Activity-Dependent Calcium Sequestration in Dendrites of Hippocampal Neurons in Brain Slices

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Volume 17, Number 22, Issue of November 15, 1997

Activity-Dependent Calcium Sequestration in Dendrites of Hippocampal Neurons in Brain Slices

Lucas D. Pozzo-Miller¹^,², Natalia B. Pivovarova¹, Richard D. Leapman³, Roger A. Buchanan¹, Thomas S. Reese¹^,², and S. Brian Andrews¹^,²
¹ Laboratory of Neurobiology, National Institute of Neurological Diseases and Stroke, National Institutes of Health, Bethesda, Maryland 20892, ² Marine Biological Laboratory, Woods Hole, Massachusetts 02543, and ³ Biomedical Engineering and Instrumentation Program, National Center for Research Resources, National Institutes of Health, Bethesda, Maryland 20892

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Synaptic activity-dependent changes in the spatio-temporal distribution of calcium ions regulate important neuronal functionssuch as dendritic integration and synaptic plasticity, but theprocesses that terminate the free Ca²⁺ transients associated with these changes remain unclear. We havecharacterized at the electron microscopic level the intracellularcompartments involved in buffering free Ca²⁺ transients in dendritic cytoplasm of CA3 neurons by measuringthe larger changes in the concentrations of total Ca that persistfor several minutes after neuronal activity. Quantitative energy-dispersivex-ray microanalysis of cryosections from hippocampal slice culturesrapidly frozen 3 min after afferent synaptic activity identifieda subset of dendritic endoplasmic reticulum (ER) as a high-capacityCa²⁺ buffer. Calcium sequestration by cisterns of this subset of ERwas graded, reversible, and dependent on a thapsigargin-sensitiveCa²⁺-ATPase. Sequestration was so robust that after repetitive high-frequencystimulation the Ca content of responsive ER cisterns increasedas much as 20-fold. These results demonstrate that a subpopulationof ER is the major dendritic Ca sequestration compartment in theminutes after neuronal activity.
Key words: calcium regulation; calcium sequestration; hippocampus; CA3; dendrites; endoplasmic reticulum; synaptic activity; hippocampal slice cultures; X-ray microanalysis

INTRODUCTION

Despite the wealth of information about the role of Ca ions in neuronal function (Miller, 1988), and especially about thechannels and stores that give rise to free Ca²⁺ transients (Tsien and Tsien, 1990; Simpson et al., 1995), theprocesses that terminate such transients are not well understood(Miller, 1991; Pozzan et al., 1994). In particular, several importantcharacteristics of neuronal Ca handling immediately after synapticactivity-induced cytosolic Ca²⁺ transients remain unclear, including the absolute size and fateof the underlying total Ca load. Likely candidates for clearingcytosolic Ca²⁺ include the same mechanisms that neurons employ to maintain lowresting levels of intracellular free Ca²⁺, namely, binding to cytoplasmic proteins, uptake into the smoothendoplasmic reticulum (ER) via a Ca²⁺-ATPase (SERCA) pump, electrochemically driven uptake into mitochondria,and extrusion across the plasma membrane by the Na⁺-Ca²⁺ exchanger and a plasma membrane Ca²⁺-ATPase (Carafoli, 1987; Miller, 1991).

The ER has been the focus of considerable attention since the original demonstrations of its Ca-sequestering activity (Henkartet al., 1978; McGraw et al., 1980). Since then, a related butdistinct Ca²⁺-regulating function of the ER, namely, that of a releasable Ca²⁺ store, has been well characterized (Alford et al., 1993; Llanoet al., 1994; Seymour-Laurent and Barish, 1995; Pozzo-Miller etal., 1996; Garaschuk et al., 1997; Golovina and Blaustein, 1997).This store, because it is engaged in cycles of Ca²⁺ uptake and release, plays an important role in neuronal Ca²⁺ buffering (Andrews et al., 1988; Markram et al., 1995). It isalso now recognized, on the basis of the heterogeneous distributionof luminal Ca-binding proteins, membrane Ca²⁺-ATPase pumps, and Ca²⁺-permeable membrane channels, that the various functional aspectsof the ER, and particularly the dendritic ER, are spatially compartmentalized(Henzi and MacDermott, 1992; Pozzan et al., 1994), even thoughthe ER forms a structurally continuous network of membranes (Martoneet al., 1993; Terasaki et al., 1994).

Direct measurements correlating neuronal activity with changes in the total Ca content of the ER would potentially revealand localize any high-capacity sequestration activity that mightfunction in signal termination and distinguish this from a Ca²⁺ release function. At present, such measurements are nonexistent,not only for the ER but also for other subcellular compartmentsof neurons. The latter is equally important, because Ca²⁺ buffering and sequestration do not reside exclusively in theER, as indicated by the high Ca²⁺-binding capacity of many cytoplasmic proteins (Miller, 1991)and by recent and accumulating evidence for the participationof mitochondrial Ca²⁺ uptake (Rizzuto et al., 1993; Friel and Tsien, 1994; Werth andThayer, 1994; White and Reynolds, 1995; Budd and Nicholls, 1996;Herrington et al., 1996; Babcock et al., 1997). As a first stepin establishing the roles of, as well as the interplay between,each of these mechanisms in dendritic Ca²⁺ handling, we have determined the amount and location of intracellularCa in proximal dendrites of CA3 pyramidal cells in hippocampalslice cultures, both at rest and at defined times after neuronalactivity. These experiments were performed by exploiting the highanalytical sensitivity and subcellular resolution of modern (Leapmanand Andrews, 1991; Buchanan et al., 1993; Andrews et al., 1994)energy-dispersive x-ray (EDX) microanalysis (Shuman et al., 1976;Hall and Gupta, 1983), a technique that $---$ in distinction to imagingwith Ca²⁺-sensitive fluoresecent dyes $---$ provides direct and quantitativemeasurements of the concentration of total Ca within identifiedsubcellular compartments.

