antibody to PSD-95,1:100 dilution; polyclonal antibody to CaMKII, 1:50 dilution)in 1%BSA-TBS for 60 min. After incubation with antibody, coverslipswere rinsed in 0.05% Tween 20-TBS for 45 min, blocked in 1%BSA-TBSfor 30 min, and incubated in secondary antibodies conjugated to10 nm gold (anti-mouse 1:100 and anti-rabbit, 1:50 dilution in1%BSA-TBS; Ted Pella). Coverslips were then rinsed in Tween 20-TBSfor 45 min, followed by another rinse in 5 mM HEPES for 30 min.Finally, samples were dipped in distilled water, mounted on freezingstages, and slam frozen using a Life Cell rapid freezing machine.Controls were treated in an identical manner except for the omissionof primary antibody; background on the glass substrate wasnegligible.

Binding of gold-conjugated calmodulin
PSD fractions were adhered to glass coverslips, washed, and blocked as detailed in the above protocol. Coverslips were thenplaced for 1 hr on 15 µl drops of gold-labeled calmodulin (1:200dilution; Sigma) in 0.1% BSA and 20 mM HEPES, pH 7.4, containingeither 1 mM CaCl₂ or 1 mM EGTA. Unbound calmodulin was rinsedoff by two quick dips (~15 sec total duration) in either 10 µMCaCl₂ or 10 µM EGTA, and samples were slam frozen asabove.

Rotary-shadowing electron microscopy
Frozen coverslips with adhered immunolabeled proteins were transferred to a Balzers-301 freeze fracture machine precooledto $-$ 110°C. Samples were freeze-dried under high vacuum by increasingthe temperature to $-$ 100°C for 1 hr and then $-$ 90°C for 45 min.Platinum and carbon replicas of freeze-dried samples were madeby shadowing platinum from a 20° angle onto the rotating specimen,followed by a layer of carbon from directly above. The carbonand platinum replicas were separated from the glass coverslipwith hydrofluoric acid, transferred to distilled water, and pickedup on 400 mesh Formvar-coated copper grids. Replicas were viewedon a JEOL (Peabody, MA) 200CX electron microscope at 120 kV. Stereomicrographs were made for three-dimensionalanalysis.
Gold particles 8-10 nm in diameter are considerably more electron-dense than the platinum shadow and therefore are visiblethrough it. The replicas are illustrated in negative view so theplatinum shadow and the gold particles are seen as white. Eachgold particle had a shell of antibody adhered to it, and the platinumaccreted on this shell during shadowing accounts for the halosurrounding most goldparticles.

Treatment of hippocampal cultures with carbonyl cyanide m-chlorophenylhydrozone
Hippocampal cultures grown on top of a layer of glial cells were prepared from 1-d-old rat brain as described by Lu et al.(1998). The neuronal cultures were maintained in an incubatorunder 90% air, 10% CO₂. Carbonyl cyanide m-chlorophenylhydrozone(CCCP) (Sigma) was dissolved in DMSO. The final concentrationof the carrier in incubation media was 0.1%. Culture dishes (35mm) containing neurons 3-4 weeks in culture were removed fromthe incubator, and culture medium was replaced with incubationmedium (124 mM NaCl, 2 mM KCl, 1.24 mM KH₂PO₄, 1.3 mM MgCl_2, 2.5mM CaCl₂, and 30 mM sucrose in 25 mM HEPES) with 2-10 µM CCCP,after one rinse with incubation medium. In control samples, CCCPwas omitted from the incubation medium, which contained 30 mMglucose instead of sucrose. The culture dishes were maintainedat ~35°C for the indicated intervals before fixation, as describedbelow.

