Cdk5/p35 Regulates Neurotransmitter Release through Phosphorylation and Downregulation of P/Q-Type Voltage-Dependent Calcium Channel Activity

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The Journal of Neuroscience, April 1, 2002, 22(7):2590-2597

Cdk5/p35 Regulates Neurotransmitter Release through Phosphorylation and Downregulation of P/Q-Type Voltage-Dependent Calcium Channel Activity
Kazuhito Tomizawa¹, Jun Ohta², Masayuki Matsushita¹, Akiyoshi Moriwaki¹, Sheng-Tian Li¹, Kohji Takei³, and Hideki Matsui¹
Departments of ¹ Physiology, ² Biochemistry, and ³ Neuroscience, Okayama University Graduate School of Medicine and Dentistry, Okayama 700-8558, Japan

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cyclin-dependent kinase 5 (Cdk5) is a proline-directed serine/threonine kinase with close structural homology to the mitoticCdks. The complex of Cdk5 and p35, the neuron-specific regulatorysubunit of Cdk5, plays important roles in brain development, suchas neuronal migration and neurite outgrowth. Moreover, Cdk5 isthought to be involved in the promotion of neurodegeneration inAlzheimer'sdisease.
Cdk5 is abundant in mature neurons; however, its physiological functions in the adult brain are unknown. Here we show thatCdk5/p35 regulates neurotransmitter release in the presynapticterminal. Both Cdk5 and p35 were abundant in the synaptosomes.Roscovitine, a specific inhibitor of Cdk5 in neurons, inducedneurotransmitter release from the synaptosomes in response tomembrane depolarization and enhanced the EPSP slopes in rat hippocampalslices. The electrophysiological study using each specific inhibitorof the voltage-dependent calcium channels (VDCCs) and calciumimaging revealed that roscovitine enhanced Ca²⁺ influx from the P/Q-type VDCC. Moreover, Cdk5/p25 phosphorylatedthe intracellular loop connecting domains II and III (L_II-III)between amino acid residues 724 and 981 of isoforms cloned fromrat brain of the $alpha$ _1A subunit of P/Q-type Ca²⁺ channels. The phosphorylation inhibited the interaction of L_II-IIIwith SNAP-25 and synaptotagmin I, which were plasma membrane solubleN-ethylmaleimide-sensitive factor attachment protein (SNAP) receptor(SNARE) proteins and were required for efficient neurotransmitterrelease. These results strongly suggest that Cdk5/p35 inhibitsneurotransmitter release through the phosphorylation of P/Q-typeVDCC and downregulation of the channelactivity.

Key words: Cdk5; presynapse; calcium channel; SNARE; p35; exocytosis

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cdk5 is a serine/threonine kinase with close structural homology to the Cdks (Lew and Wang, 1995). Cdk5 forms a complex withits activators, p35^nck5a (p35) or p39^nck5ai (p39), in neurons (Lew et al., 1994; Tsai et al., 1994; Tanget al., 1995). The association of Cdk5 with its activators isessential for the kinase activation (Lew et al., 1994; Tsai etal., 1994; Tang et al., 1995). Previous studies have shown thatthe complex of Cdk5 and p35 has multiple functions in neurons.Mice lacking p35 display defects in cortical and hippocampal laminationas well as fasciculation of the axon fibers (Chae et al., 1997).In the cortex of p35 knock-out mice, the layering of corticalneurons is inverted, because neurons born later cannot migratepast their predecessors (Chae et al., 1997). Inactivation of Cdk5in cultured cortical or cerebellar neurons inhibits neurite outgrowth(Nikolic et al., 1996). Cdk5 kinase activity and p35 expressionlevel are most prominent from newborn to 2 weeks after birth,when synaptogenesis occurs through the development of the ratbrain (Matsushita et al., 1996; Tomizawa et al., 1996). Moreover,Cdk5 kinase activity increases in the kindling rat hippocampus,in which sprouting and synaptic reorganization have also beenobserved (Stula et al., 1988; Moriwaki et al., 1996; Tomizawaet al., 2000). These previous data suggest that Cdk5/p35 playcritical roles in neural migration, differentiation, and synaptogenesisin immatureneurons.

Recent studies have shown that Cdk5/p35 is involved in neuronal degeneration in Alzheimer's brain (Patrick et al., 1999; Leeet al., 2000). Proteolytic cleavage of p35 produces p25, whichaccumulates in the brains of patients with Alzheimer's disease.The calpain-dependent proteolytic cleavage causes prolonged activationand mislocalization of Cdk5. Consequently, the Cdk5/p25 kinasehyperphosphorylates tau proteins, disrupts the cytoskeleton, andpromotes neuronal celldeath.

These previous data suggest that Cdk5/p35 plays important roles in the immature and aging brain. However, Cdk5 expressionis most prominent in mature neurons (Matsushita et al., 1996).The physiological function of Cdk5/p35 in the mature neuron isnot clear. Previous studies have shown that Cdk5 is strongly expressedin axons of the adult brain (Tsai et al., 1993; Matsushita etal., 1996). Several studies have identified Munc 18 (nSec-1) (Shuanget al., 1998), Synapsin 1 (Jovanovic et al., 1996; Matsubara etal., 1996), and Amphiphysin I (Floyd et al., 2001) as physiologicalsubstrates of Cdk5. These proteins localize in the presynapticterminal of the mature neuron and play important roles in neurotransmitterrelease. These previous observations lead to a hypothesis thatCdk5/p35 may regulate neurotransmitterrelease.