MATERIALS AND METHODS
Preparation, stimulation, recording, and rapid freezing of hippocampal slice cultures. Hippocampal slice cultures were preparedfrom postnatal d 7 rats, as described previously (Stoppini etal., 1991; Pozzo-Miller et al., 1993). Slice cultures 6-8 d invitro were transferred to an immersion chamber continuously perfused(2-4 ml/min) with artificial CSF (ACSF) at room temperature (23-24°C),containing (in mM): 124 NaCl, 2 KCl, 1.3 MgSO₄, 1.24 KH₂PO₄, 17.6NaHCO₃, 2.5 CaCl₂, and 10 D-glucose, equilibrated with 95% O₂/5%CO₂. Thapsigargin (Sigma, St. Louis MO; Research Biochemicals,Natick MA; 10 µM in 0.01% DMSO) and TTX (Sigma; 5 µM) were addedto the perfusion ACSF as indicated. Field EPSPs in CA3 stratum(st.) lucidum were evoked by stimulation of dentate gyrus st.granulosum or the mossy fiber track in CA3 st. lucidum with abipolar stainless steel electrode and recorded with a ACSF-filledglass pipette (5 M $Omega$ ) using an Axoclamp-2A amplifier (Axon Instruments,Foster City, CA). Test stimuli consisting of single monophasicpulses of 100 µsec duration were delivered by a stimulus isolator-constantcurrent unit (Axon Instruments) at an intensity of 10-100 µA at0.25-0.5 Hz. After establishing that EPSPs were stable in theslice (0.5-2 mV; 5-15 min), high-frequency stimuli consistingof one or four trains every 30 sec, each composed of 50 pulsesat 50 Hz at test intensities, were delivered to the afferent fibers.After withdrawing the recording and stimulating electrodes, sliceswere removed from the recording chamber, mounted on 400-µm-thickagar-gelatin pads, marked to locate cell layers for subsequentcryosectioning, and rapidly frozen by impact onto a liquid nitrogen-cooledcopper block using a custom-modified CF-100 machine (LifeCell,The Woodlands, TX). The interval from the last high-frequencytrain in the recording chamber to the instant of freezing was3.0 ± 0.5 min. Postsynaptic responses were digitized on-line at10 kHz (ITC-16; Instrutech, Great Neck, NY) for display and analysisand stored on magnetic media using custom-written software ina Power PC Macintosh computer (T. Inuoe, Tokyo University, Tokyo,Japan).

Electron microscopy, cryosectioning, and quantitative EDX microanalysis. For morphological evaluation, rapidly frozen slicecultures were freeze-substituted in 4% OsO₄ in acetone at $-$ 80C°over 48 hr (Pozzo-Miller and Landis, 1993), resin-embedded (Araldite)and thin-sectioned using standard techniques, and examined ina JEOL (Peabody, MA) 100-CX electron microscope. Structural preservationin rapidly frozen slice cultures (Pozzo-Miller and Landis, 1993)varies with distance from the cryogenic contact surface. To ensuretechnically satisfactory preparations that showed no evidenceof ice crystal-induced distortions, section depth was limitedto <20 µm, at which depth rapid freezing has been calculated tooccur in <2 msec (Heuser et al., 1979).

Cryosectioning was performed as described previously (Michel et al., 1992; Buchanan et al., 1993). In brief, cryosectionswere cut en face from the well frozen surface (<20 µm deep) ofpreviously marked regions of CA3 st. lucidum, trimmed to a 0.25× 0.25 mm block face. The en face orientation ensures that allmaterial was taken from the well frozen surface and has the additionaladvantage that the somatic region of pyramidal cells was oftencontained in the margin of sections, thereby aiding the identificationand location of CA3 dendrites. Cryosections were obtained as smooth,continuous ribbons at less than $-$ 160°C with a specimen advanceof 80 nm using a diamond knife in an Ultracut S/FCS ultracryomicrotome(Leica, Deerfield, IL). The actual physical section thicknessis approximately doubled on account of unrelievable compression,but the unidirectional nature of the compression only distortsorganelle shape in the direction of knife movement; it does notincrease organelle overlap relative to the original 80-nm sections(Shi et al., 1996). Therefore, such sections are suitable forelemental analysis of structures $>=$ 80 nm in the z (thickness) direction.Sections were mounted on carbon- and Formvar-coated grids andcryotransferred into an EM912 Omega electron microscope (LEO ElectronMicroscopy, Thornwood, NY) or into an HB501 field-emission scanningtransmission electron microscope (STEM) (VG Instruments, Beverly,MA) for imaging and analysis. In both instruments, sections werefreeze-dried at approximately $-$ 110°C and recooled to less than $-$ 160°C.