Thin-section immunocytochemistry
Immunocytochemistry (ICC) was performed as described by Tanner et al. (1996). Briefly, samples were fixed with 4% paraformaldehydeand 0.01% glutaraldehyde in 0.1 M phosphate buffer at pH 7.4 for20 min, washed, permeabilized, and incubated with the monoclonalantibody to CaMKII (10 µg/ml) and the secondary antibody conjugatedto Nanogold (Nanoprobes, Stoney Brook, NY), followed by washingand silver enhancement (HQ kit; Nanoprobes). Samples were treatedwith 0.2% OsO₄, dehydrated, and embedded in Epoxy resin. Pelletsfrom fractions were treated in a similar manner for ICC. Theywere fixed in centrifugation tubes and sliced into smaller piecesfor processing. In controls, the primary CaMKII antibody was eitheromitted or substituted with PSD-95antibody.

Morphometry
Diameters of the CaMKII clusters, areas of PSDs, and concentration of CaMKII clusters (see details in Table 1) were measuredusing NIH Image 1.61. PSD thickness, CaMKII labeling, and synapticvesicle depletion at synapses were qualitatively evaluated infive pairs of control and experimental cultures, and a matchedpair representing exactly the same culture conditions was selectedfor further morphometric analysis. To measure average thicknessof the PSDs in thin sections, the cytoplasmic outline of eachPSD, including the associated dense material, was traced in penon coded prints, and this area was enclosed by tracing the postsynapticmembrane. Only PSDs in which the postsynaptic membrane was cross-sectionedwere measured. The resulting area was divided by the length ofthe postsynaptic membrane to derive an average thickness for eachPSD. To estimate the intensity of the gold label, all silver enhancedgold particles within 50 nm of the cytoplasmic outline aroundeach PSD were counted, and this number was divided by the lengthof the corresponding postsynaptic membrane.


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Table 1. Proportion of neuronal somata in hippocampal cultures that develop CaMKII clusters upon exposure to energy-depleting conditions

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The distribution of CaMKII on PSDs was studied in replicas by immunogold labeling with an antibody that recognizes both $alpha$ and $beta$ isoforms of the kinase. PSDs are easily identified in replicasby their size, shape, and immunogold labeling for the PSD markerPSD-95 (Fig. 1B, top). The labeling of PSDs for CaMKII is heterogeneous.Many structures the size and shape of PSDs show little labelingfor CaMKII (Fig. 1A, top), whereas a few others show a more concentrated,patchy distribution of the label.

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Figure 1. Rotary-shadowed replicas of components of the PSD fraction labeled for either CaMKII or PSD-95. PSD fractions were adhered to coverslips and immunolabeled with an antibody to either CaMKII (A) or PSD-95 (B). Representative colloidal gold particles are indicated by arrowheads in the bottom panels. Top, Lower magnification fields showing spherical structures (arrows) and PSDs (P). Insets at top right and left corners show enlargements of PSDs, and the panels below show enlargements of spherical structures. Numbers in each panel indicate number of gold particles counted on the spherical structure shown. Spherical structures label heavily for CaMKII, whereas only a small amount of CaMKII label is present on PSDs. In contrast, PSDs label heavily for PSD-95 (B, top), whereas the spherical structures remain unlabeled (B, bottom). There is little extraneous label on the substrate. All replicas are pictured as negatives so shadow material is white. Scale bars, 100 nm.

The PSD fraction contains, in addition to PSDs, many spherical structures manifesting intense labeling for CaMKII but no labelingfor PSD-95 (Fig. 1, arrows in top panels; enlargements are shownin the bottom panels). The diameters of these spherical structuresranges from 75 to 144 nm with a mean value of 104 nm (SEM = 2.6;n = 39). The differences in the labeling in PSDs and sphericalstructures for CaMKII does not appear to be the result of post-mortemmodifications or to depend on the particular antibody used. Similarlabeling is observed when PSD fractions are prepared from rapidlyprocessed brains and/or when using an antibody that recognizesonly $alpha$ -CaMKII (Fig. 2). However, preparations from rapidly processedbrains contain fewer spherical structures as will be discussedbelow.

