Potassium Current Development and its Linkage to Membrane Expansion During Growth of Cultured Embryonic Mouse Hippocampal Neurons: Sensitivity to Inhibitors of Phosphatidylinositol 3-Kinase and Other Protein Kinases

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The Journal of Neuroscience, August 15, 1998, 18(16):6261-6278

Potassium Current Development and its Linkage to Membrane Expansion During Growth of Cultured Embryonic Mouse Hippocampal Neurons: Sensitivity to Inhibitors of Phosphatidylinositol 3-Kinase and Other Protein Kinases
Rui-Lin Wu, Donna M. Butler, and Michael E. Barish
Division of Neurosciences, Beckman Research Institute of the City of Hope, Duarte, California 91010

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Hippocampal pyramidal neurons express three major voltage-dependent potassium currents, I_A, I_D, and I_K. During hippocampaldevelopment, I_A, the rapidly activating and inactivating transientpotassium current, is detected soon after pyramidal neurons canbe morphologically identified. Appearance of I_A in developingpyramidal neurons is dependent on contact with cocultured astroglialcells; cultured pyramidal neurons not in contact with astroglialcells have reduced membrane area and I_A (Wu and Barish, 1994).
We have examined intracellular signaling pathways that could contribute to the regulation of I_A development by probing developingpyramidal neurons with kinase inhibitors. We observed that exposureto LY294002 or wortmannin, inhibitors of phosphatidylinositol(PI) 3-kinase, reduced somatic cross-sectional area, neurite outgrowth,whole-cell capacitance, I_A amplitude and density (amplitude normalizedto membrane area), and immunoreactivity for Kv4.2 and/or Kv4.3(potassium channel subunits likely to be present in the channelscarrying I_A). In contrast, exposure to ML-9 or KN-62, inhibitorsof myosin light chain kinase or Ca²⁺-calmodulin-dependent protein kinase II (CaMKII), reduced membranearea and I_A amplitude but did not affect I_A density or Kv4.2/3immunoreactivity to the same extent as inhibitors of PI 3-kinase.Unexpectedly, exposure to bisindolymaleimide I or calphostin C,inhibitors of protein kinase C (PKC), did not affect membranearea or potassium current development.
Our data suggest that PI 3-kinases regulate both A-type potassium channel synthesis and plasmalemmal insertion of vesiclesbearing these potassium channels. CaMKII appears to regulate fusionof channel-bearing vesicles with the plasmalemma and myosin lightchain kinase to regulate centripetal transport of channel-bearingvesicles from the Golgi. We further suggest that astroglial cellsexert their influence on pyramidal neuron development throughactivation of PI 3-kinases.

Key words: hippocampus; development; excitability; potassium channels; I_A; I_D; I_K; membrane expansion; neurite outgrowth; phosphatidylinositol 3-kinase; calcium-calmodulin-dependent protein kinase II; myosin light chain kinase

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Hippocampal pyramidal neurons display three major voltage-dependent potassium currents (Storm, 1990), I_A, I_D, and I_K. I_A isa rapidly activating and inactivating voltage-gated potassiumcurrent that influences the subthreshold electrical behavior ofneurons (Connor and Stevens, 1971a,b). It is a particularly importantregulator of postsynaptic efficacy and dendritic excitabilityin pyramidal neurons (Hoffman et al., 1997). Physiological evidencesuggests that the Shal-related potassium channel subunits Kv4.2and/or Kv4.3 (Serôdio et al., 1996; Tsaur et al., 1997) are likelyto be components of the dendritic potassium channels carryingI_A in hippocampal neurons (Serôdio et al., 1994; Keros and McBain,1997; Johns et al., 1997), and immunocytochemical evidence indicatesthat Kv4.2 and/or Kv4.3 protein is localized to the somatic anddendritic compartments of hippocampal pyramidal neurons (Shenget al., 1992; Maletic-Savatic et al., 1995b; Tsaur et al., 1997;see below). Control of the insertion of these channels into dendriticmembrane is thus critical for tuning the integrative propertiesof pyramidal neuron dendrites.

I_A is detected early in the development of hippocampal pyramidal neurons, and I_A amplitude increases rapidly during the lateembryonic-early postnatal developmental period (Ficker and Heinemann,1992; Spigelman et al., 1992; Wu and Barish, 1992). One factorinfluencing the development of I_A in pyramidal neurons in dissociatedcell culture is contact of individual neurons with coculturedastroglial cells (Wu and Barish, 1994; see also Barish, 1995).Pyramidal neurons in contact with astroglial cells have greatermembrane area and a prominent I_A; pyramidal neurons not in contactwith astroglial cells have reduced membrane area and are deficientin I_A. This I_A deficit is seen in both I_A amplitude and in I_Adensity (amplitude normalized to membrane area). We have suggestedthat glial-derived signals, transmitted by cell-cell contact orshort-range diffusion, promote insertion of surface membrane enrichedin A-type potassium channels. We have hypothesized, therefore,that astroglial contact is promoting two parallel processes: (1)membrane expansion and neurite outgrowth and (2) synthesis, transport,and/or insertion of A-type potassium channels into areas of expandingplasmalemma.

In the present experiments we have examined second messenger systems that may regulate I_A development by using selective inhibitorsto probe kinases implicated in receptor signaling, and/or controlof membrane trafficking and exocytosis: (1) phosphatidylinositol(PI) 3-kinase, (2) myosin light chain kinase, (3) Ca²⁺-calmodulin-dependent protein kinase II (CaMKII), and (4) proteinkinase C (PKC), as well as (5) multiple kinases (using less selectivekinase inhibitors). We made measurements of membrane area, amplitudesand densities of the three voltage-gated potassium currents, andin some particularly interesting cases, the subcellular distributionsof Kv4.2 and/or Kv4.3 potassium channel subunits.

Our results indicate that in developing hippocampal pyramidal neurons PI 3-kinases have a central role in regulating synthesisof the channels carrying I_A and in regulating insertion of vesiclesbearing these and other potassium channels into the expandingplasmalemma. Our data also indicate that CaMKII regulates fusionof channel-bearing vesicles with the plasmalemma, and that myosinlight chain kinase influences centripetal transport of channel-bearingvesicles from the Golgi. We further suggest that PI 3-kinasesmay mediate the effects of astroglial cells on dendritic growthand I_A development.