Neurotransmitter release from specialized active zones in presynaptic terminals is a critical step in synaptic transmission.Release of synaptic vesicles containing neurotransmitter is triggeredby an influx of Ca²⁺ through voltage-dependent calcium channels (VDCCs) (Catterall,1998). It has been thought that N-type and P/Q-type VDCCs mainlyregulate neurotransmitter release in the presynaptic terminals(Wheeler et al., 1996; Reid et al., 1997). Specific protein-proteininteractions between a synaptic protein interaction (synprint)site on N-type and P/Q-type channels and the presynaptic solubleN-ethylmaleimide-sensitive factor attachment protein (SNAP) receptor(SNARE) proteins, syntaxin, SNAP-25, and synaptotagmin are requiredfor efficient synchronous neurotransmitter release (Kim and Catterall,1997; Catterall, 1998). The synprint sites on N-type and P/Q-typeCa²⁺ channels locate within the intracellular loop connecting homologousdomains II and III (L_II-III) of their $alpha$ _1A and $alpha$ _1B subunits (Catterall,1998). The interaction of N-type Ca²⁺ channels with syntaxin and SNAP-25 is Ca²⁺ dependent and regulated by protein phosphorylation (Yokoyamaet al., 1997). In this study, we demonstrate direct evidence thatCdk5/p35 regulates neurotransmitter release through the phosphorylationof the L_II-III of P/Q-typeVDCC.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrophysiological recording. Field EPSP recording was performed as described previously (Lu et al., 1996, 1999). Briefly,male Wistar rats aged 7-8 weeks were killed in accordance withthe guidelines of the Health Science Division of the GraduateSchool of Medicine and Dentistry, Okayama University. The brainwas quickly removed and immersed in ice-cold artificial CSF (ACSF)bubbled with a gas mixture of 95% O₂ and 5% CO₂. The hippocampuswas dissected, and 400 µm transverse slices were prepared. Thehippocampal slices were incubated in an interface-recording chambermaintained at 28°C for at least 1.5 hr before recording and wereconstantly subfused with gas-saturated ACSF at 1.2 ml/min. Thecomposition of the ACSF was as follows (in mM): NaCl 124, KCl4.4, CaCl₂ 2.5, MgSO₄ 1.3, NaH₂PO₄ 1, NaHCO₃ 26, and glucose10.

To record the field EPSPs, a glass micropipette filled with ACSF (1-5 M $Omega$ resistance) was placed in the stratum radiatum ofthe CA1 region, and a bipolar stimulating electrode was placedalong the Schaffer collateral fibers. The intensity of the stimulationwas adjusted to produce an EPSP with a slope between 35 and 50%of the maximum. The test stimulation was delivered once per minute(0.017Hz).

The following drugs were used. Roscovitine was kindly donated by L. Meijer (Station Biologique, Bretagne, France); olomoucine, $omega$ -Conotoxin GVIA ( $omega$ -CgTX GVIA), $omega$ -Agatoxin IVA ( $omega$ -Aga IVA), andNifedipine were from RBI (Natick, MA). The drugs were preparedas stock solutions and diluted in ACSF immediately before application.Roscovitine, olomoucine, and Nifedipine were prepared in DMSO,and $omega$ -CgTX GVIA and $omega$ -Aga IVA were dissolved in H₂O. The finalconcentration of the DMSO was 0.1%.

Data are shown as mean (±SEM) percentage of the baseline EPSP slope. Data were analyzed using either the Student t test tocompare the two conditions or ANOVA followed by planned comparisonsof the multiple conditions, and p < 0.05 was consideredsignificant.

Synaptosome preparation and Western blot analysis. Synaptic fractions were prepared from rat brain as described previously(Huttner et al., 1983) with minor modifications. Briefly, thebrains from seven male Wistar rats were homogenized in 50 ml ofsucrose buffer (0.32 M sucrose/5 mM HEPES/KOH buffer, pH 7.4,containing the following protease inhibitors: 0.4 mM phenylmethylsulfonylfluoride, 0.8 mg/ml pepstatin A, 0.8 mg/ml antipain, 0.8 mg/mlleupeptin, 0.8 mg/ml benzamidine, 0.4 mg/ml aprotinin). The homogenatewas spun for 10 min at 800 × g, yielding a pellet (P1). The supernatantwas centrifuged for 15 min at 9200 × g. The resulting pellet waswashed once with sucrose buffer, yielding a crude synaptosomalpellet (P2'). The supernatant was centrifuged at 165,000 × g for2 hr, yielding a pellet (P3) and supernatant (S3). P2' was resuspendedin 4 ml of sucrose buffer and lysed by the addition of 9 vol ofdistilled water, followed by homogenization. HEPES/KOH buffer,pH 7.4, was added to a final concentration of 10 mM together withthe above protease inhibitors. The fraction was spun at 25,000× g for 20 min (pellet LP1) and the supernatant (LS1) was furthercentrifuged for 2 hr at 165,000 × g, yielding a crude synapticvesicle pellet (LP2) and a supernatant(LS2).

Western blot analysis was performed at high stringency, essentially as described previously (Tomizawa et al., 1996). Briefly,50 µg of each fraction protein was separated by electrophoresisthrough a 10-12% SDS-PAGE gel before transfer to a nitrocellulosemembrane (Amersham Biosciences). Blots were probed with primaryantibodies against Cdk5 (C-8; Santa Cruz Biotechnology, SantaCruz, CA), p35^nck5a (N-20; Santa Cruz Biotechnology), synaptophysin (Progen Biotechnik,Heidelberg, Germany), and calmodulin kinase I (kindly providedby A. C. Nairn, The Rockefeller University, New York, NY), andsecondary antibodies [anti-rabbit IgG (H+L), Pierce, Rockford,IL] before bands were visualized using a commercial ECL detectionkit (AmershamBiosciences).

Measurement of glutamate release from synaptosome. The purified synaptosomes were preincubated at 37°C with each concentrationof roscovitine or DMSO (final concentration, 0.1%) as controlsfor 30 min. Then 1 mM NADP⁺, 60 U glutamate dehydrogenase (GDH), and 1.3 mM CaCl₂ were added,and the synaptosomes were further incubated for 10 min. The suspensionwas then transferred to a stirred cuvette in the fluorescencespectrophotometer, and 1 mM 4-aminopyridine (4-AP; Sigma, St.Louis, MO) was added in solution to depolarize the cell membrane.When glutamate is oxidized to 2-oxoglutarate by GDH and NADP⁺, NADP⁺ is reduced to NADPH, and the fluorescence of NADPH can be measured(Vinje et al., 1999). Internal standards were made by adding 2nmol glutamate at the end of eachassay.

Ca²⁺-imaging experiments. For the Ca²⁺ imaging, the rat hippocampal cultures were prepared as described previously (Yan et al.,1999). The cells were plated on glass-bottom dishes (Iwaki, Tokyo,Japan) and maintained for 2 weeks. After 2 weeks of culture, themedium was changed to ACSF with 10 mM HEPES, pH 7.4, and the cellswere then loaded with 5 µM fura-2 AM for 40 min at room temperature.Then cells were washed with ACSF and incubated with 25 µM AP5,0.5 µM $omega$ -CgTx GVIA, and 10 µM Nifedipine, with or without 5 µMroscovitine to measure Ca²⁺ entry from the P/Q-type VDCC channels for 30 min at 37°C. Thecells were directly exposed to 50 mM KCl for 10 sec by a gravity-fed"sewer pipe" system (Yan et al., 1999), and fura-2 AM fluorescencewas recorded using a video image analysis system (AquaCosmos,Hamamatsu Photonics, Hamamatsu, Japan), with excitation alternativelyat 340 and 380 nm, and emission at 510 nm. Data from 20-30 individualcells were collected per experiment, and ensemble averages werecalculated for multiple experiments. Data acquisition was typicallyat 5 sec intervals and lasted for 10min.