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Figure 2. Labeling with two different CaMKII antibodies in fractions prepared by rapid post-mortem processing of brains. Cerebral cortices used for the PSD preparation were dissected and homogenized within ~2 min of decapitation. The immunolabeling was with either the polyclonal antibody as in Figure 1 (A) or a monoclonal antibody specific for $alpha$ -CaMKII (B). Top, Fields at lower magnification showing spherical structures (arrows) and PSDs (P). Panels below show enlargements of spherical structures. Numbers in each panel indicate number of gold particle on the spherical structure shown. The labeling of PSDs and spherical structures are essentially the same as those observed in Figure 1, although spherical structures are less numerous in this preparation. Scale bars, 100 nm.

As expected from their high content of CaMKII, the spherical structures bind gold-conjugated calmodulin in a Ca²⁺-dependent manner (Fig. 3). PSDs in the preparation also showheavy calmodulin binding (Fig. 3A), although it is expected thatat least part of this label corresponds to other calmodulin-bindingproteins associated with the structure.

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Figure 3. Binding of calmodulin to spherical structures. PSD fractions were adhered to a glass coverslip and, after blocking with BSA and gelatin, incubated with gold-conjugated calmodulin. They were then quickly washed and slam frozen. Spherical structures (arrow in A) show heavy labeling when incubated in the presence of Ca²⁺ (A, B), but almost no labeling when incubated in the presence of EGTA (C). Gold-conjugated calmodulin also binds PSDs (P in A), but not to other unidentified structures (asterisk). The gold particles used in this experiment are slightly smaller than the 10 nm gold particles used for immunolabeling on replicas in Figures 1 and 2. Numbers in each panel indicate number of gold particles assigned to the spherical structure shown. Scale bars, 100 nm.

A nonsynaptic cytoskeletal fraction enriched in CaMKII had been described previously (Sahyoun et al., 1985). To determinewhether CaMKII-positive spherical structures are also presentin this fraction, a similar preparation was performed (Materialsand Methods). This fraction, which we designate as "heavy microsomalcytoskeleton," should contain very little synaptic material becauseits preparation includes a centrifugation step to remove synaptosomes.Biochemical analysis indicates that the heavy microsomal cytoskeletonfraction has high levels of CaMKII and very little PSD-95 comparedwith the PSD fraction (Fig. 4B), confirming its nonsynaptic origin.CaMKII in this fraction is active and capable of autophosphorylation.In experiments comparing the heavy microsomal cytoskeleton fractionwith a crude PSD fraction, Ca²⁺/calmodulin-dependent kinase activities measured with Syntideas substrate were found to be similar (75 and 79 pmol phosphatetransferred · min¹ · µg¹ total protein, respectively), and the amount of ³²P incorporated into $alpha$ -CaMKII after incubation of fractions inthe presence of Ca²⁺/calmodulin and ATP was slightly higher in the heavy microsomalcytoskeleton (data not shown). Observation of replicas of thisfraction reveals spherical structures that label for CaMKII butnot for PSD-95 (Fig. 4A). These structures (mean diameter of 102nm; SEM = 3.0; n = 39; range, 65-137 nm) have similar size andshape to those in the PSD fraction.

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Figure 4. Structure and composition of the heavy microsomal cytoskeleton fraction. A, Rotary-shadowed replicas of this fraction labeled with antibodies to CaMKII and PSD-95. Spherical structures (enlarged in bottom panels) are labeled [for CaMkII (number of gold particles is indicated in each panel) but did not label for PSD-95]. B, Comparison of the protein staining profiles (top) and immunoblots (bottom) of the PSD (lane 1) and heavy microsomal cytoskeleton (lane 2) fractions (10 µg of protein per lane). CaMKII is a major component of both fractions (arrowhead), but immunoblots (bottom) show that the heavy microsomal cytoskeleton fraction contains relatively little PSD-95. C, Thin section through pelleted heavy microsomal cytoskeleton fraction labeled with a monoclonal antibody for $alpha$ -CaMKII. Round structures labeled for $alpha$ -CaMKII are the predominant component of this fraction; other labeled structures (arrow) are PSDs in cross-section. The diameters of CaMKII-positive round structures in the pellet (panels at right) correspond closely to those of the spherical structures in replicas (Figs. 1A, 3A), indicating that they correspond to the same structural entities. Immunolabeling here and in all subsequent thin sections uses silver-enhanced gold, which accounts for the variability in grain size. Scale bars, 100 nm.