Some of these results have previously been published in abstract form (Wu and Barish, 1996).

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Dissociated cell culture. Embryonic Swiss Webster mice were removed under sterile conditions from pregnant female mice afteranesthesia (by halothane inhalation) and cervical dislocation,using procedures meeting National Institutes of Health guidelines.Hippocampi were removed from fetuses and dissociated using papain(Worthington, Freehold, NJ), as described in Wu and Barish (1992).Dissociated cells were plated at ~22,100 cells/cm² (25,000 cells per coverslip) onto poly-D-lysine-coated and laminin-coated12 mm-diameter glass coverslips (Assistent; Carolina Biological,Burlington, NC) in a 150 µl bubble of medium (described below)supplemented to 10% total serum. After allowing 2 hr for the cellsto settle, each 35 mm-diameter Petri dish containing three coverslipswas flooded with 1 ml of low-serum (2% total) medium.

Low-serum medium, which facilitates growth of neurons on a sparse underlying layer of astroglial cells, consisted of MEM supplementedwith 1 mM glutamine, B-27 additive (1:50; Brewer et al., 1993),1% fetal bovine serum, and 1% horse serum, with total glucoseincreased to 25 mM. No antibiotics were used, and an antimitotic,ara-C (10 µM), was added after 12-48 hr to control astroglialproliferation as desired. All components of tissue culture media,including sera and B-27, were purchased from Life Technologies(Gaithersburg, MD).

Electrophysiology. Procedures for whole-cell voltage clamp of voltage-gated potassium current were standard and describedin previous publications (Wu and Barish, 1992, 1994). The internaland external solutions were designed to minimize contributionsof currents other than the three voltage-gated potassium currentsunder consideration.

Whole-cell recordings were made using an Axopatch 1B (Axon Instruments, Foster City, CA) amplifier modified for phase lagseries resistance compensation and a TL-1/pClamp6 (Axon Instruments)data acquisition and analysis system. Currents were filtered inthe Axopatch amplifier at 1 kHz ( $-$ 3 db; 4-pole Bessel filter).Currents linear with membrane voltage (leak currents and residualcapacity transients) were subtracted using a P/ $-$ 4 voltage stepprotocol. Voltages were corrected for junction potentials betweenelectrode and bath solutions, and series resistance was correctedat the amplifier to ~80%. Recordings were made at room temperature(22-24°C).

The external solution was based on HBSS and contained (in mM): 140 NaCl, 5.8 KCl, 1.8 CaCl₂, 1 MgCl₂, 4.2 NaHCO₃, 5.5 glucose,and 15 HEPES, pH 7.3. The normal internal solution contained (inmM): 59 KF, 59 KCl, 1 CaCl₂, 2 MgCl₂, 11 EGTA or BAPTA, and 10HEPES, pH 7.3. External solutions contained tetrodotoxin (1 µM)to block voltage-gated sodium conductances. Reagents for physiologicalsolutions were purchased from Sigma (St. Louis, MO).

The bath chamber (volume 0.4 ml) was continuously perfused at a rate of 0.4 ml/min using a peristaltic pump. Channel blockersand other reagents were applied using a slightly pressurized largebore (tip diameter ~400 µm) puffer pipette. The exchange timeof the solution surrounding the target cell was estimated to be250-500 msec based on the change in tip potential of a patch pipettein the normal bath solution to a puff of 100 mM KCl.

Immunocytochemistry. At the appropriate growth stage, neurons were fixed by immersing coverslips in 4% paraformaldehyde inPBS (in mM: 137 NaCl, 2.7 KCl, and 10 Sigma catalog #410-3S phosphatebuffer solution, pH 7.4) at 37°C for 1 hr, rinsed in PBS, andstored in 0.1% paraformaldehyde in PBS at 4°C until use. Afterrinsing stored coverslips in buffer, they were permeabilized inPBS containing 0.3% Triton X-100 for 15 min at 37°C, then rinsedagain and blocked for 1 hr at room temperature with 4% blockingreagent (Boehringer Mannheim, Indianapolis, IN) plus 0.1% TritonX-100 in PBS. All remaining steps were performed at room temperature.Coverslips were incubated in primary antibody for 2 hr and washedthree times for 10 min each in PBS containing 0.3% Triton X-100,and then were washed one time for 30 min in PBS. Coverslips werethen incubated in biotinylated goat anti-rabbit antibody (1:1000;Vector Laboratories, Burlingame, CA) for 1 hr, washed as above,and amplified using biotin (Berghorn et al., 1994). Coverslipswere first incubated in streptavidin-horseradish peroxidase (1:5000;TSA Indirect kit, Dupont NEN, Boston, MA), then in biotinyl tyramide(5 µl/ml, prepared as directed), and then in streptavidin-Cy3(1:2500; Jackson ImmunoResearch, West Grove, PA), each for 30min, followed by three washes for 10 min each in PBS plus 0.3%Triton X-100. They were then mounted in Vectashield (Vector Laboratories)and viewed.

Images were collected with a Zeiss 310 laser-scanning confocal microscope using 543 nm excitation and a long-pass barrierfilter (Chroma, Brattleboro, VT). The fluorescence images presentedhere were acquired at 512 × 512 or 1024 × 1024 pixels using a20 µm-diameter pin hole (depth of field ~1 µm), and were takenfrom the lower (nearer the coverslip) portions of each neuron.

Use of the Boehringer blocking reagent in conjunction with the biotin amplification procedure aided in obtaining high resolutionimages with low background fluorescence.

Morphometrics. After 4 d in culture, neurons were fixed at room temperature in 4% paraformaldehyde, and a small drop of thefluorescent lipophilic dye DiI (dissolved in cod liver oil) wasplaced on a soma. Cells were held at 4°C overnight to allow thedye to diffuse through the membrane and then imaged on the confocalmicroscope (at maximum pin hole diameter). Images were exportedin TIFF format to the Optimas image analysis package (OptimasCorporation, Bothell, WA). Measurements were made manually fromthese images by drawing a cursor across the soma or along a neurite,and length values were exported into a spreadsheet for furtheranalysis.