The National Institutes of Health STEM, as well as instrumentation and techniques for cryotransfer, freeze-drying, dark-fieldimaging and EDX analysis, have been described previously (Leapmanand Andrews, 1991; Buchanan et al., 1993). Each EDX analysis was100 sec at ~4 nA probe current rastered over a 20 × 20 nm area;doses were therefore >10⁸ e/nm². We avoid recording spectra from small ER cisterns that are notwholly contained within the section thickness; if such spectrawere inadvertently acquired, however, the calculated Ca contentwould underestimate the ER Ca content. Spectra were recorded at $-$ 160°C or below. Data were processed and quantified by establishedprocedures (Shuman et al., 1976; Hall and Gupta, 1983; Kitazawaet al., 1983; Buchanan et al., 1993) using the program DeskTopSpectrum Analyzer for the Macintosh (C. E. Fiori, C. R. Swyt,and R. L. Myklebust, Office of Standard Reference Data, NationalInstitute of Standards and Technology, Gaithersburg, MD). Concentrationsare given in millimoles per kilogram of dry weight because theHall quantification procedure (Hall and Gupta, 1983) providesthese data directly. Concentrations in millimoles per liter oforiginal wet volume, which are more intuitively useful in physiology,can be estimated by multiplying dry weight concentrations by thedry mass fraction of analyzed organelles; typical values are 15,25, and 40% dry mass for cytoplasm, ER, and mitochondria, respectively(Buchanan et al., 1993). It is further possible to convert valuesto mM, i.e., millimoles per liter of cell water, by dividing bythe water fraction of each compartment, but this is not appropriatefor total Ca measurements, because most of the Ca is not in solution.

The mean Ca concentrations of the apparently normally distributed low-Ca populations seen in Figure 5 were estimated by least-squaresfitting of Gaussians. Mean concentrations and uncertainties derivedby curve fitting are reasonable for the statistical and biologicalvariability expected from EDX analysis; curve fitting has theadditional merit of accounting for the negative concentrationvalues, which occur because of statistical fluctuations in thesubtraction of a fitted background when true Ca x-ray counts arevery low (Kitazawa et al., 1983). The minimum detectable concentrationcan be taken as twice the estimated analytical uncertainty, whichis typically 2-4 mmol/kg dry weight for a single analysis underour conditions (Andrews et al., 1994); the SEM for pooled analyses,however, is much lower (e.g., Table 1). Measured concentrationssmaller than twice their corresponding SEMs, including zero andnegative values, are equivalent to "not detected."
Fig. 5. Calcium sequestration in a subpopulation of dendritic ER. A-F, Frequency distributions of Ca concentrations within ER cisternsafter different stimulation protocols reveal that Ca²⁺ sequestration is limited to a subset of ER cisterns. The multimodalnature of these distributions was evident under conditions (B,C) in which increased Ca²⁺ influx led to the separation of the Ca-accumulating population(black bars) from a nonresponsive population (gray bars). Thus,in dendrites stimulated with one (B) and four (C) afferent trains,40 and 45% of the cisterns, respectively, accumulated enough Cato exceed the arbitrary but conservative cutoff of 15 mmol/kgdry weight. The concentrations reached by the Ca-accumulatingcisterns were nonuniformly distributed; those achieving extraordinarylevels >100 mmol/kg have been pooled at the right edges of B andC. The mean Ca concentrations of the residual nonresponsive populations,as estimated by least-squares fitting of Gaussians (solid curveswith mean ± SEM) were not significantly different one from theother, nor were they different from the mean Ca concentrationsfor the four nonaccumulating conditions (A, D-F). In the lattercases, Ca distributions of the low-Ca cisterns (gray bars) areprobably also multimodal but (apart from a few outliers) appearnormally distributed, because the population means are similarand cannot be distinguished.
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Table 1. Elemental concentrations in cellular compartments of hippocampal CA3 dendrites

n NaKCa

(mmol/kg dry weight)