The heavy microsomal cytoskeleton fraction was also analyzed by a parallel method of thin-section immunoelectron microscopythat could subsequently be applied to the examination of wholecells (Tanner et al., 1996). Pre-embedding immunogold labelingof the pelleted heavy microsomal cytoskeleton with a monoclonalantibody specific to $alpha$ -CaMKII (Fig. 4C) reveals intensely labeledround structures with a mean diameter of 110 nm (SEM = 2.6; n= 28; range, 86-147 nm). The abundance, size, shape, and CaMKIIimmunoreactivity of these structures indicate that they correspondto the spherical structures seen in replicas. The fraction containsonly a few recognizable PSDs (Fig. 4C, arrow), consistent withthe low levels of PSD-95 detected inimmunoblots.

Extraction of the Triton X-100-derived PSD preparation with the stronger detergent N-lauryl sarcosinate (NLS) is known toresult in a pellet that is greatly enriched in CaMKII (~40% oftotal protein) (Cho et al., 1992). To determine whether NLS extractionresults in enrichment of spherical structures, heavy microsomalcytoskeleton and PSD fractions were treated with a 3% solutionof thedetergent.

Coomassie blue protein-staining pattern corresponding to NLS-insoluble pellet from the PSD fraction (Fig. 5A, lane1) showsan enrichment of the ~50 kDa band that corresponds to $alpha$ -CaMKII,as well as a number of higher molecular bands. The pellet fromthe heavy microsomal cytoskeleton fraction (Fig. 5A, lane 2) showstwo main bands, ~50 and ~60 kDa, respectively. Both of these bandsare recognized by the antibody to CaMKII (Fig. 5A, lane3). Thetwo electrophoretic bands were subjected to in-gel proteolyticdigestion, and digests were analyzed by LC-MS/MS to identify theprotein. The ~50 kDa major band was identified as rat $alpha$ -CAMKIIon the basis of the following nine peptides: (K) ESSESTNTTIEDEDTK,(K) VLAGQEYAAK, (K) HPWISHR, (R) NSKPVHTTILNPH, (K) GAFSVVR, (F)AGTPGYLSPEVLR,(R) DLKPENLLLASK, (R) FTEEYQLFEELGK, and (R)FYFENLWSR, and onepeptide, (K) WQNVHFHR, which differs by a single residue fromthe rat $alpha$ -CaMKII sequence. No other proteins were identified inthat band. The ~60 kDa band was identified as containing rat $beta$ -and $gamma$ - CAMKII on the basis of the following three peptides: (R)FTDEYQLYEDIGK, (K)GSLPPAALEPQTTVIHNPVDGIK ( $beta$ -CaMKII), and (R)FTDDYQLFEELGK ( $gamma$ -CaMKII). No other proteins except human keratin,a common contaminant, were identified in this band.

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Figure 5. Purification and molecular composition of spherical structures. Heavy microsomal cytoskeleton and PSD fractions were treated with 3% NLS in 20 mM HEPES, pH 7.4, for 10 min at room temperature, at a final protein concentration of 0.43 mg/ml. Detergent-insoluble pellets were collected by centrifugation (240,000 × g for 1 hr) A, Biochemical analysis of the pellets. Lane 1, Protein staining profile of NLS-insoluble fraction from PSD. Lane 2, Protein staining profile of NLS-insoluble fraction from heavy microsomal cytoskeleton. Lane 3, Immunoblot of NLS-insoluble fraction from the heavy microsomal cytoskeleton with a polyclonal antibody to CaMKII (each lane contains pellet corresponding to 20 µg of original protein). C, Thin sections through the NLS-insoluble pellet from the heavy microsomal cytoskeleton show that the preparation consists almost entirely of spherical structures. B, Enlargements of two spherical structures from the same thin sections show that they closely resemble those in the untreated fractions (Fig. 3C). D, Thin sections through the NLS-insoluble pellet from the PSD preparation show an enrichment in spherical structures but also contain PSDs (indicated by arrows). Scale bars, 100 nm.