Phosphorylation and binding assay. Complementary DNA encoding L_II-III (amino acids 724-983) of isoforms cloned from rat brain(rbA) of the $alpha$ _1A subunit of P/Q-type Ca²⁺ channel was cloned from a rat hippocampus cDNA library (Stratagene,La Jolla, CA) by PCR with oligonucleotides 5'-GAACTCACCAAGGATGAACAAG-3'and 5'-TCTGCGCTCCCTGTCATCGTG-3'. The PCR products were subclonedinto PCR-Blunt II-TOPO vector, and the sequence was confirmed.Then, the PCR products were cleaved with BamHI and XhoI and ligatedinto pGEX-6P (AmershamBiosciences).

Glutathione S-transferase (GST)-tagged proteins were expressed and purified as described previously (Lee et al., 1996). Finally,GST-fusion proteins were dialyzed with phosphate buffer. Phosphorylationreactions were performed in a basal buffer containing 20 mM MOPS,pH 7.4, 30 mM MgCl₂, 100 µM [ $gamma$ -³²P]ATP (300 dpm/pmol), and 1 mM dithiothreitol. GST-L_II-III wasincubated with each concentration of GST-Cdk5 and/or GST-p25 at32°C for 30min.

For phosphorylation time course experiments, 1 µM GST-L_II-III was incubated with both 2 µM GST-Cdk5 and GST-p25 at 32°C. Additional[ $gamma$ -³²P]ATP, GST-Cdk5, and GST-p25 were added to the time course reactionsat 60 min to test whether these reagents were limiting the maximalincorporation. The reactions were terminated by the addition ofboiling SDS sample buffer. After SDS-PAGE, gel drying, and autoradiography,the relevant gel slices were excised and Cerenkov-counted to determinetotal ³²P incorporation. Specific radioactivity in picomoles of [ $gamma$ -³²P]ATP was determined by counting diluted aliquots of the stock,and this conversion value was used to calculate moles of ³²P incorporated and the molar ratio of ³²P to GST-L_II-III.

For binding assay, GST-L_II-III proteins were incubated with purified bovine Cdk5/p25 (Lee et al., 1996) and/or 5 µM roscovitinein a basal buffer containing 100 µM ATP instead of 100 µM [ $gamma$ -³²P]-ATP for 1 hr at 32°C. After this, the complex was incubatedwith glutathione-Agarose (Sigma) for 1 hr at 4°C. The glutathione-Agarosewas replaced in a 10 ml column, and the column was washed withwashing buffer containing Tris-HCl, pH 7.4, 150 mM NaCl, and 0.4%Triton X-100 and was then washed with PBS once. Solubilized synaptosomeprotein (300 µg) was loaded on the column. The column was washedwith washing buffer containing Tris-HCl, pH 7.4, 150 mM NaCl,20 µM CaCl₂, and 0.1% Triton X-100 three times. After the proteincomplexes were collected with glutathione-Agarose, the complexwas denatured with boiled SDS-PAGE buffer and centrifuged. Then,the supernatants were used for Western blot analysis using anti-SNAP-25antibody (Transduction Laboratories, Lexington, KY), anti-synaptotagminI antibody (Santa Cruz Biotechnology), and anti-syntaxin 1 antibody(Calbiochem, San Diego, CA),respectively.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The effect of Cdk5 inhibitors, roscovitine and olomoucine, on EPSP slopes

Roscovitine is a potent, membrane-permeable, specific Cdk5 inhibitor in neurons (Meijer et al., 1997). To demonstrate whetherCdk5 regulates neurotransmission, hippocampal slices were incubatedwith 10 µM roscovitine, and the EPSP slopes were measured. Afterthe roscovitine application, the EPSP slope gradually increased(Fig. 1A). The EPSP slope reached a maximum (178 ± 10.2% of baseline)at 40 min after the roscovitine application. After washing outthe roscovitine, the enhanced EPSP slope gradually decreased.The EPSP slope returned to the baseline 50 min after the washout,suggesting that the effect of roscovitine on the EPSP slope wasreversible. To demonstrate the dose-dependent effect of roscovitineon the EPSP slopes, hippocampal slices were incubated with eachconcentration of roscovitine until the maximal EPSP was recorded.Roscovitine dose-dependently increased the EPSP slope, and theeffect was saturated at 10 µM (Fig. 1B). Olomoucine is also apotent inhibitor of Cdks (Vesely et al., 1994). However, the IC₅₀against Cdk5/p35 is >10-fold higher than that of roscovitine (Meijeret al., 1997). Olomoucine at <10 µM had no effect on the EPSPslope (Fig. 1C). However, application of 100 µM olomoucine significantlyincreased the EPSP slope (maximum 130 ± 7.8% of baseline). Theeffect of olomoucine was also reversible (data not shown). Thesedata suggest that Cdk5 inhibitors enhance neurotransmission.

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Figure 1. Cdk5 inhibitors enhanced the field EPSP slope. A, Hippocampal slices were perfused with 10 µM roscovitine for 35 min, and then the slices were washed out by perfusion with ACSF. Inset, Representative field EPSPs before and 40 min after the perfusion of roscovitine are shown. Calibration: 20 msec, 2 mV. B, Dose-dependent effect of roscovitine on maximum EPSPs. To record the maximum EPSP, each concentration of roscovitine was applied until the maximum and stable EPSP was recorded. Each column is the mean ± SEM values of five independent slices. The significance of differences was calculated by the Scheffe's test after ANOVA. *p < 0.05 and **p < 0.01 compared with the control slices (0 µM). C, Dose-dependent effect of olomoucine on the maximum EPSPs. The conditions of drug application were the same as those of roscovitine. Values were significantly different from the control slices (0 µM); *p < 0.05.