Materials. Tetrodotoxin, LY294002, wortmannin, ML-9, KN-62, staurosporine, and K252a were all purchased from Calbiochem (SanDiego, CA).

The polyclonal antiserum against Kv4.2/3 (Barry et al., 1995) was a gift from Drs. D. M. Barry and J. M. Nerbonne (Departmentof Pharmacology, Washington University School of Medicine, St.Louis, MO).

Data presentation. All data are presented as mean ± SD. Statistical comparisons were made using either Student's t test orDunnett multiple comparisons test as appropriate (Instat; GraphPad, San Diego, CA). Significance was assessed as p < 0.05.

  RESULTS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Technical considerations

All of the data presented here were taken from morphologically identified mouse hippocampal pyramidal neurons (Banker andCowan, 1977, 1979; Kriegstein and Dichter, 1983) in cultures ofcells dissociated from hippocampi isolated from mouse fetusesat embryonic days 15 or 16 and grown in culture for 4-7 d. Kinaseinhibitors were added 2 hr after cells were plated and were presentcontinuously until cell-bearing coverslips were rinsed for electrophysiologicalrecording or for immunochemistry.

Separation of three distinct voltage-gated potassium currents, I_A, I_D, and I_K (Storm, 1990) followed procedures describedin publications from this laboratory and others (Ficker and Heinemann,1992; Wu and Barish, 1992). Briefly, sodium currents were blockedby adding TTX (1 µM) to all external solutions; calcium currentsand calcium-dependent potassium currents were minimized by usingphysiological [Ca²⁺] in external solutions (1.8 mM), by incorporating potassium fluoridein internal solutions, and by intracellular dialysis with EGTA-or BAPTA-containing solutions. Under these conditions we havenot observed any effect on potassium currents of adding Ni²⁺ or Cd²⁺ to external solutions at blocking concentrations. Neurons wereheld under voltage clamp at $-$ 80 mV, and maximal availability ofall voltage-gated currents was achieved by imposing a 1000-msec-longconditioning hyperpolarization to $-$ 120 mV. Potassium currentswere measured at a test voltage of +40 mV, at which I_A is maximallyactivated. I_A was defined as the current sensitive to a conditioning50-80-msec-long prepulse to $-$ 40 mV, I_D as the current sensitiveto 100-200 µM 4-AP, and I_K as the TEA-sensitive current remainingafter block of I_A by the prepulse and block of I_D by exposureto 4-AP. An example of this separation is shown in Figure 3.

Cell capacitance was also measured as described in previous publications (Wu and Barish, 1992). After establishing the initialhigh resistance seal and in-amplifier compensation for pipetteand patch membrane capacitance, the patch was ruptured and thewhole-cell condition was established. Before imposing any additionalcapacitance compensation, a series of 10 short (20-msec-long)depolarizations from $-$ 70 to $-$ 60 mV were delivered, and the currentswere averaged. Whole-cell capacitance was evaluated by integratingthe area under the capacity transient to measure Q (total chargetransferred) and computed from the relation C = Q/ $Delta$ V, where Cis cell capacitance and $Delta$ V is the magnitude of the voltage step.

We believe that measurements of whole-cell capacitance and voltage-gated potassium currents and analyses of membrane insertionwere all made from a somatodendritic compartment subject to reasonablevoltage control and also susceptible to inhibition of membraneinsertion. In cultured neurons A-type potassium channels are foundon somata and apical dendrites (as assessed during single channelrecording; R.-L. Wu and M. E. Barish, unpublished observations),and the cross-sectional area of this compartment, as describedbelow, was reduced by kinase inhibitors. Cable analysis of hippocampalpyramidal neurons in situ (Johnston and Brown, 1984) indicatesthat even rapid synaptic events located on the apical dendritecan be well clamped. Thus, the A-type potassium channel-bearingregion of cell membrane could be subjected to electrophysiologicalanalysis, and it was also actively inserting membrane during thisdevelopmental period.

Overview

The data that follows are grouped into three sections: first, the effects of manipulating neurite outgrowth by varying thecomposition of the culture medium; second, the effects of inhibitingkinases implicated in receptor signaling and/or in control ofexocytosis; and third, the effects of two broad spectrum kinaseinhibitors.

Culture medium and neurite outgrowth
Because we had previously observed that pyramidal neurons growing in contact with astroglial cells had enhanced membrane area,we wished to separate effects of astroglial contact from thoserelated to membrane insertion and neurite outgrowth. To do thiswe compared neurons grown in serum-containing and serum-free media.Neurons grown in serum-free medium are commonly observed to havegreater neurite outgrowth than neurons grown in serum-containingmedium (Brewer et al., 1993; Brewer, 1995), and serum-free mediumalso discourages proliferation of astroglial cells and their precursors(Brewer et al., 1993). For these particular experiments we useda serum-containing medium consisting of MEM supplemented onlywith 10% fetal calf serum (MEM-FCS) and a serum-free medium consistingof Neurobasal supplemented only with B-27 additive (Neurobasal-B-27;Brewer et al., 1993).
Images of representative pyramidal neurons grown in these two media are shown in Figure 1A. Increased neurite outgrowth inthe absence of astroglial cells is evident for the Neurobasal-B-27cultures. Neurons in the MEM-FCS cultures grew in contact witha sparse astroglial monolayer and showed fewer neurite branches.

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Figure 1. A, Comparison of neuronal morphology after culture in serum-containing (MEM-FCS) and serum-free (Neurobasal-B-27) media. The images illustrate enhanced neurite outgrowth by neurons cultured in Neurobasal-B-27 medium. Neurons had been in culture for 5 d. B, Effects of the culture medium on potassium current development. I_A was enhanced in neurons grown in Neurobasal-B-27 medium despite their lack of astroglial contact. Numbers of cells: 10 NB-B-27 and 8 MEM-FCS. In this and subsequent figures, * denotes p < 0.05; ** denotes p < 0.01; and *** denotes p < 0.001.