Electron microscopy of thin sections (Fig. 5B,C) shows that the NLS-insoluble pellet from the heavy microsomal cytoskeletonconsists almost solely of round structures of similar size (meandiameter of 112 nm; SEM = 2.4; n = 45; range, 84-145 nm) to thoseobserved in the parent fraction (Fig. 4C). Together, the resultsfrom biochemical and morphological analysis indicate that $alpha$ -CaMKIIis the main constituent of the spherical structures purified byNLS extraction. With the exception of $beta$ and $gamma$ isoforms of CaMKII,these structures do not appear to contain any other protein. Basedon these results, we decided to designate them as "CaMKII clusters."NLS extraction of the PSD preparation also yields a fraction thatis highly enriched in CaMKII clusters (Fig. 5D). However, in agreementwith the presence of other proteins in the pellets, PSDs (indicatedby arrow) are recognizable in electron micrographs of thin sections(Fig. 5D)

Are CaMKII clusters present in intact cells? To clarify this issue, we studied the distribution of CaMKII in cultured hippocampalneurons. In agreement with previous studies on adult brain (Ouimetet al., 1984; Liu and Jones, 1997), immunocytochemistry with anantibody to $alpha$ -CaMKII indicates that the protein is present incultured neurons but not in glia. Within neurons, its distributionis heterogeneous, with no label observed in the nuclei (data notshown). Diffuse immunogold labeling is observed in neuronal somaand processes, which may correspond to cytosolic CaMKII (Fig.6A). CaMKII clusters such as those observed in the subcellularfractions are, however, extremely rare.

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Figure 6. Formation of CaMKII clusters upon exposure of hippocampal cultures to energy-depleting conditions. Hippocampal cultures were exposed to glucose-free medium containing either 2 µM (C) or 10 µM (B, D) CCCP for 30 and 15 min, respectively. Control samples (A) were incubated for 30 min in corresponding glucose-containing medium with carrier only (0.1% DMSO). In thin sections of control samples, diffuse labeling for CaMKII (each spot corresponds to an individual enhanced gold complex) is observed throughout the cytoplasm of neurons. In treated samples, diffuse labeling is greatly diminished, but intense labeling of electron-dense round structures is observed (B, arrows). C and D show that these round structures are virtually identical to the CaMKII clusters observed in subcellular fractions (Figure 3C). Scale bars, 100 nm.

Is it possible that the high numbers of CaMKII clusters found in subcellular fractions are attributable to ischemic conditionsthat prevail during and right after death, but before the breakingup of the cells by homogenization? This possibility is suggestedby the observations of Suzuki et al. (1994) who reported thatthe CaMKII content of the PSD fraction increases in direct proportionto the time elapsed between decapitation and homogenization. Acomparison of the ratio of PSDs to CaMKII clusters in our PSDpreparations from brains collected by Pel-Freez (brief exposureto CO₂ before decapitation and frozen after dissection) and rapidlyprocessed brains (homogenization within 2 min of decapitation)further supports this idea. The ratio of PSDs to CaMKII clusters,estimated by counting all PSDs and CaMKII clusters within thesame fields on replicas, is 1:1.2 in the former but 1:0.3 in therapidly processedbrains.

The above observations suggest that exposure of cells to ischemic conditions may promote the formation of CaMKII clusters.In agreement with this hypothesis, PSD preparations from brainsof animals subjected to an ischemic insult contain higher levelsof CaMKII (Hu et al., 1998). To test whether the formation ofCaMKII clusters is promoted by conditions related to ischemicstress, hippocampal neurons were exposed to conditions designedto deplete their energystores.