Roscovitine affects paired-pulse facilitation

To clarify that the effect of Cdk5 inhibitors on the neurotransmission is in presynapse or in postsynapse, we examined thepaired-pulse facilitation (PPF). PPF is a more transient formof presynaptic plasticity in which the second of two closely spacedstimuli elicits enhanced transmitter release, because of residualcalcium in the presynaptic terminal after the first stimulus (Zucker,1989). The PPF was markedly reduced in the roscovitine-perfusedhippocampal slices compared with the control slices when paired-pulsestimuli of 50-100 msec intervals were applied (Fig. 2). Thesedata suggest that roscovitine acts in the presynaptic terminaland regulates neurotransmission.

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Figure 2. Roscovitine reduced PPF in hippocampal slices. The hippocampal slices were incubated with each concentration of roscovitine (, 0 µM; $black-diamond$ , 1 µM; $open circle$ , 5 µM; $black-triangle$ , 10 µM) for 50 min, after which PPF was induced by two pulses of stimulation separated by intervals of 50, 100, 150, and 200 msec. Data show the ratios of the second EPSP slopes and the first EPSP slopes. The significance of difference was calculated by the Scheffe's test after ANOVA. *p < 0.05 and **p < 0.01 compared with the control slices (0 µM).

The expressions of Cdk5 and p35 in purified synaptosomes

To demonstrate whether both Cdk5 and p35 exist in the presynaptic terminal, we tested the expressions of Cdk5 and p35 in thepurified synaptosomes (Fig. 3). Subcellular fractionation showedthat Cdk5 was widely expressed, with no obvious concentrationin one fraction. In contrast, p35 was enriched in isolated nerveterminals (P3 and LP2 fractions) to approximately the same extentas an insoluble presynapse marker, synaptophysin. In purifiedsynaptosomes, Cdk5 existed in both the soluble (LS2) and insoluble(LP2) fractions. In contrast, p35 was expressed only in LP2 butnot seen in LS2, as with Amphiphysin, which tightly associatedwith the synaptic vesicles (Fig. 3). These results suggest thatCdk5 and its activator, p35, are expressed in the presynapticterminal and that p35 may be tightly associated with membranesor vesicles.

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Figure 3. Both Cdk5 and p35 were enriched in purified synaptosomes. Western blot analyses for Cdk5, p35, calmodulin kinase I (CaM KI, soluble presynapse fraction marker), and synaptophysin (insoluble presynapse fraction marker) of the rat brain subcellular fractions are shown. Each fraction is shown in Materials and Methods. H, Total homogenate; P2, crude synaptosomes; LP2, membrane fraction of the purified synaptosomes; LS2, cytosolic fraction of the purified synaptosomes.

Roscovitine upregulates glutamate release from synaptosomes

The present data show that Cdk5 inhibitors block the Cdk5 activity in the presynaptic terminal, resulting in the inductionof neurotransmission. These data lead to a hypothesis that Cdk5regulates neurotransmitter release. We demonstrated the effectof roscovitine on glutamate release from the synaptosomes (Fig.4). Preincubation of the synaptosomes with roscovitine (5 or 10µM) resulted in a significant increase in the 4AP-evoked glutamaterelease compared with the control (5 µM roscovitine, 7.2 ± 0.4nmol/mg per 4 min; 10 µM roscovitine, 9.0 ± 1.7 nmol/mg per 4min; control, 5.5 ± 1.1 nmol/mg per 4 min). This result indicatesthat Cdk5 inhibits neurotransmitter release.

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Figure 4. The effect of roscovitine on Ca²⁺-dependent glutamate release from synaptosomes prepared from rat brains in response to membrane depolarization with 1 mM 4-AP (n = 5). Data represent the mean ± SEM values of five independent experiments. The synaptosomes were incubated with each concentration of roscovitine (, 0 µM; $open circle$ , 5 µM; $black-triangle$ , 10 µM) for 30 min, and then 4-AP was added at 0 sec. Values significantly different from the control synaptosomes (0 µM roscovitine) are indicated (*p < 0.05; **p < 0.01; Scheffe's test).

Roscovitine enhances the activation of P/Q-type voltage-dependent calcium channel

Bibb et al. (1999) have reported that the application of roscovitine enhanced whole-cell Ca²⁺ current in striatum neurons. These data and our results leadto a hypothesis that Cdk5 may enhance the activity of presynapticVDCC, resulting in increased neurotransmitter release. In thecultured hippocampal neurons, N- and P/Q-type VDCCs predominantlymediate excitatory synaptic transmission (Wheeler et al., 1996;Reid et al., 1997). Coapplication of $omega$ -CgTx GVIA and $omega$ -Aga IVA,which are specific inhibitors of N-type and P/Q-type VDCCs, respectively,completely blocked the EPSP slope (>98%) in the hippocampal slices,suggesting that N- and P/Q-type VDCCs specifically regulated neurotransmitterrelease in the hippocampal slices (Fig. 5A). To investigate whetherroscovitine affects the activity of theses VDCCs, its effect oneach channel-dependent EPSP slope was examined. An applicationof $omega$ -CgTx GVIA reduced the EPSP slope by 44 ± 3.6%. After theEPSP slopes became stable, 5 µM roscovitine was applied. An applicationof roscovitine gradually induced the EPSP slope by 31.5 ± 4.9%(Fig. 5B). In contrast, $omega$ -Aga IVA, a specific blocker of P/Q-typeVDCC, significantly reduced the EPSP slope (21 ± 8.1%) 25 minafter the application), and an application of roscovitine hadno effect on the $omega$ -Aga IVA-reduced EPSP slope (Fig. 5C). Thesedata suggest that roscovitine specifically enhances P/Q-type VDCCactivity.

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Figure 5. The effect of roscovitine on the EPSP slope in the presence of $omega$ -CgTx GVIA and $omega$ -Aga IVA. Hippocampal slices were incubated with 1 µM $omega$ -CgTx GVIA and 0.5 µM $omega$ -Aga IVA (A), 1 µM $omega$ -CgTx GVIA (B), or 0.5 µM $omega$ -Aga IVA (C). Then, 10 µM roscovitine was applied after recording stable EPSP slopes. The drugs were perfused continuously until the end of the experiment.