Comparison of the electrophysiological properties of these neurons (Fig. 1B) suggests that neurite outgrowth (membrane expansion)may regulate I_A development, and this process may be downstreamof contact with astroglial cells. Although membrane area (determinedas whole-cell capacitance) was comparable in the two neuronalpopulations, I_A amplitude (top row) and I_A density (current amplitudenormalized to cell capacitance and expressed as picoamperes perpicofarad; bottom row) was increased significantly in neuronsgrown under serum-free conditions. This result is contrary towhat would be expected if astroglial contact alone was regulatingappearance of I_A and instead suggests that, in these cultures,greater neurite outgrowth was responsible for enhanced I_A development.
Interestingly, I_D amplitude and density showed some reciprocity with I_A; this reached statistical significance for I_D density.A similar relationship between I_A and I_D was seen in our previousinvestigation of the effects of astroglial contact (Wu and Barish,1994).
Because the growth-promoting effects of glial cells on neurons are well known (Noble et al., 1984; Fallon, 1985; Pixley etal., 1987), the results of this experiment further suggested thatastroglial cells might exert their influence on I_A development(Wu and Barish, 1994) through programs of membrane expansion andneurite outgrowth and parallel insertion of A-type potassium channels.We therefore examined intracellular signaling pathways that maybe involved in these processes.

Kinases implicated in control of membrane trafficking and exocytosis
The experiments presented in this section were all performed using neurons growing on a cocultured astroglial monolayer andwere designed to perturb the potassium current development promotedby astrocyte contact. The kinases targeted by the inhibitors usedwere as follows: PI 3-kinases by LY294002 or wortmannin; myosinlight chain kinase by ML-9; CaMKII by KN-62; PKC by bisindolymaleimide,calphostin C, or K-252b; and multiple serine-threonine and tyrosinekinases by staurosporine or K-252a.
Inhibition of phosphatidylinositol 3-kinase by LY294002 and wortmannin. PI 3-kinases are a family of lipid kinases (Zvelebilet al., 1996) that catalyze phosphorylation of inositol at theD-3 position. PI 3-kinases are elements in the signaling pathwaysinitiated by receptor tyrosine kinases (Kapeller and Cantley,1994), and regulate, among other activities, membrane trafficking(De Camilli et al., 1996; Shepherd et al., 1996). Wortmannin andLY294002 (Vlahos et al., 1994) are structurally unrelated membrane-permeantinhibitors of PI 3-kinases.
Exposure of developing neurons to micromolar concentrations of LY294002 or wortmannin reduced both membrane area and neuriteoutgrowth. Shown in Figure 2, A1 and A2, are fluorescence imagesof individual neurons labeled with the membrane probe DiI. Thecontrol (Fig. 2A1a,A2a) and experimental (Fig. 2A1b,c,A2b,c) fieldspresented illustrate the reduced somatic diameters and neuritenumbers of neurons grown in the presence of LY294002 (5 µM) orwortmannin (2 µM).

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Figure 2. A, Morphology of neurons grown in the presence of PI 3-kinase inhibitors; exposure to LY294002 (A1) or wortmannin (A2) reduced soma size and neurite outgrowth. Neurons were labeled by placing a small drop of DiI dissolved in oil on a neuron soma, as described in Materials and Methods. Shown for each inhibitor are representative examples of a control image (note that two neurons are labeled in the wortmannin control) and two experimental images. B, Measurements of neurons imaged as above. Inhibition of PI 3-kinase reduced somatic cross-sectional area (B1) and numbers of neurites (B2). The lengths of shorter neurites (i.e., lengths <30-40 µm) were minimally effected, but exposure to LY294002 affected growth of longer neurites (B3, cumulative analysis). Numbers of cells analyzed: 10 control, 17 LY294002, and 10 wortmannin.

We quantified membrane area and neuronal morphology in terms of (1) somatic cross-sectional area, approximated as an ellipseand determined from measurements of major and minor axes, (2)numbers of first order (1^o) neurites emerging from the soma or apical dendrite, and (3)the lengths of these neurites. The major effects of PI 3-kinaseinhibitors were to reduce somatic size and numbers of 1^o neurites, with smaller effects on the lengths of individual neurites.Somatic cross-sectional area (Fig. 2B1) was reduced to ~62% ofcontrol by LY294002 and to ~75% of control by wortmannin. Numbersof 1^o neurites per cell (Fig. 2B2) were reduced to ~60% of controlby LY294002 and to ~47% of control by wortmannin. Surprisingly,exposure to LY294002 or wortmannin did not noticeably affect thegrowth of those shorter neurites that did emerge (i.e., neuriteswith lengths <30-40 µm), but growth of longer neurites (i.e.,with lengths more than ~50 µm) was selectively disturbed by LY294002(Fig. 2B3).
Growth in the presence of PI 3-kinase inhibitors also affected development of voltage-gated potassium currents. Recordingsshown in Figure 3, made from a control neuron and a neuron exposedto LY294002, illustrate the selective deficit in I_A induced bythe inhibitor. Shown in the top row are the total potassium currentsrecorded during test depolarizations to +40 mV after conditioningprepulses to $-$ 120 or $-$ 40 mV (solid lines). An additional trace(dotted line) shows total current recorded after a prepulse to $-$ 120 mV in the presence of 100 µM 4-AP. The traces below showI_A, I_D, and I_K isolated as described above and illustrate thealmost total loss of I_A in the neuron exposed to LY294002. I_Dand I_K are also reduced in amplitude but not eliminated, as expectedgiven the reduced size of neurons grown in the presence of LY294002.

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Figure 3. Whole-cell potassium currents recorded at +40 mV from control and LY294002-treated neurons. The traces in the top row are currents recorded after conditioning prepulses to $-$ 120 and $-$ 40 mV (solid traces). Addition of 100 µM 4-AP to the bath reduced the current evoked after the prepulse to $-$ 120 mV (dotted trace). The traces in the bottom rows illustrate isolation of the individual currents, as described in Results. In this example, I_A was almost completely eliminated in the cell grown for 4 d in the presence of LY294002 (5 µM). I_D and I_K were smaller in the LY294002-exposed neuron, as expected from the reduced membrane area of these cells.