Cultured hippocampal cells were incubated in glucose-free medium in the presence of CCCP, an uncoupler of oxidative phosphorylationthat acts by dissipating the proton gradient across the mitochondrialmembrane. Incubation of hippocampal neurons with either 10 µMCCCP for 15 min or 2 µM CCCP for 30 min in glucose-free mediumpromotes the formation in cell bodies and dendrites of neuronsof round, electron-dense structures that label intensely for $alpha$ -CaMKII(Fig. 6B-D). Comparison of these structures with the CaMKII clustersin subcellular fractions visualized by the same technique (Figs.4C, 6, bottom panels) indicates that they are indistinguishable,in terms of either shape or size (mean diameter of 108 nm; SEM= 3.9; n = 27; range, 79-150 nm). Serial thin sections (at anaverage thickness of 70 nm) revealed that none of the CaMKII clustersexisted in more than three consecutive sections, demonstratingthat these clusters are not interconnected and, indeed, are sphericalin structure. Although some patchy condensation of the chromatinin the nucleus was observed in CCCP-treated neurons, these manifestednone of the typical signs of cell death, such as swollen mitochondriaand endoplasmic reticulum, fragmented nuclei, and blebbing ofthe plasma membrane, at either the light or electron microscopiclevels.

Formation of CaMKII clusters is observed in up to 83% of neurons in treated samples (Table 1). Some of the treated neuronslacking clusters showed no label at all, suggesting that theydo not express $alpha$ -CaMKII. After exposure to 10 µM CCCP, the densityof clusters was found to be as high as one to three clusters persquare micrometer in sections through neurons that contain CaMKIIclusters. The size of the clusters does not appear to increasewith increasing exposure to energy-depleting conditions. In amatching set of experiments, the average diameters after 15, 60,and 90 min incubation in 10 µM CCCP were 105 ± 2 (n = 45), 110± 2.9 (n = 47), and 113 ± 3.6 (n = 30) nm, respectively. The observationof an upper limit for diameter would indicate that these clustersmay be ordered arrays of molecules rather than randomaggregates.

Exposure of cultures to 10 µM CCCP in glucose-free medium for 15 min causes a 50% decrease (p < 0.05; t test; 24 synapsesper group) in the number of synaptic vesicles within 150 nm ofthe presynaptic membrane, indicating massive neurotransmitterrelease (Fig. 7). Thus, it is likely that the conditions usedin these experiments, a combination of glucose deprivation andinhibition of oxidative phosphorylation, induce extracellularaccumulation of excitatory neurotransmitters, a well documentedconsequence of ischemic stress (Benveniste et al., 1984; Globuset al., 1988). The resulting increase in intracellular Ca²⁺ levels is likely to be further potentiated because of the inhibitionof mitochondrial Ca²⁺ uptake by CCCP.

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Figure 7. Changes in synapses upon exposure of hippocampal cultures to energy-depleting conditions. Hippocampal cultures were exposed to glucose-free medium with 10 µM CCCP for 15 min. Control samples were incubated in corresponding glucose-containing medium with carrier alone for a total of 30 min. CCCP-treated and control samples were labeled with a monoclonal antibody to $alpha$ -CaMKII before embedding. Thin sections through synapses in control (A) and treated (B) samples are shown. In neurons exposed to CCCP, there is a marked decrease in the number of synaptic vesicles clustered near the active zone, and the material adhering to the cytoplasmic side of the PSD increases in thickness. Also, the labeling density for CaMKII around the PSD increases (measurements in Results). Scale bars, 100 nm.