Endoplasmic reticulum^a

  Control ± TTX 56 76 ± 7 571 ± 20 5.1 ± 1.1

  Single train 68 91 ± 8 626 ± 24 17.8 ± 3.5^*

  4 Trains 68 181 ± 13^* 505 ± 14 35.5 ± 5.4^*

  4 Trains + TTX 39 152 ± 11^*^,^** 683 ± 39 6.2 ± 2.3^**

  4 Trains + recovery 47 41 ± 5^** 509 ± 21 8.0 ± 1.5^**

  4 Trains + thapsigargin 54 101 ± 14^** 497 ± 18 5.0 ± 0.8^**

Mitochondria

  Control ± TTX 22 32 ± 4 286 ± 12 0.3 ± 1.0^***

  Single train 8 17 ± 4 239 ± 22 1.8 ± 2.0^***

  4 Trains 21 62 ± 7^* 288 ± 14 1.3 ± 0.6

  4 Trains + TTX 12 44 ± 7 267 ± 12 $-$ 1.3 ± 0.9^***

  4 Trains + recovery 32 19 ± 3^** 232 ± 11 0.6 ± 0.8^***

  4 Trains + thapsigargin 29 63 ± 10^* 258 ± 14

    Matrices 13 3.7 ± 1.4^*^,^**

    Inclusions 16 165 ± 94

Cytoplasm

  Control ± TTX 18 77 ± 16 854 ± 61 0.7 ± 1.1^***

  Single train 16 72 ± 12 990 ± 88 3.5 ± 3.4^***

  4 Trains 63 266 ± 28^* 772 ± 30 4.2 ± 0.9^*

  4 Trains + TTX 14 147 ± 16^*^,^** 854 ± 93 1.2 ± 1.5^**^,^***

  4 Trains + recovery 18 70 ± 17^** 864 ± 97 0.4 ± 1.9^**^,^***

  4 Trains + thapsigargin 28 179 ± 39^*^,^** 599 ± 35^*^,^** 1.8 ± 1.6^***

Data are given as mean ± SEM, where column n is the number of compartments analyzed; the number of ER analyzed ranged fromthree to seven per dendrite (fewer for other compartments). Therewere at least two slices for each condition, with dendrites distributedas follows: control ± TTX, 21 dendrites; single train, 25; 4 trains,31; 4, trains + TTX, 9; 4 trains + recovery, 15; 4 trains + thapsigargin,28. SE and n values are based on compartmental analyses, becausea statistical evaluation of the data indicated that dendrite-to-dendriteand slice-to-slice variabilities were small compared with compartment-to-compartmentvariability. The quantification procedure provides concentrationsin units of millimoles per kilogram of dry weight; conversionto millimoles per liter of hydrated cell volume is described inMaterials and Methods. ^a Morphologically defined ER consisted of multiple populations with differing Ca uptake capacities, as discussed in the textand illustrated in Figure 5. Therefore, mean concentrations reportedin this table are not necessarily derived from normal distributions.Large SEs result when the underlying populations are different,for example, ER Ca concentrations after one or four stimulus trains. ^* Significantly higher than corresponding values from resting control cultures, except cytoplasmic K⁺ after four trains in the presence of thapsigargin, which is lower;t test, p < 0.05. ^** Significantly lower than corresponding values from cultures subjected to four stimulus trains, except Ca in mitochondrialmatrices after four trains in the presence of thapsigargin, whichis higher; t test, p < 0.05. ^*** Not significantly different from zero. However, the data are given to indicate the errors of Ca analyses, which in this caseare mainly limited by counting times. Negative values, reflectingstatistical fluctuations, sometimes occur for populations thatare not significantly different from zero.

RESULTS

Structural characterization of organelles and compartments in CA3 dendrites
Proximal apical dendrites of CA3 pyramidal neurons within st. lucidum (<100 µm from cell bodies) of rapidly frozen, freeze-substitutedhippocampal slice cultures (Pozzo-Miller and Landis, 1993) displayedthe characteristic complement of membrane-bound organelles describedin more conventional preparations of nervous tissue (Peters etal., 1991) (Fig. 1). Most dendritic branches contained abundantmitochondria, usually elongated and oriented along the longitudinalaxis of the dendrite. The ER network consisted of pleomorphiccisterns and tubules of variable dimensions coursing among longitudinalarrays of microtubules; frequently, cisterns ran in close proximityto the plasma membrane. The number and size of ER cisterns andmitochondria varied between dendritic branches (Fig. 1, compareA, B). However, the volume-fractions occupied by these organellesappeared on average similar to those found in hippocampal CA1pyramidal and Purkinje cell dendrites, which in the case of theER is ~10% of dendritic volume (Martone et al., 1993; Spacek andHarris, 1997). Although Golgi cisterns have been observed in dendritesnear the cell body (Peters et al., 1991; Krijnse-Locker et al.,1995), they were rarely, if ever, encountered in the more distalportions selected for the present study.
Fig. 1. Subcellular organization of CA3 hippocampal dendrites in slice culture. A, B, Transmission electron micrographs of dendritesin CA3 st. lucidum from thin sections of rapidly frozen, freeze-substitutedslice cultures of hippocampus. These fields illustrate proximalapical dendrites in which mitochondria (M) and cisterns of ER(arrows) are essentially the only intracellular organelles; theremaining dendritic volume is occupied by microtubule-rich cytoplasm.The general organization is similar in both larger dendrites withsparse organelles (A) and in smaller dendrites with a higher densityof ER and mitochondria (B). Synapses (S) directly on the dendriticshaft are evident (B). The typical pleomorphic appearance of smooth-membranecisterns and tubules was consistent with the organization of dendriticER as a physically interconnected network (Martone et al., 1993;Terasaki et al., 1994). All such cisterns and tubules were definedas ER, because there was no structural basis for making finerdistinctions, even though it was recognized that the ER compartmentso defined would be functionally heterogeneous (Henzi and MacDermott,1992; Pozzan et al., 1994). Scale bars, 0.5 µm.
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All of the the major dendritic compartments found in freeze-substituted, plastic-embedded cultures, as just described, canalso be unambiguously identified in en face ultrathin (80 nm effectivethickness) cryosections from the superficial 5-20 µm of unfixed,unstained, rapidly frozen slice cultures (Fig. 2). Elemental analysiswas performed on apical dendrites within CA3 st. lucidum whichwere considered as divided into three compartments: ER (includingboth cisterns and tubules), mitochondria, and a third compartment,referred to as cytoplasm, that consisted mainly of soluble proteinsand the cytoskeleton. The justification for this simplified viewof dendritic structure lies in the fact that these three compartmentsinclude all the structures likely to be involved in dendriticCa²⁺ homeostasis, even while encompassing >95% of the total volumeof the dendrite. Thus, the intrusion of unaccounted organelles,e.g., multivesicular bodies or Golgi cisterns, would representonly a minor contribution and not significantly affect the conclusionsof the present study.
Fig. 2. Dendritic structure in cryosections. A-D, Electron micrographs of dendrites in CA3 st. lucidum from rapidly frozen slice culturesof hippocampus. Micrographs of unstained, freeze-dried, ultrathinen face cryosections from the superficial 5-20 µm of slices (B-D)were digitally recorded (1024 × 1024 pixels) at approximately $-$ 170°C and low electron dose (~10³ e nm²), either in the zero loss mode of an energy-filtering TEM equippedwith a slow-scan CCD camera or in STEM elastic dark-field mode.Structural organization and preservation in cryosections (B-D)allow direct correlation with structures seen in plastic-embeddedpreparations (A). Compartments targeted for EDX analysis, namely,ER (arrows), mitochondria (M), and microtubule-rich cytoplasm,can be readily identified, whether from well frozen areas of thespecimen (C, D) or from less well preserved areas (B). In fact,visualization of membrane-bound organelles is easier in cryosectionsfrom deeper areas of the slice, which exhibit some degree of freezingdamage, because aggregation of cytoplasmic material creates acoarser matrix in which organelles stand out. The small blacksquare within the box in cracked area of cryosection (B) indicatessize of a typical 20 × 20 nm analysis raster. Scale bar, 0.5 µm.
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Basal elemental concentrations in dendritic compartments
Cryosections of rapidly frozen tissue were prepared from unstimulated control slices incubated in normal ACSF and also fromcontrol slices after incubation in 5 µM TTX for 15-30 min to blockspontaneous synaptic activity. EDX analysis of both preparationsrevealed that the concentrations of total Ca, as well as of otherelements, in the three target compartments of CA3 apical dendrites(Table 1) were comparable to basal concentrations in other excitableand nonexcitable cells (Somlyo et al., 1977, 1985; Andrews etal., 1988). The mean concentration of Ca within dendritic ER was5.1 ± 1.1 mmol/kg dry weight (mean ± SEM; Table 1), although,as discussed below, this morphologically identified set of ERconsists of at least two functionally distinct populations that,under basal conditions, coincidentally display similar low Caconcentrations. This value corresponds to ~1.3 mmol/l hydratedcell volume. (In general, the values for Ca concentrations withinER, given in mmoles per kilogram of dry weight throughout thetext, can be converted to millimoles per liter of cell volumeby multiplying by 0.25; see Materials and Methods for assumptionsand calculations, as well as conversion factors for other compartments).