Comparison of electrophysiological measurements made from populations of pyramidal neurons exposed to either LY294002 or wortmanninwith control neurons showed reduced total cell capacitance (anindex of membrane area; Fig. 4A1,2), and reduced amplitudes ofI_A, I_D, and I_K (Fig. 5A1,2). For example, exposure to LY294002reduced total cell capacitance to 47% of control, I_A amplitudeto 18% of control, I_D amplitude to 51% of control, and I_K amplitudeto 37% of control. When expressed as current density (Fig. 6A1,2),LY294002 reduced I_A density to 40% of control without significantlyaffecting densities of I_D or I_K, and the same pattern was seenwith wortmannin. Thus, LY294002 and wortmannin reduced I_D andI_K in proportion to their effects on membrane area, whereas thereduction in I_A was greater than expected based on cell size.

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Figure 4. Effects of growth in the presence of kinase inhibitors on whole-cell capacitance, determined as described in the Results. Shown are data for LY294002 (A1), wortmannin (A2), ML-9 (B), KN-62 (C), and calphostin C (D); putative targets of these inhibitors are indicated in parentheses. Membrane area was reduced by all inhibitors except calphostin C. Data presented in Figures 4-6 are drawn from the same population of neurons, and for all three figures numbers of cells are: wortmannin, 10 control, 11 experimental; LY294002, 3 control, 5 experimental; ML-9, 13 control, 10 experimental; KN-62, 8 control, 8 experimental; and calphostin C, 14 control, 17 experimental.

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Figure 5. Effects of growth in the presence of kinase inhibitors on amplitudes (as picoamperes measured at +40 mV) of voltage-gated potassium currents, determined as described in Results. Shown are data for LY294002 (A1), wortmannin (A2), ML-9 (B), KN-62 (C), and calphostin C (D); putative targets of these inhibitors are indicated in parentheses. I_A, I_D, and I_K amplitudes were all reduced by all inhibitors except calphostin C; the largest and the most significant effects were seen for inhibitors of PI 3-kinases and for I_A and I_K (a clear trend was seen for I_D).

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Figure 6. Effects of growth in the presence of kinase inhibitors on densities (as picoamperes per picofarad measured at +40 mV) of voltage-gated potassium currents, determined as described in Results. Shown are data for LY294002 (A1), wortmannin (A2), ML-9 (B), KN-62 (C), and calphostin C (D); putative targets of these inhibitors are indicated in parentheses. I_A density was significantly reduced only by LY294002 and wortmannin; a trend that did not reach significance was evident for ML-9. In contrast, I_A density was not altered by exposure to KN-62 or calphostin C, nor were densities of I_D or I_K affected by kinase inhibition.

The multimeric ion channels mediating I_A (referred to here as A-type potassium channels) are likely to incorporate Kv4.2 and/orKv4.3 protein in their pore-forming subunits (Serôdio et al.,1994; Keros and McBain, 1997; Johns et al., 1997), although theymay well not be composed exclusively of Kv4.2 and/or Kv4.3 subunits.We examined the subcellular localization of A-type potassium channelsunder control conditions and after exposure to kinase inhibitorsusing an antiserum raised against a C-terminal sequence foundin both Kv4.2 and Kv4.3 subunits (Barry et al., 1995). The stainingpattern observed by immunofluorescence using this antiserum isreferred to here as Kv4.2/3 immunoreactivity. Note that this antiserumwas raised against an intracellular epitope and, therefore, thatall images were acquired from permeabilized cells and, therefore,portray both internal and plasmalemmal distributions of immunoreactivity.
The images presented in Figures 7 and 8 indicate that Kv4.2/3 immunoreactivity was profoundly altered by exposure to LY294002.In control neurons illustrated in Figure 7A1-A4 (shown are pairsof Nomarski DIC and confocal immunofluorescence images for tworepresentative neurons), Kv4.2/3 immunoreactivity was dense, granular,and distributed throughout somata and dendritic processes. A voidarea created by the nucleus was faintly seen in these neurons.In neurons examined in other experiments this void area was oftenless apparent. Immunoreactivity was not evident in longer, moretubular axonal processes (Fig. 7A2,A4, arrowheads).

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Figure 7. Distributions of Kv4.2/3 immunoreactivity in control pyramidal neurons (A) and alterations induced by growth in the presence of the kinase inhibitors LY294002 (B), ML-9 (C), and KN-62 (D). In each case, Nomarski DIC and fluorescence images are shown for two representative neurons. The arrows in the fluorescence images indicate areas enlarged in Figure 8. A, Control neurons demonstrating the disperse and granular character of the Kv4.2/3 immunoreactivity. Strong Kv4.2/3 immunoreactivity is found only in somata and dendrites; tubular axonal structures (A2, A4, arrowheads) are devoid of signal. B, In neurons exposed to LY294002, the density of Kv4.2/3-immunoreactive punctata was greatly reduced, but their distribution was not significantly affected. C, In neurons exposed to ML-9, the density of Kv4.2/3-immunoreactive punctata was reduced but not to the extent seen with LY294002. In somata, punctata were found in a perinuclear array surrounding a void volume occupied by the nucleus; this was much more evident in ML-9-treated neurons than in control neurons or neurons exposed to the other inhibitors. D, In neurons exposed to KN-62, the density of Kv4.2/3-immunoreactive punctata was only slightly reduced from the control, and, as in control neurons, punctata were distributed throughout the soma and major dendrites. (Figure and legend continue)The images in Figures 7 and 8 were all acquired from two sets of sister coverslips that were grown, processed for immunochemistry, and imaged in parallel. Numbers of neurons analyzed: 17 control, 10 LY294002, 24 ML-9, and 10 KN-62. In general, comparisons of Kv4.2/3 immunoreactivity were performed 2-4 times for each kinase inhibitor. The luminance scale applies to all fluorescence images. Control images, in which the primary antibody was omitted, showed only background luminance (as between punctata; images not shown).

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Figure 8. Enlarged portions of fluorescence images near the regions indicated by the arrows in Figure 7, illustrating punctate areas of Kv4.2/3 immunoreactivity. Individual punctata had diameters of 0.5-0.75 µm, because each pixel represents ~0.2 × 0.2 µm in the image plane. In neurons exposed to LY294002 (B), ML-9 (C), or KN-62 (D), the maximum luminance of individual punctata was comparable to that of control neurons (A), as indicated by the luminance scale; only punctata densities and distributions appeared to be affected by the kinase inhibitors.