In agreement with changes observed previously in ischemic brains (Hu et al., 1998; Martone et al., 1999), the average overallthickness (see Materials and Methods) of the PSD in treated samples(10 µM CCCP in glucose-free medium for 15 min) increased by 75%(47.2 ± 2.5 nm compared with 27.0 ± 1.6 nm in controls; 24 synapsesper group). These conditions also resulted in increased accumulationof CaMKII label at the peripheries of PSDs (see Materials andMethods). In treated samples, the density of silver-enhanced goldlabel for CaMKII at the peripheries of PSDs increased 2.4-foldcompared with controls (p < 0.05; t test; 24 synapses pergroup).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present study describes a novel particulate form of CaMKII organized as spherical structures with average diameters of~100 nm. Their detection in the PSD fraction, as well as in anotherdetergent-insoluble fraction from brain, was made possible bya sensitive structural approach that allows localization of proteinsat the level of individual structures. Particulate material fromfractions was adhered to glass, labeled with gold-conjugated antibodies,freeze-dried, and shadowed. Electron microscopy showed that thespherical structures contain large amounts of CaMKII, but littleor no PSD-95, a marker for PSDs. It became possible to analyzethe molecular composition of the spherical structures after theywere purified to near homogeneity by extraction of the heavy microsomalcytoskeleton fraction with the relatively strong detergent NLS.Biochemical analysis of the purified preparation detected no proteinsother than CaMKII, prompting us to designate these structuresas CaMKII clusters. The presence CaMKII clusters in subcellularfractions is not an artifact of detergent treatment because theycan be induced in intactneurons.

Formation of CaMKII clusters is promoted by exposure of hippocampal cultures to a mitochondrial uncoupler in the absence ofglucose. These conditions are likely to simulate some of the consequencesof ischemic stress, such as energy depletion and an increase in[Ca²⁺]_i. When treated with 10 µM CCCP in glucose-free medium for 15min, the majority of neurons within the culture develop CaMKIIclusters. Possibly all neurons containing $alpha$ -CaMKII are able toform clusters because the presence of GABAergic and other neuronsnot expressing CaMKII account for the neurons lacking clusters.Energy-depleting conditions also promote an accumulation of CaMKIInear thePSDs.

Earlier studies have established that CaMKII levels increase in particulate fractions from brain after ischemia (Aronowskiet al., 1992; Hu and Wieloch, 1995; Shackelford et al., 1995).The present work demonstrates that under conditions that simulateaspects of ischemic stress CaMKII accumulates around the PSD andassembles into spherical clusters of uniform shape and size distributedthroughout the neuron, thus explaining how CaMKII becomes partof the particulatefraction.

It is likely that the previously reported increase in the CaMKII content of the PSD fractions after ischemia (Hu et al., 1998)is attributable, not only to a translocation of CaMKII to thePSDs, but also to an increase in the number CaMKII clusters. Similarly,ischemia-like conditions that follow decapitation are probablyresponsible for the presence of CaMKII clusters in PSD fractions,as well as for the observed increases in the CaMKII content ofthe fraction upon increasing the interval between decapitationand homogenization (Suzuki et al., 1994). Indeed, CaMKII clustersappear to be major contaminants of the PSD fraction and, therefore,changes in the CaMKII content of the fraction should not be interpretednecessarily as changes in the PSDcomposition.

Biochemical analysis of the nearly homogeneous preparation obtained by extraction with NLS suggests that the entire volumeof CaMKII clusters consists of self-associated CaMKII. This conclusion,however, does not exclude the possibility that certain peripheralproteins originally attached to the core structure may have beenremoved by NLS. Also, the two other visible bands in the NLS-insolublepellet, a faint band between $alpha$ - and $beta$ -subunits and the materialrunning at the dye front, have not been identified. The mechanismfor CaMKII self-association in vivo is at the present unclear.An earlier in vitro study by Hudmon et al. (1996), however, suggeststhat a combination of conditions, including high [Ca²⁺], low [ATP], and acidic pH may be necessary. Indeed, the authorsobserve that incubation of purified CaMKII in 0.01 mM ATP at pH6.5 in the presence of Ca²⁺ promotes self-association, whereas increasing the ATP concentrationto 1 mM, or bringing the pH to 7.5, prevents the formation ofaggregates.