Dendritic endoplasmic reticulum is the major calcium sequestration organelle after synaptic activity
Knowing the basal Ca levels, we next determined which dendritic organelles showed changes in total Ca concentration afterafferent stimulation. For these experiments, EPSPs in CA3 st.lucidum were evoked by extracellular stimulation of granule cellsin dentate gyrus st. granulosum or mossy fiber tracks in CA3 st.lucidum (Fig. 3A,B). After establishing a stimulus intensity thatevoked stable EPSPs, afferent fibers received either a singletetanus (1 sec, 50 Hz; Fig. 3C) or four such tetani at 30 secintervals. Such high-frequency afferent stimulation is sufficientto activate most, if not all, mechanisms of dendritic Ca²⁺ entry, including influx through locally activated low-voltage-gatedCa²⁺ channels (Magee et al., 1995) and NMDA receptors (Perkel et al.,1993; Petrozzino et al., 1995), plus more widespread voltage-gatedinflux triggered by back-propagating action potentials (Jaffeet al., 1992; Miyakawa et al., 1992; Spruston et al., 1995). InCA3 and CA1 apical dendrites in slice cultures, this stimulationprotocol is known to evoke micromolar free Ca²⁺ transients, which decay to approximately prestimulus levels in20-30 sec (Pozzo-Miller et al., 1993; Petrozzino et al., 1995).
Fig. 3. Stimulation and recording of EPSPs in hippocampal slice cultures. A, Infrared bright-field image of 9 d in vitro hippocampalslice culture showing the placement of recording electrode inCA3 st. lucidum (asterisk) and stimulating electrode in dentategranule cells. B, Postsynaptic response to a single afferent pulseto dentate granule cells (average of 10 traces). C, Postsynapticresponse to a 1 sec, 50 Hz train of afferent pulses to dentategranule cells (single trace; stimulus artifacts were trimmed forillustration). sl, St. lucidum; sp, st. pyramidale.
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In slices in which the distribution of Ca ions was preserved by rapid freezing 3 min after a single tetanus, i.e., at a timechosen to be well after the decay of free Ca²⁺ transients, the total Ca concentration had increased to >15 mmol/kgdry weight in 40% of dendritic ER cisterns; this population ofcisterns had a mean of 41 ± 7 mmol/kg (Fig. 4). Because Ca concentrations>15 mmol/kg dry weight clearly indicate a significant increasein Ca content, we propose that the population of responsive cisternsshowing such increases represents a Ca sequestering componentof the ER. In contrast to the large increase in Ca within someER cisterns, there was no change in the Ca content of dendriticmitochondria, and only a small, statistically insignificant increasein cytoplasmic Ca after a single tetanus (Fig. 4). There was nosignificant change in any other measured element in any cellularcompartment (Table 1).
Fig. 4. Calcium sequestration in dendritic ER after synaptic activity. Histograms comparing Ca concentrations within dendritic organelles3 min after afferent stimulation reveal that Ca was sequesteredpredominantly in a responsive population of ER (1 Train, 4 Trains).Uptake into ER was graded with increased number of afferent trains(1 Train vs 4 Trains) and inhibited by blocking action potential-mediatedsynaptic transmission (4 Trains+TTX). In contrast, elemental Caconcentrations in dendritic compartments of control slices rapidlyfrozen with no afferent stimulation, either in normal ACSF orin the presence of TTX, were uniformly low (Control±TTX). (Slicesfrozen untreated and after incubation in TTX were indistinguishableand therefore were pooled.) Cytoplasmic Ca was slightly but significantlyelevated after four afferent stimulus trains; no other differencesare statistically significant (*) at p < 0.05 level.
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Three minutes after four tetani at 30 sec intervals, total Ca increased to a mean of 72 ± 8 mmol/kg in the slightly larger(45%) subset of ER cisterns that exceeded 15 mmol/kg (Fig. 4).The Ca concentrations achieved in the most avidly accumulatingcisterns approached, and even occasionally exceeded, 100 mmol/kg,a level otherwise found only in the sarcoplasmic reticulum ofskeletal muscle (Somlyo et al., 1977). Again, there was no increasein mitochondrial Ca and only a modest but statistically significantrise in cytoplasmic total Ca. The latter result suggests thatthis mode of ER sequestration is proportional to the cytoplasmicCa load, as would be expected if saturation of cytoplasmic buffersis a prerequisite to ER accumulation. Among the other elements,only Na⁺ showed significant increases (Table 1). Increases in Na⁺ content (relative to resting cultures) also occurred in otherexperiments using the four-train protocol (see below), and presumablyreflect a combination of opening Na⁺ channels by membrane depolarization (Jaffe et al., 1992), permeationthrough AMPA/kainate subtype of glutamate receptors, and enhancedactivity of the Na⁺-Ca²⁺ exchanger (Blaustein, 1988; Kiedrowski et al., 1994).