We further demonstrated the effect of roscovitine on calcium entry from the P/Q-type VDCC channel using Ca²⁺ imaging. To record the specific Ca²⁺ influx from the P/Q-type VDCC channel, the hippocampal neuronswere incubated with 25 µM AP5, 0.5 µM $omega$ -CgTx GVIA, and 10 µM Nifedipine,which were specific inhibitors of other types of VDCCs and NMDAreceptor. The cells were then stimulated by high K⁺ in the presence or absence of roscovitine. In the control neurons,the intracellular Ca²⁺ concentration increased after the high K⁺ stimulation (Fig. 6A). The increased Ca²⁺ influx gradually decreased after washing out, and Ca²⁺ entry was not recorded 3 min after the high K⁺ stimulation. An application of roscovitine significantly enhancedthe maximal Ca²⁺ influx from the P/Q-type VDCC channel compared with that in thecontrol neurons (Fig. 6A,B). The enhanced Ca²⁺ influx was rapidly decreased after washing out KCl (Fig. 6A).A significant Ca²⁺ influx was observed 20 sec after the high K⁺ stimulation but not observed 40 sec after the stimulation (Fig.6B). Moreover, $omega$ -Aga IVA, a specific blocker of the P/Q-type VDCCblocker, significantly reduced the roscovitine-induced Ca²⁺ influx from P/Q-type VDCC. These results directly showed thatthe inhibition of Cdk5 activity enhanced the Ca²⁺ influx from the P/Q-type VDCC channel.

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Figure 6. Roscovitine enhanced Ca²⁺ influx from P/Q-type VDCCs. A, Primary cultured hippocampal neurons were incubated with $omega$ -CgTx GVIA, Nifedipine, and AP-5 to measure the Ca²⁺ influx specific from P/Q-type VDCCs for 30 min. Roscovitine was also applied 30 min before depolarization. The cells were exposed with 50 mM KCl for 10 sec, and fura-2 AM fluorescence was recorded using a video image analysis system (AquaCosmos, Hamamatsu Photonics), with excitation alternatively at 340 and 380 nm, and emission at 510 nm (, control; , 5 µM roscovitine; $open circle$ , roscovitine and $omega$ -Aga IVA). B, Comparison of Ca²⁺ influx from P/Q-type VDCCs at 20 and 40 sec after depolarization. Data from 20-30 individual cells were collected per experiment, and ensemble averages were calculated for multiple experiments (n > 30). Data were analyzed using ANOVA followed by planned comparisons of the multiple conditions. *p < 0.01.

Cdk5/p35-dependent phosphorylation of L_II-III of rbA isoform of the $alpha$ _1A subunit of P/Q-type Ca²⁺ channels and the regulation of the interaction with SNAP-25 and synaptotagmin

What is the mechanism of the induction of the activity of P/Q-type VDCCs by Cdk5-specific inhibitors? P/Q-type Ca²⁺ channels contain pore-forming $alpha$ _1A subunits in association with $beta$ and $alpha$ ₂ subunits (Catterall, 1998). Thedistinct $alpha$ _1A isoforms cloned from rat brain (rbA) and rabbit brain(BI) have synprint sites with different specificities for interactionswith plasma-membrane SNARE proteins, such as SNAP-25, synaptotagmin,and syntaxin (Catterall, 1998; Seagar and Takahashi, 1998). Disruptinginteractions between these SNARE proteins and Ca²⁺ channels inhibits neurotransmission, demonstrating that suchinteraction is required for efficient neurotransmitter release(Catterall, 1998). Phosphorylation of the synaptic protein interactionsite on N-type calcium channels inhibits the interaction withSNAP-25 and syntaxin, resulting in the inhibition of channel activity(Yokoyama et al., 1997). These results lead to a hypothesis thatCdk5 directly phosphorylates the $alpha$ _1A isoform of P/Q-type VDCCs,resulting in the inhibition of the interaction with SNAREproteins.

To clarify the hypothesis, we demonstrated whether Cdk5/p25 phosphorylated L_II-III (synprint site) of the rbA isoform of the $alpha$ _1A subunit (Fig. 7). Cdk5/p25 phosphorylated synprint polypeptides(Fig. 7A). Stoichiometric analysis revealed that the synprint $alpha$ _1A was a good substrate for Cdk5/p25, with a maximal stoichiometryof 1.5 mol/mol. Although the correlation of stoichiometry measurementswith the precise number of phosphorylated residues is not possiblefrom this analysis, there are clearly multiple good substratesites for Cdk5 in the synprint peptide. The rbA isoform of $alpha$ _1Abinds SNAP-25 in a calcium-independent manner. In contrast, thebinding of the isoform with synaptotagmin is calcium dependent,with maximum binding at 10-30 µM (Catterall, 1998). Therefore,we incubated phospho- and dephospho-GST-L_II-III proteins withsynaptosomes in HEPES buffer with 20 µM calcium. Phosphorylationof the synprint peptides blocked the binding of the peptides withboth SNAP-25 and synaptotagmin I (Fig. 7C). These inhibitionsof the phosphorylation-dependent binding with SNAP-25 and synaptotagminI were blocked by an application of roscovitine (Fig. 7C). Onthe other hand, syntaxin I did not bind to the synprint peptidesof P/Q-type VDCCs regardless of the phosphorylation and dephosphorylation(data not shown). These data suggest that Cdk5/p25 phosphorylatesL_II-III of the rbA isoform of the $alpha$ _1A subunit of P/Q-type VDCCs,resulting in the inhibition of the association with SNAP-25 andsynaptotagmin, and roscovitine blocked the Cdk5-dependent inhibitionof these associations. In contrast, Cdk5/p25 did not phosphorylateL_II-III (718-963) of the $alpha$ _1B subunit of rat N-type calcium channel,which is phosphorylated by protein kinase A and CaM KII, and regulatedthe interaction with SNARE proteins (data not shown).

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Figure 7. Cdk5/p35-dependent phosphorylation of L_II-III of rbA isoform of the $alpha$ _1A subunit of P/Q-type Ca²⁺ channels and the regulation of the interaction with SNARE proteins. A, Purified GST-L_II-III peptides were incubated with GST-Cdk5 or each concentration of GST-p25 at 32°C for 30 min. GST-L_II-III peptides were phosphorylated by GST-Cdk5 correlating with GST-p25 concentration. B, Stoichiometry of phosphorylation for GST-L_II-III. Polypeptides of GST-L_II-III were phosphorylated with GST-Cdk5/p25 for the indicated time periods. C, Phosphorylation of GST-L_II-III inhibited the interaction with SNAP-25 and synaptotagmin. Polypeptides of GST-L_II-III were incubated with purified Cdk5/p25 or 5 µM roscovitine. Then the complex was incubated with glutathione-Agarose. The glutathione-Agarose was replaced in a 10 ml column. After the column was washed, the solubilized synaptosome protein (300 µg) in HEPES buffer with 20 µM CaCl₂ was loaded on the column, and the column was washed. After the protein complexes were collected with glutathione-Agarose, the complex was denatured with boiled SDS-PAGE buffer. The supernatants were then used for Western blot analysis using anti-SNAP-25 antibody, anti-synaptotagmin I antibody, and anti-syntaxin I antibody, respectively. Top panel, Result of Western blot analysis with anti-SNAP-25 antibody. Middle panel, Result of Western blot analysis with anti-synaptotagmin I antibody. Bottom panel, After the complex was collected with glutathione-Agarose, the proteins were separated in SDS-PAGE gel. Then, the gel was stained by Coomassie blue, and the polypeptides of GST-L_II-III were visualized.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