Processes displaying Kv4.2/3 immunoreactivity were identified as dendritic because of their tapering morphology and relativelyshort length (Bartlett and Banker, 1984a,b; Dotti et al., 1988)and because they express the dendritic marker MAP2 (Caceres etal., 1984; data not shown). These observations are consistentwith other reports of Kv4.2/3 immunoreactivity localization tosomata and dendrites of hippocampal pyramidal neurons in situand in culture (Sheng et al., 1992; Maletic-Savatic et al., 1995b;Tsaur et al., 1997).
The size and distribution of the granular Kv4.2/3-immunoreactive punctata are shown in more detail in Figure 8A, which istaken from the region of the soma of the neuron in Figure 7A3indicated by the arrow. In this enlargement each pixel representsa square ~0.2 × 0.2 µm; individual punctata had diameters of 0.5-0.75µm. We assume that these punctata represent aggregates of membranousstructures bearing Kv4.2/3 subunits, perhaps the tubulovesiculartransport vesicles described by Nakata et al. (1998).
For neurons grown in the presence of LY294002, Kv4.2/3 immunoreactivity was dramatically reduced, as judged by the much lowerdensity of immunoreactive punctata (Fig. 7B3,4). These punctatawere distributed as in control neurons; throughout somata anddendrites but not axons and without significant accumulation inany one region. Exposure to LY294002 reduced the density of punctata,but those punctata that were evident had diameters and luminancevalues similar to those seen in control neurons (Fig. 8B).
Inhibition of myosin light chain kinase by ML-9. Multiple members of the myosin superfamily are found in brain and may participatein aspects of membrane trafficking, including exocytosis (Mermallet al., 1998). We used the myosin light chain kinase inhibitorML-9 (Saitoh et al., 1986).
In electrophysiological experiments, ML-9 reduced total cell capacitance in a dose-dependent manner, with reduction to 60%of control by 10 µM ML-9 (Fig. 4B). At this concentration ML-9also reduced I_A amplitude to 37% of control, I_D amplitude to 58%of control, and I_K amplitude to 51% of control (Fig. 5B). ML-9reduced I_A density (although this did not quite reach statisticalsignificance) without affecting the densities of the other potassiumcurrents (Fig. 6B).
Nomarski DIC images of pyramidal neurons grown in the presence of ML-9 (Fig. 7C1,2) indicated that exposure to ML-9 re- sultedin somata that were less triangular and more rounded than thoseof control neurons (Fig. 7A1,2). ML-9-treated neurons showed reduceddensity of Kv4.2/3-immunoreactive punctata (Fig. 7C3,4), and thesepunctata showed greater accumulation in a perinuclear rind thanwas evident in control neurons or neurons exposed to inhibitors.Diameters of these punctata and their maximum luminance were similarto values seen in control neurons (Fig. 8C).
Inhibition of Ca²⁺-calmodulin-dependent protein kinase II by KN-62. Multiple lines of investigation point to a role for CaMKIIin control of exocytosis (see Discussion). We used the CaMKIIinhibitor KN-62 (Tokumitsu et al., 1990).
Electrophysiological measurements indicated that growth in the presence of KN-62 (10 µM) reduced whole-cell capacitance to65% of control (Fig. 4C) and reduced I_A amplitude to 60% of control,I_D amplitude to 60% of control, and I_K amplitude to 52% of control(Fig. 5C). However, neither I_A, I_D, nor I_K densities were affected(Fig. 6C), despite the clear reduction in membrane area.
Images of Kv4.2/3 immunoreactivity (Fig. 7D3,4) showed a slight reduction in overall luminance as compared with control neurons(Fig. 7A3,4), but no change in its almost uniform distribution.As was true for the other inhibitors, this appeared to be attributableto a reduction in the density of Kv4.2/3-immunoreactive punctatarather than to decreases in their diameter or maximum luminance(Fig. 8D).
Inhibition of protein kinase C by calphostin C, bisindolymaleimide I, or K-252b. We explored the role of PKC in regulationof potassium current development using the inhibitors calphostinC (Kobayashi et al., 1989; Tamaoki, 1991), K-252b (Kase et al.,1987), and bisindolymaleimide I (and its inactive variant bisindolymaleimideV; Toullec et al., 1991).
Electrophysiological measurements indicated that neurons grown in the presence of bisindolymaleimide I (data not shown), calphostinC (Figs. 4D, 5D, 6D), or K-252b (Fig. 10) displayed patterns oftotal cell capacitance and potassium current development thatwere similar to those of control neurons. This was in contrastto the clear effects of K-252a (see below), a structural relativeof K-252b.

Broad spectrum kinase inhibitors
These experiments used two compounds, staurosporine and K-252a, that inhibit a broad spectrum of kinases (Tamaoki, 1991) andillustrate two additional points.
First, experiments with staurosporine indicated that growth in serum-free medium could mimic the effects of astroglial contact,in that membrane expansion and potassium current development showedthe same sensitivity to kinase inhibition. Comparison of resultsobtained with 20 nM staurosporine show that neurons exposed inserum-containing medium had reduced total cell capacitance (72%of control), I_A amplitude (33% of control), and I_A density (41%of control), but essentially unaffected I_D or I_K (Fig. 9A), whereasneurons exposed in serum-free medium (Neurobasal-B-27) also hadreduced total cell capacitance (56% of control), I_A amplitude(20% of control), and I_A density (36% of control) but essentiallyunaffected I_D and I_K (Fig. 9B).

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Figure 9. Effects of growth in the presence of staurosporine on total cell capacitance and potassium current development when neurons were grown in normal (low serum) medium (A), or serum-free Neurobasal-B-27 medium (B). Comparable results were obtained under both conditions, a result indicating that neither serum nor astroglial contact were required for kinase-sensitive control of I_A development. A, Numbers of cells: 7 Control, 14 2 nM, and 7 20 nM. B, Numbers of cells: 4 Control, 4 2 nM, and 2 20 nM (neurons exposed to staurosporine in Neurobasal-B-27 medium were extremely fragile, and recordings sufficiently stable for acquisition of all data were difficult to maintain).