After four tetani at 30 sec intervals in the presence of 5 µM TTX, no Ca uptake occurred in any cellular compartment, includingthe ER (Table 1, Fig. 4). The TTX dependence of Ca uptake suggeststhat the observed Ca sequestration in ER is a consequence of synapticactivity. The Na⁺ elevation observed after four-train stimulation was significantlyreduced in cultures given four stimulus trains in the presenceof 5 µM TTX (Table 1). A residual increase in cellular Na⁺ after high-frequency stimulation in TTX (compared with restingcultures) may reflect the activity of TTX-insensitive Na⁺ channels (Yoshida, 1994).

Calcium sequestration only occurs in a subset of dendritic endoplasmic reticulum
Analysis of the frequency distributions of ER Ca content under different conditions of stimulation provided evidence for atleast two subpopulations of ER cisterns, only one of which wasinvolved in Ca sequestration. In resting dendrites and in dendritesstimulated in the presence of TTX, the distributions of Ca contentfor all cisterns, which presumably included both responsive andnonresponsive organelles, are well described as normal populationswith means of 3.5 ± 0.7 and 1.7 ± 0.9 mmol/kg, respectively (Fig.5A,D). In contrast, the distribution of Ca content after a singletetanus is multimodal (Fig. 5B). Nevertheless, the distributionof Ca concentrations in the ~60% of nonresponsive cisterns thatdid not exceed the 15 mmol/kg threshold still fits a normal distributionwith a mean, 3.7 ± 0.7 mmol/kg, indistinguishable from those ofunstimulated dendritic ER (Fig. 5, compare A, D with B).

As with the single afferent train, there was also a residual pool of nonresponsive ER cisterns after four tetani (Fig. 5C).The size of this pool, 55% of all cisterns, was reduced only slightlyby the recruitment of cisterns into the responsive pool, eventhough the Ca content of responsive cisterns was dramaticallyincreased (Fig. 4; also compare black bars in Fig. 5B,C); thisfurther suggests, in view of the significantly higher Ca loadafter four trains, that nonresponsive cisterns lack the capacityto accumulate or store Ca. No spatial or structural differencesbetween accumulating and nonaccumulating cisterns were apparent.It was noted that the two types of cisterns, although apparentlyrandomly distributed within dendrites, frequently occurred inclose proximity (Fig. 6).
Fig. 6. Ca-accumulating and nonaccumulating cisterns of ER. Electron micrograph of a cryosection showing a representative dendriteof CA3 st. lucidum from a rapidly frozen slice culture of hippocampus,recorded as described in legend to Figure 2. This culture wasfrozen 3 min after the last of four afferent trains. The fieldillustrates a pair of ER cisterns (arrows) that are structurallyand spatially similar, as far as can be determined in cryosections.Nevertheless, the bottom left member of the pair had a total Cacontent exceeding 70 mmol/kg dry weight, while the top right cisterncontained only 5 mmol/kg. Although the low-calcium cistern isapparently closer to the plasma membrane in this dendrite, thisis not reliably the case. Scale bar, 0.5 µm.
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Calcium sequestration in endoplasmic reticulum is reversible and dependent on a Ca²⁺-ATPase pump
Additional experiments further characterized the Ca²⁺-buffering organelles by demonstrating reversibility and identifying theuptake mechanism. In slices rapidly frozen after a recovery periodof 15-30 min after high-frequency stimulation, Ca distributions,both between compartments and within ER, were indistinguishablefrom those of resting control slices (Figs. 5E, 7). This indicatesthat the ER can unload Ca²⁺, presumably via a leak or by spontaneous Ca²⁺ release. The Ca sequestration activity of the ER was abolishedby incubation in 10 µM thapsigargin, an inhibitor of the ER Ca²⁺-ATPase (Figs. 5F, 7). Although thapsigargin at these concentrationsis known to affect voltage-gated Ca²⁺ channels (Shmigol et al., 1995), blockade of voltage-gated Ca²⁺ influx does not appear to be the major effect here, because alarge component of Ca sequestration was diverted to dendriticmitochondria. Thus, a small but significant increase, to 3.7 ±1.4 mmol/kg, was observed in the mean Ca content of mitochondrialmatrices, whereas the number of mitochondria that exhibited largefocal increases in Ca was dramatically increased (Fig. 7, Table1). These sites of elevated Ca generally appeared as dense matrixinclusions with highly variable Ca contents, frequently well inexcess of 100 mmol/kg dry weight.
Fig. 7. Reversibility and inhibition of ER calcium sequestration. Comparison of Ca concentrations within dendritic organelles at 3min (4 Trains) and 15 min (4 Trains+Rec) after four afferent stimulationtrains reveals that Ca²⁺ uptake into ER was reversible. Ca²⁺ uptake into ER was dependent on a thapsigargin-sensitive Ca²⁺-ATPase pump (4 Trains+TG). Ca accumulated within mitochondria,either diffusely within the matrix (gray bar) or in the form ofsmall inclusions (hatched bar), only when ER Ca²⁺-ATPase pumps were inhibited; under these conditions there wereno large increases in the Ca content of any other organelle. Asterisksindicate statistical significance (p <0.05) relative to 4 Trainsstimulation.
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DISCUSSION
This study provides the first direct correlation $---$ at the electron microscopic level $---$ of the concentrations of total Ca withinidentified subcellular compartments with the physiological activityof central vertebrate neurons. Our approach depended on combiningthe physiological control available in hippocampal slices, theability of rapid freezing (Van Harreveld and Crowell, 1964) toimmobilize diffusible ions in <2 msec (Heuser et al., 1979), andthe high spatial resolution of modern quantitative EDX microanalysis(Leapman and Andrews, 1991; Buchanan et al., 1993; Andrews etal., 1994). The latter is a well established technique for quantitativelymeasuring total element concentrations with submicrometer spatialresolution. Furthermore, because it detects the large fractionof Ca (>99.9% in the case of the cytoplasm) that constitutes thebound Ca pool, it provides valuable complementary informationto the free Ca²⁺ measurements obtained by optical methods using Ca²⁺-sensitive fluorescent dyes in living slice preparations.