These results provide four important findings as follows. First, Cdk5 inhibitors enhanced neurotransmission in hippocampalslices. Second, the regulation of neurotransmission by Cdk5 isperformed in the presynaptic terminal. Third, Cdk5 inhibitorsenhanced Ca²⁺ entry from P/Q-type VDCCs. Fourth, Cdk5/p25 phosphorylated theintracellular loop connecting domains II and III correspondingto amino acid residues 724 and 981 of the rbA isoform of the $alpha$ _1Asubunit of P/Q-type Ca²⁺ channels, and the phosphorylation inhibited the interaction withSNAP-25 andsynaptotagmin.

Cdk5 is a multifunctional kinase in the developing, adult, and aging brain

Cdk5/p35 plays an important role in neuronal migration and differentiation in immature neurons (Nikolic et al., 1996; Chaeet al., 1997). The complex of Cdk5/p35 is colocalized with Pak1in the axonal growth cone, and the kinase downregulates Pak1 kinaseactivity (Nikolic et al., 1998), resulting in neurite outgrowth.Moreover, it has recently been reported that Cdk5 phosphorylatedNUDEL, a novel LIS-1-interacting protein in the growth cone (Niethammeret al., 2000). The inhibition of Cdk5 activity with roscovitinealters NUDEL localization and its association with the dyneincomplex, resulting in the alteration of neuronal migration (Niethammeret al., 2000). These data suggest that in the immature neuron,the Cdk5/p35 complex localizes in the growth cones and regulatesneuronal migration, differentiation, andsynaptogenesis.

In the mature neuron, in contrast, Cdk5 is expressed in the presynaptic terminals (Matsushita et al., 1996) (present results),and the enzyme phosphorylates presynaptic proteins such as Munc18(Shuang et al., 1998), Synapsin I (Jovanovic et al., 1996), andAmphiphysin I (Rosales et al., 2000). These data suggest thatCdk5 changes localization from the growth cone to the axon (presynapticterminal) and regulates neurotransmitter release in the adultbrain.

Moreover, recent studies have shown that in Alzheimer's brain, p35 is truncated to p25, and the complex of Cdk5 and p25 leadsto mislocalization of the kinase to the soma, resulting in neuronaldegeneration (Patrick et al., 1999; Lee et al., 2000). These studiessuggest that Cdk5 has multiple and different functions in thedeveloping, adult, and aging neuron and that the change in localizationof Cdk5 is an important mechanism underlying the different functionsofCdk5.

The mechanism of Cdk5-dependent regulation of P/Q-type VDCC activity

Our data first showed that Cdk5 inhibitors enhanced neurotransmitter release via enhancement of the activity of P/Q-type VDCCs.Moreover, we showed that Cdk5 phosphorylated the L_II-III of P/Q-typecalcium channels, and the phosphorylation inhibited the interactionwith SNAP-25 andsynaptotagmin.

The synprint site on the N-type VDCC $alpha$ _1B subunit is phosphorylated, and the phosphorylation inhibits interaction with SNAREproteins such as syntaxin and SNAP-25 (Yokoyama et al., 1997).We demonstrated that Cdk5 phosphorylated the synprint site onN-type VDCCs; however, Cdk5 did not phosphorylate the L_II-IIIpeptides of the VDCCs. Immunocytochemical and pharmacologicalexperiments provide evidence that N-type VDCCs regulate neurotransmitterrelease at both peripheral and central synapses (Westenbroek etal., 1992). In contrast, P/Q-type VDCCs are present in high densityat central synapses (Westenbroek et al., 1995), and transmitterrelease primarily requires P/Q-type channels, with N-type channelsplaying a secondary role (Catterall, 1998). The present resultsshowed that the inhibition of the EPSP slope by $omega$ -Aga IVA, a specificblocker of P/Q-type VDCCs, is much greater than that by $omega$ -CgTxGVIA, a specific blocker of N-type VDCCs in the hippocampus. Theseresults suggest that Ca²⁺ entry from P/Q-type VDCCs might be more important in regulatingneurotransmitter release than that from N-type VDCCs in thehippocampus.

The synaptic vesicle proteins synaptotagmin and synaptobrevin/vesicle-associated membrane protein bind to the synaptic plasmamembrane SNARE proteins syntaxin and SNAP-25 to form a core compleximplicated in synaptic vesicle docking and membrane fusion (Hansonet al., 1997). This core complex associates with N-type and P/Q-typeVDCCs via L_II-III (Catterall, 1998). Disruption of interactionsbetween SNARE proteins and these Ca²⁺ channels inhibits neurotransmission, demonstrating that suchinteraction is required for efficient neurotransmitter release(Catterall, 1998). These previous data agree with our presentresults that Cdk5 phosphorylated L_II-III of P/Q-type VDCCs, resultingin the disruption of the interaction with SNAP-25 and synaptotagminI. These data suggest that Cdk5 might downregulate the activityof the rbA isoform of P/Q-type VDCCs through phosphorylation ofL_II-III of the calcium channel and inhibition of the interactionwith SNARE proteins. The present results showed that syntaxinI did not bind to L_II-III of the rbA isoform of P/Q-type VDCCsregardless of the phosphorylation and dephosphorylation. Thesedata agree with the previous results that the rbA isoform of P/Q-typeVDCCs binds SNAP-25 but not syntaxin (Rettig et al., 1996; Zhonget al., 1999).

Voltage-dependent calcium channels, which are involved in neurotransmitter release, are strictly regulated by the activityof the specific SNARE proteins (Sheng et al., 1996; Catterall,1998). The interaction of N-type Ca²⁺ channels with syntaxin and SNAP-25 is Ca²⁺ dependent and regulated by protein phosphorylation (Yokoyamaet al., 1997). The interaction of the calcium channels with SNAREproteins may be regulated by phosphorylation and dephosphorylation.Cdk5 may be one of the most important kinases that regulate neurotransmitterrelease.