Second, comparison of results obtained with K-252a and K-252b confirms the general pattern of kinase sensitivities observedabove. K-252a affects multiple protein kinases including PKC,cyclic nucleotide-dependent protein kinases, CaMKII, and proteintyrosine kinase, whereas K-252b is more selective for PKC (Lazaroviciet al., 1996). As illustrated in Figure 10, exposure to K-252areduced whole-cell capacitance to 56% of control, I_A amplitudeto 41% of control, I_D amplitude to 61% of control, and I_K amplitudeto 37% of control, while reducing I_A density to 51% of control,not affecting I_D density, and reducing I_K density to 45% of control.In parallel cultures, exposure to K-252b did not affect totalcell capacitance or development of potassium currents.

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Figure 10. Effects of growth in the presence of the broad spectrum kinase inhibitor K-252a and its PKC-preferring variant K-252b on total cell capacitance and potassium current development. Exposure to K-252a affected membrane area, the amplitudes of I_A, I_D, and I_K, and densities of I_A and I_K. In contrast, exposure to K252b did not affect membrane area or development of any of the potassium currents. Numbers of cells: 21 control, 14 K252a, and 9 K252b.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Regulation of electrogenesis

A major implication of these experiments is that growth of particular neuronal regions may be driving targeted insertion ofspecific ion channels. Thus, whereas some channels may be uniformlydistributed over the neuronal surface, membrane expansion mayalso result in selective insertion of particular channels to createa mosaic of channel types over the neuronal surface.

For developing hippocampal neurons, PI 3-kinases may be critical elements of signaling pathways regulating both A-type potassiumchannel synthesis and fusion of channel-bearing vesicles intoregions of expanding membrane. The late embryonic and early postnatalperiod examined here (corresponding to the first 7-10 d in culture)is characterized by the initial preferential development of I_A(Ficker and Heinemann, 1992; Wu and Barish, 1992; Spigelman etal., 1992), and this process was disrupted by exposure of neuronsgrowing in contact with astroglial cells to inhibitors of PI 3-kinases.

Further, dendritic growth may occur by insertion of membrane specifically enriched in A-type potassium channels. Localizationof both I_A (Spigelman et al., 1992; Hoffman et al., 1997) andKv4.2/3 immunoreactivity (Sheng et al., 1992; Maletic-Savaticet al., 1995b; Tsaur et al., 1997; this report) to somata anddendrites suggests the presence of a population of targeted vesiclesbearing A-type potassium channels. These vesicles may be the Kv4.2/3-immunoreactivepunctata illustrated (Figs. 7, 8), because their density was reducedby exposure to LY294002, and they were similar in appearance tothe mobile tubulovesicular transport vesicles recently describedby Nakata et al. (1998). However, we have not yet compared thedistributions of Kv4.2/3-immunoreactive structures to markersof compartments of the secretory pathway (Krijnse-Locker et al.,1995), or determined if LY294002 perturbs generation of all transportvesicles, the presence of Kv4.2/3 immunoreactivity on transportvesicles, or both.

Unlike observations on I_A, changes in I_D and I_K amplitudes after inhibition of PI 3-kinases were in proportion to reductionsin membrane area (compare Figs. 5A1,2, 6A1,2). This suggests either(1) that minimal synthesis of the subunits comprising these channelswas occurring during this period and that insertion was drawingon a preexisting subunit pool, or (2) that subunit synthesis wasminimally affected by kinase inhibition. Regardless, these dataalso suggest regulation of channel insertion by PI 3-kinases.

Role of PI 3-kinases

How valid is our interpretation implicating PI 3-kinases in regulation of development of excitability?

First, the specificity of the inhibitors used suggests involvement of PI 3-kinases. We used unrelated membrane-permeant inhibitorsof PI 3-kinases, either LY294002 or wortmannin. LY294002 was effectiveat the micromolar concentration for which it is selective forPI 3-kinases (Vlahos et al., 1994) over PI 4-kinases (Vlahos etal., 1994) or myosin light chain kinase (Yano et al., 1995). Unlikewortmannin, LY294002 is stable when added to cultures (Vlahoset al., 1994). Wortmannin at nanomolar concentrations is selectivefor PI 3-kinases (Shepherd et al., 1996), but at higher (micromolar)concentrations affects other kinases, including PI 4-kinases (Nakanishiet al., 1995) and myosin light chain kinase (Nakanishi et al.,1992). Wortmannin was used at micromolar concentrations, whichappears inconsistent with actions restricted to PI 3-kinases.However, wortmannin is notoriously unstable, and in serum-containingcultures loses effectiveness after ~5 hr (Kimura et al., 1994).Because wortmannin was added to cultures at intervals of 8 and16 hr, its concentration was almost certainly below its nominalvalue. Therefore, although we do not exclude the possibility thatwortmannin was affecting other targets, we suggest that a majoraction of wortmannin was on PI 3-kinases.

Second, because the PI 3-kinases are a family of related kinases (Zvelebil et al., 1996), particular PI 3-kinases might influencehippocampal neuron development at different sites (Ward et al.,1996). PI 3-kinases appear to serve two major overlapping classesof functions. Some PI 3-kinases are activated as part of the signalingcascade initiated by protein tyrosine kinases and may regulateadditional kinases potentially linked to control of transcriptionfactor activity (Kapeller and Cantley, 1994) as well as to controlof intracellular membrane trafficking (De Camilli et al., 1996;Shepherd et al., 1996). Other PI 3-kinases may directly regulateintracellular membrane trafficking (De Camilli et al., 1996; Shepherdet al., 1996).

Although no other studies have directly addressed involvement of PI 3-kinases in the development of excitability, in studiesof PC12 cells, neurite growth was induced by introduction of aconstitutively active PI 3-kinase and inhibited by wortmannin(Kimura et al., 1994; Kobayashi et al., 1997). Other studies inneurons have examined PI 3-kinases in relation to regulation ofapoptosis (Nomomura et al., 1996; D'Mello et al., 1997; Milleret al., 1997).

Relation to the association of I_A development with astroglial contact

The similarity of the results obtained with inhibitors of PI 3-kinases to our previous observations of the effects of astroglialcontact (Wu and Barish, 1994), control of I_A amplitude and densityin association with changes in membrane area, suggests that PI3-kinases may be elements of intracellular signaling pathwaysin neurons whose activation is linked to astroglial contact. Inthis model, reception of signals originating in astroglial cellswould activate tyrosine kinases (possibly receptor tyrosine kinases),and subsequent activation of PI 3-kinases could regulate I_A development.Future work will be directed toward identification of the neuronalreceptor(s) responding to astroglial contact and their linkagesto particular PI 3-kinases.