What would be the consequence of clustering? This question may be explored by considering the functions of CaMKII in neurons.CaMKII is a Ca²⁺-activated protein kinase whose activation leads to the inductionof synaptic potentiation in certain regions of the brain. Underconditions of Ca²⁺ overload, overactivation of CaMKII may have a deleterious effect,possibly by causing a sustained and generalized potentiation.Indeed, inhibition of CaMKII provides protection against NMDA-and hypoxia-hypoglycemia-induced cell death in cultured corticalneurons (Hajimohammadreza et al., 1995). Assembly of CaMKII intodensely packed clusters should lower its access to fixed substratesand thus limit the damage. Indeed, a particle that is as largeas 100 nm would have almost no diffusion capacity within a cell,and the phosphorylation of a fixed substrate would be impossibleunless a cluster is formed right next to it. Also, clusteringwould cause the effective concentration of the kinase to be reduceddrastically. For example, whereas 10 molecules of CaMKII can,in theory, reach 10 fixed substrates placed more than 100 nm apartsimultaneously, a cluster of 10 molecules can reach only one ofthem at a time. In addition, clustering may by itself inactivatethe enzyme, as suggested by observations that under ischemic conditionsCaMKII activity is reduced in parallel with its translocationto particulate fractions (Aronowski et al., 1992; Hu and Wieloch,1995; Shackelford et al., 1995).

In addition to its role as a protein kinase, a calmodulin-trapping function has been proposed for CaMKII (Meyer et al., 1992;Mayford et al., 1995). Indeed, CaMKII makes up ~1-2% of the totalprotein in certain brain areas, including the cerebral cortexand the hippocampus (Erondu and Kennedy, 1985), quantities muchgreater than would be expected for an enzyme but enough to bindan appreciable portion of the intracellular calmodulin. Becausetrapping by CaMKII would limit calmodulin availability to othercalmodulin-regulated molecules, such as nitric oxide synthase,calcineurin, and adenylate cyclase, retention of this calmodulinbuffering function could be essential under conditions of excessiveCa²⁺ build-up. In fact, a participation of calmodulin-mediated pathwaysin ischemic damage is well established (Pohorecki et al., 1990;Kuroda et al., 1997; Sun et al., 1997). In contrast to its effecton the phosphorylation function discussed above, clustering ofCaMKII is not expected to inhibit the capability of CaMKII totrap calmodulin. This proposition is supported by our in vitroexperiments demonstrating Ca²⁺-dependent specific binding of gold-conjugated calmodulin to CaMKIIclusters.

As implied by the above discussion, CaMKII has a dual function in neurons, as a kinase and as a calmodulin trap. During episodesof Ca²⁺ overload, the suppression of kinase function but the preservationof calmodulin-trapping function would be essential in limitingcellular damage. Clustering of CaMKII into spherical structures,by dissociating its two functions, appears to achieve both ofthese goals. Thus, we regard CaMKII clustering as a protectivemechanism that can be induced under certain pathological conditions,in anticipation of a continued loss of Ca²⁺ homeostasis. We speculate that, within the confine of a synapticspine, sustained synaptic activity may also promote CaMKII clusteringaround the PSD in a synapse-specific manner. The existence ofsuch a mechanism and its relevance in activity-dependent synapticmodification are interesting possibilities that remain to beexplored.

  FOOTNOTES

Received Nov. 10, 1999; revised Jan. 27, 2000; accepted Feb. 17, 2000.

We thank Dr. Howard Jaffe (Laboratory of Neurochemistry, Protein/Peptide Sequencing Facility, National Institute of NeurologicalDisorders and Stroke) for LC-MS analysis, Dr. Lucia Vinade forher help in preparing PSD fractions, Virginia Tanner Crocker forher meticulous work on electron microscopy of cultures and cellfractions, John Chludzinski for his work and support of the digitalphotography, and Pat Zerfas for photography. We are particularlygrateful to Christine Winters for providing the numerous hippocampalcultures needed for ourstudy.
Correspondence should be addressed to Ayse Dosemeci at her present address: Marine Biological Laboratory, 7 MBL Street, WoodsHole, MA 02543. E-mail: dosemeci{at}marinebiombl.edu.

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RESULTS
DISCUSSION
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