Calcium sequestration by dendritic endoplasmic reticulum
The results demonstrate that the Ca load associated with dendritic Ca²⁺ transients persists for many minutes after the decay of thesetransients, and that in this time frame and in terms of achievableCa concentration, the ER is the dominant sequestering compartment.When viewed in terms of total Ca-binding capacity, the ER andcytoplasmic buffers appear to be approximately equal, mainly becausethe volume fraction of the cytoplas-mic compartment is so muchlarger that a sixfold increase in total cytoplasmic Ca, as observedafter four tetani, is roughly equivalent to the concomitant 20-foldincrease in the ER. Nevertheless, the Ca load attained by someER cisterns is extraordinary, reaching levels (>100 mmol/kg dryweight) that are unknown outside of the sarcoplasmic reticulumof skeletal muscle (Somlyo et al., 1977). Even so, this largeaccumulation is apparently within the range of normal physiologicalactivity for these dendrites, as indicated by the modest, parallelelevation of cytoplasmic total Ca in comparison with unstimulateddendrites, and by the reversibility of ER and cytoplasmic Ca sequestrationwhen slices were allowed a recovery period. This recovery presumablyreflects the action of slow-acting plasma membrane pumps and exchangersreturning intracellular Ca $---$ including ER Ca that unloads by equilibrationbetween ER and cytosolic free Ca²⁺ $---$ to resting levels (also see Pozzo-Miller et al., 1996). Becausethe recovery phase has a lifetime of 15-30 min, the total Ca contentwithin ER stores available for release by IP₃ and/or ryanodinereceptor signaling pathways during this time could serve as amemory trace of previous strong neuronal activity. Ca²⁺ extrusion, and not just redistribution, is most likely occurringduring the recovery period, because EDX analysis records a decreasein total Ca content integrated over all cellular compartments.

Functional heterogeneity and molecular identity of Ca-sequestering cisterns
Under conditions of Ca²⁺ entry, we observed a clear distinction between a non-normally distributed, Ca-sequestering pool ofER and a normally distributed, nonresponsive pool. The invariantCa content of the nonresponsive pool under conditions that inducelarge changes in both free and total Ca indicates that this poolis incapable of Ca accumulation or storage. It further impliesthat avid Ca accumulation in responsive cisterns occurs becausethis is a specific property of that subpopulation and not merelya consequence of variability in sampling or in dendritic activityor geometry. The heterogeneous response in stimulated dendritescannot be explained by gradients or heterogeneities in free Ca²⁺ concentrations, because responsive and nonresponsive ER cisternswere intermixed and similarly situated within the same dendriticsegments. These results add additional support to the emergingconcept (Henzi and MacDermott, 1992; Pozzan et al., 1994; Golovinaand Blaustein, 1997; Korkotian and Segal, 1997) that the ER consistsof several subtypes of spatially and functionally distinct membrane-boundorganelles, some fraction of which are specialized to play a criticalrole in Ca²⁺ regulation.

An extensive literature describes the distribution of various membrane and luminal proteins regulating Ca²⁺ homeostasis in dendrites of different brain regions and in differentspecies (for review, see Henzi and MacDermott, 1992; Pozzan etal., 1994). In the case of rodent hippocampal pyramidal dendrites,the present observation of thapsigargin-sensitive Ca sequestrationinto ER cisterns implies the presence of a SERCA pump, while thepresence of IP₃- and ryanodine-sensitive release channels hasbeen shown immunocytochemically (Sharp et al., 1993), and by opticalimaging of Ca²⁺-sensitive dyes (Seymour-Laurent and Barish, 1995; Pozzo-Milleret al., 1996; Garaschuk et al., 1997; Korkotian and Segal, 1997).Our finding that approximately half of the smooth membrane organellesstructurally identified as ER appear to function as Ca²⁺ sinks or sources is consistent, in light of recent observationsof others (Golovina and Blaustein, 1997), with the tentative identificationof dendritic Ca sequestration organelles as identical to Ca²⁺ release organelles, sequestration being an alternative functionalresponse to a different physiological demand. The remaining nonresponsiveER would then consist of molecularly different cisterns involvedin other functions, such as synthesis and transport of cell components.