In conclusion, we have shown that both Cdk5 and p35 are abundant in the presynaptic terminals and that Cdk5 inhibitors enhanceneurotransmitter release. The induction of the neurotransmitterrelease by Cdk5 inhibitors is caused by the regulation of P/Q-typevoltage-dependent Ca²⁺ channel activity. Our results indicate that Cdk5 regulates theneurotransmitter release in the presynaptic terminals of the adultbrain.

  FOOTNOTES

Received Oct. 31, 2001; revised Jan. 23, 2002; accepted Jan. 23, 2002.

This work was supported by a Grant-in-Aid for Scientific Research from the Ministry of Education, Science, Sports and Cultureof Japan and by Industrial Technology Research Grant Program in'01 from New Energy and Industrial Technology Development Organization,Japan. We are grateful to Dr. L. Meijer for roscovitine and toDr. A. Nairn for CaM KIantibodies.

Correspondence should be addressed to Kazuhito Tomizawa, Department of Physiology, Okayama University Graduate School of Medicineand Dentistry, Shikata-cho 2-5-1, Okayama 700-8558, Japan. E-mail:tomikt{at}md.okayama-u.ac.jp.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Bibb JA, Snyder GL, Nishi A, Yan Z, Meijer L, Fienberg AA, Tsai LH, Kwon YT, Girault JA, Czernik AJ, Huganir RL, Hemmings Jr HC, Nairn AC, Greengard P (1999) Phosphorylation of DARPP-32 by Cdk5 modulates dopamine signalling in neurons. Nature 402:669-671[Medline].
Catterall WA (1998) Structure and function of neuronal Ca²⁺ channels and their role in neurotransmitter release. Cell Calcium 24:307-323[Web of Science][Medline].
Chae T, Kwon YT, Bronson R, Dikkes P, Li E, Tsai LH (1997) Mice lacking p35, a neuronal specific activator of Cdk5, display cortical lamination defects, seizures, and adult lethality. Neuron 18:29-42[Web of Science][Medline].
Dunlap K, Luebke JI, Turner TJ (1995) Exocytotic Ca²⁺ channels in mammalian central neurons. Trends Neurosci 18:89-98[Web of Science][Medline].
Floyd SR, Porro EB, Slepnev VI, Ochoa GC, Tsai LH, De Camilli P (2001) Amphiphysin binds the cdk5 regulatory subunit p35 and is phosphorylated by cdk5 and cdc2. J Biol Chem 276:8104-8110[Abstract/Free Full Text].
Hanson PI, Heuser JE, Jahn R (1997) Neurotransmitter release: four years of SNARE complexes. Curr Opin Neurobiol 7:310-315[Web of Science][Medline].
Huttner WB, Schiebler W, Greengard P, De Camilli P (1983) Synapsin I (protein I), a nerve terminal-specific phosphoprotein. III. Its association with synaptic vesicles studied in a highly purified synaptic vesicle preparation. J Cell Biol 96:1374-1388[Abstract/Free Full Text].
Jovanovic JN, Benfenati F, Siow YL, Sihra TS, Sanghera JS, Pelech SL, Greengard P, Czernik AJ (1996) Neurotrophins stimulate phosphorylation of synapsin I by MAP kinase and regulate synapsin I-actin interactions. Proc Natl Acad Sci USA 93:3679-3683[Abstract/Free Full Text].
Kim DK, Catterall WA (1997) Ca²⁺-dependent and -independent interactions of the isoforms of the $alpha$ _1A subunit of brain Ca²⁺ channels with presynaptic SNARE proteins. Proc Natl Acad Sci USA 94:14782-14786[Abstract/Free Full Text].
Lee K-Y, Rosales JL, Tang D, Wang JH (1996) Interaction of cyclin-dependent kinase 5 (Cdk5) and neuronal Cdk5 activator in bovine brain. J Biol Chem 271:1538-1543[Abstract/Free Full Text].
Lee M-S, Kwon YT, Li M, Peng J, Friedlander RM, Tsai L-H (2000) Neurotoxicity induces cleavage of p35 to p25 by calpain. Nature 405:360-364[Medline].
Lew J, Wang JH (1995) Neuronal cdc2-like kinase. Trends Biochem Sci 20:33-37[Web of Science][Medline].
Lew J, Winkfein RJ, Huang QQ, Qi Z, Aebersold R, Hunt T, Wang JH (1994) Neuronal cdc2-like kinase is a complex of cyclin-dependent kinase 5 and a novel brain-specific regulatory subunit. Nature 371:423-426[Medline].
Lu Y-F, Tomizawa K, Moriwaki A, Hayashi Y, Tokuda M, Itano T, Hatase O, Matsui H (1996) Calcineurin inhibitors, FK506 and cyclosporin A, suppress the NMDA receptor-mediated potentials and LTP, but not depotentiation in the rat hippocampus. Brain Res 729:142-146[Medline].
Lu Y-F, Kandel ER, Hawkins RD (1999) Nitric oxide signaling contributes to late-phase LTP and CREB phosphorylation in the hippocampus. J Neurosci 19:10250-10261[Abstract/Free Full Text].
Matsubara M, Kusubata M, Ishiguro K, Uchida T, Titani K, Taniguchi H (1996) Site-specific phosphorylation of synapsin I by mitogen-activated protein kinase and Cdk5 and its effects on physiological functions. J Biol Chem 271:21108-21113[Abstract/Free Full Text].
Matsushita M, Tomizawa K, Lu YF, Moriwaki A, Tokuda M, Itano T, Wang JH, Osamu H, Matsui H (1996) Distinct cellular compartment of cyclin-dependent kinase 5 (Cdk5) and neuron-specific Cdk5 activator protein (p35^nck5a) in the developing rat cerebellum. Brain Res 734:319-322[Medline].
Meijer L, Borgne A, Mulner O, Chong JP, Blow JJ, Inagaki N, Inagaki M, Delcros JG, Moulinoux JP (1997) Biochemical and cellular effects of roscovitine, a potent and selective inhibitor of the cyclin-dependent kinases cdc2, cdk2 and cdk5. Eur J Biochem 243:527-536[Web of Science][Medline].
Moriwaki A, Lu YF, Hayashi Y, Tomizawa K, Tokuda M, Itano T, Hatase O, Matsui H (1996) Immunosuppressant FK506 prevents mossy fiber sprouting induced by kindling stimulation. Neurosci Res 25:191-194[Medline].