Role of myosin light chain kinase

Our observations suggest involvement of myosin and myosin light chain kinase in regulation of vesicle populations availablefor exocytosis, because exposure to ML-9 reduced membrane areaand potassium current amplitudes and the overall luminance ofKv4.2/3 immunoreactivity. Significantly, Kv4.2/3 immunoreactivityshowed greater restriction to perinuclear portions than was evidentin control neurons or in neurons exposed to the CaMKII inhibitorKN-62, suggesting inhibition of peripheral migration of Kv4.2/3immunoreactivity. This process was not totally arrested, perhapsbecause cells possess multiple vesicle transport systems (Fathand Burgess, 1994). Nevertheless, our interpretation is consistentwith other analyses of myosin functions (Mermall et al., 1998)because: (1) the subcellular distributions of myosins and theirassociations with vesicles suggest a transport function in somata(Mermall et al., 1998), and (2) functional analyses of myosinssuggest involvement in vesicle transport and exocytosis (Ohara-Imaizumiet al., 1992; Kumakura et al., 1994; Mermall et al., 1994; Mochidaet al., 1994; Rao et al., 1997).

Role of calcium-calmodulin-dependent protein kinase II

Our observations also suggest that CaMKII regulates fusion of transport vesicles with the plasmalemma at a site close to theexocytotic step, because growth in the presence of a CaMKII inhibitorreduced membrane area and potassium current amplitudes proportionatelywithout substantially affecting the intensity or distributionof Kv4.2/3 immunoreactivity. This model is consistent with recentobservations of chronic CaMKII-sensitive membrane cycling at nonsynapticas well as synaptic sites on developing hippocampal neurons (Matteoliet al., 1992; Maletic-Savatic et al., 1995a, 1996).

Other studies have also reported a relationship between CaMKII activity and neuronal growth, in particular with neurite extensionand branching, and growth cone motility (Cabell and Audesirk,1993; Goshima et al., 1993; Williams et al., 1995; Audesirk etal., 1997).

Studies of neurotransmitter release indicate that CaMKII may affect exocytosis by regulating vesicle mobility and availabilityfor docking and eventual membrane fusion (Llinás et al., 1985;Greengard et al., 1993; Ceccaldi et al., 1995; Nielander et al.,1995; Maletic-Savatic et al., 1995a, 1996). Similar mechanismsmay be involved in neuronal growth regulation.

Role of protein kinase C

Growth in the presence of PKC inhibitors did not affect membrane area (measured electrophysiologically) or potassium currentdevelopment, an observation consistent with our notion that membraneexpansion and potassium channel insertion are linked. This insensitivityto PKC inhibitors was unexpected because PKC regulates a numberof processes involving vesicle fusion (Strong et al., 1987; Finchand Jackson, 1990; Parfitt and Madison, 1993; Corey et al., 1994;Billiard et al., 1997). However, in a broad way our observationsare consistent with studies indicating that inhibition of PKCwith calphostin C reduced only axon branching, but not dendritenumber, branching, or length (Cabell and Audesirk, 1993; Audesirket al., 1997) because we believe A-type potassium channels incorporatingKv4.2/3 subunits to be restricted to somatic and dendritic membrane.

Other studies linking membrane expansion to ion channel insertion and the potential significance of linked growth and excitability

The first studies linking changes in excitability (hyperpolarization of developing bastomeres) with membrane expansion wereexperiments on dividing early amphibian embryos (Woodward, 1968;de Laat and Bluemink, 1974), which demonstrated enhanced potassiumpermeability in membrane newly inserted at the cleavage furrow.

More recently, several studies have examined episodes of membrane expansion linked to regulation of excitability. In Aplysiabag cell neurons, appearance of action potential-triggered Ca²⁺ influx at the distal edges of expanding lamellipodia (Knox etal., 1992) is attributable to PKC-regulated recruitment of "covert"calcium channels to the surface membrane (Strong et al., 1987)from a pool of vesicular calcium channels (White and Kaczmarek,1997). In neuroblastoma cells, continuous exposure to $omega$ -conotoxinGVIA ( $omega$ -CgTX) GVIA or Cd²⁺ increases I_Ca and depolarization-induced intracellular Ca²⁺ transients (Passafaro et al., 1992, 1994, 1996) by processesassociated with increase in the number of surface ¹²⁵I- $omega$ -CgTX GVIA-binding sites and parallel loss of internal bindingsites. In growth cone particles derived from fetal rat brain,externalization of voltage-gated sodium channels from intracellularreservoirs (Schmidt et al., 1985) is sensitive to disruption ofthe membrane fusion apparatus (Wood et al., 1992), as may be channelsin these other examples.

More generally, the experiments presented here have significance for our understanding of nervous system assembly and signalingplasticity, because they imply that the morphological transformationsthat accompany both development (Harris et al., 1992; Purves etal., 1994) and use-dependent synaptic modifications (Bailey andChen, 1989; Glanzman et al., 1990; Hosokawa et al., 1995) maybe accompanied by changes in channel or receptor numbers and distributions.A specific suggestion is the possibility of "silent" glutamatereceptors potentially exposed at central synapses during the developmentand/or expression phases of hippocampal long-term synaptic potentiation(Isaac et al., 1995; Liao et al., 1995; Durand et al., 1996; Wuet al., 1996). A critical issue is thus elucidation of the rulesgoverning specific forms of membrane expansion and linkages toparticular ion channel and neurotransmitter receptor subunits.

  FOOTNOTES

Received Feb. 18, 1998; revised June 1, 1998; accepted June 9, 1998.

This work was supported by National Institutes of Health National Institute of Neurological Diseases and Stroke Grant R01NS23857. We thank Arlene Y. Chiu and Charles E. Niesen for theirhelpful comments on this manuscript, Dianne M. Barry and JeanneM. Nerbonne for their generous gifts of antibodies, and M. JillFlanagan for her assistance with manuscript preparation.
Correspondence should be addressed to Dr. Michael E. Barish, Division of Neurosciences, Beckman Research Institute of theCity of Hope, Duarte, CA 91010.

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