The role of mitochondrial Ca sequestration
The complete dominance of ER Ca sequestration over mitochondrial uptake at 3 min after stimulation provides no support formitochondrial involvement at this rather late time but does notnecessarily contradict recent studies demonstrating a significantrole for mitochondrial Ca²⁺ buffering at early times after cytoplasmic Ca²⁺ elevation (Herrington et al., 1996; Babcock et al., 1997). Thefact that mitochondrial uptake is transient and followed by extrusionwithin 1 min after Ca²⁺ elevation (Herrington et al., 1996; Padua et al., 1996) $---$ a processthat is much faster than release from the ER $---$ is in good agreementwith our measurements of low mitochondrial Ca content 3 min afterstimulation. Nonetheless, the elevated levels of mitochondrialCa observed at 3 min after synaptic stimulation in the presenceof an ER Ca²⁺-ATPase inhibitor show that dendritic mitochondria are capableof accumulating and retaining Ca. Additionally, preliminary resultsindicate that when hippocampal slices were rapidly frozen 30 secafter a single tetanus, i.e., just after termination of the freedendritic Ca²⁺ transient (Pozzo-Miller et al., 1993; Petrozzino et al., 1995),significant Ca accumulation occurred in both mitochondria andER cisterns (Pivovarova et al., 1997). Taken together, these resultsindicate that mitochondria may well participate in dendritic Ca²⁺ clearance when their "set point" (Carafoli, 1987) for cytoplasmicCa²⁺ concentration has been exceeded during the seconds after synapticactivity but will retain Ca at later times only in the absenceof a functional ER sequestration mechanism. Considering that resultsfrom several new (Markram et al., 1995; Budd and Nicholls, 1996),as well as earlier (Somlyo et al., 1985) studies argue againstsignificant mitochondrial participation under other physiologicalconditions, more work will be necessary to understand the comparativeimportance of and interplay between these two organelles in dendriticCa²⁺ buffering.

Methodological considerations
Studies such as this one have only recently become feasible, thanks to technical advances in the development of stable organotypicslice cultures of hippocampus (Stoppini et al., 1991; Pozzo-Milleret al., 1993), as well as methodological advances in biologicalEDX microanalysis (Buchanan et al., 1993; Andrews et al., 1994).Organotypic slice cultures of deep brain structures offer theadvantage of an intact and living surface that can be studiedoptically and electrophysiologically and subsequently directlyfrozen using cold metal block techniques (Pozzo-Miller and Landis,1993; Pozzo-Miller et al., 1993). Because neuronal cell bodiesand processes, including axons, dendrites, and synapses, are presentwithin 5-20 µm of the exposed surface of such slices (L. D. Pozzo-Miller,T. S. Reese, and S. B. Andrews, unpublished observations), thesecomponents are structurally well preserved (Figs. 1, 2) and $---$ mostimportantly for this study $---$ also maintain on a millisecond timescale (Heuser et al., 1979) their native distributions of intracellulardiffusible ions (Somlyo et al., 1977).

These slice cultures are also well suited for en face cryosectioning, which, using newer sectioning techniques (Michel etal., 1992; Buchanan et al., 1993) produces uniform, truly ultrathincryosections in which even small organelles such as cisterns ofER are unambiguously recognizable (Fig. 2). After freeze-drying,these cryosections are suitable for EDX analysis, which is theprincipal established method for obtaining direct, quantitativemeasurements of the total concentrations of Ca, as well as ofseveral other physiologically important chemical elements in parallel,within identified subcellular compartments. It is important toemphasize that over the past decade there have been major technicaland instrumental advances in biological EDX analysis (summarizedby Buchanan et al., 1993; Andrews et al., 1994). These advanceshave largely eliminated the problems that plagued many early attemptsat biological microanalysis using immature techniques and instruments.Claims for the performance of modern EDX analysis are now welljustified (Leapman and Andrews, 1991; Buchanan et al., 1993),with a demonstrated sensitivity of <50 atoms of Ca in analyticalvolumes smaller than 20 × 20 × 60 nm (Andrews et al., 1994; Shiet al., 1996).

Conclusions
Ca sequestration by ER possesses several of the characteristics expected of an intracellular Ca²⁺ buffering system: (1) it is graded and dependent on neuronalactivity; (2) it is reversible, even in the extreme case of repetitivehigh-frequency stimulus trains; and (3) it is dependent on a SERCApump, implying a molecular similarity to, even possibly an identitywith, IP₃- and/or ryanodine-sensitive Ca²⁺ release organelles. Taken together, these results directly demonstratethat in CA3 dendrites specific cisterns of ER constitute the majorsubcellular compartment responsible for Ca sequestration in theminutes after neuronal activity.

FOOTNOTES

Received June 3, 1997; revised Aug. 29, 1997; accepted Sept. 8, 1997.

This work was supported by the National Institutes of Health Intramural Research Program. We thank M. F. O'Connell and J.Chludzinski for expert technical assistance, especially Ms. O'Connell'selegant cryosectioning. We also acknowledge Drs. J. A. Connorand J. J. Petrozzino for advice and equipment at the Roche Instituteof Molecular Biology, B. Lu for equipment at the National Institutesof Health, and D. M. D. Landis (Case Western Reserve University)for discussions and suggestions during the early phases of thisstudy. L.D.P.-M. also acknowledges support at the Marine BiologicalLaboratory from the Grass Foundation and the Lakian Foundation.

L.D.P.-M., N.B.P., and R.D.L. contributed equally to this manuscript.

Correspondence should be addressed to S. B. Andrews, Building 36, Room 2A-21, National Institutes of Health, Bethesda, MD20892-4062. E-mail: sba{at}helix.nih.gov

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