Nikolic M, Dudek H, Kwon YT, Ramos YF, Tsai LH (1996) The cdk5/p35 kinase is essential for neurite outgrowth during neuronal differentiation. Genes Dev 10:816-825[Abstract/Free Full Text].
Nikolic M, Chou MM, Lu W, Mayer BJ, Tsai LH (1998) The p35/Cdk5 kinase is a neuron-specific rac effector that inhibits Pak1 activity. Nature 395:194-198[Medline].
Niethammer M, Smith DS, Ayala R, Peng J, Ko J, Lee M-S, Morabito M, Tsai LH (2000) NUDEL is a novel Cdk5 substrate that associates with LIS1 and cytoplasmic dynein. Neuron 28:367-711.
Patrick GN, Zukerberg L, Nikolic M, de la Monte S, Dikkes P, Tsai LH (1999) Conversion of p35 to p25 deregulates Cdk5 activity and promotes neurodegeneration. Nature 402:615-622[Medline].
Reid CA, Clements JD, Bekkers JM (1997) Nonuniform distribution of Ca²⁺ channel subtypes on presynaptic terminals of excitatory synapses in hippocampal cultures. J Neurosci 15:2738-2745.
Rettig J, Sheng ZH, Kim DK, Hodson CD, Snutch TP, Catterall WA (1996) Isoform-specific interaction of the alpha1A subunits of brain Ca²⁺ channels with the presynaptic proteins syntaxin and SNAP-25. Proc Natl Acad Sci USA 93:7363-7368[Abstract/Free Full Text].
Rosales JL, Nodwell MJ, Johnston RN, Lee KY (2000) Cdk5/p25^nck5a interaction with synaptic proteins in bovine brain. J Cell Biochem 78:151-159[Medline].
Seagar M, Takahashi M (1998) Interactions between presynaptic calcium channels and proteins implicated in synaptic vesicle trafficking and exocytosis. J Bioenerg Biomembr 30:347-356[Web of Science][Medline].
Sheng ZH, Rettig J, Takahashi M, Catterall WA (1996) Calcium-dependent interaction of N-type calcium channels with the synaptic core complex. Nature 379:451-454[Medline].
Shuang R, Zhang L, Fletcher A, Groblewski GE, Pevsner J, Stuenkel EL (1998) Regulation of Munc-18/syntaxin 1A interaction by cyclin-dependent kinase 5 in nerve endings. J Biol Chem 273:4957-4966[Abstract/Free Full Text].
Stula T, Xiao-Xian H, Cavazos J, Scott G (1988) Synaptic reorganization in the hippocampus induced by abnormal functional activity. Science 239:1147-1150[Abstract/Free Full Text].
Tang D, Yeung J, Li K-Y, Matsushita M, Tomizawa K, Matsui H, Hatase O, Wang JH (1995) An isoform of neuronal cyclin-dependent kinase 5 (Cdk5) activator. J Biol Chem 270:26897-26903[Abstract/Free Full Text].
Tomizawa K, Matsui H, Matsushita M, Lew J, Tokuda M, Itano T, Konishi R, Wang JH, Hatase O (1996) Localization and developmental changes in the neuron-specific cyclin-dependent kinase 5 activator (p35^nck5a) in the rat brain. Neuroscience 74:519-529[Web of Science][Medline].
Tomizawa K, Cai X-H, Moriwaki A, Matsushita M, Matsui H (2000) Involvement of cyclin-dependent kinase 5/p35^nck5a in the synaptic reorganization of the rat hippocampus during kindling progression. Jpn J Physiol 50:525-532[Medline].
Tsai LH, Takahashi T, Caviness Jr V, Harlow E (1993) Activity and expression pattern of cyclin-dependent kinase 5 in the embryonic mouse nervous system. Development 119:1029-1040[Abstract].
Tsai LH, Deialle I, Caviness Jr V, Chae T, Harlow E (1994) p35, a neuronal specific regulatory subunit of the cdk5 kinase. Nature 371:419-423[Medline].
Vesely J, Havlicek L, Strnad M, Blow JJ, Donella-Deana A, Pinna L, Letham DS, Kato J, Detivaud L, Leclerc S, Meijer L (1994) Inhibition of cyclin-dependent kinases by purine analogues. Eur J Biochem 224:771-786[Web of Science][Medline].
Vinje ML, Valø ET, Røste GK, Berg-Johnsen J (1999) Measured increase in intracellular Ca2+ during stimulated release of endogenous glutamate from human cerebrocortical synaptosomes. Brain Res 843:199-201[Medline].
Westenbroek RE, Hell JW, Warner C, Dubel SJ, Snutch TP, Catterall WA (1992) Biochemical properties and subcellular distribution of an N-type calcium channel $alpha$ 1 subunit. Neuron 9:1099-1115[Web of Science][Medline].
Westenbroek RE, Sakurai T, Elliott EM, Hell JW, Starr TVB, Snutch TP, Catterall WA (1995) Immunochemical identification and subcellular distribution of the $alpha$ 1A subunits of brain calcium channels. J Neurosci 15:6403-6418[Abstract/Free Full Text].
Wheeler DB, Randall A, Tsien RW (1996) Change in action potential duration alters reliance of excitatory synaptic transmission on multiple types of Ca²⁺ channels in rat hippocampus. J Neurosci 16:2226-2237[Abstract/Free Full Text].
Yan Z, Hsieh-Wilson L, Feng J, Tomizawa K, Allen PB, Feinberg AA, Nairn AC, Greengard P (1999) Protein phosphatase 1 modulation of neostriatal AMPA channels: regulation by DARPP-32 and spinophilin. Nat Neurosci 2:13-17[Web of Science][Medline].
Yokoyama CT, Sheng ZH, Catterall WA (1997) Phosphorylation of the synaptic protein interaction site on N-type calcium channels inhibits interactions with SNARE proteins. J Neurosci 17:6929-6938[Abstract/Free Full Text].
Zhong H, Yokoyama CT, Scheuer T, Catterall WA (1999) Reciprocal regulation of P/Q-type Ca2+ channels by SNAP-25, syntaxin and synaptotagmin. Nat Neurosci 2:939-941[Web of Science][Medline].
Zucker RS (1989) Short-term synaptic plasticity. Annu Rev Neurosci 12:13-31[Web of Science][Medline].

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